MEMORANDUM AND ORDER
I. INTRODUCTION
This patent infringement action concerns patents held by Amgen, Inc. (“Am-gen”), relating to the manufacture of a recombinant (genetically engineered) DNA
1
product, known as epoietin alfa,
2
that is similar to natural erythropoietin (“EPO”), a hormone that stimulates production of red blood cells, and is useful in, among other things, treating patients who need blood transfusions and suffer from blood composition disorders such as hemophilia, anemia, and sickle cell disease. This product and this case are not new to the public or to this Court. The ease began brewing in 1997, when Amgen filed a declaratory judgment in the United States District Court for the District of Massachusetts against Defendants Hoechst Marion Roussel, Inc.
3
and Tran-skaryotic Therapies, Inc. (collectively “HMR/TKT”) claiming that three of its patents were infringed by HMR/TKT’s human EPO product, “HMR 4396,” produced from the R223 cell line grown in culture.
See Amgen, Inc. v. Hoechst Marion Rous-sel, Inc.,
II. BACKGROUND: PROCEDURAL AND SUBSTANTIVE HISTORY
A. The Patents, at Issue
There were originally five patents at issue in this case. Only four, however, remain on remand. The patents and claims now at issue are: Claim 1 of U.S. Patent No. 5,955,422 (issued Sept. 21, 1999) (“ ’422 patent”); Claims 2-4 of U.S. Patent No. 5,621,080 (issued Apr. 15, 1997) (“ ’080 patent”); Claims 4-9 of U.S. Patent No. 5,618,698 (issued Apr. 8, 1997) (“ ’698 patent”); and Claims 1, 3, 4, 6, and 7 of U.S. Patent No. 5,756,349 (issued May 26, 1998) (“ ’349 patent”).
Amgen I,
*214
Although the patents vary, they all share a common disclosure and identical specifications.
Amgen I,
B. The Technology
As
Amgen I
set out the basics of the underlying technology in detail, only a brief summary is provided here. EPO is a naturally occurring hormone that controls erythropoiesis, the production of red blood cells in bone marrow. ’933 Patent, Ex. 1, col. 5: 39-67. Erythropoiesis occurs continuously to offset cell destruction.
Id.
It enables a sufficient (but not excessive) amount of red blood cells to be available in the blood to provide tissue oxygenation.
Id.
Hemoglobin is the protein in the red blood cells that actually transports the oxygen.
Amgen I,
EPO is produced in the kidney and liver. Therefore, patients with chronic renal failure lack normal levels of EPO and suffer from anemia.
Amgen II,
Early attempts to obtain EPO from plasma or urine proved unsuccessful 'because the body only produces human EPO in very small amounts, ’933 Patent, Ex. 1, col. 5: 54-58, and the techniques were very complicated and resulted in the collection of very small amounts of impure and unstable amounts of EPO, id. at col. 6: 60-65. Amgen is recognized as the pioneer in the production of a therapeutically effective amount of EPO via recombinant EPO (“rEPO”) techniques. See, e.g., Molecular Biology and Biotechnology: A Comprehensive Desk Reference 108 (Robert A. Meyers ed., VCH Publishers 1995).
Dr. Fu-Kuen Lin (“Lin”), the named inventor of all the patents in issue, isolated and characterized DNA sequences encoding EPO from humans and monkeys. ’933 Patent, Ex. 1, col. 13: 50-53. Lin determined the DNA sequence of human EPO and its predicted amino acid sequence. ’933 Patent, Ex. 1, col. 10: 65-11: 2. Lin then produced large amounts of EPO by using recombinant DNA technology. Id. at col. 14: 23-29. In the patent specification, many methods of producing EPO are described. EPOGEN® is pro *215 duced by the method described in Example 10, wherein human EPO is produced by introducing exogenous DNA into host Chinese hamster ovary (“CHO”) cells. Id. at col. 25: 30-29: 7. 6 The rEPO that is produced has the same or similar amino acid sequences or primary structural conformation as that of naturally-occurring EPO. Id. at col. 29: 1-7. As a result, it possesses one or more the biological properties of naturally-occurring EPO but differs from natural EPO in its “glycosylation,” that is, it has a different average carbohydrate composition. Id. at col. 10: 35-41.
HMR/TKT, in producing its human er-ythropoietin, HMR 4396 (also called Gene-Activated EPO “GA-EPO”), also uses recombinant technology. HMR/TKT, however, does not use a host cell from a nonhuman species but manipulates the ordinarily unexpressed human EPO gene where it naturally resides.
Amgen I,
C. The Federal Circuit’s Decision
A brief review of the key rulings and findings that were affirmed and remanded on appeal follows:
1. Claim Construction
a. Affirmed
The Federal Circuit upheld all of the Court’s claim constructions.
Amgen II,
The Federal Circuit also upheld the Court’s determination that claim 1 of the ’422 patent, claims 2, 3, and 4 of the ’080 patent, and claims 1, 3, 4, and 6 of the ’349 patent are product claims (not process claims) and thus are not restricted or defined by any method of production or any particular source, other than what is specifically excluded.
Amgen II,
b. Remanded
Although all the terms that this Court construed in
Amgen I
under the principles of
Markman v. Westview Instruments, Inc.,
2. Infringement
a. Affirmed
The Federal Circuit affirmed this Court’s ruling on summary judgment that claim 1 of the ’422 patent is literally infringed.
Amgen II,
b. Remanded
(1) The ’080 Patent
After finding that HMR 4396 did not literally infringe claims 2, 3, and 4 of the ’080 patent because HMR 4396 comprised only 165 amino acids,
Amgen I,
In response to HMR/TKT’s argument that Amgen should be estopped from arguing equivalent infringement, this Court ruled that prosecution history estoppel did not apply because Amgen did not add the “mature amino acid sequence of Figure 6” limitation “in an attempt to overcome a rejection [or] to avoid prior art,” but, instead, to “demonstrate that ‘same invention’ type double patenting did not apply,” — that is, to distinguish the ’080 patent from the ’933 patent. Id. at 134-35.
The Federal Circuit agreed that the amendment was made for this purpose but made clear that under
Festo Corp. v. Shoketsu Kinzoku Kogyo Kabushiki,
(2) The ’698 Patent
On appeal, the Federal Circuit vacated and remanded this Court’s ruling regarding infringement of the ’698 patent because this Court had compared the accused device to the preferred or commercial embodiments of the patent instead of to the properly construed claims themselves.
Amgen II,
(3) The ’349 patent
Although this Court found that claims 1, 3, 4, and 6 of the ’349 patent are literally infringed by HMR/TKT’s 4396, it held that HMR/TKT did not literally or equivalently infringe claim 7, the process claim, of the ’349 patent.
Amgen I,
3.Inequitable Conduct
The Court’s determination that HMR/ TKT had not proven by clear and convincing evidence that the ’933, ’080, ’349 and ’422 patents were unenforceable due to inequitable conduct was affirmed on appeal.
Amgen II,
4. Written Description, Definiteness, and Enablement
a. Affirmed
The Federal Circuit affirmed this Court’s rulings that the ’422, ’080, and ’349 patents are adequately described and enabled. Id. at 1337. In so ruling, the Federal Circuit explained that this Court “carefully considered these issues, finding in the end that HMR/TKT had not met its clear and convincing burden of proof.” Id. Because the Federal Circuit found “no clear error in these factual determinations,” and the parties did not allege any legal error, it reasoned that it would “not disturb [this Court’s] holding that the asserted patents are not invalid for failure to meet the enablement requirement of § 112 ¶ 1.” Id.
As mentioned in an earlier footnote,
see
note 3,
supra,
this Court held and the Federal Circuit affirmed that the ’933 patent (specifically the claims requiring “gly-cosylation which differs”) was invalid for indefiniteness under section 112.
Amgen I,
5. Anticipation and Obviousness
a. Affirmed
The Court’s ruling that the asserted claims of the ’080, ’349, and ’933 patents are not anticipated under 35 U.S.C. § 102 by the Sugimoto reference was affirmed by the Federal Circuit. Id. at 1320, 1356. 8 *218 In affirming, however, the Federal Circuit made clear that the Court’s determination that Sugimoto was not enabled was an error, though harmless, because the Court put the burden of proving enablement of Sugimoto on HMR/TKT when the burden of proving non-enablement should have been put on Amgen. Id. at 1356. 9
b. Remanded
The Federal Circuit remanded, however, the Court’s findings that Sugimoto does not anticipate claim 1 of the ’422 patent stating that the “district court should consider whether claim 1 of the ’422 patent is novel over Sugimoto in light of the court’s new definition of ‘therapeutically effective’ ” and be “mindful of the principle that source limitations cannot impart novelty to old compositions.” Id. at 1356. 10 Additionally, the Federal Circuit remanded this Court’s finding that the ’422, ’080, and ’349 patents were not obvious in light of Sugi-moto because this Court based its decision, in part, on the fact that it concluded that Sugimoto was not enabled. Id. at 1357. The Federal Circuit explained that under section 103, a reference need not be enabled to qualify as prior art. Id.
In
Amgen I,
this Court found that the asserted claims of the ’080, ’422 and ’349 patents were not anticipated or rendered obvious by the Goldwasser reference.
Amgen I,
D. Procedural and Substantive History Since Amgen II
The Federal Circuit’s decision issued on January 6, 2003. This Court received the action on remand on March 13, 2003 [Doc. No. 653], and it held a status conference on April 16, 2003 [Doc. No. 657]. On May 16, 2003, Amgen moved for: (1) judgment under Federal Rule of Civil Procedure 52(c) that claims 2-4 of the ’080 patent were infringed under the doctrine of equivalents [Doc. No. 659]; (2) summary judgment of infringement of claims 4-9 of the ’698 patent [Doc. No. 663]; (3) judgment pursuant to Rule 52(c) that claim 1 of the ’422 patent and claim 4 of the ’080 patent are valid [Doc. No. 670]; and (4) judgment pursuant to Rule 52(c) that claims 1, 3, 4, 6, and 7 of the ’349 patent are valid and that claim 7 of the ’349 patent is infringed [Doc. No. 674]. HMR/TKT simultaneously moved for: (1) judgment that Amgen is estopped from asserting infringement of the ’080 patent pursuant to the doctrine of equivalents [Doc. No. 678]; (2) judgment that claim 1 of the ’422 patent is invalid as *219 anticipated [Doc. No. 682]; (3) judgment pursuant to Rule 52(c) that the asserted process claims of the ’698 patent and ’349 patents are not infringed [Doc. No. 686]; and (4) judgment that the ’422, ’080, and ’349 claims are invalid for obviousness [Doc. No. 690],
The memoranda in support of and in opposition to these motions raised additional issues that are reviewed in this opinion. They are described briefly below.
In its opposition to Amgen’s renewed motion for summary judgment of infringement of the ’698 patent, 11 HMR/TKT argued, among other things, that Amgen’s proposed construction of the words “DNA encoding” found in claims 4 and 6 of the ’698 patent is incorrect. HMR/TKT’s Mem. in Opp’n re ’698 [Doc. No. 700] at 7-8. Second, HMR/TKT argued that in claims 4 and 6 of the ’698 patent, Amgen set forth a step-plus-function claim in referring to the “steps of ... growing, under suitable nutrient conditions” and that an assessment of whether HMR/TKT infringed this aspect of the claim must focus on a comparison between HMR/TKT’s process for growing and the process for growing described by Amgen in the specification. Id. at 9. Finally, HMR/TKT argued that even if there is literal infringement here, it can justifiably invoke the defense of the reverse doctrine of equivalents. Id. at 13. 12
With regard to claim 7 of the ’349 patent, HMR/TKT made four “new” arguments, two of which are very similar to those made in conjunction with the ’698 patent. First, HMR/TKT contended that its process does not infringe claim 7 of the ’349 patent when considered in light of its proposed claim construction of “DNA encoding.” HMR/TKT’s Mem. in Support re ’698/’349 [Doc. No. 687] at 8-9. Second, HMR/TKT argued that its process does not infringe claim 7 of the ’349 patent because claim 7 is a step-plus-function limitation; and, as such, HMR/TKT’s process does not literally infringe the “step of culturing” found in claim 7 because it does not involve the culturing procedures set forth in Amgen’s specification. Id. at 12-15. Third, HMR/TKT claimed that its process does not infringe the process claim under the reverse doctrine of equivalents. Id. at 15-18. Fourth and lastly, HMR/ TKT argued that if the Court construes the term “DNA encoding” as Amgen urges, then the validity of the asserted claim of the ’349 patent is called into question. Id. at 12.
Amgen, in response, did not dispute that “DNA encoding” needs to be construed by the Court. See, e.g., Amgen’s Reply re ’698 [Doc. No. 731] at 6-10. It did, however, assert that HMR/TKT should not be allowed to make its “new” arguments relating to step-plus-function and the reverse doctrine of equivalents given the procedural posture of the case. 13 See, e.g., id. at 10-15.
*220 On July 29, 2003, this Court held a Markman hearing regarding those terms in dispute and in need of construction and considered other pending motions, including motions for summary judgment. At the end of the Markman portion of the hearing, the Court tentatively construed the terms “DNA encoding” and “therapeutically effective,” providing two constructions for the latter, one being an alternate. 7/29/03 Hr’g Tr. at 55: 1-56: 23. It then continued to hear argument. At the end of the day, the Court noted that it would determine whether the asserted claims of the ’698 and ’349 patents were step-plus-function claims at a later date. Id. at 176: 1-10. It then continued the motion hearing to July 31, 2003. Id. at 176: 11-15.
During a hearing two days later, the Court retracted the alternative construction and reiterated its primary “working construction,” retaining its right to revise it after a more careful review of the claims, specification, and prosecution history. 7/31/03 Hr’g Tr. at 87: 5-88: 7. Additionally, it ruled that claims 4 and 6 of the ’698 patent and claim 7 of the ’349 patent were not step-plus-function claims pursuant to 35 U.S.C. § 112. Id. at 88: 8-89: 9. It then denied Amgen’s motion for summary judgment of infringement of the ’698 patent, citing Arthur Miller’s recent article, The Pretrial Rush to Judgment. Id. at 89: 23-90: 25; see Miller, supra. The Court took everything else under advisement and set the final pretrial conference for September 18, 2003. Id. at 91: 25-92: 2.
On August 5, 2003, the Court entered an order regarding the pending motions. [Doc. No. 740], It denied HMR/TKT’s motions for summary judgment with respect to the validity of the asserted claims of the ’422, ’080 and ’349 patents. Order of 8/5/03 at 1. It denied in part and allowed in part Amgen’s motions, under Rule 52(c), for judgment that claim 1 of the ’422 patent and claim 4 of the ’080 patent are valid and that claims 1, 3, 4, 6, and 7 of the ’349 patent are valid. Id. Because HMR/TKT did not dispute that the ’080 and ’349 patents are not anticipated by Goldwasser and that the ’349 patent is not rendered obvious by Goldwasser, the Court allowed Amgen’s motions with respect to these matters. Id. at 1-2. Specifically, the Court held that claim 4 of the ’080 patent is not anticipated by Goldwasser and that claims 1, 3, 4, 6, and 7 of the ’349 patent are not anticipated or rendered obvious by Goldwasser. Id. at 2. Because Amgen did not have the opportunity to rebut HMR/ TKT’s remaining validity arguments concerning the ’422, ’080, and ’349 patents during trial in 2000, the Court stated that Amgen would have that opportunity at the October trial. Id.
On September 18, 2003, the Court held a final pretrial conference. After explaining that this case will not “turn into a patent version of Penelope’s robe,” in other words, that the Court and the parties were “not going to unravel anything [that the Court has] woven thus far which has not been unraveled by a higher court,” the Court made the following findings and rulings. First, it ruled that it would hear and take evidence on the reverse doctrine of equivalents as it related to the ’698 patent and that HMR/TKT could address other patent defenses. 9/18/03 Final Pretrial Conf. Tr. at 6: 4-16. Second, it ruled that Amgen had met its burden (outlined in Festo II) of proving that the prosecution history does not estop it from arguing equivalent infringement with regard to the ’080 patent and it affirmed its earlier *221 finding that HMR/TKT infringes claims 2-4 of the ’080 patent. Id. at 7: 17-8: 5. It explained that it would issue a full opinion at a later date but that it might have to revisit the Festo issue due to the rapidly-developing law in that area. Id. at 7: 19-25. The Court then turned to the ’349 patent and explained that it would allow Amgen to put on rebuttal evidence as to the matter of obviousness and Sugimoto only and it made clear that the Court would not accept other evidence from HMR/TKT regarding the ’349 patent. Id. at 8: 12-19, 16: 5-6 (“As far as evidence goes, ’349 is in the can and I’m done with it.”). The Court then issued a revised claim construction of “therapeutically effective” based on a more thorough analysis of the claims, specification, and prosecution history. Id. at 9: 3-10: 25. The Court mentioned, however, that this revision may have made the third sentence of the construction unnecessary and, therefore, reserved its right to further consider the proper construction. Id. at 10: 21-25. It directed the parties to try the case based on the construction it had just issued along with a construction that eliminated the third sentence. Id. at 11: 1-5. The pretrial conference was continued until September 24, 2003. Id. at 30: 22-23.
During the further pretrial conference, the Court reviewed the issues to be tried and outlined the procedure for trial and the parameters for the introduction of evidence and expert testimony. See 9/24/03 Final Pretrial Conf. Tr. After the Court provided both parties with an opportunity to be heard on the subject, pursuant to Federal Rule of Civil Procedure 53(b)(1), the Court appointed Michele D. Beardslee as Special Master, beginning January 1, 2004, to assist the Court in research, analysis, and drafting of the forthcoming opinion. Order re Special Master [Doc. No. 801]; see also 11/07/03 Beardslee Aff. [Doc. No. 799]. 14 The trial on remand was set to commence on October 7, 2003. 9/24/03 Final Pretrial Conf. Tr. at 40: 23.
On October 30, 2003, the Court issued an opinion supporting its ruling that Am-gen had successfully rebutted the presumption of prosecution history estoppel as outlined in
Festo II
and, therefore, was not estopped from asserting equivalent infringement of the ’080 patent.
Amgen, Inc. v. Hoechst Manon Roussel, Inc.,
The remanded trial lasted nine days over the course of four and a half weeks. 16 *222 All the remaining issues — those remanded to the Court from the Federal Circuit and those raised by the parties in the course of this remanded trial — are addressed herein. 17
III. CLAIM CONSTRUCTION
As expounded in great detail in
Amgen I,
this Court strongly believes in the importance of construing patent claims without regard to the alleged infringement issues.
Amgen I,
The Court followed its usual procedure in conducting the Markman hearing. The Court entertained oral argument from counsel for each party. Counsel referred the Court to the relevant portions of the patent, specification, and prosecution history. Demonstrative exhibits were presented and references were made to certain expert testimony, but extrinsic evidence was not admitted.
At the conclusion of the Markman portion of the hearing the Court interpreted “therapeutically effective” and “DNA encoding”' — cautioning that they were “working constructions” — and held off deciding whether the asserted claims of the ’349 and ’698 patent were step-plus-function claims. The Court then announced during the July 31, 2003 hearing that it did not construe the asserted claims of the ’349 and ’698 patents as step-plus-function claims. During the pretrial conference on September 18, 2003, after the Court had engaged in a more careful review of the patents, specification, and prosecution history, the Court issued a revised claim construction for “therapeutically effective.” The final claim constructions are reproduced and explained below. 18
A. “Therapeutically Effective”
1. Background
The term “therapeutically effective” is contained in claim 1 of the ’422 patent and claim 4 of the ’080 patent. 19 As *223 mentioned above, although this phrase was not construed during the first trial, in determining whether prior art anticipated the ’422 and ’080 patents, the Court interpreted the term to mean an increase in hematocrit:
Such evidence [of e.g., increased eryth-roid marrow stimulation] should be outweighed by the fact that the actual production of mature red blood cells was not achieved and, as a result, hematocrit levels were unchanged. Because an increase in hematocrit and hemoglobin levels is the true mark of therapeutic effectiveness, Dr. Goldwasser’s study, which revealed only inchoate indicators of red blood cell production, falls far short of anticipating claims requiring a therapeutic amount of human EPO.
Amgen I,
The Federal Circuit, in addition to remanding so that the Court could construe the term pursuant to
Markman,
provided some guidance. It agreed that the “endgame in the treatment of chronically anemic patients is to increase the hematocrit,” but pointed out that the term should be construed in light of the specification.
Amgen II,
2. The Claims at Issue
The actual words of the claims are as follows:
*224 ’422 Claim 1: A pharmaceutical composition comprising a therapeutically effective amount of human erythropoietin and a pharmaceutically acceptable diluent, adjuvant or carrier, where insaid erythropoietin is purified from mammalian cells grown in culture.
’422 Patent, Ex. 1, col. 88: 36-41 (emphasis added). 21
’080 Claim 4: A pharmaceutical composition comprising a therapeutically effective amount of an erythropoietin gly-coprotein product according to Claim 1, 2, or 3.
’080 Patent, Ex. 1, col. 38: 51-53 (emphasis added).
3. Summary of the Parties’ Arguments
Amgen urges adoption of the ordinary meaning of “therapeutically effective” given by those skilled in the art. Amgen’s Mem. in Support re ’422/’080 [Doc. No. 671] at 7. Specifically, it argues that (1) expert testimony shows that the ordinary meaning of “therapeutically effective” is “sufficient to produce a sustained increase in hematocrit,” and that the term requires a therapeutic — not merely biological — effect; (2) the other effects listed in the specification, to which the Federal Circuit referred, are known biological effects of EPO, not the intended therapeutic effects; (3) the specification taken as a whole supports the plain meaning of “therapeutically effective,” and that no special meaning was given to the term; (4) the prosecution history shows that Amgen specifically noted that its invention shares the same in vivo biological activity as naturally occurring human EPO, but differentiated its invention from prior art by pointing out that human recombinant EPO (unlike naturally-occurring human EPO) is not a viable, effective human therapeutic product; and (5) the doctrine of claim differentiation requires that this term have a different meaning than the recitation of EPO’s biological activities. Id. at 8-17. In its reply memorandum, Amgen also argues that the dictionary definition of the term supports its asserted meaning. Amgen’s Reply re ’422/’080 [Doc. No. 730] at 5-6.
HMR/TKT, on the other hand, argues that the Federal Circuit made clear that it believed that the term “therapeutically effective” encompasses all of the effects set forth in the specification described. HMR/ TKT’s Mem. in Opp’n re ’422/’080 [Doc. No. 702] at 5. Thus, it argues, the term encompasses those effects observed in the Goldwasser study. Id. at 6. Moreover, it asserts that Amgen is trying to import limitations from the specification to make the claims require an increase in the he-matocrit levels when the claims contain no language indicating such a requirement and the specification language itself is actually inconsistent with such a requirement. HMR/TKT points to the same section of the specification as did the Federal Circuit did to make its point:
[T]o the extent that polypeptide products of the invention share the in vivo activity of natural EPO isolates they are conspicuously suitable for use in erythropoietin therapy procedures practiced on mammals, including humans, to develop any or all of the effects herefore attributed in vivo to EPO, e.g., stimulation of reticulocyte response, development of ferrokinetic effects ... erythrocyte mass changes, stimulation of hemoglobin C syntheses ... and, as in *225 dicated in Example 10, increasing he-matocrit levels in mammals.
Id. at 13 (quoting ’933 Patent, Ex. 1, col. 33: 19-31). This, HMR/TKT asserts, makes clear that “erythropoietin therapy procedures” include procedures that “develop any or all of the effects heretofore attributed in vivo to EPO,” and, therefore, “therapeutically effective amount” includes any or all of the effects listed in this portion of the specification — which, HMR/ TKT argues, are defined in terms of biological effects. Id. at 14. HMR/TKT further argues that Amgen is trying to rely on isolated references of the specification to restrict the term meaning when these restrictions are not apparent in the plain language, and when the intrinsic record, as a whole, supports a broader interpretation. Id. at 16.
4. Discussion
While the Federal Circuit indeed mentioned that the term “therapeutically effective” appeared to encompass the biological effects listed within lines 19-31 of column 33, the Court notes that the Federal Circuit did not, in
Amgen II,
actually construe the term “therapeutically effective.”
See Amgen II,
a. The Plain and Ordinary Meaning
Generally, it is the plain and ordinary meaning of the words — as defined by one skilled in the relevant art — that governs.
Vitronics,
Amgen, on the other hand, grounds its assertion of the plain and customary meaning of the disputed term upon expert testimony. This, however, is extrinsic evidence to which resort ought be had only
“if necessary.” Vitronics,
*228 The dictionary definition of “therapeutic” is “[h]aving healing or curative powers,” or “[o]f or relating to the treatment of disease or disorders by remedial agents or methods.” The American Heritage Dictionary 1260 (2d college ed.1985); Webster’s Ninth New Collegiate Dictionary 1223 (1984), attached as Tab X to Supp.App. [Doc. No. 735] to Amgen’s Reply re ’422/’080; see also Chamber’s Technical Dictionary 844 (3d ed.1961), attached as Tab W to Supp.App. to Amgen’s Reply re ’422/’080 (“Of, or pertaining to, the medical treatment of disease: remedial: curative”). The definition of therapeutics is “[t]he medical treatment of disease.” The American Heritage Dictionary, supra, at 1260. The dictionary definition of “effective” is “[h]aving an intended or expected effect” or “[pjroducing or designed to produce the desired impression or response.” Id. at 439.
Based on these definitions alone, one would surmise that a “therapeutically effective” amount is one that produces healing or curing as it relates to medical treatment of disease. 24 This is, in essence, consistent with the definition that Amgen proposes. See Amgen’s Mem. in Support re ’422/’080 [Doc. No. 671] at 14 (arguing that the ordinary meaning is an amount sufficient to “cure or relieve a disease state” and “require[s] a meaningful benefit to the health of patients”). Amgen, however, goes further, asserting that the plain and ordinary meaning of “therapeutically effective amount,” to one skilled in the art, taken in the context of this patent, is an amount that provides more than the biological effects of EPO and “produce[s] a *229 sustained increase in hematocrit,” because only this result provides a meaningful benefit to the health of patients suffering from anemia. 25 Id. at 7-8, 14. Neither the claims, the specification, nor the prosecution history, however, demonstrate clearly that the plain and ordinary meaning of the term to one skilled in the art involves an increase in hematocrit. Therefore, the Court begins with the assumption that the plain and ordinary meaning of “therapeutically effective amount” is one in line with that found in the dictionaries and treatises noted above — i.e., one that heals or cures as it relates to medical treatment of disease.
The next step is to look to the claims, specification, and prosecution history to see if Amgen redefined the term in the file wrapper. In addition, the Court will look to these sources to determine whether the file wrapper indicates clearly the types of patients for which this product is “therapeutically effective” and thus infuses the term with real meaning. Indeed, this is the elephant in the room. Without tackling this question, the term “therapeutically effective” or “therapeutically effective amount” is vague and meaningless. The public must know upon reading the patent what disease state is cured or healed by the product.
26
As the Federal Circuit pointed out, “indiscriminate reliance on definitions found in dictionaries can often produce absurd results.... One need not arbitrarily pick and choose from the various accepted definitions of a word to decide which meaning was intended .... The subject matter, the context, etc., will more often than not lead to the correct conclusion.”
Renishaw PLC v. Marposs Societa’ per Azioni,
b. The Claims
“The name of the game is the claim.”
Amgen I,
Do the claims redefine the plain and ordinary meaning of the terms used? Am-gen asserts that the claims do not support HMR/TKT’s argument that it has redefined the term to include the biological effects of EPO. Amgen asserts that be
*230
cause claim terms are construed to give each term meaning,
Lantech, Inc. v. Keip Mack Co.,
’080 Claim, 4: A pharmaceutical composition comprising a therapeutically effective amount of an erythropoietin gly-coprotein product according to claim 1, 2, or 3.
’080 Claim 2: An isolated erythro-poietin glycoprotein having the in vivo biological activity of causing bone marrow cells to increase production of reti-culocytes and red blood cells, wherein said erythropoietin glycoprotein comprises the mature erythropoietin amino acid sequence of FIG. 6 and is not isolated from human urine.
Amgen asserts that under the doctrine of claim differentiation, claim 4 of the ’080 patent must not include any or all of the effects listed in the specification because otherwise claim 4 would be identical to that of claim 2. Specifically, it points out that claim 4 of the ’080 patent requires “[a] pharmaceutical composition comprising a therapeutically effective amount” of EPO according to claim 1, 2, or 3. Amgen’s Mem. re ’422/’080 at 15-16. It then asserts that the claim 2 requires the “in vivo biological activity of causing bone marrow cells to increase production of reticulocytes and red blood cells.” Therefore, if “therapeutically effective” included the effects listed in the specification to which the Federal Circuit pointed, Amgen argues, it would include the in vivo biological activity cited by claims 1, 2, or 3 of the ’080 patent and render claim 4 of the ’080 patent superfluous. Id. at 16.
As HMR/TKT urges, however, this argument is flawed because claim 4 concerns a pharmaceutical composition comprising a “therapeutically effective amount” of an EPO that happens to have the qualities described in claim 2. HMR/TKT’s Opp’s re ’422/’080 at 22. HMR/TKT correctly points out that claim 2 recites an isolated EPO glycoprotein and therefore refers to biological effects whereas claim 4 recites a pharmaceutical composition and involves therapeutic effects. Id. at 21-22. Hence, claim 2 would not be rendered superfluous if this Court construed “therapeutically effective” to include the biological effects listed in the specification. Id. at 22.
Another equally flawed argument is that claim 4, by encompassing claim 2 (in referring to a “therapeutically effective” amount of the product claimed in claim 2), indicates that a
“therapeutically effective
amount” is one that does more than cause the in vivo biological activities described in claim 2. After a careful review of the technology and its history, it is clear that this is not a correct reading of the claims. This review relied on extrinsic evidence, as is permissible under Federal Circuit precedent.
Vitronics,
*231 Before Amgen’s invention, human EPO was known to elicit certain biological effects, but it was impossible to extract an efficient amount of it for use in treatment of patients with anemias and other low red blood cell disorders. Amgen invented a product, recombinant EPO, that had the same in vivo biological effects as natural EPO but differed in its carbohydrate composition and was capable of manufacture in quantities large enough to provide effective treatment.
With this understanding of the technology, it is clear that claims 2 and 4 of the ’080 patent, by themselves, do not define “therapeutically effective” beyond its plain and ordinary meaning, nor do they indicate that a “therapeutically effective amount” of EPO is one that does more than elicit the biological effects noted in claim 2. Instead, claim 2 stakes out Am-gen’s novel recombinant EPO that has the same in vivo biological activities of natural EPO (causing bone marrow cells to increase production of reticulocytes and red blood cells). Claim 4 sets out a pharmaceutical composition that has a novel amount of the EPO — an amount that can actually treat or cure patients. Notably, these claims do not indicate whether biological effects are themselves sufficient to treat or cure patients.
Similarly, the claims of the ’422 patent do not define a “therapeutically effective amount” as one that does something above and beyond eliciting the biological effects of EPO listed in the specification.
The next question is whether the claims themselves indicate for what types of patients this product is “therapeutically effective.” Amgen contends that its EPO is specifically designed for those suffering from anemias and thus only an increase in hematocrit is “therapeutically effective.” Indeed, the record shows that Amgen’s product
can
be used to increase levels of hematocrit, in other words, it
can
be used to “cure” or “relieve” the diseased state brought on by anemia.
Amgen I,
The problem with Amgen’s argument, however, is that the claims that contain the disputed term do not themselves include a limitation directed to the specific clinical benefit of correcting anemia. Therefore, the plain and ordinary meaning of “therapeutically effective” cannot be limited to curing anemia, i.e., producing an increase in hematocrit levels based on the claims *232 alone. The claim language simply does not allow for such a specific interpretation. This conclusion is further supported by the fact that claim 6 of the ’080 patent (unlike claim 4) does indeed specify the type of treatment (kidney dialysis) for which the EPO should be used and calls out, in that context, that an effective amount is one that increases hematocrit:
’080 Claim 6: A method for treating a kidney dialysis patient which comprises administering a pharmaceutical composition of claim 4 in an amount effective to increase the hematocrit level of said patient.
’080 Patent, Ex. 1, col. 38: 57-60. Had Amgen used similar claim language in claim 4 — that is, had it referred specifically to anemia — then its argument would have merit. Based on the non-specific language of claim 4, however, this argument fails.
In sum, the claim language supports only the plain and ordinary definition of “therapeutically effective” — an amount that produces a result that, in and of itself, helps to heal or cure. The language of the claims at issue does not delineate the type of disease for which the EPO is “therapeutically effective.” Therefore, the Court must now turn to the specification and the prosecution history to determine whether Amgen has limited or altered the plain meaning of the term either by defining the term or specifying the disease states for which the product is intended.
c. The Specification
The second step in claim construction is to review the specification to determine whether the patentee has used terms in a manner inconsistent with the ordinary meaning or has become his own lexicographer.
Vitronics,
The part of the specification to which the Federal Circuit in Amgen II pointed is as follows:
Similarly, to the extent that polypeptide products of the invention share the in vivo activity of natural EPO isolates they are conspicuously suitable for use in erythropoietin therapy procedures practiced on mammals, including humans, to develop any or all of the effects herefore attributed in vivo to EPO, e.g., stimulation of reticulocyte response, development of ferrokinetie effects (such as plasma iron turnover effects and marrow transit time effects), erythrocyte mass changes, stimulation of hemoglobin C synthesis (see, Eschbach, et al., supra) and, as indicated in Example 10, increasing hematocrit levels in mammals.
’933 Patent, Ex. 1, col. 33: 19-31 (emphases added).
The Court begins by analyzing whether this section defines therapeutically effective to include the effects listed above. It is undisputed that this section declares that Amgen’s recombinant EPO is similar to natural EPO in that it shares some of the same in vivo activity. Id. at col. 33: *233 19-22. “[T]o the extent ” that it does so— to the extent that it is similar to natural EPO — Amgen’s EPO are “conspicuously suitable for use in erythropoeitin therapy procedures” to develop any or all of the effects that were “herefore” (before) attributed in vivo to EPO, such as the stimulation of reticulocyte response, development of ferrokinectic effects, erythrocyte mass changes, and stimulation of hemoglobin C synthesis. What is unclear and disputed, however, is whether the section that begins with “and, as indicated in Example 10, increasing hematocrit levels in mammals” is part of the laundry list of effects previously attributed in vivo to EPO or a separate suitable use for the product. In other words, this portion of the specification can be interpreted one of the following two ways:
1) Amgen’s EPO is “conspicuously suitable for use in erythropoietin therapy procedures practiced on mammals, including humans, to develop any or all of the effects herefore attributed in vivo to EPO, e.g., stimulation of reticulocyte response, ... and, as indicated in Example 10, increasing hematocrit levels in mammals.”
2) Amgen’s EPO is “conspicuously suitable for” (a) “use in erythropoietin therapy procedures practiced on mammals, including humans, to develop any or all of the effects herefore attributed in vivo to EPO, e.g., stimulation of reticulocyte response, ...” and, (b) “as indicated in Example 10, increasing hematocrit levels in mammals.”
The former interpretation — a direct quote of the specification — suggests that an increase in hematocrit level was an effect previously attributed to natural EPO and that it, along with the biological effects, are a type of effective therapy. In other words, it includes “increasing the hematocrit levels” as
one of the many effects
of EPO that were previously identified and that are now produced by this product and useful in “erythropoietin
therapy
procedures.” The problem with this reading is that the intrinsic evidence (the claims, the specification, and the prosecution history) and extrinsic evidence suggest that an increase in hematocrit levels was
not
previously attributed to natural EPO.
29
In remarks following an amendment made during prosecution of the ’080 patent, Amgen explained to the Patent, and Trademark Office (“PTO”) that Example 10 is novel in that it is the first therapeutic procedure ever practiced with EPO to demonstrate that EPO has the capacity to generate an increase in hematocrit in vivo. Amgen’s ’422/’080 App., Tab G (Ex. 2), at Tab 6, at 179. The extrinsic record also suggests that an increase in hematocrit was not previously attributed to natural EPO.
Vitronics,
The latter interpretation — and the one that the Court adopts — suggests that an increase in hematocrit is independent or different from the in vivo effects previously attributed to natural EPO. In other words, in this section, Amgen calls out that its recombinant EPO can elicit “any or all” of the effects that natural EPO does — and more. Admittedly, the use of the words “therapy procedures” supports the interpretation that a “therapeutically effective amount” encompasses an amount that would result in the biological effects because it implies that the effects are a part *234 of therapy. That being said, however, the way in which the increase in hematocrit is set off from the rest of the language suggests that this product elicits something in addition to what the prior art elicited, something more than the biological effects. Moreover, it makes clear that “any or all” only modifies those effects previously attributed to natural EPO — not the increase in hematocrit. Indeed, if the phrase “as indicated in Example 10, increasing hemat-ocrit levels in mammals” were merely an item in the list of “any or all of the effects herefore attributed in vivo to EPO,” then the words “in mammals” would be redundant. The list of items refers to “effects herefore attributed in vivo to EPO” for “use in erythropoietin therapy procedures practiced on mammals ”, so “increasing hematocrit levels in mammals ” must be a second end for which Amgen’s EPO is “conspicuously suitable.”
This interpretation comports with the Court’s understanding — developed over the course of two intensive trials — of what hematocrit actually measures. Hematocrit measures the ability of the blood to supply oxygen to the body. It indicates the relative proportion of red blood cells to the total volume of blood. By introducing additional EPO into the patient’s body, a patient’s hematocrit level can be increased to and sustained at or near normal levels. In other words, the blood is able to provide a steady supply of sufficient oxygen to the tissues. It is the Court’s understanding that, in most cases, an increase in hemato-crit is accompanied, if not preceded, by “any or all” of the biological effects listed in the specification. 30 In other words, this portion of the specification explains what happens when a “therapeutically effective amount” of EPO is used — that is, it produces an increase in hematocrit — along with any or all of the biological affects previously attributed to natural EPO. As will be discussed below, this reading is further supported by other parts of the specification and the prosecution history.
Therefore, while this Court agrees with the Federal Circuit that therapeutic effectiveness “encompasses the patient responses described in the specification,” this part of the specification does not indicate that these biological responses are sufficient or that Amgen “broadened” the plain meaning of the term “therapeutically effective” to encompass the elicitation of biological effects alone regardless of whether they heal or cure. Indeed, the term “therapeutically effective” is never even mentioned in this section of the specification. While guidance as to a claim term’s meaning or a claim’s scope need not be provided in explicit definitional format,
SciMed Life Systems,
Amgen points to a few other portions of the specification in support of its argument that while it did not alter the meaning of “therapeutically effective” to include the biological effects, it did limit the claimed therapy to patients suffering from anemia and anemia-like disorders and likewise limited the claim to an increase in hemato-crit. 32
The first such passage is the one immediately following the portion of the specification cited by the Federal Circuit:
Included within the class of humans treatable with products of the invention are patients generally requiring blood transfusion and including trauma victims, surgical patients, renal disease patients including dialysis patients, and patients with a variety of blood composition affecting disorders, such as hemophilia, sickle cell disease, physiologic anemias, and the like.
’933 Patent, Ex. 1, col. 83: 31-36 (emphasis added).
33
As HMR/TKT correctly points out, this list of patients is obviously incomplete as it begins with the words “included within,” which suggests that there are other types of patients for which the product is intended. HMR/TKT’s Posb-Hr’g Mem. [Doc. No. 747] at 4. While this is true, it still provides insight into the type of patients who may receive a therapeutic benefit from the pharmaceutical compositions of the invention. Therefore, while the specification does not actively limit the term to this class of patients, it provides guidance to the Court in defining the term.
Vitronics,
Other portions of the specification support interpreting the claims with reference to the class of patients listed in the specification. For example, the specification states: “The minimization of the need for transfusion therapy through use of EPO therapy can be expected to result in reduced transmission of infectious agents.” ’933 Patent, Ex. 1., col. 33: 37-39. While this is only one example of how the product is useful or advantageous, it falls within the class of patients listed in the specification. 35
Other pertinent sections are as follows:
It has recently been estimated that the availability of erythropoietin in quantity would allow for treatment each year of anemias of 1,600,000 persons in the United States alone.
Id. at col. 6: 35-39.
... clinical testing and potential wide-ranging therapeutic use of [Lin’s recombinant EPO] in treatment of e.g., chronic kidney disease wherein diseased tissues fail to sustain production of er-ythropoietin.
Id. at col. 9: 6-9 (emphasis added).
Also comprehended by the invention are pharmaceutical compositions comprising effective amounts of polypeptide products of the invention together with suitable diluents, adjuvants and/or carriers which allow for provision of erythro-poietin therapy, especially in the treatment of anemic disease states and most especially such anemic states as attend chronic renal failure.
Id. at col. 12: 1-7 (emphasis added).
Because erythropoietin is essential in the process of red blood cell formation, the hormone has potential useful application in both the diagnosis and the treatment of blood disorders characterized by low or defective red blood cell production.
*237 Id. at col. 6: 20-24 (emphasis added). 36
Amgen also points to column 6, lines 28-33 of the ’933 patent, which cites a study-done by Eschbaeh:
See, generally, ... Eschbaeh, et al[.] ... describing a therapeutic regimen for uremic sheep based on in vivo response to erythropoietin-rich plasma infusions and proposing a dosage of 10 U EPO/kg per day for 15-40 days as corrective of anemia of the type associated with chronic renal failure.
That Amgen intended its invention to treat anemic patients is clear from these sections (along with the prosecution history, as will be discussed below) and is pertinent to the analysis.
Renishaw,
While these sections do not suggest that the product is solely intended for anemic patients and to increase hematocrit, they do imply, in combination, that it is designed for the class of patients listed in column 33 and noted above.
37
That being said, it seems to stretch the doctrine of claim construction too far to incorporate into the plain and ordinary meaning a reference to a class of patients that at best is only implied in the specification.
Northern Telecom Ltd. v. Samsung Elees. Co.,
*238 d. The Prosecution History
The third step in claim construction is to consider the prosecution history to determine whether the applicant has made any express representations regarding the claim’s scope.
Vitronics,
The amendments made early on in pursuance of the patents support HMR/TKT’s contention that Amgen defined a “therapeutically effective amount” of EPO to encompass an amount sufficient to elicit any or all of the biological effects that were attributed to natural EPO.
On December 5, 1988, in response to a rejection under 35 U.S.C. §§ 112, 102(b) and 103 of what eventually became the ’080 patent, Amgen submitted independent claim 41 and dependent claims 55-57 and 61-66. The pertinent amendments are claim 41 (which relates to claim 2 of the ’080 patent), claim 55 (which relates to claim 4 of the ’080 patent), claim 57 (which relates to claim 6 of the ’080 patent), and claim 56 (because it is referenced in claim 57).
Claim 41: A glycoprotein product having a primary structural conformation and glycosylation sufficiently duplicative of that of a naturally occurring human erythropoietin to allow possession of the in vivo biological property of causing bone marrow cells to increase production of reticulocytes and red blood cells and having an average carbohydrate composition which differs from that of naturally occurring human erythropoiet-in.
Claim 55: A pharmaceutical composition comprising an effective amount of a glycoprotein product according to claim 41 and a pharmaceutically acceptable diluent, adjuvant or carrier.
Claim 56: A method for providing er-ythropoietin therapy to a mammal comprising administering an effective amount of a glycoprotein product according to claim 41.
Claim 57: A method according to claim 56 wherein the therapy comprises enhancing hematocrit levels.
Amgen’s ’422/’080 App., Tab G (Ex. 2), at Tab 6, at 174-75.
These claims make clear that Amgen’s product purposefully duplicates natural EPO in that it elicits the in vivo biological activity of causing bone marrow cells to increase production of reticulocytes and red blood cells, but that it differs from natural EPO in its carbohydrate composition. These claims also make clear that claim 55 (similar to claim 4 in the ’080 patent) is not limited to increasing hemato-crit because that is precisely what claim 57 does (and what claim 6 in the ’080 patent how does). In the remarks accompanying the amendment, Amgen twice explained that its product produces the same in vivo biological activity as that of natural EPO:
Applicant’s novel glycoprotein preparations ... hav[e] the glycosylation-requir-ing in vivo biological activity (promoting reticulocyte and red blood cell production) characteristics of naturally occurring human erythropoietin.
Amgen’s ’422/’080 App., Tab G (Ex. 2), at Tab 6, at 175.
[T]he glycoprotein products herein claimed ... possess the essential in vivo biological activity of naturally occurring erythropoietin.
*239 Amgen’s ’422/’080 App., Tab G (Ex. 2), at Tab 6, at 181. It then explained, with reference to claim 56, that Amgen “first developed knowledge of the full amino acid sequence of erythropoietin and first generated the presently claimed glycoprotien products which allowed for full scale clinical application to provide therapeutic effects consistent with the in vivo activity of naturally occurring erythropoietin.” Id. at 177 (first emphasis added). With reference to claim 41, it stated that Amgen “was the first to provide a glycoprotein which is both different from previously isolated urinary erythropoietin in its glycoys-lation and yet sufficiently like the natural product ... in terms of its glycosylation to allow it to fill the long-felt need (unsatisfiable by urinary isolates) for life-sustaining human therapeutic agents for, e.g., the anemia associated with dialysis in renal failure patients.” Id. at 178. It then explained that the product is “sufficiently like” natural EPO in glycosylation because it “allow[s] for in vivo biological activity.” Id. at 179. Later, it explained that Example 10 is novel in that it is the first therapeutic procedure ever practiced with EPO to demonstrate that EPO has the capacity to generate in vivo an increase in hemato-crit. Id.
Taken in combination, the amendments and these remarks support the interpretation that Amgen intended “therapeutically effective amounts” of EPO to encompass an amount that elicited in patients any or all of the biological effects previously attributed to natural EPO and that it did not limit the term to an increase in hemato-crit. 39 Such an effect is separately claimed in claim 6 (here claim 57).
Were this the entire prosecution history, the Court would agree with HMR/TKT and the Federal Circuit that Amgen broadened the term to mean one that elicits any or all of the in vivo effects before attributed to natural EPO regardless of whether they actually heal or cure the patient. In the course of overcoming two additional rejections later on in the process, however, Amgen differentiated its product from natural EPO (i.e., it overcame rejection) by asserting that natural EPO — which elicits the biological effects— was not therapeutically viable, whereas its product was clinically effective and designed specifically for a class of patients for which the product was intended. In doing so, Amgen avowed that its invention produced enough quantity of EPO to elicit responses that actually healed or cured the patient.
Renishaw,
For example, in a June 5, 1989 amendment, in response to a PTO rejection under 35 U.S.C. § 103 for obviousness, Am-gen distinguished its recombinant EPO product from natural EPO by claiming natural EPO was “not a viable therapeutic product” whereas its recombinant EPO was “clinically effective” and the “first *240 therapeutic product” successfully to treat anemia and other disorders involving low red blood cell counts:
All of the references cited by the Examiner in this rejection relate to naturally occurring erythropoietin. The claims of the subject invention relate to erythro-poeitin which is produced through recombinant DNA techniques. Recombinant erythropoietin is different from naturally occurring erythropoietin... Moreover, naturally occurring human erythropoietin is not a viable human therapeutic product; human recombinant erythropoietin, on the other hand, has been proven to be clinically effective, and is the first therapeutic product which can be used to effectively treat the hundreds of thousands of patients who suffer from anemia and other disorders involving low red blood cell counts.
Amgen’s ’422/’080 App., Tab G (Ex. 2), at Tab 11, at 227 (emphasis omitted). Amgen further explained that “[i]n contrast to recombinant erythropoietin, naturally occurring human erythropoietin is not used to treat patients. In the past, efforts were made to obtain purified erythropoietin from natural sources .... The results of these efforts however yielded only a small amount of material which was far too little for clinical research.”
Id.
at 229. As the FDA stated in its approval of recombinant EPO “there is not enough naturally occurring enthropoetin produced to collect it from healthy persons for use in treatment,” but “gene splicing techniques have permitted its production.”
Id.
Thus, in response to this rejection, Amgen differentiated its EPO from natural EPO in two respects. First, Amgen claimed its invention allowed for a sufficient amount of EPO actually to treat patients — as opposed to natural EPO which was not available in large enough quantities. Second, it claimed its EPO, as opposed to prior art, effectively treated patients suffering from anemia or other disorders involving low red blood cell count.
40
This was a clear and definitive statement about what the invention “envelopes.”
Renishaw,
*241 That Amgen intended its invention to provide a meaningful health benefit to the list of patients expressly mentioned in the specification is supported by another portion of the prosecution history. On November 6, 1990, Amgen claimed the following in an application that eventually resulted in the ’422 patent:
Claim 61: An erythropoietin-containing, pharmaceutically-acceptable composition wherein human serum albumin is mixed with erythropoietin.
Claim 62: A composition according to claim 61 containing a therapeutically effective amount of erythropoietin.
Claim 63: A composition according to claim 61 containing a therapeutically effective amount of recombinant erythro-poietin. 41
HMR/TKT’s App. to Opp’n [Doc. No. 705], Tab 2 (Ex.2003, 11/6/90 Preliminary Amendment) at 9. The examiner rejected claims 62 and 63 as “being indefinite for failing to particularly point out and distinctly claim the subject matter which [the] applicant regard[ed] as the invention.” Id. (Ex.2003, 6/1/94 Examiner’s Action) at 2. Claim 62 was rejected for being “vague and indefinite because it is unclear what the claimed composition is required to be ‘effective’ for,” and claim 63 was rejected as “vague and indefinite because it is unclear as to how the recitation that the claimed erythropoietin is ‘recombinant’ modifies the physical erythropoietin composition[;] ... while the claimed erythro-poietin may be prepared using recombinant techniques, the product would not necessarily distinguish over that found in nature.” Id. In essence, then, the examiner rejected Amgen’s patent because it did not specify for what type of patients the product was intended to be “therapeutieally effective” and it did not distinguish how the recombinant EPO was different than natural EPO besides its preparation. In other words, it did not differentiate what recombinant EPO provided to patients that natural EPO did not.
Amgen requested reconsideration, stating that the terms “effective” and “recombinant” are, “in view of the extensive disclosure of the specification,” well-defined and understood by a person of skilled in the art. Id. (Ex.2003, 12/1/94 Request for Reconsideration) at 1. Amgen argued that “the specification indicates several potential therapeutic uses for the claimed invention.” Id. at 2 (emphasis added). It then quoted the exact portion of the specification to which the Federal Circuit had pointed, where the in vivo effects along with the effect of an increase in hematocrit levels are mentioned. Id. Importantly, however, Amgen also quoted the following sections regarding the class of humans treatable with products:
Similarly, to the extent that polypeptide products of the invention share the in vivo activity of natural EPO isolates they are conspicuously suitable for use in erythropoietin therapy procedures practiced on mammals, including humans, to develop any or all of the effects heretofore attributed in vivo to EPO e.g., stimulation of reticulocyte response, development of ferrokinetie effects (such as plasma iron turnover effects and marrow transit time effects), erythrocyte mass changes, stimulation of hemoglobin C synthesis (see, Eschbach, et al[.], supra) and[,] as indicated in Example 10, increasing hematocrit levels in mammals. Included within the class of humans treatable with products of the invention are patients generally requiring *242 blood transfusions and including trauma victims, surgical patients, renal disease patients including dialysis patients, and patients with a variety of blood composition affecting disorders, such as hemophilia, sickle cell disease, physiologic anemias[,] and the like.
Id. (Ex.2003, 12/1/94 Request for Reconsideration) at 2 (emphasis omitted) (quoting ’933 Patent, Ex. 1, col. 33: 19-36). According to Amgen,
these sentences from the specification and others provide a clear and definite description of the uses for which the claimed erythropoietin compositions would be therapeutically effective. A person of skill in the art would understand that the amount of erythropoeitin necessary to achieve these defined therapeutic results would vary for each use. However, clinicians can readily determine the “therapeutically effective” amounts for each condition, and indeed for each patient.
Id. (emphasis added).
The question then is what are the “uses” to which Amgen refers. At first blush, it may appear that the “therapeutic uses” are the effects listed in the specification. A close reading of the remarks, however, makes clear that the words “uses” and “use” refer to treatment of the conditions listed in the specification — not to eliciting the effects. If this were not the case, the following sentence would not make sense: “A person of skill in the art would understand that the amount of erythropoeitin necessary to achieve these defined therapeutic results would vary for each
use.” Id.
(emphasis added). Amgen overcame a rejection of indefiniteness, in part by claiming that its product was specifically designed to treat patients suffering from the types of disease listed in the specification. Such a clear avowal — when considered alone or along with the other parts of the prosecution history and specification— would estop Amgen now were it to try to claim that its product was “therapeutically effective” in treating patients with
high
red blood cell counts.
Alpex Computer Corp.,
The trickier question, however, is whether these remarks define the disputed term to include the in vivo effects of EPO regardless of whether they heal or cure this *243 class of patients. 43 While it is a close call, the Court does not so read these remarks. Admittedly, all of the effects — the in vivo effects and an increase in hematocrit — are labeled together as “therapeutic results.” What is not made clear, however, is whether “therapeutic results” equates with “therapeutically effective.” While there is support for reading the terms as coextensive, there is also support for viewing them differently. Amgen specifically differentiates between an amount that achieves therapeutic results and a “therapeutically effective amount:”
A person of skill in the art would understand that the amount of erythropoeitin necessary to achieve these defined therapeutic results would vary for each use. However, clinicians can readily determine the “therapeutically effective” amounts for each condition, and indeed for each patient.
HMR/TKT’s App. to Opp’n, Tab 2 (Ex. 2003, 12/1/94 Request for Reconsideration), at 2 (emphasis added). These two sentences indicate that a different amount of EPO is used to achieve each of the effects listed in the specification — including the in vivo effects — depending on the condition and needs of the patient, but that a clinician can determine the amount that would be “therapeutically effective.” Thus, when read together, these sentences indicate that (1) the biological effects listed in the specification are part- of the “therapy” but not necessarily “therapeutically effective,” i.e., they do not necessarily heal or cure the patient, and (2) the amount necessary for therapeutic effectiveness — an amount that heals or cures — depends on the types of patients to which the recombinant EPO is being administered.
Because these remarks do not clearly disavow the ordinary and customary meaning of the disputed term and can actually be interpreted to support the ordinary and customary meaning of the disputed term,
44
the Court does not construe “therapeutically effective” to encompass any or all of the biological effects regardless of whether they work to heal or cure.
Amgen II,
5. Conclusion and Claim Construction of “Therapeutically Effective”
The Federal Circuit has stated that “any interpretation [of a patent claim term] that is provided or disavowed in the prosecution history shapes the claim scope.”
Renishaw,
A therapeutically effective amount is a quantity that produces a result that in and of itself helps to heal or cure. A therapeutically effective amount is one that elicits in vivo biological activity of natural EPO such as those listed in the specification, column 33, lines 24 through 28: stimulation of reticulocyte response, development of ferrokinetic effects (such as plasma iron turnover effects and marrow transit time effects), erythrocyte mass changes, stimulation of hemoglobin C synthesis (see, Eschbach, et al., supra) and, as indicated in Example 10, increasing hematocrit levels in mammals.
Therapeutically effective is to be interpreted as being therapeutically effective with respect to the class of patients listed in the specification, column 33 lines 31 through 36: patients generally requiring blood transfusions and including trauma victims, surgical patients, renal disease patients including dialysis patients, and patients with a variety of *246 blood composition affecting disorders, such as hemophilia, sickle cell disease, physiologic anemias, and the like.
See 9/18/03 Pretrial Conference Tr. at 9-11.
As will be discussed further below, in deciding whether the Goldwasser reference anticipates Amgen’s patents, this construction leaves the Court with a very fact-intensive task: determining which, if any, of the effects listed in the specification actually heal or cure the class of patients referred to therein.
B. “DNA Encoding”
1. Background
At the close of Amgen’s case-in-chief during the first trial, this Court granted HMR/TKT’s Fed.R.Civ.P. 52(c) motions for judgment of non-infringement of claims 4-9 of Amgen’s ’698 process patent.
Amgen I,
In the memoranda in support and in opposition to each party’s motions regarding infringement of the ’698 patent, the parties argued different interpretations of the term “DNA encoding” found in claims 4 and 6 of the ’698 patent. Thus, the Court concluded that the term is in dispute and needed to be construed in order properly to determine the issue of literal infringement. 48
2. The Claims at Issue
Claim 4 of the ’698 Patent:
A process for the production of a glyco-sylated erythropoietin polypeptide having the in vivo biological property of causing bone marrow cells to increase production of reticulocytes and red blood cells comprising the steps of: (a) growing, under suitable nutrient conditions, vertebrate cells comprising promoter DNA, other than human erythropoietin promoter DNA, operatively linked to DNA encoding the mature erythropoiet-in amino acid sequence of FIG. 6; and (b) isolating said glycosylated erythro-poietin polypeptide expressed by said cells.
’698 Patent, Ex. 1, col. 38: 37-47 (emphasis added) (paragraph structure altered).
Claim 6 of the ’698 Patent:
A process for the production of a glyco-sylated erythropoietin polypeptide having the in vivo biological property of causing bone marrow cells to increase production of reticulocytes and red blood cells comprising the steps of: (a) growing under suitable nutrient conditions, vertebrate cells comprising amplified DNA encoding the mature erythropoiet-in amino acid sequence of FIG. 6; and (b) isolating said glycoslated erythro-poietin polypeptide expressed by said cells.
Id. at col. 38: 50-59 (emphasis added) (paragraph structure altered).
3.Summary of the Parties’ Arguments
HMR/TKT’s proposed claim construction rests on the argument that the word “encoding” means “producing.” HMR/ TKT’s Mem. in Opp’n re ’698 [Doc. No. 700] at 8. HMR/TKT argues that the phrase at issue in Amgen’s ’698 patent means that the DNA actually produces a *247 glycosylated erythropoietin polypeptide having a 166 amino acid sequence. Id. In other words, HMR/TKT argues that section (a) of claims 4 and 6 of the ’698 patent should be construed to require the production of an EPO protein with 166 amino acids. Id. at 1; HMR/TKT’s Reply re ’698 [Doc. No. 725] at 3.
Amgen agrees that the term “mature erythropoietin amino acid sequence of FIG 6” refers to a fully processed EPO glyco-protein having a 166 amino acid sequence. Amgen argues, however, that section (a) of the disputed claims refers to the DNA that encodes the fully processed EPO glycopro-tein — not to the EPO glycoprotein itself. In other words, Amgen argues that the disputed claims refer to the type of DNA that is involved and describe that DNA as one that has a certain sequence, the genetic code, for the amino acid sequence spanning +1 through +166 of Figure 6. Am-gen’s Reply re ’698 [Doc. No. 731] at 6. Amgen asserts that the proper construction of the claim language is “a DNA sequence that contains the genetic code for the amino acid sequence spanning from position +1 through position +166 of Figure 6.” Amgen’s Reply re ’698 at 6. Amgen contends that a process can contain DNA that encodes the full 166 amino acids but result in an end-product that does not have the full 166 amino acid sequence. Thus, according to Amgen, this portion of the disputed claims refers to a type of DNA and to what that DNA encodes — not the end-protein that is ultimately produced.
4. Discussion
It is true that the Court construed the “mature erythropoietin amino acid sequence of FIG. 6,” as stated in both the ’080 and ’698 patent, to mean a mature (fully realized) erythropoietin having 166 amino acids.
Amgen I,
The Court notes that HMR/TKT supports its definition of “encoding” primarily with extrinsic evidence — evidence to which resort ought be had only “if necessary.”
Vitronics,
Furthermore, the extrinsic evidence adduced during the second trial shows that “DNA encoding” in these claims does not mean that the end product must be produced. Dr. Lodish testified that those of skill in the art at the time would understand the plain meaning of the disputed term to mean “a DNA which when copied into RNA, and if necessary spliced, specifies the order of amino acids that are the mature erythropoietin amino-acid sequence depicted in Figure 6 of the patent.” 49 Lodish Test., R. Trial Tr. at 1054: 17-22, 1058: 10, 1059: 1-3 (explaining that genes have two parts, one of which involves the “coding sequence, the piece of DNA that actually specifies the amino acids in the encoded product” and stating that it is this part that is the subject of the claim, “that is, it is an issue of DNA encoding specifying an amino-acid sequence as determined by the genetic code”); id. at 1059: 16-21 (stating that “DNA encoding the mature erythropoietin amino acid sequence of FIG. 6” refers to “the DNA sequences that encode all of the amino acids from +1 to +166 of the EPO sequence”); id. at 1063: 17-19 (explaining that “DNA encoding” refers to DNA in the cell, not to “the polypeptide that is ultimately secreted by the cell. It’s a statement of the coding capacity of the DNA in the cell”); id. at 1055: 13-18 (“It simply refers to a sequence of DNA which has the capability of encoding, which encodes, a particular protein. It is not a statement about a protein that the cell actually makes or secretes.”). Indeed, even Dr. Kingston, HMR/TKT’s expert, admitted that one way the word “encoding” “could be used very precisely is to describe a very, very precise small bit of the gene, and that is the codons.” Kingston Test., R. Trial Tr. at 163: 2-16. 50 Further, consistent with Dr. Lodish’s testimony, Dr. Kingston stated that the phrase “DNA encoding the mature erythropoietin amino acid sequence of FIG. 6” means “DNA that provides the instruction to make th[e] protein which would be the sequences” found in Figure 6 and depicted as the codons encoding amino acids +1 through +166. Kingston Test., R. Trial Tr. at 135: 2-142: 7 (circling the entire sequence of Figure 6); Lodish Test., R. Trial Tr. at 1059: 22-1060: 25 (same).
Again, however, none of this evidence is necessary to the Court’s construction because an examination of the plain and ordinary meaning of the words, the claims themselves, and the specification demonstrates that HMR/TKT’s asserted construction is off base.
Vitronics,
a. The Plain and Ordinary Meaning
The plain and ordinary meaning of “encode” is to “convert from one system of communication to another” and “to convert (a message) into code.” Webster’s Ninth New Collegiate Dictionary 1990. This implies that “DNA encoding” is DNA that converts one type of message or text into *249 another type of message and that it provides information to the cell.
b. The Claims
The claim language supports the plain and ordinary meaning of the term. The claim language establishes that “DNA encoding” refers to DNA that contains a certain sequence in the cells. Both claims 4 and 6 describe processes for producing a glycosylated erythropoietin polypeptide. The sentences in section (a) of the disputed claims do not, as HMR/TKT argues, require the production of the end-product of the claimed processes — an EPO polypeptide with 166 amino acids. To the contrary, the claims clearly distinguish between the cells grown in step (a) (which comprise “DNA encoding the mature er-ythropoietin amino acid sequence of Figure 6”) and the EPO glycoprotein itself that is isolated in step (b). Here, the “mature erythropoietin amino acid sequence of FIG. 6” modifies “DNA encoding” in the cells grown in step (a) — not the “glycosylated erythropoietin polypeptide” isolated in step (b). Therefore, based on the claim language and the ordinary meaning of the words, it appears that the sentences containing the disputed phrase mean, in conjunction, that the DNA must provide or contain the code or instructions for the “mature erythropoietin amino acid sequence of FIG. 6.”
The claims do not, however, imply that a protein with the “mature erythropoietin amino acid sequence of FIG. 6” must at the end of the process be produced. This point becomes clear when comparing these claims to that of the ’080 patent. The ’698 claims recite a “DNA encoding the mature erythropoietin amino acid sequence of FIG. 6.” as opposed to the claims of the ’080 patent that specifically recite an EPO glycoprotein that “comprises the mature erythropoietin amino acid sequence of FIG. 6.” ’080 Patent, Ex. 1, col. 38: 42-43.
In a nutshell, HMR/TKT’s construction conflates the concept of DNA that encodes for a protein with requiring the production of a specific protein and in so doing ignores how proteins are actually produced. The DNA encodes the protein. It provides the instruction set used by the cell to synthesize a polypeptide that is later processed to its final form. DNA encoding a specific amino acid sequence, however, does not necessarily determine the final length of the polypeptide produced by the cell. The testimony adduced at trial regarding the 166th arginine makes this clear. Dr. Lodish explained that “as long as that DNA encodes the mature erythro-poietin — mature EPO sequence, it matters not at all how many other amino acids might be there. Whatever it is, as long as it encodes that sequence, it’s fine.” Lodish Test., Trial Tr. at 248: 23-249: 1.
HMR/TKT counterargues that it is the protein that is produced by the cell that determines what instructions were actually present in the cell and used in the process, that is, that erroneous instructions are not really instructions at all. See, e.g., 7/28/03 Hr’g Tr. at 52: 1-9 (explaining that “there’s no proof one way or another as to what the intermediary is,” and “the only proof that there is in this case is as to the end product”). 52
The Court, however, is not persuaded. The evidence adduced at the first trial overwhelmingly suggested that although
*250
the DNA encodes for a 166 amino acid sequence, ultimately, the
cell
cleaves off the last amino acid residue prior to secretion of the final protein, EPO that has a 165 amino acid sequence.
Amgen I,
Moreover, as Amgen argues, HMR/ TKT’s construction makes the claims illogical. With HMR/TKT’s construction, the claimed processes would require the use of a cell containing “a promoter DNA opera-tively linked to an EPO protein” or “an amplified EPO protein.” Amgen’s Mem. In Opp’n re ’698 [Doc. No. 717] at 6-7. As asserted by Amgen and undisputed by HMR/TKT, this does not make sense.
In sum, any argument based on the claims that the words “producing” or “that produces” should be inserted in lieu of “encoding” fails along with HMR/TKT’s argument that “encoding” refers to the EPO protein itself. 54
c. The Specification
Like the claims, the specification supports the.plain and ordinary meaning of the word “DNA encoding.” It demonstrates that one skilled in the art at the time would have defined “encoding” as providing genetic instructions, that is, the sequence.
At the Markman hearing, HMR/TKT pointed to columns 11 and 13 in the specification to support its argument that DNA encoding means producing or that the protein is actually produced. 7/28/03 Hr’g Tr. at 51: 6-11. Those sections state that:
The isolation of the desired cDNA clones containing EPO encoding DNA was accomplished through the use of DNA/DNA colony hybridization.
’933 Patent, Ex. 1, col. 13: 64-66.
Specifically comprehended in part (b) are genomic DNA sequences encoding allelic variant forms of monkey and human erythropoietin and/or encoding other mammalian species of erythropoietin. Specifically comprehended by part (c) *251 are manufactured DNA sequences encoding EPO, EPO fragments and EPO analogs which DNA sequences may incorporate codons facilitating translation of messenger RNA in non-vertebrate hosts.
’933 Patent, Ex. 1, col. 11: 54-61.
As this Court pointed out during the hearing, however, neither of these sections equates “encoding” with producing. 7/28/03 Hr’g Tr. at 51: 12-15. Likewise, neither shows a clear and deliberate attempt by the patentee to become its own lexicographer.
See Renishaw,
5. Conclusion and Claim Construction of “DNA Encoding”
Accordingly, the Court construed “DNA encoding” to mean “the genetic instructions for.” 7/28/03 Hr’g Tr. at 56: 18-23. 55 TKT/HMR, however, did not give up. As a last-ditch effort to win on literal infringement — which is what claim construction is really all about — HMR/TKT argued at the second trial via Dr. Kingston’s testimony that “genetic instructions for,” the Court’s construction of DNA encoding, could mean either the codons for the amino acids plus 1 to 166 of Figure 6 of the patent, or alternatively, all the instructions to make the mature protein including the regulatory sequences. Kingston, R. Trial Tr. at 161-163. Dr. Kingston explained that a scientist could use the term differently depending on the context. Id. To be clear, in this context, the Court interprets the claim to be referring to the coding sequence, the piece of DNA that actually specifies the amino acid sequence — not the regulatory sequences that determine when and under what conditions the cells copy the gene into RNA. 56 This interpretation is supported by the claims themselves, which refer to DNA that encodes — provides the genetic instructions for — “the mature er-ythropoietin amino acid sequence of FIG. 6.” Figure 6 indeed depicts, among other things, the deduced amino acid sequence that is arrived at by reading the codons of the DNA encoding the protein. Importantly, HMR/TKT points to no support in the prosecution history for its argument on this point. Thus, the Court interprets the claims to require the use of cells contain *252 ing DNA that provides the genetic instructions, the codons, for a 166 amino acid sequence.
C. Are Claims 4 and 6 of the ’698 Patent Step-Plus-Function Claims?
1. Background 57 and Summary of The Parties’ Arguments
Whether Amgen, in referring to the “step[ ] of ... growing under suitable nutrient conditions” in claims 4 and 6 of the ’698 patent, was making step-plus-function claims is an issue raised for the first time by HMR/TKT in its Memorandum in Opposition to Amgen’s Renewed Motion for Summary Judgment of infringement of claims 4-9 of the ’698 patent. HMR/TKT’s Mem. In Opp’n re ’698 [Doc. No. 700] at 9. Paragraph 6 of 35 U.S.C. § 112, which sets forth the notion of step-plus-function and means-plus-function, “obligates this court to interpret each functional element in a combination claim by reference to the corresponding structure, material, or acts described in the
specification and their equivalents.” Seal-Flex, Inc. v. Athletic Trade and Court Const.,
Ironically, this is exactly what the Court did — in error— in the first go-round. In Amgen I, the Court based its holding of non-infringement of the ’698 patent on a comparison of HMR/TKT’s process to the processes outlined in the patent specification. 59 This was error because the Court had never ruled that the relevant claims qualified as a step-plus-function claims. 60 HMR/TKT now presses the Court to address the issue and so to rule.
The wrinkle here is whether the Court now can address this issue — that is, whether the Court can or should permit HMR/ TKT to raise the argument at this stage. After all, in 2000, the Court issued a sanction order against HMR/TKT limiting it to *253 the contentions specifically described in its responses to interrogatories. Amgen’s Mem. in Opp’n re ’698 & ’349 [Doc. No. 717] at 4; Amgen’s App. to Mem. in Opp’n re ’698 & ’349 [Doc. No. 719], Ex. A (1/28/00 Order Granting Sanction). HMR/ TKT never identified its step-plus-function theory in its responses to Amgen’s contention interrogatories as a basis for non-infringement of the ’698 patent. Amgen’s App. to Mem. in Opp’n re ’698 & ’349, Tab C (12/7/99 HMR/TKT’s Supplemental Answers and Objections to Amgen’s Interrog. Nos. 2, 3, and 9) at 5-7, 17. Moreover, HMR/TKT never stated that this aspect of the ’698 patent (i.e., whether it included a step-plus-function claim) needed to be resolved through a Markman hearing. Am-gen asserts that the Court should therefore not allow this argument, and, at a minimum, the Court should afford Amgen the opportunity to present evidence directed to this new step-plus-function argument. Id. at 4-5. Moreover, Amgen argues that even if the Court allows such an argument, it lacks merit because “growing” is an “act,” not a “function.”
2. Discussion 61
a. Should the Court Allow HMR/ TKT to Make Its Step-Plus-Function Argument?
Whether the language of a claim is in step-plus-function format is a question of claim construction.
See, e.g., Kemco Sales, Inc. v. Control Papers Co., Inc.,
The situation here is unusual. First, this is not a new claim construction argument raised on appeal but instead a new claim construction argument raised on remand to the trial court. Second, counsel for Amgen—the party now seeking to have the issue deemed waived—acknowledged the possible applicability of the step-plus-function doctrine to the Court. On June 9, *254 2000, after the Court made its finding of non-infringement of the ’698 patent, Am-gen queried whether the Court was construing the ’698 process claims as “means plus function” claims. Trial Tr. at 1308-1309. The Court replied as follows:
I don’t mean to be elliptical. That is my analogy. That’s right.... Now I think you’ve missed on the ’698 patent. I think that because I do think you have to spell out a means-plus-function. And I have read this patent with great care and I’ve reflected on it throughout the testimony of all the witnesses. I don’t see either by equivalent or by literal infringement.
Trial Tr. at 1309-1310. Thus, the Court referred to the means-plus-function doctrine in relation to the ’698 patent 62 but, as noted earlier, did not definitively rule that the asserted claims were in means or step-plus-function format nor even mention step-plus-function in the opinion despite applying the infringement analysis required when a claim is in step-plus-function format.
Although the situation is not straightforward, it is clear that Amgen was on notice of the issue but did not get an opportunity to argue it. Given the procedural posture of the case with respect to the ’698 patent specifically, Amgen was fully afforded the opportunity during the remand trial to address the issue, which substantially reduces any prejudice to it.
Indeed, the Federal Circuit has suggested that it is appropriate to consider whether a claim is in means-plus-function or step-plus-function format even when one party has essentially waived the issue.
Rodime PLC v. Seagate Technology, Inc.,
[The plaintiffs] concession ... does not relieve this court of its responsibility to interpret the claims as a matter of law. To interpret the claims, this court must decide the subsidiary question of whether the claim element disputed by the parties invokes § 112, ¶ 6 in the first instance.... Only by undertaking this inquiry can this court ensure consistency in statutory application. Moreover, this court’s claim interpretation affects entities beyond the parties to this case. Therefore, this court examines the district court’s decision that this claim falls under § 112, ¶ 6.
Id. (internal citations omitted). The Federal Circuit subsequently concluded that the district court had erred and that the claim was not in means-plus-function format.
*255 Similarly, in this case, whether this portion of the ’698 patent is in step-plus-function format determines the entire analytic framework for analyzing whether HMR/TKT’s process infringes this part of the patent. To make this assessment, therefore, this Court needs to determine which analytic framework is implicated. The Court can either make this decision on the merits or can simply decide that the regular infringement framework must be used because HMR/TKT waived its argument that the step-plus-function framework should be used. The problem with the latter approach is that, if the step-plus function framework is truly the applicable one, and the Court nonetheless declines to use it on grounds of waiver, the Court will essentially be applying the wrong law to this aspect of the claim. This, in turn, undermines consistency in statutory application.
For these prudential reasons, this Court analyses whether claims 4 and 6 of the patent are step-plus-function claims. It does so in the course of construing the claims because, as noted above, whether the language of a claim is in step-plus-function format is a question of claim construction.
See, e.g., Kemco Sales, Inc.,
b. Are Claims 4 and 6 of the ’698 Patent Step-Plus-Function Claims?
This is a close question, but, on balance, claims 4 and 6 of the ’698 patent do not qualify as step-plus-function claims. 63 Five reasons support this conclusion.
First — although this is not dispositive— the words “steps of’ are used in the claim. Such a grammatical structure indicates that this is not a step-plus-function claim, because the phrase “steps of’ colloquially signals the introduction of specific acts, rather than functions.
See Seal-Flex,
Second, upon examination, the claim element “growing” appears to recite a specific act for performing an ultimate function, that is, it appears to explain how the function is accomplished, rather than reciting the ultimate function itself. This is a key distinction. As Judge Rader explained in his concurrence in
Seal-Flex,
“the ‘underlying function’ of a method claim element corresponds to
what
that element ultimately accomplishes in relationship to what the other elements of the claim and the claim as a whole accomplish. ‘Acts,’ on the other hand, correspond to
how
the function is accomplished.”
Sealr-Flex,
Third, HMR/TKT does not even attempt to explain, much less show, how Amgen’s language — “growing under suitable nutrient conditions”' — -fails to describe an act. “[W]here a method claim does not contain the term ‘step[s] for,’ a limitation of that claim cannot be construed as a step-plus-function limitation
without
a showing that the limitation contains no act.”
Masco,
Fourth, the Federal Circuit has made clear that “claiming a step by itself, or even a series of steps, does not implicate section 112, ¶ 6,” and that courts must be
careful not to extend the language of this provision to situations not contemplated by Congress. If we were to construe every process claim containing steps described by an “ing” verb, such as passing, heating, reacting, transferring, etc. into a step-plus-function limitation, we would be limiting process claims in a manner never intended by Congress.
O.I. Corp.,
As a final matter, the Federal Circuit’s silence as to whether these claims are step-plus-function claims may be indicative. True, the Federal Circuit probably may not even have considered the possibility.
66
Alternatively, however, the Federal Circuit may have considered the step-plus-function possibility but rejected it as without merit. This latter interpretation of the Federal Court’s silence is supported by the Federal Circuit’s statement that this Court’s analysis (comparing HMR/TKT’s process to the specification) was “legally unsupportable.”
Amgen II,
3. Conclusion and Claim Construction
Though it is a close question, this Court rules that claims 4 and 6 of the ’698 patent, in referring to the “steps of: (a) growing under suitable nutrient conditions ...,” are not step-plus-function claims and that the regular infringement framework should therefore apply.
D. Is Claim 7 of the ’349 Patent a Step-Plus-Function Claim?
1.Background
Amgen’s ’349 patent contains six product claims (claims 1-6) and one process claim (claim 7). ’349 Patent, Ex. 1. This Court held, and the Federal Circuit affirmed, that HMR/TKT’s HMR 4396 literally infringes the product claims of the ’349 patent.
Amgen II,
2. The Claim at Issue
Claim 7 of the ’349 Patent:
A process for producing erythropoietin comprising the step of culturing, under suitable nutrient conditions, vertebrate cells according to claim 1, 2, 3, 4, 5 or 6.
’349 Patent, Ex. 1, col. 38: 34-36.
3. Summary of the Parties’ Arguments
HMR/TKT, in an effort to establish non-infringement of claim 7, has argued, as it did with claims 4 and 6 of the ’698 patent, that claim 7 is a step-plus-function claim and that 35 U.S.C. § 112, ¶ 6 therefore applies. As such, it contends that its product does not literally infringe the “step of culturing” because HMR/TKT’s process does not involve the culturing procedures set forth in Amgen’s specification. HMR/ TKT’s Mem. in Supp. [Doc. No. 687] at 12-13. As with the ’698 patent, Amgen argues, as a preliminary matter, that HMR/ TKT is improperly basing its motion under Fed.R.Civ.P. 52(c) on new arguments and defenses, given the previous orders of this Court and Amgen’s lack of opportunity to address these issues. Amgen’s Mem. In Opp’n re ’698 & ’349 [Doc. No. 717] at 3-5. Furthermore, Amgen points out, the procedural context here is different than it was with the ’698 patent, as this Court heard the entirety of both parties’ arguments and evidence concerning ’349 claims 1, 3, 4, 6, and 7. Lastly, Amgen argues, for the same reasons that it did regarding the ’698 patent, that claim 7 is not a step-plus-function claim. Id. at 11-14.
4. Discussion
a. Should the Court Allow HMR/ TKT to Make Its Step-Plus-Function Argument?
Here, there is the same wrinkle that there was with the step-plus-function argument respecting the ’698 patent: *259 should the Court permit HMR/TKT to raise this argument at this late stage in the game? There are two differences, however, that make the wrinkle, in the context of this patent, harder to iron out. First, the Court did not remark on the record, as it did with the ’698 patent, that it was making a means-plus-function analogy in ruling on the ’349 patent claims. Second, HMR/TKT has already presented its case of non-infringement regarding all the claims of the ’349 patent.
Neither of these differences, however, prevents the Court from allowing HMR/ TKT to make this argument at this point. The fact that the Court did not make a means-plus analogy to this patent is easily overcome since the Court, in Amgen I, explained that it found non-infringement of claim 7 of the ’349 patent for the same reasons as it did the ’698 patent. Thus, the parties were on notice that any analysis regarding the process claims of the ’698 patent would necessarily apply to the ’349 patent. The procedural landscape ought not prevent the Court from construing whether this is a step-plus-function claim. If it is such a claim, the Court ought not conduct its infringement analysis as though it were not. This claim is here on remand and this Court must construe it in accordance with the law. Thus, the Court reaches the same conclusion as it did with the ’698 patent, that is, that it can and should address HMR/TKT’s step-plus-function argument.
b. Is Claim 7 of the ’349 Patent a Step-PIus-Punction Claim?
The determination of whether claim 7 of the ’349 patent is a step-plus-function claim must be made in the same way as any other determination regarding claim construction. As such, the Court must principally rely on intrinsic evidence and refer to extrinsic evidence only if necessary, with the exception that a dictionary or treatise — which qualifies as extrinsic evidence — can be consulted freely as long as it does not contradict the patent language.
The Court’s assessment of whether “culturing” is a function rather than an act, such that the step-plus-function framework applies, tracks the analysis provided above with respect to the whether “growing” is a function rather than an act in the ’698 patent. Just as the Court ruled that growing is an act, it rules that culturing is an act, and claim 7, therefore, does not state a step-plus-function limitation.
Like the asserted claims of the ’698 patent, claim 7 contains the phrase “step of,” rather than the phrase “step for.” Accordingly, there is a presumption that section 112, paragraph 6 does not apply — that this is not a step-plus-function.
Generation II Orthotics Inc.,
HMR/TKT argues that “culturing” is the claimed function of claim 7. HMR/ TKT’s Mem. in Supp. re ’698 & ’349 [Doc. No. 687] at 13. Specifically, it claims that the “what” is “culturing.” In other words, HMR/TKT argues that “culturing” is “what” the claim ultimately accomplishes, and nothing else in the claim describes “how” the culturing is accomplished. HMR/TKT’s Reply Mem. re ’698 & ’349 [Doc. No. 725] at 9. While at first blush this argument makes sense, the Federal Circuit, in
Masco,
interpreted Judge Rad-er’s formulation as requiring analysis of “what th[e] limitations ultimately accomplish in relation to what the other limitations and each claim as a whole accomplish.”
Masco,
Claim 1: Vertebrate cells which can be propagated in vitro and which are capable upon growth in culture of producing erythropoietin in the medium of their growth in excess of 100 U of erythro-poietin per 106 cells in 48 hours ...
Claim 4: Vertebrate cells which can be propagated in vitro which comprise transcription control DNA sequences ... for production of human erythropoietin, and which upon growth in culture are capable of producing in the medium of their growth in excess of 100 U of eryth-ropoietin per 106 cells in 48 hours ...
’349 Patent, Ex. 1, col. 38: 8-14, 21-27 (emphasis added). Hence, when considering what the “other limitations and each claim as a whole accomplish,” it appears that “culturing” is not the claimed function but instead a single step or act of a process claim that
“ultimately accomplishes
” the production of erythropoietin at a certain rate.
Masco,
There are two other pieces of support for construing “culturing” as an act. First, both parties agreed that the claim term “culturing under suitable conditions” means “growing in vitro under appropriate [or suitable] conditions.” Amgen’s App. to Mem. in Opp’n re ’698 & ’349, Tab P (9/20/99 App. to Amgen’s Claim Construction Submission) at 7;
id.,
Tab Q (10/18/99 App. to HMR/TKT’s Claim Construction Submission) at 5. Thus, implicitly HMR/ TKT admitted that “culturing” and “growing” are essentially interchangeable terms. This, considered in combination with the Joint Pretrial Memorandum itself, which states that HMR/TKT’s HMR 4396 is produced by “growing, under suitable nutrient conditions R223 cells,” 4/26/00 Corrected Joint Pretrial Mem. at 5, ¶ 25, suggests that even HMR/TKT at one point did not believe that “growing” — and by extension, “culturing” — was a function that needed further explanation. This strongly suggests that the term “culturing” was one reasonably well understood by those skilled in the art, a relevant consideration in determining whether a term is an act.
Cf. Greenberg v. Ethicon Endo-Surgery, Inc.,
Second, dictionary definitions of “culturing” define this word as an act. A standard medical dictionary,
Dorland’s Medi
*261
cal Dictionary,
defines “culture” as “propagation of ... living tissue cells in special media conducive to their growth.” Amgen’s App. to Mem. in Opp’n re ’698 & ’849, Tab R
(Borland’s Illustrated Med. Dictionary
(27th ed.1988)), at 384; see,
e.g., Masco,
In sum, HMR/TKT has failed to show that the “limitation contains nothing that can be construed as an act.”
Sealr-Flex,
As a final matter, the Court notes the same concerns it had with construing “growing” as a step-plus-function limitation. If the Court were to construe “culturing” as a step-plus-function limitation, it would run the risk of interpreting the process claim of the ’349 patent in a way that Congress never intended, rendering the scope of coverage of the patent uncertain and disrupting the patentee’s settled expectations regarding the scope of the claims.
Masco,
5. Conclusion and Claim Construction
Accordingly, the Court rules that claim 7 of the ’349 patent does not contain a step-plus-function limitation and that the regular framework for assessing infringement therefore applies. 69
IV. VALIDITY CHALLENGES UNDER 35 U.S.C. § 112
When claims are construed broadly, alleged infringers commonly challenge validity under 35 U.S.C. § 112, ¶¶ 1, 2 in light of the broad construction.
Amgen II,
As with any validity challenge, the Court begins by presuming that the patents are valid.
Amgen II,
A. Definiteness
1. The ’698 and ’349 Patent 71
a. Discussion
Paragraph 2 of section 112 requires that a patent specification include one or more claims “particularly pointing out and distinctly claiming subject matter which the applicant regards as his invention.” 35 U.S.C. § 112, ¶ 2 (2000). The Federal Circuit has stated that the standard for determining whether a claim is sufficiently definite is “[i]f one skilled in the art would understand the bounds of the claim when read in light of the specification.”
Exxon Research and Eng’g Co. v. United States,
HMR/TKT argues that under the Court’s construction of “DNA encoding” the asserted claims of the ’698 patent and claim 7 of the ’349 patent are invalid as indefinite because they include within their scope many embodiments that will not make EPO. HMR/TKT’s Opening Br. After Trial [Doc. No. 808] at 47-48. Specifically, it argues that the Court’s construction of the term requires only that the DNA provide the requisite letters or co-dons, regardless of what protein is actually made, and that the evidence demonstrates that while many cells contain the same DNA codons, only those in which certain particular DNA codons are contiguous will actually produce EPO. Further, it asserts that Amgen has changed its stance and now claims that “genetic instructions for” includes not only the codons but also the splicing instructions for putting those co-dons together in the correct order. 72 The claims, it asserts, say nothing about splicing instructions or messages and, as such, are indefinite and inoperative.
*263 Amgen responds primarily by arguing that the evidence demonstrates that skilled artisans using the teachings of Amgen’s patents would have been able to produce EPO using cells comprising non-contiguous DNA encoding the “mature erythro-poietin amino acid sequence of FIG. 6.” Amgen’s Reply to HMR/TKT’s Opening Br. After Trial [Doc. No. 815] at 33-34. 73 Further, it claims that this very evidence establishes that those skilled in the art would have known how to determine which processes fell within the ’698 and ’349 claims.
The primary dispute, then, is whether the specification teaches skilled artisans to splice the codons into the correct order when the codons are not contiguous but need to be in order to make EPO. If it does, then the claims are not indefinite as they do not cover embodiments that do not make EPO.
While it may be true, as Dr. Kingston originally stated, that “only those cells in which the DNA letters were contiguous would actually produce EPO,” Kingston Test., R. Trial Tr. at 56-60, 164: 2-7, Dr. Kingston admitted that the cells from Example 10 of Amgen’s specification produce EPO even though the Figure 6 codons for the mature erythropoietin sequence in the Example 10 cells are not contiguous. Id. at 164: 8-22; 170: 4-10. Either Dr. Kingston was blatantly contradicting his original statement, or — as the Court concludes is more likely — Example 10 and Figure 6 communicate to Dr. Kingston, one skilled in the art, how non-contiguous codons can be manipulated to produce EPO. This belies HMR/TKT’s argument that the claims are vague or indefinite for not including splicing instructions and for covering contiguous and noncontiguous codons because the specification provides the information that Dr. Kingston believed was missing from the claims.
This deduction — that the specification makes the term “DNA encoding” understandable to the skilled artisan,
Exxon Research and Engineering Co.,
According to Dr. Lodish, Dr. Lin’s patent taught those skilled in the art in 1983 to produce DNA sequences encoding EPO that are either contiguous
or noncontiguous.
Lodish Test., R. Trial Tr. at 1061: 4-1063: 4. In other words, Dr. Lodish testified that those skilled in the art would not
*264
consider the phrase “DNA encoding” to require the presence of contiguous codons of the mature EPO sequence of Figure 6. The main support for this contention stems from the fact that the codons were non-contiguous in Figure 6 of the patent. As mentioned earlier in the claim construction portion of this memorandum and order, Dr. Lodish testified that those of ordinary skill in the art at the time would have understood the disputed term to mean “a DNA which when copied into RNA, and
if necessary
spliced, specifies the order of amino acids that are the mature erythro-poietin amino-acid sequence depicted in Figure 6 of the patent.” Lodish Test., R. Trial Tr. at 1054: 17-22 (emphasis added);
id.
at 1058: 10-1059: 3. He explained that Figure 6 disclosed to those skilled in the art the codons for the mature EPO amino acid sequence, the introns, exons, and splice donor and acceptor sites of the human genomic EPO sequence.
Id.
Indeed, Dr. Kingston admitted that Lin’s specification discloses the EPO gene sequence, the EPO splice donor and acceptor sites, and the linkage of a non-human promoter with the EPO gene. Kingston Test., R. Trial Tr. 116: 23-117: 2. According to Dr. Lodish (and not directly disputed by Dr. Kingston), this information, along with what was known in the art, enabled skilled artisans to alter the codons, to alter or eliminate the introns, and to make many DNA sequences that would encode human EPO and work in the claimed processes.
Id.
Thus, contrary to HMR/TKT’s assertions, expert testimony from both sides shows that those skilled in the art would understand the claims to cover contiguous and non-contiguous DNA sequences that when necessary could be spliced into a correct and contiguous order to produce EPO.
Union Pacific Resources Co.,
b. Conclusion
HMR/TKT has failed to establish by clear and convincing evidence that “DNA encoding” is a vague, ambiguous, or undefined term not understandable to a skilled artisan when read in light of the specification. Accordingly, the Court rejects HMR/TKT’s argument that the disputed claims of the ’349 and ’698 patent are indefinite.
B. Written Description 74
1. The ’698 and ’349 Patents
a. Discussion
The basic requirements for the content of a patent specification are found in 35 U.S.C. § 112, ¶ 1:
The specification shall contain a written description of the invention, and of the manner and process of making and using it, in such full, clear, concise, and exact terms as to enable any person skilled in the art to which it pertains ... to make and use the same ....
35 U.S.C. § 112, ¶ 1 (2000). “The purpose of this provision is to ensure that the scope of the right to exclude, as set forth in the claims, does not overreach the scope of the inventor’s contribution to the field of art as described in the patent specification.”
Reiffin v. Microsoft Corp.,
HMR/TKT contends that Amgen’s claims, as construed by the Court, have a scope far greater than the written description of Amgen’s patents and are, therefore, invalid. HMR/TKT’s Opening Br. After Trial at 47-48. Primarily, it makes two arguments in support of this contention. First, HMR/TKT argues that the specification “repeatedly describes [the] DNA, cells, processes and proteins in terms of only exogenous DNA and heterologous recombination,” whereas the Court construed the asserted claims in the ’698 and ’349 patents to cover both exogenous and endogenous DNA and homologuous and heterologous recombination. 75 HMR/TKT’s Opening Br. After Trial at 47-48. Second, HMR/TKT points to the undisputed fact that the specification provides only an example of a process which places the promoter just upstream of the ATG initiation codon of a cloned and isolated EPO gene, although the Court construed “operatively linked,” as found in the ’698 patent, 76 to cover placement much farther upstream. Id. 77 As such, HMR/ TKT argues, the asserted process claims of the ’698 patent fail to provide adequate written description. Id.
(1) HMR/TKT’s First Argument: Endogenous DNA and Homologous Recombination
Although HMR/TKT’s first argument is, in part, factually correct — the specification explicitly discloses only exogenous EPO DNA expression systems and heterologous recombination techniques
78
— it is misdirected. The section
*266
112 inquiry focuses on what was known by those skilled in the art at the time of the filing of the application. Here, it is undisputed that in 1983-84 (the time period of the application filing date), endogenous activation technology and homologous recombination were not known to skilled artisans. HMR/TKT’s Findings of Fact ¶ 488; Amgen’s Reply to HMR/TKT’s Opening Br. After Trial at 34-35.
79
Therefore, this technology is irrelevant to the written description analysis, and for good reason. “If later states of the art could be employed as a basis for rejection under 35 U.S.C. § 112, the opportunity for obtaining a basic patent upon early disclosure of pioneer inventions would be abolished.”
Application of Hogan,
HMR/TKT incorrectly assumes that the Court’s construction of Amgen’s claims to cover this later developed technology changes the analysis.
Application of Koller,
a case similar to this one, shows the fallacy of HMR/TKT’s assumption. In that case, the Federal Circuit upheld a broad construction of the term “liquid medium” that covered all solvents (including the later developed water-immiscible solvents) despite a specification that only described water and water-miscible solvents — and not water-immiscible solvents. It reversed, however, the decision of the United States Patent and Trademark Office Board of Appeals that had found,
inter alia,
that the claims failed to provide adequate description. The Federal Circuit conducted its section 112 analysis based on what was claimed and known at the time of the application filing date. Because water-immiscible solvents were not known at the time of the application filing date, the Federal Circuit found that the term “liquid medium” was adequately described.
Koller,
Here, the situation is very similar. Because homologous recombination and use of endogenous DNA were not known to those skilled in the art at the time of the application, HMR/TKT’s first argument
*267
for inadequate written description fails. As the Federal Circuit explained in
Application of Hogan,
“the Courts have consistently considered subsequently existing states of the art as raising questions of infringement but never of validity.”
Hogan,
HMR/TKT’s arguments are more properly reserved for invoking the judicially developed reverse doctrine of equivalents defense which allows interpretation of the claims in light of the specification,
inter alia,
and precludes improper enforcement against later developers.
Hogan,
(2) HMR/TKT’s Second Argument: Placement of the Promoter
HMR/TKT’s second argument and Amgen’s response thereto, as they relate to the ’698 patent, render determination of the written description a bit more squirrelly. As stated above, HMR/TKT correctly argues that the specification only describes insertion of the promoter just upstream of the ATG initiation codon of the EPO gene to be expressed while the Court construed the claims to cover HMR/ TKT’s process of inserting the promoter far upstream leaving multiple ATGs between the promoter and the gene to be expressed. 81 Instead of counter-arguing, as it did in response to HMR/TKT’s first argument, that HMR/TKT’s placement technique was a post-filing advance which need not be described, Amgen contends that by 1984, artisans of ordinary skill could have placed a promoter DNA in such a position that multiple ATGs would exist between it and the gene to be expressed, and they knew how to express proteins in vertebrate cells by positioning a promoter upstream of exon coding sequences and removing unwanted DNA by manipulating splice sites. Amgen’s Reply to HMR/ TKT’s Opening Br. After Trial at 34-35; Amgen’s Reply to HMR/TKT’s Findings of Fact ¶ 67. Further, Amgen asserts, evidence shows that those of skill in the art would have understood the patent to describe operative linkages of far greater distances than 44 pairs and that skilled artisans would have understood from Lin’s patent how to avoid potentially interfering ATG sequences and thereby successfully position the promoter further upstream of DNA encoding EPO. Id. ¶ 68, ¶ 342. 82
*268
This argument is curious because the easier path would have been to argue that placement so far upstream was a post-filing advance. Indeed, the Court’s factual findings in
Amgen I
would have supported such an argument.
See, e.g., Amgen I,
Stuck in a similar catch-22, HMR/TKT argues with respect to section 112 that Amgen should have described upstream placement of the promoter, yet, in furtherance of its reverse doctrine of equivalents argument, HMR/TKT argues with equal passion that a process for producing EPO by linking the promoter and transcription control sequences far upstream of the EPO gene had never been done before HMR/TKT developed its patented gene activation process. HMR/TKT’s Reply Br. After Trial [Doc. No. 819] at 29, 34. Further, it argues that those skilled in the art recognized that promoter linkages further upstream of the initiation codon would not work to produce EPO. HMR/TKT’s Findings of Fact ¶493. Thus, HMR/TKT’s reverse doctrine of equivalents argument belies its argument that Amgen should have described placement of the promoter further upstream of the EPO gene to be expressed since, according to HMR/TKT, this had never been done before. Thus, both parties, to a degree, have argued against their best interests on this issue because to do otherwise would weaken their positions with respect to application of the reverse doctrine of equivalents.
However the parties may frame the issue, this Court, as trier of fact in this case, must determine whether placing the promoter farther upstream was a concept sufficiently known to those skilled in the art at the time of filing such that the claims would have been understood to encompass such a technique.
United States Steel Corp.,
After careful review of the evidence from the first and second trials, the Court now concludes that placement of the promoter further upstream of the EPO coding region and splicing out deleterious ATGs was indeed a concept known and understood — albeit not practiced — by those skilled in the art at the time Amgen filed its application (1983-84).
Dr. Lodish and Dr. Kingston testified that both Amgen and HMR/TKT use a technique of linking two different pieces of DNA together with a splice donor site and a splice acceptor to express a protein and that this was a standard technique in 1983. Kingston Test., Trial Tr. at 1428-30, 1433, 1434: 12-19; Lodish Test., R. Trial Tr. at 1081 (claiming that at the time of the patent application this type of splicing was common). While Dr. Lodish did indeed admit that Dr. Lin did not know what sequences were upstream of the EPO gene, and that it was intuitive to place the promoter close to the EPO coding region because the “longer the distance the more problems you’re likely to encounter,” he clarified that those skilled in the art knew that it was possible to vary the distance and still cause transcription and proteins to be made, because the sequences that are unwanted are readily identifiable and can be avoided. Lodish Test., Trial Tr. at 255-58. Further, he explained, those skilled in the art in 1983 did indeed know that a promoter could be placed 8,000-10,000 bases upstream and that very long intervening sequences could be spliced out. Lodish Test., R. Trial at 1081. Even Dr. Kingston himself admitted that in 1983 those skilled in the art knew how to place a promoter much further upstream than 44 base pairs, the location identified in Example 7 of Dr. Lin’s patent. Kingston Test., Trial Tr. at 1436-38.
Additionally, there were published articles showing that those skilled in the art possessed this knowledge. Dr. Kingston’s mentor, Dr. Sharp, published an article in 1983 that, according to Dr. Kingston, showed a construct in which a splice donor site was added to splice out approximately a 700 base pair fragment of DNA (“a 5 prime splice and a 3 prime splice”) from the message. Kingston Test., Trial Tr. at 1435-36. Indeed, Dr. Kingston himself published an article in 1982 that disclosed that the way to discard a portion of the DNA that was not wanted in the vector was to put a downstream splice receptor or *270 acceptor site and splice it out. Id. at 1436-37. In the constructs discussed in the article, the distance between the 5 prime and 3 prime splice sites was, according to Dr. Kingston, between 180 and 500 pairs. Id. at 1438.
HMR/TKT argues, however, that the evidence shows that no one had in fact used those splice sites the way that HMR/TKT eventually did — in other words, that placing the promoter upstream as HMR/TKT did was novel. HMR/TKT’s Response to Amgen’s Findings at 130. HMR/TKT also suggests that the situations to which reference has just been made appear only in nature; that is, they were not human constructs or experiments. See, e.g., Lodish Test., R. Trial Tr. at 1104: 15-1105: 5. The Court is not persuaded that the evidence shows what HMR/TKT claims it does. First, Dr. Sharp’s article, Trial Ex. 247, discloses actual experiments showing upstream placement, see, e.g., R. Trial Tr. at 1134-35. HMR/TKT produced no evidence to the contrary. Tellingly, HMR/ TKT’s counsel neither asked Dr. Kingston whether actual experiments had been conducted in 1983-1984 nor asserted in any of its post-trial memoranda the absence of actual experimentation. Second, and perhaps most enlightening, the only support HMR/TKT offers for its contention that no one skilled in the art had in 1983-84 placed the promoter upstream as HMR/TKT did, or even would have dared to do so, is the Court’s previous factual findings, which were made with respect to a different legal issue. See, e.g., HMR/TKT’s Opening Br. After Trial at 15 (citing only this Court’s opinion in support); HMR/TKT’s Reply Br. After Trial at 29 (citing this Court’s opinion and unsupportable testimony by Dr. Lodish (inaccurately referred to as “Kingston Tr. 162-167”) and irrelevant testimony by Dr. Kingston, “Kingston R. Tr. 177, 181”); HMR/TKT’s Proposed Findings of Fact ¶¶ 111, 112, 114, 116 (citing this Court’s opinion and irrelevant testimony from Dr. Lodish, admitting that he did not include homologous recombination in the first edition of his textbook). The Court finds that placement of the promoter further upstream, as HMR/TKT does with its HMR 4396, was a technique known to those skilled in the art at the time of Amgen’s application filing. 84
Because upstream placement of the promoter was known at the time of Amgen’s application, however, the Court now addresses whether HMR/TKT has shown by clear and convincing evidence that Amgen did not adequately describe such a placement. The Court agrees with HMR/ TKT’s central contention that the specification explicitly refers only to placement of the promoter in close proximity (within 44 base pairs) of the EPO gene to be expressed, leaving only one ATG adjacent to the amino terminal coding region. ’933 Patent, Ex. 1, col. 24: 15-32. “The test for determining compliance with the written description requirement,” however “is whether the disclosure of the application as originally filed reasonably conveys to the artisan that the inventor had possession at that time of the later claimed subject matter,” rather than the presence or absence of literal support in the specification for the claim language.
Kaslow,
First, as Amgen rightly points out, the ’698 claims themselves have no limitations specifying the promoter distance or the number of ATGs. Instead, the claims state that the promoter DNA must be “operatively linked” to the “DNA encoding the mature erythropoietin amino acid sequence of FIG. 6.” The Court in
Amgen I
construed this to mean “the promoter DNA is linked to the EPO DNA in a way that maintains the capability of the promoter DNA to initiate transcription of the EPO DNA.”
Amgen I,
Second, as was determined in
Am-gen I,
the specification does not clearly communicate a locational restriction.
Am-gen I,
The only support in the specification that the invention is of a narrower scope than the claims is the absence of specific examples showing an alternate location for the promoter. The specification, however, does not limit the patent to the examples therein. It does not clearly identify placement within 44 base pairs as the only possible location from which to conduct the process nor does it indicate that this exact location was an essential element of the invention or that placement farther upstream is “outside the stated purpose of the invention.”
Cf. Amgen II,
That Amgen chose to show placement of the promoter in very close proximity is only evidence that this was perceived to be the best location to achieve operative linkage — as Dr. Lodish testified — not the only location. Lodish Test., Trial Tr. at 258 (explaining that the longer the distance the
*272
higher likelihood that problems might occur and that “there’s no reason one would want to put it very far upstream. But one could,” with a little bit of work);
id.
at 553 (commenting that “in practice in the laboratory one does what is most expeditious”); Lodish Test., R. Trial Tr. at 1131 (explaining that Dr. Lin had no reason even to consider other sequences of pieces of DNA);
cf.
Kingston Test., R. Trial Tr. at 41: 20-21 (testifying that standard practice in 1984 was to place the promoter in a position such that there was not another ATG present). True, Dr. Lodish stated that the patent teaches that by
linking
a strong promoter or
placing it near
the first codon for the signal sequence of EPO, one could overcome the natural suppression of EPO expression in vertebrate cells. Lodish Test., R. Trial Tr. at 1070, 1077-78. This, however, does not unambiguously limit the location of the promoter to a distance of 44 base pairs or indicate that further upstream placement was not part of the invention. As Dr. Lodish explained, placement of the promoter thousands of base pairs upstream, as HMR/TKT does, is only a “minor difference” that is “irrelevant in the final process.”
Id.
at 1077: 1-6.
86
Thus, as testified to by Dr. Lodish, the specification teaches that putting a strong viral promoter upstream of the human EPO gene is the important feature— not how far upstream — as long as the intervening sequences are spliced out. Lodish Test., Trial Tr. at 173, 549;
see also
Lodish Test., R. Trial Tr. at 1081 (noting that “there’s nothing different about a large intro spliced out and a small intron spliced out”);
Cooper Cameron Corp. v. Kvaerner Oilfield Products, Inc.,
Therefore, the Court infers that though the examples may show linkage that is
directly
upstream, those skilled in the art would not, nor does the Court, read the specification so to limit the process.
United States Steel Corp.,
Third, although HMR/TKT has shown that the specification lacks literal support for a process that places the promoter further upstream, it has failed to show by
*273
clear and convincing evidence that Am-gen’s patent does not “reasonably convey to the artisan that [Amgen] had possession at that time of the later claimed subject matter.”
Kaslow,
While it appears that the scope of the right to exclude as set forth in the claims does not overreach the scope of Amgen’s contribution to the field of the art as described in the specification,
see Reiffin,
Although this evidence is compelling, when considered in light of prior case law and HMR/TKT’s high burden of proof, it fails to persuade the Court that Amgen’s specification is invalid for lack of written description. As discussed, the techniques disclosed in the specification are the same ones used in a process that places the promoter further upstream. Simply because further upstream placement was possible and applicants could have, as testified to by Dr. Lodish, done it and then described it in an example does not mean that the applicant must describe it. This is just the sort of argument rejected in
In re Vickers,
The exclusive right to the thing patented is not secured, if the public are at liberty to make substantial copies of it, varying its form or proportions. And, therefore, the patentee, having described his invention, and shown its principles, and claimed it in that form which most perfectly embodies it, is, in contemplation of law, deemed to claim every form in which his invention may be copied, unless he manifests an intention to disclaim some of those forms.
In re Kirschbraun,
Moreover, this admission can be distinguished from the admission in
Gentry Gallery, Inc. v. Berkline Corp.,
upon which HMR/TKT relies for support. There, Gentry admitted he broadened his claims to cover placement of the controls outside the console only after competitors engaged in such placement.
Gentry,
Here, according to undisputed expert testimony, the specification communicates that in order to achieve “operative link[age],” what is important is placing a strong promoter upstream of the ATG initiating codon of the EPO gene and splicing out unwanted ATGs. One skilled in the art who read Amgen’s specification would understand that it is unimportant where upstream the promoter is placed, so long as it is genuinely “operatively linked.”
Cf. Rasmussen,
In a nutshell, HMR/TKT misconstrues the focus of the section 112 inquiry, to wit, whether the claimed subject matter is adequately described,
see, e.g., Ralston Purina Co. v. Far-Mar-Co., Inc.,
b. Conclusion
Accordingly, the Court holds that HMR/ TKT has failed to show by clear and convincing evidence that the asserted claims of the ’698 patent and claim 7 of the ’349 patent are invalid for lack of written description under 35 U.S.C. § 112, ¶ 1.
C. Enablement
1. The ’698 and ’349 Patents
a. Discussion
A patent application must “contain a written description of the invention, and of the manner and process of making and using it ... as to enable any person skilled in the art to which it pertains, or with which it is most nearly connected to make and use the same.” 35 U.S.C. § 112, ¶ 1 (2000). “To be enabling, the specification of the patent must teach those skilled in the art how to make and use the full scope of the claimed invention without ‘undue experimentation.’ ”
Genentech, Inc. v. Novo Nordisk A/S,
The parties’ arguments for non-enablement run parallel to those regarding written description. Although the enablement requirement is separate and distinct from the written description requirement, the
*277
written description requirement is broader than the enablement requirement.
Vas-Cath,
(1) HMR/TKT’s First Argument: Endogenous DNA and Homologuous Recombination
HMR/TKT rightly claims that under the Court’s claim construction, the asserted process claims of the ’698 and ’349 patents “do not enable one of skill in the art to produce EPO from vertebrate cells other than those transfected with exogenous cloned EPO DNA.” HMR/TKT’s Opening Br. After Trial at 48. As discussed above, however, it is undisputed that in 1983-84, endogenous activation technology and homologous recombination were not known to skilled artisans. HMR/ TKT’s Findings of Fact ¶ 488; Amgen’s Reply to HMR/TKT’s Opening Br. After Trial at 34-35. As with the written description requirement, when considering enablement, later states of art cannot be employed as a basis for rejection.
Hogan,
(2) HMR/TKT’s Second Argument: Placement of the Promoter
HMR/TKT argues that Amgen’s specification only enables operative linkage of promoter DNA and EPO DNA near or adjacent to the ATG initiation codon of a cloned and isolated EPO gene and that skilled artisans at the time would not have expected promoters placed further upstream to produce EPO. Furthermore, HMR/TKT contends that Amgen’s argument — that enablement of one way to make a claimed product suffices — does not apply, because these are process claims not product claims. As a result, HMR/ TKT argues, Amgen has forfeited its patent under 35 U.S.C. § 112, ¶ 1 by claiming all processes for making EPO but enabling only one.
HMR/TKT cites no cases that actually support its contention that process claims are somehow different than product claims when it comes to the enablement inquiry. HMR/TKT’s Opening Br. After Trial at 49-50. The two cases that HMR/TKT does cite,
Genentech,
Here, HMR/TKT has not proved that the disclosure fails adequately to guide the skilled artisan to a process that places the promoter further upstream without undue experimentation. The thrust of HMR/ TKT’s argument — that the skilled worker would not have expected promoter linkages further upstream to produce EPO — has already been rejected by the Court. As discussed in the written description analysis, this Court finds as a factual matter that skilled artisans at the time of the application filing were aware of how to place promoters further upstream than is shown in example 7 of the ’698 patent specification. Moreover, this Court found that all the techniques required to achieve such placement were taught in the specification. According to Dr. Lodish, using the specification, one skilled in the art could have placed a promoter further upstream and produced EPO. While he admitted that some problems might have occurred and that it would have taken a little bit of work, Lodish Test., Trial Tr. at 258, this does not necessarily equate to undue experimentation.
See In re Vaeck,
Tellingly, HMR/TKT has neither addressed in its memorandum nor pointed to record evidence regarding the amount of experimentation required by one of skill in the art to use the specification to place the promoter further upstream. Rather, it implicitly asks the Court to infer undue experimentation from general testimony about the development of the technology, the admission that Dr. Lin had not actually tried to place the promoter further upstream and did not know what was upstream of the EPO gene, and the absence of working examples disclosing placement of the promoter further upstream.
92
Given this lack of. specific evidence, HMR/TKT
*279
simply has not met its burden to prove undue experimentation.
See Moba,
b. Conclusion
Accordingly, the Court holds that HMR/ TKT has failed to show by clear and convincing evidence that the process claims of the ’349 and ’698 patents were not enabled.
V. INFRINGEMENT
A. The ’698 Patent: Claim 4-9
1. Background
At the close of Amgen’s case-in-chief in the first trial, and before HMR/TKT had presented its case, this Court granted HMR/TKT’s motions for judgments of non-infringement under Fed.R.Civ.P. 52(c), both literally and under the doctrine of equivalents of claims 4-9 of the ’698 patent.
Amgen I,
On appeal, the Federal Circuit vacated and remanded this Court’s ruling regarding infringement of the ’698 patent because the Court had erroneously compared the accused device to the preferred or commercial embodiments of the patent instead of to the properly construed claims themselves.
Amgen II,
As discussed briefly in the procedural history portion of this memorandum and order, the Court denied both Amgen’s and HMR/TKT’s renewed motions for summary judgment regarding infringement of the ’698 patent [Doc. Nos. 664 and 665]. As a result, HMR/TKT presented its case on these issues at the remand trial.
HMR/TKT was also allowed to present its defense that it does not literally infringe claims 4-9 of the ’698 patent under the reverse doctrine of equivalents. The Court decided to entertain such an argument because the facts that form the reverse doctrine of equivalents defense were always a part of HMR/TKT’s interrogatory responses. In
Wright Medical Technology, Inc. v. Osteonics Corp.,
2. The Claims at Issue
Claims 4 and 6 are the critical claims for resolving the infringement issue, as claims 5, 7, 8, and 9 are dependent.
Claim 4:
*281 A process for the production of a glyco-sylated erythropoietin polypeptide having the in vivo biological property of causing bone marrow cells to increase production of reticulocytes and red blood cells comprising the steps of: (a) growing, under suitable nutrient conditions, vertebrate cells comprising promoter DNA, other than human erythropoietin promoter DNA, operatively linked to DNA encoding the mature erythropoiet-in amino acid sequence of FIG. 6; and (b) isolating said glycosylated erythro-poietin polypeptide expressed by said cells.
’698 Patent, Ex. 1, col. 38: 37-47 (paragraph structure altered).
Claim 6:
A process for the production of a glyco-sylated erythropoietin polypeptide having the in vivo biological property of causing bone marrow cells to increase production of reticulocytes and red blood cells comprising the steps of: (a) growing under suitable nutrient conditions, vertebrate cells comprising amplified DNA encoding the mature erythropoiet-in amino acid sequence of FIG. 6; and (b) isolating said glycoslated erythro-poietin polypeptide expressed by said cells.
Id. at col. 38: 50-58 (paragraph structure altered).
3. Literal Infringement
a. Discussion
To determine whether an accused device literally infringes a patent claim, courts apply a two-step analysis.
See, e.g., Watts v. XL Sys., Inc.,
The only limitation of claims 4-9 of the ’698 patent that HMR/TKT asserts it does not literally infringe is “DNA encoding the mature erythropoietin amino acid sequence of FIG. 6.”
See, e.g.,
HMR/ TKT’s Reply Br. After Trial at 26-27; HMR/TKT’s Opening Br. After Trial at 10-11. As discussed,
supra,
the Court conducted the first step of the inquiry and construed the term “DNA encoding” to mean “the genetic instructions for” the “mature erythropoietin amino acid sequence of FIG. 6.” To conduct the second step, the Court must compare the properly construed claim with the accused product to determine whether the accused product meets each and every limitation.
Bayer AG v. Elan Pharm. Research Corp.,
HMR/TKT argues that the claims require the genetic instructions for an EPO with the fully realized, secreted 166 amino acid sequence of Figure 6.
See
HMR/ TKT’s Reply Br. After Trial at 26-27; HMR/TKT’s Opening Br. After Trial at 10-11. In support it points to the Court’s ruling in
Amgen I,
in the context of the ’080 patent, that the “mature erythro-poietin amino acid sequence of FIG. 6” is “the fully realized form of the amino acid sequence of Figure 6,”
Amgen I,
HMR/TKT’s argument fails to persuade the Court because “the mature erythro-poietin amino acid sequence of FIG 6” in the context of the ’080 patent refers to the structure of the claimed glycoprotein
*282
whereas in the ’698 claims it refers to the structure of a DNA in the claims.
94
This is not to suggest that the phrase should have different meanings in different contexts. Indeed, the parties agreed in
Am-gen I
that the meaning of the term should be the same in both settings.
Amgen I,
HMR/TKT argues that “Amgen ignores that the ‘cDNA’ sequence it relies upon has a ‘methionine, alanine, threonine’ amino acid sequence, which is exon 1” and is derived from human growth hormone, not from EPO. HMR/TKT’s Findings of Fact After Trial at 24, ¶ 104. This argument, however, is irrelevant. First, as Amgen points out — and HMR/TKT does not dispute — this argument involves the amino acids of the leader sequence in HMR/ TKT’s R223 cells, yet the claims do not specifically address the leader sequence. Amgen’s Reply to HMR/TKT’s Findings of Fact at 36. The Court held, in
Amgen I,
that the mature EPO amino acid sequence of Figure 6 included only 166 amino acids, that is, positions +1 through +166.
Am-gen I,
Even so, HMR/TKT argues that proof that its DNA is the same as Amgen’s DNA is not enough. It contends that the claims require production of an EPO product with 166 amino acids because “the mature er-ythropoietin amino acid sequence of Fig. 6” is followed in the claims by a clause which states “said glycosylated erythro-poietin polypeptide” is “isolated.” HMR/ TKT’s Opening Br. After Trial at 11.
Based on the language of the claims, including the preambles, the Court rejects this argument and concludes that “the mature erythropoietin amino acid sequence of FIG. 6” modifies the words “DNA encoding” in the cells grown in step (a)—and does not modify “glycosylated erythro-poietin polypeptide” isolated in step (b). This interpretation is supported by evidence, proffered by Amgen and undisputed by HMR/TKT, that the proper antecedent basis is provided only by use of prior identical language in the claim. See Manual of Patent Examining Procedure 2173.05(e) (6th ed.1997); Amgen’s Reply to HMR/TKT’s Findings of Fact at 37. Here, “glycosylated erythropoietin polypeptide” is previously found only in the preamble and not in part (a) of the claim. 96 Part (a), although it refers to the “mature erythropoietin amino acid sequence of Fig. 6,” concerns the DNA that is doing the encoding—not the EPO itself. Part (b) merely addresses the next step in the process which is the step of isolating. Thus, “said glycosylated erythropoietin polypeptide” refers back to the preamble before steps (a) and (b) are described. This is the only reading that makes grammatical sense. Moreover, it is consistent with how the claims of the ’080 patent are read. There, “said erythropoietin glycoprotein” always refers back to the exact identical language at the beginning of the claim and not to the attributes of the glycoprotein itself. ’080 Patent, Ex. 1, col. 38: 39-50.
b. Conclusion
In sum, Amgen has shown by a preponderance of the evidence that HMR/TKT’s HMR 4396 does indeed literally infringe claims 4-9 of the ’698 patent. Before ruling that Amgen prevails on this issue, however, the Court must address HMR/TKT’s reverse doctrine of equivalents defense.
4. Reverse Doctrine of Equivalents
a. Overview of the Doctrine
The reverse doctrine of equivalents is an equitable doctrine that a court applies when it finds that the accused device literally infringes a patented invention, but is so fundamentally different from the patented invention that a judgment of infringement would be inappropriate.
Texas Instruments, Inc. v. United States
*284
International Trade Commission,
The reverse doctrine of equivalents is applied equitably based upon factual determinations made after “the accused infringer proves that, despite the asserted claims literally reading on the accused devise, ‘it has been so changed that it is no longer the same invention.’ ”
Amgen II,
The patentee may bring the defendant within the letter of his claims, but if the latter has so far changed the principle of the device that the claims of the patent, literally construed, have ceased to represent his actual invention, he is as little *285 subject to be adjudged an infringer as one who has violated the letter of a statute has to be convicted, when he has done nothing in conflict with its spirit and intent.
Although the Federal Circuit recognizes this doctrine, it is rarely invoked successfully. Shyh-Jen Wang & Shyh-Yau Wang,
The Verification Flow Chart of Patent Infringement,
86 J. Pat.
&
Trademark Off. Soc’y 74, 78 (2004) (“[I]t is not often raised and even less frequently successful.”); Burk & Lemley,
supra,
at 1657. Indeed, according to the Federal Circuit, it has never upheld a decision of non-infringement based on the reverse doctrine of equivalents.
Tate,
The reverse doctrine of equivalents is invoked when claims are written more broadly than the disclosure warrants. The purpose of restricting the scope of such claims is not only to avoid a holding of infringement when a court deems it appropriate, but often is to preserve the validity of the claims with respect to their original intended scope.
Despite the paucity of cases relying on the reverse doctrine, the doctrine is not yet dead.
102
Indeed, just last year, the Federal Circuit implied in two separate cases that the reverse doctrine of equiva
*287
lents still had a heart beat, albeit a faint one.
See Amgen II,
Although both the reverse doctrine of equivalents and section 112 spring from the same roots and very often take account of the same factors and considerations,”
Texas Instruments II,
This is not to suggest that the reverse doctrine of equivalents should be invoked frequently. To the contrary, it should be saved — and apparently is — for the inventor that
radically,
not just modestly, improves upon the prior art such that there is a “manifest departure • from the principle in the [patentee’s] patent.”
Westinghouse,
b. Discussion
HMR/TKT argues that it does not infringe claims 4-9 of the ’698 patent because its process is “so far removed in terms of its principles of operation from the process Amgen disclosed.” HMR/ TKT’s Opening Br. After Trial at 18. Although HMR/TKT proffers many reasons in support of its position, it has failed to make out a prima facie case.
107
As Amgen aptly points out, HMR/TKT makes the same mistake with each of its arguments. It repeatedly compares its process to the examples disclosed in Amgen’s patent specification instead of to the “equitable scope of the claims.”
Scripps,
(1) Homologous Recombination, Endogenous EPO DNA, and The Neighborhood’s Effect on the Production of EPO
(a) Homologous Recombination and Endogenous EPO DNA 109
HMR/TKT repeatedly asserts that (1) its process is different because it uses homologous recombination (as opposed to heterologous recombination); and (2) its EPO gene is different in structure because HMR/TKT’s EPO DNA is endogenous and Amgen’s is exogenous. HMR/TKT’s Opening Br. After Trial at 13; HMR/TKT’s Proposed Findings of Fact ¶ 141; HMR/TKT’s Reply Br. After Trial at 28. 110
Tellingly, aside from the neighborhood theory (discussed immediately below),
*291
HMR/TKT does not even attempt to explain how these differences matter — that is, how they are different in principle from the processes disclosed in Amgen’s patents. Instead, it primarily relies on this Court’s prior findings, in the equivalent infringement context, that HMR/TKT’s process is not substantially similar to Am-gen’s because,
inter alia,
it uses homologous recombination and endogenous activation techniques.
See, e.g., Amgen I,
True, heterologous recombination and endogenous activation techniques were not known by skilled artisans at the time Amgen filed its application. Equivalent infringement, however, is evaluated based on the date of infringement.
Warner-Jenkinson,
(b) The Endogenous EPO Neighborhood and Its Effect on EPO Production
HMR/TKT argues that how the gene construct “functions with the surrounding neighborhood to produce EPO is completely different in HMR/TKT’s and Amgen’s cells.” HMR/TKT’s Proposed Findings of Fact at 29-32; HMR/TKT’s Opening Br. After Trial at 16 (claiming that the way in which expression of human EPO is accomplished is significantly different in HMR/TKT’s process). In support, it explains that HMR/TKT activates the normally silent EPO gene and inserts it amidst the endogenous EPO neighborhood. HMR/TKT’s Proposed Findings of Fact ¶¶ 122-125. This, according to HMR/ TKT, enables the promoter “to work with other nearby enhancers and the EPO gene neighborhood to contribute to the gene’s transcriptional activity,” id. ¶ 124, and to “produce higher levels of EPO,” id. ¶ 129. See id. ¶¶ 126-138. 111
While this theory is intriguing — and might well have justified invocation of the reverse doctrine of equivalents — the evidence HMR/TKT presented fails sufficiently to support it.
HMR/TKT relied primarily on Dr. Kingston’s testimony to elucidate its neighborhood theory. Dr. Kingston testified that the neighborhood around the EPO gene affects expression capability. See, e.g., Kingston Test., R. Trial Tr. at 36. He explained that HMR/TKT uses an endogenous EPO promoter in a region that is normally set up to express EPO. Therefore, like a hotel that is positioned in the heart of the city, he argued, it is helped by its surroundings, that is, the nearby regulatory sites “all work together to help keep this gene on.” See, e.g., Kingston Test., R. Trial Tr. at 26-28. This is different, according to Dr. Kingston, than Amgen’s process which, as explained in the specification, randomly integrates exogenous DNA, leaving the potential surroundings up to chance. Id. at 26-28 (“A gene that has gone into an open region that doesn’t happen to be near any other regulatory elements” may have “nothing in its surroundings to help it stay on.”); id. at 151. Dr. Kingston opined that it was the neighborhood — and not the difference in promoter strength, culture conditions, media, *293 or cell type, or any other factors — that caused HMR/TKT’s construct to express more EPO per gene copy than the cells made following example 10 in Amgen’s patent. Id. at 29-33.
Although this testimony is compelling, it fails to persuade the Court for three reasons. First, notwithstanding Dr. Kingston’s testimony to the contrary, the bulk of the credible evidence demonstrates that the endogenous regulatory sequences surrounding the EPO gene in HMR/TKT’s construct are “inactive” and actually do not work with the CMV promoter to enhance EPO reproduction in the R223 cells. Dr. Wall testified that the EPO neighborhood in HRM/TKT’s cells does not enhance their ability to produce EPO. Wall Test., R. Trial Tr. at 1149: 3-5, 1161-62. Specifically, he explained
The genomic neighborhood around the EPO gene is there to constrain the expression of the EPO gene in very specific cells; and in all the rest of the cells in the body the genomic neighborhood is silent, it’s shut down, it’s not responsive to hypoxia. So the genomic neighborhood is not set there to somehow enhance the activity of this really robust viral promoter. Instead, it’s there to exquisitely restrict the level and the tissue-specific activity of the EPO gene expression.
Id. at 1161: 18-1162: 2; id. at 1148: 13-25, 1149: 5-9, 1162: 15-1163: 11. See also Lodish Test., R. Trial Tr. at 1085-86 (disagreeing with Kingston’s neighborhood theory). Moreover, contrary evidence exists not merely from Amgen but also from HMR/TKT itself. In its own FDA filings, HMR/TKT admitted that the regulatory sequences surrounding the EPO gene in HMR/TKT’s construct are not active and actually are bypassed. HMR/TKT’s IND, Ex. 18, at 16 (stating that HMR/TKT’s technology works by “bypassing regulatory DNA sequences set in the “off position” ”); HMR/TKT’s IND, Ex. 19, at 561.
Second, Dr. Kingston — the sole exponent of the neighborhood theory — did not perform any experiment to validate his conclusions. Kingston Test., Trial Tr. at 1495: 9-1496: 16; Kingston Test., R. Trial Tr. at 189: 14-16; Lodish Test., R. Trial Tr. at 1086 (noting that there is no evidence that supports Dr. Kingston’s contention); id. at 1096: 1-5. He merely compared HMR/TKT’s R223 cell experiments with Amgen’s Example 10 cell experiments. These comparisons do not, on their own, establish Dr. Kingston’s conclusions. As both Dr. Lodish and Dr. Wall pointed out — and Dr. Kingston did not dispute — Dr. Kingstown compared EPO production per gene copy by looking at experiments with cells grown in different locations under different conditions by different people without controlling for other variables that could have affected the amount of EPO produced per gene copy. Id. at 1095-98, 1091 (explaining that Dr. Kingston’s comparison did not account for the different growing conditions, different promoters, and many other variables in the experiment that are evidenced by the thousand-fold variance in data points for one construct and pointing out that Kingston relied on only a single data point); Wall Test., R. Trial Tr. at 1155, 1157-1158 (objecting to Dr. Kingston’s conclusions because there is not a reliably established significant difference; “you can’t really compare these two cells. They’re like apples and oranges” due to “time differences” and a “large number of variables that could affect the expression level of EPO in those cells”); cf. Kingston Test., R. Trial Tr. at 190-91, 199-202, 205-06 (conceding that no other experiments were conducted, that the experiments were based on a single data point, and that he could not do a statistical analysis to determine if there was an outlier, but *294 asserting that he still considered them to be controlled experiments); Kingston Test., Trial Tr. at 1484-85, 1490-91 (acknowledging that factors other than “neighborhood” effects can affect the amount of EPO produced per gene copy). Even Dr. Kingston admitted that a failure to use controls can lead to erroneous or misleading results and that a competent technician controls for the variables that could cause certain results. Kingston Test., R. Trial Tr. at 120: 10-18, 119: 9-120: 3. Furthermore, the evidence at trial suggested that HMR/TKT’s experimental data itself was inconsistent. A single data point was an 800-fold difference from all the other data points' — a variance greater than the alleged 500-fold difference between the single data point for pREP026 and the highest value reported for pRE-P022. Kingston Test., R. Trial Tr. at 190: 16-25, 201: 1-10; see also 12-17-96 Memo from Fike to Hermentin, Ex. 165. Thus, there is no reliable experimental data supporting the contention that it is the neighborhood, as opposed to some other factor, that accounts for HMR/TKT’s expression capabilities.
Third, even if HMR/TKT had proven that the genomic EPO regulatory sequences in the EPO neighborhood — and not other factors like nutritional growth conditions, limits in cellular folding, strength of promoter, number of enhancers, and the Kozak sequence — affected the amount of EPO produced per gene copy, that would not have proved a meaningful change or substantial difference in actual EPO production.
SRI Int’l,
Had HMR/TKT proven that its new technology of using homologous recombination or endogenous activation actually worked in some substantially different way due to the neighborhood and enabled it to produce significantly more EPO or EPO that somehow differed in its biologic or therapeutic effects (which would have supported HMR/TKT’s contention that its technology functions differently), it might well have demonstrated sufficient grounds for invoking the reverse doctrine of equivalents.
Cf. Scripps,
Thus, despite the fact that HMR/TKT’s process employs homologous recombination and endogenous DNA and produces more EPO per gene copy than Amgen’s Example 10 cells, it appears that its process does exactly that which Amgen’s patent teaches: it introduces a strong viral promoter and non-human enhancers to overcome the naturally restrictive neighborhood in the R223 cells. See Wall Test., R. Trial Tr. at 1149: 3-14, 1159: 6-1161: 13; Lodish Test., R. Trial Tr. at 1097; Lodish Test., Trial Tr. at 165: 1-11, 178: 4-12; Kingston Test., Trial Tr. at 1382-1386. 114
(2) Different Promoter Placement, Splice Sites, and Leader Sequences
HMR/TKT argues that it places its promoter much farther upstream of the EPO gene to be expressed than does Am-gen and that this was something those skilled in the art in 1984 would not have dared to attempt. HMR/TKT’s Opening Br. After Trial at 13. As a result, it contends, HMR/TKT’s process for producing EPO uses primary RNA transcripts and splice sites that differ from those used in Amgen’s process, and results in a different EPO mRNA in HMR/TKT’s and Am-gen’s cells and a different primary EPO protein product. HMR/TKT’s Proposed Findings of Fact at 33-36; HMR/TKT’s Opening Br. After Trial at 15.
(a) Upstream Promoter Placement and Splice Sites
Although it is undisputed that HMR/ TKT places its promoter much farther upstream than 44 base pairs (the position described in one example in Amgen’s specification), the Court has now found that placement of the promoter further upstream of the EPO coding region and splicing out deleterious ATGs was indeed a concept known and understood to those *296 skilled in the art at the time Amgen filed its application (1983-84). 115 Furthermore, the Court has held that Amgen’s process covers, adequately describes, and enables such upstream promoter placement.
In terms of the EPO splice donor sites, it is undisputed that absent the exons, the splice donor sites are the same and that the intended effect of both processes was to splice out what is in between including intervening sequences and any deleterious ATGs. See, e.g., Kingston Test., Trial Tr. at 1431: 10-19, 1432: 14-24, 1433: 1-22, 1440: 19-25, 2094-2102 (admitting that what HMR/TKT labeled as its splice donor site is identical to the human splice donor site disclosed by Amgen in Figure 6). HMR/TKT argues, however, that its splice site is not the same as Amgen’s because the left portion (the exon) is different. HMR/TKT’s Opening Br. After Trial at 15; HMR/TKT’s Proposed Findings of Fact at 35. It asserts that “it is the exon portion that matters” because it creates the leader sequence for the expressed polypeptide, that is, the exons remain to encode the polypeptide while the introns are removed. HMR/TKT’s Opening Br. After Trial at 15. Amgen argues that the exon is irrelevant and not part of the splice site. Therefore, the key factual question for the Court is whether exons are included when one skilled in the art refers to the splice sites.
To the extent .that the experts disagreed, the Court credits Dr. Lodish’s testimony explaining that the exons are not included. Lodish Test., R. Trial Tr. at 1107-10; id. at 1132-33 (explaining that it is the splice donor sequence, not the splice junction, that will determine where downstream and with what corresponding DNA downstream a splice junction will splice and stating that “the splice donor is the sequence ... that is removed during the splicing process,” the splice acceptor is the sequence that is removed downstream, and “it’s the regions on either side that are linked together”). This accreditation of Dr. Lodish’s testimony is supported by evidence that HMR/TKT itself did not consider the hgH exon 1 to be part of the splice donor sequence. In its Investiga-tional New Drug Application (IND) and in its patent, HMR/TKT identifies the splice donor site to be separate from the growth hormone exon 1 sequence. See, e.g., HMR/TKT’s IND, Ex. 19, at 554; HRM7 TKT’s IND, Ex. 20, at 830; U.S. Patent No. 5,641,670 (“Treco’s Patent”), Ex. 12, col. 50: 53-55; see also Kingston Test., Trial Tr. at 2094-2102 (conceding that this interpretation of the IND and patent is correct — that is, that HMR/TKT did not include the three nucleotides in exon 1 as part of the splice donor sequence). Moreover, in the IND, HMR/TKT identifies the splice donor sequence to be the first 10 nucleotides of intron 1: GTGAGTACTC, which is identical to the sequence in Am-gen’s patent. See, e.g., HMR/TKT’s IND, Ex. 19, at 554; HRM/TKT’s IND, Ex. 20, at 830; see also Demonstrative Aids 7 & 8 from Lodish Rebuttal Examination, R. Trial.
Thus, as alluded to earlier in the written description analysis, this Court finds that the fair preponderance of the evidence shows, by a slight margin, that HMR 4396 uses the same splice donor site as that disclosed in Amgen’s specification. Kingston Test., Trial Tr. at 1431: 10-19, 1432: 14-24, 1433: 1-22, 1440: 19-25 (admitting that absent the exons, the splice donor sites were the same and that the intended effect was to splice out what is in between, including intervening sequences and the
*297
deleterious ATGs). The only difference is that Amgen takes the genomic EPO splice donor site disclosed in Amgen’s Figure 6 and moves it upstream. Placing the promoter further upstream of DNA encoding a protein using the identical splice site is simply not a fundamental change in principal, because the intervening DNA is spliced out when the mRNA is formed. As discussed
supra,
skilled artisans could have done this at the time Amgen filed its application, and, more importantly, skilled artisans could easily have done it at the time of the alleged infringement — -the relevant time period for analyzing equivalent infringement.
Warner-Jenkinson,
(b) Different Leader Sequences in the Primary EPO Protein Product
HMR/TKT argues that its primary EPO protein product is different from Amgen’s product because it contains a hybrid leader sequence containing both hGH and human EPO amino acids, whereas Amgen’s only contains EPO leader sequences. HMR/ TKT’s Proposed Findings of Fact at 36; HMR/TKT’s Opening Br. After Trial at 15. 117 At trial, Dr. Lodish conceded that in Amgen’s Example 10, exon 1 comes from the EPO gene whereas in HMR/TKT’s process, it comes from the human growth hormone gene. Lodish Test., Trial Tr. at 174. He explained that the difference be *298 tween the leader peptides is a “minor” one because they both function in exactly the same way and both are removed. Id.; see also id. at 433-34 (stating that the leader peptides are different but perform the same function and are ultimately cleaved); id. at 159-160. Evidently, exons 2-5 of the EPO structural genes are what encode amino acids in the mature secreted form of the protein. Id. at 173; id. at 160 (“[E]xon 1 ... encodes part of the leader peptide which is removed from the cell and has no other function.”). Furthermore, what is ultimately secreted from the cell is the same polypeptide with three n-linked oligosacharides, sialic acids ... and one o-linked oligosacharide.” Id. at 174; id. at 160 (“Exon 1 ... has no effect whatsoever on the secreted mature EPO glycopro-tein.”). HMR/TKT points to no evidence disputing this testimony nor does it even attempt to explain how this difference presents a change in principle from Am-gen’s patented process.
(3) Method of Growing Cells
HMR/TKT argues that it grows its cells in a substantially different manner from that described in the ’698 patent. HMR/TKT’s Opening Br. After Trial at 18-19; HMR/TKT’s Proposed Findings of Fact at 38-41. It points out that Amgen’s specification describes a process of growing vertebrate cells that uses a roller bottle system to obtain adhesion of the cell line to the bottle surface. HMR/TKT’s Opening Br. After Trial at 19. HMR/ TKT, on the other hand, uses an air-lift technology that “works in a completely different way from roller bottle technology”. Id.
These arguments fail for the same reasons that all of HMR/TKT’s other reverse doctrine of equivalents arguments fail. First, HMR/TKT compares its process to the method of culturing described in an embodiment in the specification instead of to the spirit and intent of the claims. Second, it has not even argued how its culturing process is changed in principle from that explicated in Amgen’s patent.
The Court begins by pointing out that it has not construed the claims to require roller bottle culturing. Nor has HMR/ TKT pointed to anything in the patent, specification, or prosecution history to compel it to do so. HMR/TKT simply argues that because a roller bottle system is the only type of culturing actually described in the specification, the claims should be limited to this type of culturing. The Court has already explained at length that a patent’s scope is not limited to those embodiments described in the specification, absent concerns about invalidity, prosecution history estoppel, or other such grounds.
Moreover, after a careful review of the specification, it is clear that it does anything but imply that use of roller bottles is the only way to culture or grow the cells. The specification states that productivity can be improved “by appropriate cell culture techniques.” ’933 Patent, Ex. 1, col. 27: 7-9. Then it makes a general statement that “[the] propagation of mammalian cells in culture generally requires the presence of serum in the growth media,” but that “a method” that does not contain serum can “greatly facilitate” the process. Id. at col. 27: 10-14 (emphasis added). The implication of these two sentences is (a) more than one culturing technique is contemplated, and (b) both serum and serum-free culturing can be used to propagate mammalian cells, but serum-free is preferred. The specification then goes on to describe one such preferred method that happens to use roller bottles. Id. at col. 27: 15-53. Later, the specification also teaches, in the preferred method, growing suspension cell cultures in spinner *299 flasks — yet another type of culturing or growing process. Id. at col. 27: 19-21. Thus, the specification does not only teach culturing via the roller-bottle but also teaches culturing in spinner flasks. 118 Indeed, HMR/TKT’s expert testimony confirms this interpretation of the specification. See Hancock Test., R. Trial Tr. at 259: 20-260: 21, 262: 16-263: 24 (admitting that in 1984 roller-bottles were not the only method for culturing mammalian cells and that the specification teaches growing up the suspension cell cultures in spinner flasks, which grow the cells in suspension).
Since HMR/TKT points to nothing in the patent or prosecution history to support adding a limitation to the claims, the Court refuses to do so. The equitable scope of the claim is broader than roller-bottle culturing.
Scripps,
Even if the Court were to limit the claims to a roller bottle system of culturing, HRM/TKT would still fall short of making a prima facie showing that the reverse doctrine of equivalents is applicable. HMR/TKT does not even attempt to explain how using an air-lift fermenter to grow its cells (as opposed to roller bottles) justifies invoking the reverse doctrine of equivalents, that is, it does not show how this difference is a “manifest departure in principle” or even novel, for that matter.
Westinghouse,
Indeed, HMR/TKT did not even show that air-lift fermenting was superior let alone a substantial or radical improvement. Dr. Hancock basically testified as to how the processes were different, but said nothing about how these differences mattered.
See generally
Hancock Test., R. Trial Tr. at 232-39. True, Dr. Hancock testified there is a risk of contamination when using fetal calf serum and that the air-lift fermenter allows for more uniform monitoring and control of conditions since it only uses one vessel.
Id.
at 234-35, 241, 256;
see also id.
at 238-399. He did not,
*300
however, loop it back together. He did not present or refer to any controlled experimental data comparing the two processes that showed that fetal calf serum caused contamination that affected the process.
Id.
at 256-57. Moreover, he did not testify as to how or even whether the additional level of control in air-lift fermenting is beneficial or superior.
Id.
at 239. He merely made some vague statements that in the air lift fermentation technology, the process could potentially be optimized because the medium can be defined.
Id.
at 242-43. Even if there had been a more concrete showing that serum-free medium was advantageous to fetal-calf serum medium, it would not have been enough to show a substantial change or manifest departure in principle. As discussed earlier, the mere fact that something is improved or better does not justify invoking the reverse doctrine.
See, e.g., Studiengesellschaft,
Further, HMR/TKT’s own expert implicitly admitted that growing cells in an air-lift fermenter is equivalent to many culture methods including the roller bottles or spinner flasks exemplified in Am-gen’s patent. Hancock Test., R. Trial Tr. at 264: 12-265: 12, 261: 23-262: 24 (conceding that regardless of whether roller bottle spinner cells are used or other types of culturing techniques, the objectives are the same and can be met by mixing or agitating the cell culture by spinning, rolling, or mixing it with air bubbles from an air-lift fermenter).
As the Federal Circuit has noted many times in the past, “[ejquivalence and non-equivalence, as the terms indicate, are but opposite sides of the same coin.”
SRI International,
(4) HMR/TKT’s Process Was Patented
HMR/TKT seems to believe that since the United States Patent and Trademark Office granted it a patent on its culturing process, the two processes must be so substantially different that the reverse doctrine of equivalents can justifiably be invoked.
See, e.g.,
HMR/TKT’s Reply Br. After Trial at 28; HMR/TKT’s Proposed Findings of Fact ¶ 121. While attainment of a patent may aid in making a prima facie case in support of the reverse doctrine of equivalents,
see, e.g., Jewish Hosp. of St. Louis v. IDEXX Laboratories,
c. Conclusion
HMR/TKT has succeeded in proving that its process differs in many respects from those specifically exemplified in the Amgen’s specification and even is advanced technologically in at least one way. As the Supreme Court explained in Graver Tank, however,
Equivalence, in the patent law, is not the prisoner of a formula and is not an absolute to be considered in a vacuum. It does not require complete identity for every purpose in every respect. In determining equivalents, things equal to the same thing may not be equal to each other and, by the same token, things for most purposes different may sometimes be equivalents. Consideration must be given to the purpose for which [some aspect of the invention] is used in a patent, the qualities it has when combined with the other [aspects], and the function which it is intended to perform.
While the Court affirms the viability of the reverse doctrine of equivalents for those rare cases where the claims read on a new device or process despite its use of a new technology that makes a real difference in how the process works pr what is produced, HMR/TKT has failed to meet its burden in establishing the defense here *302 (although the neighborhood theory potentially could have carried the day, had it been thoroughly demonstrated through experimentation at trial).
5. Ultimate Conclusion Concerning Infringement of the ’698 Process Patent
The Court holds that Amgen has carried its burden of proving by a fair preponderance of the evidence that HMR/TKT’s process infringes the ’698 patent, claims 4-9.
B. The ’349 Patent: Claim 7
1.Background
In
Amgen I,
the Court held that HMR/ TKT did not literally or equivalently infringe claim 7, the process claim, of the ’349 patent.
Amgen I,
Since the Court heard the entirety of both parties’ arguments and evidence concerning the ’349 patent at the first trial, no new evidence with respect to this patent was taken on remand. The parties, however, were given the opportunity to brief the issues remanded to this Court in pre and post-trial memoranda. Before the Court are both parties’ motions for judgment pursuant to rule 52(c) [Doc. Nos. 674 & 686],
In HMR/TKT’s motion for judgment pursuant to rule 52(c), it argued a new defense, the reverse doctrine of equivalents. Although the Court allowed the defense as it related to the ’698 patent, it did not definitively do so for the ’349 patent, because the procedural postures of the two patents were different. HMR/TKT never had a chance to present its case of non-infringement with regard to the ’698 patent in Amgen I, but it did with regard to the ’349 patent. As it ends up, this procedural dispute is moot. Even if the Court were to allow the defense at this stage, it would fail for lack of merit.
2. The Claim At Issue
Amgen’s ’349 patent contains six product claims regarding types of vertebrate cells grown in culture and one process claim, claim 7. The issue is whether HMR/TKT infringed claim 7, the process claim:
A process for producing erythropoietin comprising the step of culturing, under suitable nutrient conditions, vertebrate cells according to claim 1, 2, 3, 4, 5 or 6.
’349 Patent, Ex. 1, col. 38: 34-36.
3. Literal Infringement
a. Discussion
Since literal infringement of claims 1, 2, 4, and 6 has been established and affirmed,
Amgen II,
First, Dr. Lodish specifically testified that “I guess there is no dispute that [HMR/TKT’s] cells are cultured and they’re clearly vertebrate cells.” Am-gen’s ’349 App., Tab I (Lodish Test., Trial Tr.) at 300: 22-301: 8. HMR/TKT’s assertion that Dr. Lodish’s testimony makes clear that he was only guessing does not cast any affirmative doubt on Dr. Lodish’s statements, which this Court credits.
Second, as discussed earlier, the Joint Pretrial Memorandum itself states that HMR/TKT’s HMR 4396 is produced by “growing, under suitable nutrient conditions R223 cells,” Amgen’s ’349 App., Tab M (4/26/00 Corrected Joint Pretrial Mem.), ¶ 25, and that its cells are cultured, id. ¶ 13 (“HMR 4396 is produced from the R223 cell line grown in culture.”). Since HMR/TKT has admitted in various contexts that culturing and growing basically mean the same thing, it has implicitly admitted that its process literally infringes claim 7. 122
Last, this Court’s factual findings support the holding that HMR/TKT’s process cultures the cells. In finding literal infringement of claims 1 and 4 of the ’349 patent, this Court found that HMR/TKT’s R223 cells are “capable, upon growth in culture, of producing erythropoietin in the medium of their growth in excess of 100 units of erythropoietin per 10 cells in forty-eight hours as determined by RIA (ra-dioimmunoassay),” just like Amgen’s cells.
Amgen I,
Tellingly, HMR/TKT did not even argue in its post-trial submissions that its process did not literally infringe claim 7 of the ’349 patent.
b. Conclusion Concerning Infringement: ’349 Patent, Claim 7
Amgen has shown by a fair preponderance of the evidence that HMR/TKT’s HMR 4396 literally infringes claim 7 of the ’349 patent.
4. Reverse Doctrine of Equivalents
HMR/TKT presented the exact same arguments in furtherance of its reverse doctrine of equivalents arguments for the ’349 patent as it did for the ’698 patent. Given that it points to nothing in the claims or prosecution history of the ’349 patent specifically in support, and the specifications are the same as between the two patents, the above analysis with respect to the ’698 patent applies here. 123
*304 5. Ultimate Conclusion Concerning Infringement of Claim 7 of the ’349 Patent
The Court rules that Amgen has shown by a fair • preponderance of the evidence that HMR/TKT’s process literally infringes Amgen’s ’349 patent. Therefore, HMR/TKT’s Fed.R.Civ.P. 52(c) motion regarding infringement of the ’349 patent [Doc. No. 686] is DENIED and Amgen’s Fed.R.Civ.P. 52(c) motion regarding infringement of the ’349 patent [Doc. No. 674] is ALLOWED.
VI. VALIDITY CHALLENGES UNDER 35 U.S.C. §§ 102(a) & 103
HMR/TKT argues that the asserted claims of the ’422, ’080, ’698, and ’349 patents are either anticipated or rendered obvious by Sugimoto, Goldwasser, or both. Since these patents are presumed valid, HMR/TKT bears the burden of proving its contentions by clear and convincing evidence. 35 U.S.C. § 282 (2000);
Amgen II,
A. Sugimoto
1. Background
a. Overview of Sugimoto
U.S. Patent No. 4,377,513 (Sugimoto’s patent) was filed in 1981 and issued to Sugimoto on March 22, 1983. Sugimoto’s patent, Ex. 2229, at 1. Sugimoto claims a process for producing human erythropoiet-in comprising “multiplying human lym-phoblastoid cells capable of producing er-ythropoietin by transplanting said cells into a non-human warm-blooded animal body,” or, alternatively, multiplying said cells “by allowing said cells to multiply with a device by which the nutrient body fluid of a non-human warm-blooded animal is supplied to said cells,” and allowing the cells multiplied by either of the above multiplications procedures to release human erythropoietin.
Id.
at col. 6: 46-59. Put another way, Sugimoto claims that when a human cell line that produces EPO is fused with a human lymphoblastoid cell line, the resulting fused cells produce higher amounts of EPO in culture than the original fusion partners.
Amgen I,
b. The Court’s Decisions in Amgen I
(1) Anticipation
This Court held that HMR/TKT failed to show by clear and convincing evidence that Sugimoto’s patent anticipated Am-gen’s ’422, ’080, and ’349 patents. Id. at 110. In support of this holding, it found that Sugimoto was not enabled and that none of the cited references disclose each and every limitation of any of Amgen’s individual claims. Id. at 109. With respect specifically to claim 1 of the ’422 patent, the Court found that none of the cited references disclose a therapeutically effective amount of EPO or the purification of human EPO from mammalian cells grown in culture. Id.
(2) Obviousness
Because the Court had already held that HMR/TKT failed to prove that Sugimoto was enabled, it held that Amgen’s claims were also not invalid due to obviousness. The Court noted in a footnote, however, that had the Court found the Sugimoto patent enabled, it would have “go[ne] a long way toward proving HMR/TKT’s ob
*305
viousness defense.”
Id.
at 114. This is because the patent itself suggested combining its invention with prior art sources relating to both purification and therapeutic delivery. The Court noted that if one of ordinary skill could actually make the EPO-producing cells described in the Sugi-moto patent, a point on which HMR/TKT failed to persuade this Court, such a combination of prior art material might render invalid the pharmaceutical composition claims of the ’080, and ’422 patents.
Am-gen I,
c. The Federal Circuit’s Opinion
The Federal Circuit ruled that the Court erred in placing the burden of proving enablement of Sugimoto on HMR/ TKT.
Amgen II,
The Federal Circuit noted that the Court could not have found that Amgen met its burden based solely on Dr. Er-slev’s testimony that “no one reported using Sugimoto’s process to make a pharmaceutical composition of human EPO, nor has any patient ever been treated by any EPO produced by Sugimoto procedure.” Id. at 1356. “The mere fact that no one has so used the Sugimoto process is only minimally probative of non-enablement: a conclusion that no one could have used Sugimoto.” Id. at 1356. Moreover, the Federal Circuit stated, the fact that Am-gen argued non-enablement of Sugimoto before the patent examiner during prosecution of Amgen’s patents is only minimally probative of the issue since this was only one argument out of many and “we cannot assume the acceptance of every argument presented during prosecution.” Id. Thus, the Federal Circuit concluded that Amgen had not presented evidence sufficient to meet its burden.
The Federal Circuit clarified that the Court’s error was harmless for the most part because the Court had conducted a detailed anticipation analysis. With respect to claim 1 of the ’422 patent, however, the Federal Circuit directed the Court to consider, on remand, whether it is novel over Sugimoto in light of the Court’s new definition of “therapeutically effective” while being “mindful of the principle that source limitations cannot impart novelty to old compositions.” Id.
Additionally, the Federal Circuit remanded to this Court the issue of obviousness in light of Sugimoto, because a *306 reference need not be enabled to prove invalidity under section 103. Id. at 1537.
2. The Claims at Issue
HMR/TKT argues that Sugimoto (1) anticipates claim 1 of the ’422 patent and claims 6 and 9 of the ’698 patent and (2) renders obvious claim 1 of the ’422 patent, claims 2-4 of the ’080 patent, and the asserted claims of the ’349 and ’698 patents.
3. Discussion
a. Anticipation: Does Sugimoto Anticipate Any of the Asserted Claims of the ’422 and ’698 Patents?
“[I]nvalidity by anticipation requires that the four corners of a single, prior art document describe every element of the claimed invention, either expressly or inherently, such that a person of ordinary skill in the art could practice the invention without undue experimentation.”
Advanced Display Sys., Inc. v. Kent State Univ.,
(1) Has Amgen Shown that Sugimoto Was Not Enabled?
As the Federal Circuit explained in
Amgen II,
“a non-enabled disclosure cannot be anticipatory (because it is not truly prior art) if that disclosure fails to enable one of skill in the art to reduce the disclosed invention to practice.”
*307
For the following reasons, the Court finds that Amgen has shown by a preponderance of the evidence that Sugimoto is not enabled — that is, that Sugimoto’s specification does not teach skilled artisans how to make and use the entire scope of the claimed invention without undue experimentation.
See
35 U.S.C. § 112, ¶ 1 (2000);
Genentech,
(a) The Starting Materials Were Neither Described Nor Made Available to the Public
First, the Sugimoto starting materials were not deposited, not described so that one skilled in the art could obtain them, and not otherwise made available to the public. Both Dr. Lodish and Dr. Green testified that Sugimoto’s failure to deposit the starting materials, or to make them available to the public in some way, was critical in this case, because Sugimoto also failed to describe the starting kidney cells in a manner that would enable one skilled in the art to reproduce the method. See Lodish Test., R. Trial Tr. at 287: 3-288: 16 (explaining that Sugimoto only loosely describes the kidney tumor cells as “carcinomas,” when he should have characterized the cells as to karyotype and morphology so that one could repeat the experiments); Green Test., R. Trial Tr. at 421: 4-422: 2 (hypothesizing that one reason why HMR/TKT’s attempts to reproduce Sugimoto’s hybridization failed might be that HMR/TKT was unable to obtain the starting kidney tumor line described by Sugimoto).
That this failure to teach how to obtain the starting materials or to deposit them was debilitating is evidenced by both parties’ unsuccessful attempts to procure such cells. Amgen, after many attempts, was unsuccessful at locating or obtaining any of the human kidney tumor cells used by Sugimoto or any cells capable of producing EPO at the levels reported by Sugimoto in his patent. Lin Test., R. Trial Tr. at 562: 19-563: ll.
126
Moreover, as this Court found in
Amgen I,
after an arduous search, even HMR/TKT’s star witness, Dr. Heart-lein, was unable to obtain any of the human kidney tumor cells used by Sugimoto,
HMR/TKT urges that Dr. Heartlein did not duplicate Sugimoto and, therefore, that his experiments cannot be used to show
*308
that Sugimoto was not enabled.
Johns Hopkins Univ. v. CellPro, Inc.,
HMR/TKT argues that EPO-producing cells such as the human cell line that Gold-wasser obtained from Abbott and from the American Type Culture Collection (ATCC) were available to the public and that, as of 1984, several groups of researchers had reported human kidney tumor cells capable of production of human EPO. See, e.g., HMR/TKT’s Proposed Findings of Fact ¶¶ 281-85; HMR/TKT’s Response to Am-gen’s Proposed Conclusions of Law and Findings of Fact ¶ 21. The evidence shows, however, that these cells were not comparable to the starting materials reported by Sugimoto. Lin Test., R. Trial Tr. at 562: 19-563: 11 (testifying that Amgen was never successful in obtaining EPO producing human cells or tissue sources). The Abbott cells were normal embryonic kidney cells, not kidney tumor cells, and they did not produce EPO. Id. at 541-42; Amgen Project Update, Ex. 234 (providing that Abbott cells did not make EPO). None of the cells Amgen obtained from the ATCC made EPO or could be induced to produce EPO at the levels reported in Sugimoto. Lin Test., R. Trial Tr. at 559: 21-560: 2; 1/20/83 Memo from Browne to Distribution, Ex. 235; Excerpts from Lab Notes, Ex. 236; 3/23/83 Summary Notes from Lin, Ex. 237. As to the other reported EPO producing kidney tumor cells, Dr. Sherwood would not make her cells available, Lin Test., R. Trial Tr. at 540, and Dr. Green testified that none of the cell lines made appreciable amounts of EPO, Green Test., R. Trial Tr. at 421, 471: 6-19, 478: 3-15 (explaining that he was not aware that any of these researchers showed that production of EPO was sustained to the same level over time, and testifying that in 1984, several groups of researchers had reported human kidney tumor cells capable of production of human EPO, but they were “all poor producers of the EPO”); Joseph W. Eschbach, The History of Renal Anemia (Anemia and Er-ythropoietin), Nephrology 4:279-287 (1998), Ex. 48, at 280 (noting that Lin’s invention was a “difficult feat” because, inter alia, “there was no source of eryth-ropoietin mRNA”).
While it is true, as HMR/TKT points out, that Sugimoto’s method is not limited to starting cells that produce a certain threshold amount of EPO, even HMR/TKT itself was unable to find
any
prior art EPO-producing cell lines that could be fused successfully to lymphoblastoid cells to do as Sugimoto claimed.
Amgen I,
Although it is not always necessary to deposit starting materials,
Wands,
858
*309
F.2d at 736; 35 U.S.C. § 112, deposit is required “[w]here an invention depends on the use of living materials such as microorganisms or cultured cells” and it is “impossible to enable the public to make the invention (i.e., to obtain these living materials) solely by means of a written disclosure.”
Wands,
(b) Sugimoto Did Not Teach How To Select EPO-Producing Hybrid Cells
Second, Sugimoto neither deposited his putative “hybrids” nor taught how to select true hybrids. Dr. Green’s testimony that the formation of hybrid cells — incorporating the material of two parental nuclei into a single nucleus — is “a rare event,” went undisputed.
See
Green Test., R. Trial Tr. at 414: 1-8, 415: 2-9. Because most of the cells in a culture following a fusion event are not true hybrids, use of a selection method to remove all cells which are not hybrids is a very important step.
Id.
at 414-16. Sugimoto did not describe any selection method. As a result, according to Dr. Green, if skilled artisans tried to reproduce his experiments as described, “they would have no benefit of the selective system and therefore the amount of work which would be required might make it impossible for them to succeed in isolating such a hybrid.”
Id.
at 422: 21-25;
see also Elan Pharms., Inc. v. Mayo Found. for Med. Educ. and Research,
Although Dr. Green admitted that methods to select hybrid cells were available to those skilled in the art at the time, Green Test., R. Trial Tr. at 423: 14-16, 507, he explained that execution of the methods was not routine, because the methods sometimes worked and sometimes did not, and that without publishing which methods to use and whether they worked, “there’s no reason to suppose that you can apply it routinely to any combination of cells and have it work correctly.” Id. at 425: 3-5; see id. at 420: 10-14, 422: 16-25, 424: 19-425: 5, 520: 2-24. According to Dr. Green, this lack of selection method, along with the fact that Sugimoto neither deposited nor characterized the cells, i.e., proved that they were hybrids, posed great difficulties to one skilled in the art attempting to reproduce the procedure. Id. at 425: 22-426: 8. 127
*310
HMR/TKT attempts to rely on Dr. Kingston’s testimony to lessen the weight the Court accords Dr. Green’s testimony. This attempt is unsuccessful because HMR/TKT points to no testimony by Dr. Kingston addressing selection methods specifically, let alone the potential problems identified by Dr. Green. Furthermore, although the Court has indeed considered both Dr. Kingston’s and Dr. Green’s testimony regarding the amount of experimentation due,
Elan Pharmaceuticals,
Moreover, that these deficiencies were debilitating to those skilled in the art trying to reproduce the procedure, and thus required undue experimentation to be overcome, is supported by HMR/TKT’s failed attempt to repeat Sugimoto’s process to obtain an EPO-producing hybrid cell. Green Test., R. Trial Tr. at 427: 10-22. Dr. Heartlein could not even obtain a putative hybrid when he used multiple selective markers, which make the job of selection easier.
Id.
at 427: 10-428: 12 (noting that he tried unsuccessfully with one marker ten times and then with multiple markers twenty-seven separate times, finding no putative hybrids on any occasion). While it is true, as mentioned earli
*311
er, that Dr. Heartlein did not exactly duplicate Sugimoto’s process, he
could not
for the reasons stated above. Moreover, as Dr. Green pointed out, even when he used advanced technology, had even more resources at his disposal than Sugimoto had, and had every incentive to achieve, he could not make any hybrid cells.
Id.
at 430: 3-7. Thus, the evidence shows that undue experimentation would have been required to select a hybrid human kidney tumor/lympohblastoid cell having the EPO-producing properties reported by Sugimoto.
See Genentech,
(c) Purification of EPO To Be Used To Treat Anemia Was Claimed But Not Taught, and Prior Art Techniques Were Insufficient
Third, Sugimoto did not enable a purification method. Sugimoto’s specification states that “conventional procedures” for purification may be used to purify EPO from the lysate produced in Sugimoto’s experiments and can be used “in the prevention and treatment of human diseases such as anaemia.” Sugimoto’s patent, Ex. 2229, at col. 3: 50-65, col. 3: 66-4: 2. HMR/ TKT’s experts rendered opinions that an ordinarily skilled artisan, combining procedures of Yanagawa, Chiba, and Erslev, could have purified EPO from serum or cell culture medium. See, e.g., Erslev Test., Trial Tr. at 1751: 15-1754: 3; Robbins Test., Trial Tr. 1984: 7-1987: 5; Mat-sudaira Test., R. Trial Tr. at 910-14. Notwithstanding this testimony, the Court is persuaded that one of ordinary skill in the art could not have used the prior art purification methods to purify to substantial homogeneity the EPO produced in tumor cell cultures.
Given the state of the art and the skill level at the time, purification of EPO in the context of the Sugimoto patent was not as simple as it seemed; that is, it was not simply a matter of applying
generic
protein purification procedures already well known in the art to purify EPO produced in tumor cell cultures.
See Wands,
Moreover, no one to this day has been reported as being able successfully to purify to homogeneity therapeutically effective human EPO from non-recombinant cells grown in culture, nor has any patient ever been treated by any EPO produced by the Sugimoto procedure. Even HMR/ TKT’s witnesses, Dr. Matsudaira and Dr. Erslev, admitted this. Matsudaira Test., R. Trial Tr. at 930: 16-23; Erslev Test., Trial Tr. at 1755: 17-1756: 3.
129
As this Court pointed out in
Amgen I,
“in light of the intense competition that grew out of the race to make human EPO suitable for treatment of chronic anemia, one would imagine that if Sugimoto’s invention were truly enabling then he would have won that lucrative race.”
*313
Thus, given the state of the art and the level of skill at the time — proven by testimony about the prior art and subsequent art — Sugimoto’s failure to provide any guidance as to what combination of purification techniques is likely to produce substantially homogenous human EPO from Sugimoto’s cell extracts that could potentially be used to treat patients means his patent is nothing more than an “invitation” to experiment — and this is simply not sufficient to satisfy the enablement requirement.
Enzo,
(2) Conclusion
Patent protection is granted in return for an enabling disclosure of an invention, not for vague intimations of general ideas that may or may not work.
Genen-tech,
Like in
Chugai,
here a substantial discovery is claimed, yet there is no credible evidence that the claimed EPO can be purified and produced by skilled artisans by the disclosed process. Indeed, all evidence — even that from HMR/TKT itself— is to the contrary.
Chugai,
b. Obviousness: Does Sugimoto Render Obvious Any of the Asserted Claims of the ’422, ’080, ’698, and 349 Patents?
A patent is invalid under 35 U.S.C. § 103 if the differences between the patented subject matter and the prior art are small enough that the patented subject matter “as a whole” would have been obvious at the time of the invention to a person having ordinary skill in the art. 35 U.S.C. § 103 (2001);
SIBIA Neurosciences, Inc. v. Cadus Pharm. Corp.,
The “objective indicia of non-obviousness,” referred to as secondary considerations, include (1) commercial suc
*315
cess; (2) copying; (3) long-felt, but unresolved need; (4) the failure of others; (5) commercial success; (6) unexpected result created by claimed inventions; (7) unexpected properties of the claimed inventions; (8) licenses revealing industry respect for the invention; and (9) skepticism of skilled artisans before the invention.
Graham,
Importantly, the defense of obviousness can be based on a single prior art reference or more than one prior art reference. In other words, if it is shown that it would have been obvious to one skilled in the art to modify the teachings of a reference or combine the teachings of more than one reference to accomplish the claimed invention, then the patent for the claimed invention is invalid.
SIBIA Neurosciences,
(1) Claim 1 of the ’422 Patent and Claims 2-4 of the ’080 Patent
HMR/TKT argues that Sugimoto afforded the skilled worker a reasonable expectation of success in obtaining the claimed invention of the asserted claims of the ’422 and ’080 patents because Sugimo-to discloses on its face every specific element of those claims, except for the extra 166th amino acid. HMR/TKT’s Reply Br. After Trial at 10. In other words, it urges, that
because
Sugimoto discloses all the elements of the asserted claims, it necessarily shows that those skilled in the art would have had a reasonable expectation of success in practicing Amgen’s claimed invention. This, however, erroneously conflates into a single issue what the Federal Circuit has defined as a two-part inquiry.
See, e.g., Brown & Williamson Tobacco,
(a) Scope and Content of the Prior Art/Differences Between the Claimed Invention and the Prior Art
HMR/TKT contends that Sugimoto alone, along with what was known by those skilled in the art, renders obvious the asserted claims of the ’422 and ’080 patents. As stated in
Amgen I,
Sugimoto itself “suggested combining its invention with prior art sources relating to both purification and therapeutic delivery.”
Amgen I,
The differences between Sugimoto (combined with prior art knowledge) and claim 1 of the ’422 patent and the asserted claims of the ’080 patent, however, can be summarized easily.
Sugimoto does suggest all that is contained in claim 1 of the ’422 patent. Am-gen contends that ’Sugimoto does not disclose “therapeutically effective” because it does not use those words nor describe an increase in hematocrit. While this argument may indeed have merit in an anticipation analysis, where more complete detail and description may be required, it fails here. Sugimoto suggests (if not teaches) EPO that is therapeutically effective when it claims that its EPO is useful in the treatment of patient diseases such as anemia. Sugimoto Patent, Ex. 2229, col. 3: 66 — 4: 2;
see also
Kingston Test., Trial Tr. at 1227, 1234. Moreover, it is undisputed that Sugimoto claims it produced human EPO in excess of 1000 units/10 (6) cells, a range HMR/TKT asserts, and Amgen does not dispute, to be
*317
therapeutically effective. Sugimoto Patent, Ex. 2229, col. 6: 27-39. Amgen argues in defense that Sugimoto does not suggest purification
from mammalian cells grown in culture
specifically. The Federal Circuit made clear in
Amgen II,
however, that when considering obviousness with respect to the ’422 and ’080 product claims, “a claimed product shown to be present in the prior art cannot be rendered patentable solely by the addition of source or process limitations.”
Amgen II,
There are more differences between Sugimoto and the asserted claims of the ’080 patent than there are between Sugimoto and claim 1 of the ’422 patent. As the Court explained in
Amgen I,
claims 2, 3, and 4 (by dependency) make reference to the mature erythropoietin amino acid sequence of Figure 6, which is unique to and at the heart of Amgen’s invention. Sugimoto does not discuss in any way the amino acid sequence of human EPO. HMR/TKT assumes that because Sugimoto discloses human EPO, it necessarily discloses human EPO with either a 165 amino acid sequence or 166 amino acid sequence. HMR/TKT’s Reply Br. After Trial at 12. This, however, is not necessarily true. As Amgen points out, Reply to HMR/TKT’s Findings of Fact ¶ 149, this Court already found that changes at the C-terminus neither affect the biological activity of the protein nor inhibit proper secretion from the cells.
Amgen I,
Amgen also claims, correctly, that Sugi-moto does not examine the in vivo biological activity of causing bone marrow cells to increase production of reticulocytes and red blood cells, a limitation found in claims 2 and 3 of the ’080 patent. While this argument supports a finding that Sugimo-to does not anticipate these claims, it does not work here in an obviousness inquiry. As discussed above, Sugimoto claimed its EPO was “advantageously useable .... in the prevention or treatment of human diseases such as anaemia” Sugimoto Patent, Ex. 2229, at col. 3: 66-4: 2. This necessarily suggests an increase in reticulocytes and red blood cells since, as Dr. Schu-macher explained and Amgen did not dispute, these side affects necessarily coincide with therapeutically effective treatment. Schumacher Test., R. Trial Tr. at 824-25.
(b) Level of Ordinary Skill in the Art 134 and Reasonable Expectation of Success
This Court has already found that those skilled in the art at the time Sugimo-
*318
to patented his invention would not have been able to use Sugimoto — along with knowledge and skill in the art — to select the hybrids or purify the EPO without undue experimentation. HMR/TKT does not suggest that at the time that Amgen made its claims — as opposed to the time that Sugimoto filed its patent — common knowledge in the art about these procedures had advanced. Moreover, there is no proof on record — aside from that discussed and rejected — that those skilled in the art would have been capable of practicing Sugimoto let alone practicing Amgen’s claimed invention based on Sugimoto and general knowledge of skilled artisans. Indeed, there is proof to the contrary. No one has ever purified EPO from non-recombinant cells to substantial homogeneity and all attempts to obtain a therapeutic result had failed. Although a particular reference need not be enabling to be considered in the obviousness inquiry, the asserted combination (here Sugimoto combined with knowledge of one skilled in the art) must provide a reasonable expectation of successfully practicing the claimed invention.
Boehringer Ingelheim Vetmedica, Inc. v. Schering-Plough Corp.,
(c) Secondary Considerations
As discussed in great detail in
Amgen I,
HMR/TKT argues, however, that Am-gen did not explain to which claims its success was attributable, and that the mapping of the EPO gene was claimed in .Dr. Lin’s ’008 patent. HMR/TKT’s Response to Amgen’s Proposed Findings of Fact ¶ 46. In support, it cites
Riverwood International Corp. v. Mead Corp.,
(2) Claims 4-9 of the ’698 Patent and Claims 1, 3, 4, 6, and 7 of the ’349 Patent
HMR/TKT contends that every element of the asserted claims of the ’698 *320 and ’349 patents is found in Sugimoto except the 166th amino acid of Figure 6, the “non-human” or non-EPO promoter or transcription control sequences and the amplified marker DNA. HMR/TKT’s Opening Br. After Trial at 41-44. The missing elements, it argues, were available and routinely used in the art in 1983-84. Specifically, it asserts that
[g]iven the teachings of Sugimoto, it would have been obvious for the ordinary skilled worker to use retroviral insertion to operatively link a retroviral promoter and its transcription control sequences to the erythropoietin production genetic sites in a kidney or liver tumor cell that produced EPO and to transfer those production sites ... with an amplifiable marker DNA if desired, to a lymphoblastoid cell.
Id. at 41-42. HMR/TKT, however, fails to show a suggestion or motivation to modify the teachings of Sugimoto to create what Amgen claims. Moreover, it has not shown with clear and convincing evidence that one of skill in the art would have had a reasonable expectation of success in achieving Amgen’s ’349 or ’698 claimed inventions using such techniques. Finally, as they did in the context of the ’080 and ’422 claims, the secondary factors weigh heavily in Amgen’s favor on the issue.
(a) Scope and Content of the Prior Art/Differences Between the Claimed Invention and the Prior Art
Sugimoto differs from the asserted claims of the ’349 patent in that it does not disclose the “non-human” or non-EPO promoter or transcription control sequences as claimed in the asserted claims of the ’349 patent. Sugimoto differs from the asserted claims of the ’698 patent in that it does not disclose the amino acid sequence of Figure 6, 137 amplified marker DNA, the “dihydrofolate reductase (DHFR) gene DNA,” or use of a non-EPO promoter operatively linked to the EPO gene. 138
With respect to amplified marker DNA, HMR/TKT asserts that Sugimoto’s claimed hybrid cells comprise amplified DNA because they have more copies of the EPO gene than are found in normal cells. HMR/TKT Proposed Findings of Fact at 94. Dr. Lodish testified, however, that amplified EPO DNA refers to an increase in the “number of copies of EPO DNA *321 relative to other DNA sequences in the genome.” Lodish Test., R. Trial Tr. at 1099: 25-1100: 1 (emphasis added); see also James Darnell, Harvey Lodish & David Baltimore, Molecular Cell Biology (1st ed.1986), Ex. 2394, at 457 (“When mammalian cells are grown in culture, specific sites on their DNA can become amplified.” (emphasis added)); id. at 461 (showing in a diagram that DHFR gene copy numbers increase, but does not depict a change in the chromosome copy numbers). As HMR/TKT admits, Sugimoto’s claimed hybrid cells had potentially 4 copies of every gene on every chromosome (two from each parental cell). See, e.g., HMR/ TKT’s Proposed Findings of Fact at 94; Kingston Test., R. Trial Tr. at 98: 19-99: 5. This does not represent an increase in the relative amount of EPO DNA compared to other DNA sequences.
Notwithstanding this, HMR/TKT argues that Dr. Lodish’s testimony regarding amplification supports its argument that Sugimoto’s hybrid cells will often have more than four copies of the EPO gene. See, e.g., HMR/TKT’s Proposed Findings of Fact at 94 (citing Lodish Test., Trial Tr. at 160: 24-161: 10, 494: 24-495: 3). The Court, however, is not convinced that Dr. Lodish’s testimony supports this conclusion. Instead, it appears that in the testimony on which HMR/TKT relies, Dr. Lodish was addressing selection for amplification events using the DHRF gene as a selectable marker — a feature totally missing from Sugimioto.
With respect to the other missing elements, including amplification, HMR/TKT argues that they were available and routinely used in the art in 1983-84.
See, e.g.,
HMR/TKT’s Opening Br. After Trial at 41. Instead of focusing on the invention as a whole, however, as required under 35 U.S.C. § 103, HMR/TKT approaches the obviousness inquiry on a piecemeal basis, arguing that the separate elements of Am-gen’s invention existed in the prior art and, separately, “could” have been done easily.
See, e.g.,
HMR/TKT’s Opening Br. at 43-44; HMR/TKT’s Proposed Findings of Fact After Trial at 93-115. “[AJbsent some teaching or suggestion, in the prior art, to combine the elements,” however, this is “insufficient.”
Arkie Lures,
HMR/TKT tries to hang its hat on the statements in Sugimoto regarding genetic sites and recombinant techniques. See Sugimoto Patent, Ex. 2229, col. 1: 55-2: 3. It argues that Sugimoto’s reference to “genetic recombination techniques” suggests combining Sugimoto with retroviral insertion art, that is, that Sugimoto suggested the insertion of non-human transcription control sequences. HMR/TKT’s Reply Br. at 13. The Court is not convinced. Sugi-moto nowhere suggests using “retroviral insertion” to induce expression of EPO. That the specification specifically defines recombination techniques as those “using DNA ligase, nuclease and DNA polymerase,” Sugimoto Patent, Ex. 2229, col. 2: 2-3, argues against interpreting a suggestion of retroviral insertion. Similarly, both Dr. Lodish and Dr. Green testified that an ordinarily skilled artisan reading Sugimoto *322 would not have interpreted the section relied on by HMR/TKT as teaching a way to make cells capable of producing human EPO by recombinant DNA techniques. Lodish Test., R. Trial Tr. at 281: 10-282: 4, 285: 6-23; Green Test., R. Trial Tr. at 405: 19-409: 6. While Dr. Kingston testified that the most commonly used technology to increase expression of the EPO gene in 1983-84 was retroviral insertion, Kingston Test., R. Trial Tr. at 99: 14-23, when asked how Sugimoto teaches recombinant DNA techniques to increase expression of the EPO coating region, he stated that Sugimoto did so by using “ligases and nucleases and polymerases,” id. at 104: 14-19 — not retroviral insertion.
Moreover, it is not as if “retroviral insertion” was a commonly understood technique that could simply be applied by any skilled artisan in 1983-84. Instead, as Dr. Kingston explained, a skilled artisan would have to rely on many different prior art references to achieve it. See Kingston Test., R. Trial Tr. at 99-112 (relying on at least six other references in combination in forming opinion about process of inserting a retrovirus and producing erythropoietin from the resulting cell). That all of these references, save one, were published after Sugimoto’s patent issued (after 1983) also supports the conclusion that Sugimoto was not suggesting a combination with retrovi-ral insertion. See John M. Coffin, Stephen H. Hughes & Harold E. Varmus, Retro viruses (1997), Ex. 2481; Roger D. Cone & Richard C. Mulligan, High-efficiency Gene Transfer Into Mammalian Cells, 81 Proc. Nat’l Acad. Sci. 6349 (1984), Ex. 2479; Randal J. Kaufman & Phillip A. Sharp, Amplification and Expression of Sequences Cotransfected with a Modular Dihydrofolate Reductase Complementary DNA Gene, 159 J. Molecular Biol. 601 (1982), Ex. 2239; David L. Nelson et al., Metaphase Chromosome Transfer of Introduced Selectable Markers, 2 J. Molecular & Applied Genetics 563 (1984), Ex. 2476; Munehisa Ueno et al., Enhanced Erythropoietin Secretion in Hepatoblasto-ma Cells in Response to Hypoxia, 257 Am. J. Physiology C743 (1989), Ex. 2480; John H. Weis et al., Eukaryotic Chromosome Transfer, 81 Proc. Nat’l Acad. Sci. 4879 (1984), Ex. 2477.
While the motivation to modify can be found outside the reference itself,
SIBIA Neurosciences,
HMR/TKT fails to show a suggestion to modify Sugimoto or combine it with prior art with respect to amplification as well. With respect to claims 6, 7, and 8, HMR/ TKT merely asserts that although Sugimo-to does not disclose or teach a means to position a selection marker such as DHFR next to the EPO gene, it renders this element of the claim obvious because “it was well-known in 1983-84 that the DHFR marker gene can be used to transfer and amplify co-transferred DNA sequences when transfected into CHO cells.” HMR/ TKT’s Proposed Findings of Fact ¶ 448; HMR/TKT’s Response to Amgen’s Proposed Findings ¶40; HMR/TKT’s Reply Br. After Trial at 15. While HMR/TKT may have something with respect to this element, fatally, it neither identified any. motivation or suggestion to combine this supposed common knowledge with Sugi-moto nor demonstrated how this motivation can be found in the prior art or the problem to be solved. HMR/TKT’s Proposed Findings of Fact ¶¶ 448, 452. Given that HMR/TKT shoulders the burden here, this lack of evidence and argument is fatal.
(b) Level of Ordinary Skill in the Art and Reasonable Expectation of Success
Even if one could glean the motivation to modify Sugimoto by applying knowledge in the art to create the claimed invention, HMR/TKT would not prevail here. HMR/ TKT has not shown that a skilled artisan would reasonably expect to have succeeded in achieving Dr. Lin’s claimed ’349 or ’698 inventions using such known techniques.
139
As mentioned earlier, HMR/TKT parses elements that comprise one limitation. For example, in its Proposed Findings of Fact, it separates the element “comprising promoter DNA, other than human EPO promoter DNA, operatively linked” from the element “DNA encoding the mature erythropoietin amino acid sequence of FIG. 6.” In doing so, it fails to recognize the import of the combination of elements. As this Court pointed out in
Amgen I,
in the context of the ’349 patent and tumor cell references, the identity of the sequence of the DNA encoding human eryth-ropoietin was critical.
Amgen I,
Moreover, the Court does not overlook the fact that HMR/TKT’s only evidence on this issue comes from testimony by Dr. Kingston, who earlier testified that a person of ordinary skill in the art, applying Dr. Lin’s specification — which includes the identification of the EPO gene sequence, splice, donor, and restriction sites, and much more detail than Sugimoto’s patent — would not have been able to produce EPO using a cell’s endogenous EPO gene. Kingston Test., R. Trial Tr. at 116: 23-117: 24 (testifying that an ordinarily skilled worker could not have taken Lin’s teaching to insert randomly a retrovirus into a cell and to obtain an EPO-producing cell with a reasonable likelihood of success). His testimony that ordinarily skilled artisans could have combined Sugi-moto with references regarding retroviral insertion is seemingly incongruous, Kingston Test., R. Trial Tr. at 100: 11-101: 19; 116: 11-16; 117: 15-24, not to mention inconsistent with yet other testimony by the doctor. In the first trial, Dr. Kingston stated that before Dr. Lin cloned the EPO gene, it would not have been obvious for one skilled in the art to do what he did. Kingston Test., Trial Tr. at 1357: 11-1358: 12 (explaining why he retracted yet another inconsistent statement). The Court does not, therefore, lend Dr. Kingston’s oscillatory testimony on this issue much weight — especially when considered in light of Dr. Green’s and Dr. Lodish’s testimony that one skilled in the art, lacking knowledge of EPO’s DNA sequence, would not have had a reasonable expectation of successfully making EPO-producing cells by genetic recombination. Green Test., R. Trial Tr. at 406: 17-22; 409: 3-6 (explaining that in order to use any of the recombinant methods mentioned in Sugimoto, “you must know the sequence of the eryth-ropoietin gene and that information ... did not become available until Dr. Lin’s inventions”); Lodish Test., R. Trial Tr. at 285: 21-23. Indeed, Dr. Kingston implicitly admitted the importance of knowing EPO’s DNA sequence when he testified that the first step in genetic recombination is to isolate the EPO-neo fragment, which suggests that the gene must first have been cloned. Kingston Test., R. Trial Tr. at 103: 17-104: 18 (using Demonstrative Exhibit TX II W as support for conclusion that Sugimoto teaches this type of genetic recombination); Demonstrative Ex. TX II W. 142
Thus, HMR/TKT has failed to prove that skilled artisans, without knowing EPO’s DNA sequence, would reasonably expect that combining Sugimoto with prior art references regarding retro viral insertion and knowledge regarding amplifica *325 tion would successfully achieve what Am-gen claims.
(c) Secondary Considerations
As with the claims of the ’422 and ’080 patent, the secondary considerations play a large role in the Court’s decision with respect to obviousness. For the reasons discussed above and in
Amgen I,
(3) Conclusion
Having considered the scope and content of the prior art references, the differences between such references and the claimed inventions, how one skilled in the art might combine such references in order to make what Amgen claimed, and the objective secondary considerations, the Court concludes the HMR/TKT has failed to persuade the Court by clear and convincing evidence that the asserted claims of the ’080, ’422, ’349, and ’698, patents were obvious in light of Sugimoto and the prior art.
B. Goldwasser 143
1. Background
a. Overview of Goldwasser
Dr. Goldwasser obtained a preparation of highly purified erythropoietin derived from human urine i.e., it was naturally-occurring EPO.
Amgen I,
b. The Court’s Holdings in Amgen J 145
(1) Anticipation
In
Amgen I,
the Court held that Dr. Goldwasser’s study did not anticipate the asserted claims in the ’422 and ’080 patents, because the accepted standard by which physicians measure a therapeutic response to EPO is an increase in hemato-crit, and Dr. Goldwasser admitted that “there was no significant change in hemat-ocrit in any patient” and that the trial was a failure.
Amgen I,
Further, the Court pointed to other differences between Goldwasser’s study and Amgen’s claims. First, the Court stated that Amgen specifically excluded urinary EPO preparations from the scope of the claims by including the claim limitations “non-naturally occurring” and “not isolated from human urine.” Thus, it concluded that claims 2 and 3 of the ’080 patent do not encompass Goldwasser’s urinary EPO treatment. Id. at 112. Second, Goldwas-ser’s study does not involve cells that have been altered by recombinant means, and therefore, it held that none of the ’349 claims are implicated. Id.
(2) Obviousness
The Court held that because Dr. Gold-wasser’s study was a failure and a person skilled in the art “would not reasonably have expected that Dr. Goldwasser’s work would eventually bear fruit,” none of Am-gen’s patents were invalid for obviousness. Amgen I, 126 F. Supp 2d at 114. The Court also found, inter alia, that HMR/ TKT “failed to prove the existence of any suggestion in the prior art to combine [Essers or Goldwasser and Yanagawa or Chiba] so as to produce the pharmaceutical compositions claimed in the ... ’080, and ’422 patents.” Id. It explained that “the fact that no one has ever — then or now— attempted to determine if a pharmaceutical composition comprising human EPO could be made from these cultured prior art cells also informs the Court’s decision.” Id. Therefore, the Court stated that “the contention that these various references could be combined to produce a pharmaceutical composition meeting the limitations of ... claim 4 of the ’080 patent and claim 1 of the 422 patent is simply unsubstantiated conjecture.” Id. Lastly, the Court stated that the secondary considerations counseled strongly against a finding of obviousness. Thus, at the close of HMR/TKT’s defensive case, the Court granted Amgen’s 52(c) motion for judgment of validity with respect to the defense of obviousness.
c. The Federal Circuit’s Opinion
HMR/TKT challenged, on appeal, the Court’s acceptance of Goldwasser’s assertion that his test was a failure in light of the testimony of Dr. Baron, Goldwasser’s collaborator.
Amgen II,
2. The Claims at Issue
On remand, HMR/TKT argues that Goldwasser anticipates claim 1 of the ’422 *327 patent and renders obvious claim 1 of the ’422 patent and claims 2-4 of the ’080 patent. 147 The relevant claims are as follows:
’422 Claim 1: A pharmaceutical composition comprising a therapeutically effective amount of human erythropoietin and a pharmaceutically acceptable diluent, adjuvant or carrier, where in said erythropoietin is purified from mammalian cells grown in culture.
’422 Patent, Ex. 1, col. 38: 36-41 (emphasis added).
’080 Claim 2: An isolated erythro-poietin glycoprotein having the in vivo biological activity of causing bone marrow cells to increase production of reti-culocytes and red blood cells, wherein said erythropoietin glycoprotein comprises the mature erythropoietin amino acid sequence of FIG. 6 and is not isolated from human urine.
’080 Patent, Ex. 1, col. 38: 39-44.
’080 Claim 3: A non-naturally occurring erythropoietin glycoprotein having the in vivo biological activity of causing bone marrow cells to increase production of reticulocytes and red blood cells, wherein said erythropoietin glycoprotein comprises the mature erythropoietin amino acid sequence of FIG. 6.
’080 Patent, Ex. 1, col. 38: 45-50.
’080 Claim 4: A pharmaceutical composition comprising a therapeutically effective amount of an erythropoietin gly-coprotein product according to Claim 1, 2 or 3.
’080 Patent, Ex. 1, at col. 38: 51-53 (emphasis added).
3. Discussion
a. Anticipation
(1) Claim 1 of the ’422 Patent
Given the Court’s construction of the term “therapeutically effective,” a critical factor in the anticipation analysis is whether any of the effects elicited by Gold-wasser actually, in and of themselves, helped to heal or cure the class of patients listed in column 33 of the specification. 148 Therefore, the Court will review, in turn, the responses elicited by Goldwasser — and asserted by HMR/TKT to be “therapeutically effective.” 149
(a) Increase in Reticulocytes
HMR/TKT argues that a “therapeutically effective amount” of EPO encompasses an amount that results in an increase in *328 reticulocyte count, whether or not there is an increase in hematocrit, because this increase, in and of itself, helps to heal or cure anemia. See, e.g., HMR/TKT’s Proposed Findings of Fact ¶¶ 28-31. In support, it explains that reticulocytes function like normal red blood cells and deliver greater amounts of oxygen to the body’s tissues than do older red blood cells. Id. The increased oxygen delivery to the tissues, it asserts, “confers health benefits on the patient — it can help to resolve anemia and possibly prevent strokes and heart attacks.” Id. In support of this contention, it relies mainly on the testimony of Drs. Schumacher and Foster. Id.
HMR/TKT overemphasizes the relative significance of reticulocytes in the oxygenation of the body’s tissue. Experts from both sides agree that reticulocytes comprise only one percent of all red blood cells. Schumacher Test., R. Trial Tr. at 829: 18-20; Erslev Test., Trial Tr. at 1685: 5-7. They exist for about three days, whereas mature red blood cells exist for 100-120 days. Erslev Test., Trial Tr: at 1684: 21-1685: 7. Moreover, no expert testified that a transitory increase in reti-culocytes meaningfully elevates the oxygen levels of the body as a whole. Dr. Schu-macher did not testify that a mere increase in reticulocytes increases oxygen supply to these tissues. Instead, she carefully testified that “if you are increasing the oxygen supply,” there would be a reduction in the risk of stroke or heart attacks. Schu-macher Test., R. Trial Tr. at 813-14 (emphasis added). 150 Both Drs. Erslev and Eschbach testified that reticulocytes are not the accepted reference standard for oxygenation of the body as a whole; that is, recticulocyte counts do not provide direct evidence of the number of red blood cells in circulation and do not always reflect the amount of red blood cells in the body. Erselv Test., Trial Tr. at 1687: 14-1689: 7; Eschbach Test., R. Trial Tr. at 653: 6-14 (stating that the number of circulating red blood cells is determined by the hematocrit). 151 This is because measurements of reticulocytes only reflect the production of red blood cells — not the destruction. Erslev Test., Trial Tr. at 1687: 14-1689: 7; Eschbach Test., R. Trial Tr. at 662-64, 670: 8-10. Reticulocytes do not account for the rate of red cell loss, which could exceed the rate of production. As explained by Dr. Eschbach, reticulocytes may never mature into red blood cells, because of intervening factors such as iron deficiency, infection, inflammation, blood loss, or rapid red cell destruction. Esch-bach Test., R. Trial Tr. at 662-64; 670: 21-25. 152
*329 Perhaps most telling is the fact that experts from both sides agreed that an increase in reticulocytes is merely an indication or “surrogate marker” that a therapeutic effect, i.e., one that actually helps to heal or one that makes the patient feel better, is going to follow. See, e.g., Foster Test., R. Trial Tr. at 965: 3-7 (describing an increase in reticulocytes as a “surrogate marker” of activity and of therapeutic effect); Schumacher Test., R. Trial Tr. at 807: 3-5 (testifying that increase in reticu-locytes is “the first indication of a therapeutic response”); id. at 813: 3-18 (“[T]he reticulocyte response is the first response that gives you a clue that you’re getting a response from your therapy ... the early harbinger of the cure or treatment.” (emphasis added)); Eschbach Test., R. Trial Tr. at 766: 4-17 (agreeing that an increase in reticulocytes puts a physician “on the lookout for the hematocrit to rise”); id. at 660: 22-661: 8, 669: 10-670: 2; Christensen Test., R. Trial Tr. at 1186: 9-24 (testifying that reticulocytes are a “marker ... that the marrow is putting out more blood cells,” which “signals that there will ultimately be [a benefit]”); id. at 1185: 1-17. That Amgen administered more EPO to those patients that showed an increase in reticulocytes and ferrokinetics and told the FDA that “[t]he first evidence of a response to three times weekly ... administration of EPOGEN® is an increase in the reticulocyte count within ten days,” Physicians’ Desk Reference (56th ed.2002), Ex. 2497, at 582 (describing Amgen’s EPO-GEN product) (emphasis added), merely supports the point made by HMR/TKT’s own witnesses: an increase in reticulocytes is an indicator or marker that an increase in hematocrit will follow.
The bulk of the testimony indicates that an increase in reticulocytes alone does not help patients feel better. Indeed, HMR/ TKT’s Dr. Erslev conceded that only by increasing and maintaining hematocrit is the patient able to gain energy and feel better. Erslev Test., Trial Tr. at 1681: 18-1683: 2. Even HMR/TKT’s Dr. Foster — a pharmacist arguably not qualified to testify in the area — admitted after a series of direct questions from the Court that an increase in reticulocytes such as that exemplified in Goldwasser would not in and of itself help patients feel better. Foster Test., R. Trial Tr. at 964-66.
HMR/TKT places a great deal of weight on Dr. Ohls’ testimony regarding the anemia of prematurity. She testified that an increase in reticulocytes is typically accompanied by an improvement in an infant’s overall condition that does not necessarily correspond to an increase in hematocrit, and that clinical signs that an infant is doing better as a result of EPO therapy can occur even with a decrease in hemato-crit. Ohls Test., R. Trial Tr. at 1020-21 (noting that conditions like tachycardia, apnea, and poor weight gain improve with an increase in reticulocytes, even if the hematocrit stays the same or decreases); id. at 1025. While this testimony may seem at first glance to support HMR/ TKT’s case on this point, after a careful review of the testimony of Dr. Ohls and her mentor, Dr. Christensen, it is clear that it does not.
Importantly, Dr. Ohls carefully qualified her testimony by stating that the clinical signs of anemia “gradually disappear” after a moderate increase in reticulocytes. Id. at 1021: 2-4 (emphasis added); see also Christensen Test., R. Trial Tr. at *330 1185: 1-17 (pointing out that Dr. Ohls said “gradually,” and explaining that a rise in reticulocyte count, in and of itself, has “no medical meaning,” except to “help you predict that eventually this baby is going to have a hematocrit that is stable”). Dr. Ohls’ testimony is further qualified by the biological facts associated with babies and anemia. As Dr. Ohls explained, babies, unlike adults, are constantly growing. As they grow, their blood volume also constantly grows in proportion to their size. Ohls Test., R. Trial Tr. at 1022: 9-21. While, in adults, one can measure the percentage of red blood cells in a sampled blood cell volume to get an accurate reading of hematocrit, 153 in babies, hematocrit is a constantly moving target, because as babies grow their blood volume increases. Id.; see also Christensen Test., R. Trial Tr. at 1184: 7-15 (noting that an infant’s growth rate complicates the measuring of hematocrit). Therefore, even an actual increase in red cell mass (versus just an increase in reticulocytes) can .result in a constant or even decreased hematocrit. Ohls Test., R. Trial Tr. at 1024. 154 Moreover, Dr. Ohls stated that a neonatologist would use reticulocytes to measure EPO’s efficiency — not because it necessarily had a therapeutic effect — but because it “means that the EPO is working to stimulate the bone marrow to make new red blood cells.” Id. at 1026; see also id. at 1029: 20-23 (“But in general, when we treat these babies with EPO they start making new reticulocytes, new red blood cells; they stimulate the circulation, build up the red-cell mass, the hematocrit.”). As discussed above, however, just because a person’s body is making new red blood cells does not mean that it is doing so fast enough to make up for continuing destruction of red blood cells. Presumably, this is why Dr. Ohls and her peers, in their clinical research, measure the hematocrit, the amount of blood drawn out for laboratory evaluation, and the number of transfusions and the volume of transfusions the babies receive in addition to the reticulocyte count. Id. at 1040-41,1043: 21-24. 155
The significance of Dr. Ohls’ testimony is further diminished by the testimony of her mentor, Dr. Christensen. He stated repeatedly that the reticulocyte count, in and of itself, does not have any effect on the baby and does not help the baby in any way. Id. at 1183: 15-22, 1185: 1-17, 1186: 6-24. Instead it is merely a biological indicator that a benefit will ultimately follow. Id. Further, he clarified that an infant’s growth rate does not invalidate he-matocrit as a measure of therapeutic efficacy. Id. at 1183: 23-1184: 15. Instead, a physician has to consider the growth factor in infants much like a physician takes into account an adult patient’s age, *331 sex, disease state, etc., in order to understand the meaning of the patient’s hemato-crit. Id. Dr. Christensen made clear that EPO is used to stabilize an infant’s hemat-ocrit and to prevent it from falling to a level that would require a transfusion. Christensen Test., R. Trial Tr. at 1189: 23-1190: 4.
In further support of the conclusion that reticulocytes in and of themselves do not help to heal or cure babies suffering from anemia is the fact that a decision whether to transfuse a baby (the goal of using EPO on infants is to avoid the necessity of a transfusion) 156 is never based on reticulo-cytes alone. Id. at 1116-17. Evidently, the reticulocytes can be high and the he-matocrit low, and in that situation, the baby will still need the transfusion.
In light of Dr. Christensen’s testimony and the other testimony discussed above regarding reticulocytes in adults, Dr. Ohls’ testimony is unpersuasive. Although, as Dr. Schumacher testified, “therapeutic response” may be “related to the reticulo-cytes response,” Schumacher Test., R. Trial Tr. at 811: 11-12, the evidence does not show that a reticulocyte response, in and of itself, helps to heal or cure patients suffering from anemia or from any of the other diseases listed in column 33 of the specification.
For these reasons, after a careful review of all the evidence, this Court finds that an increase in reticulocytes alone does not in and of itself help to heal or cure a patient suffering from anemia or any of the diseases listed in the specification.
(b) Increase in Plasma Iron Clearance Rate (i.e., Ferrokinetics)
HMR/TKT next contends that increases in the plasma iron clearance rate are an indication that red blood cell production has increased and that there is a therapeutic response to EPO. HMR/TKT’s Proposed Findings of Fact ¶ 51. 157 As with reticulocytes, however, HMR/TKT has failed to show that an increase in plasma iron clearance rate is “therapeutically effective.”
First, an increase in the plasma iron clearance rate indicates an increase in reti-culocytes, but not necessarily an increase in red blood cell mass. As discussed above, there are a number of intervening events, such as cell death and destruction, which preclude one from concluding that the reticulocytes become red blood cells. See, e.g., Eschbach Test., R. Trial Tr. at 670: 3-25 (noting that ferrokinetics only reflect red blood cell production, not destruction); id. at 658: 2-8.
Second, Dr. Eschbach testified that fer-rokinetic measurements were understood to be a biological effect that did not guarantee that a therapeutic response would follow. Eschbach R. Trial Tr. at 660: 22-661: 8; id. at 658: 2-8 (“Ferrokinetics is an investigational tool. It does not ... tell you anything about therapeutic response.”).
Third, Dr. Schumacher admitted that inferences as to the rate of red blood cell production cannot be drawn from the plasma iron disappearance rate without also measuring the plasma iron concentration *332 (serum iron) at the beginning and the end of the trial. Schumacher Test., R. Trial Tr. at 835: 17-836: 9, 837: 4-21; Eschbach Test., R. Trial Tr. at 689: 13-691: 20, 693: 21-25; Allan J. Erslev, Anemia of Chronic Renal Failure, in Hematology (3rd ed.1983), Ex. 249, at 399. Although the plasma concentration was measured at the beginning of the Goldwasser study, it was not measured at the end. Schumacher Test., R. Trial Tr. at 841: 24-842: 2.
Because HMR/TKT points to no other persuasive evidence on the point, 158 the Court finds that it has failed to prove that an increase in the plasma iron clearance rate, in and of itself, helps to heal or cure anemia or any of the diseases referred to in column 33 of the specification.
(c) Erythrocite (Red Cell) Mass Changes
An increase in erythrocite mass, i.e., an increase in red cell mass, is an increase in the number of erythrocytes. That is, it reflects an increase in the aggregate number of red blood cells. Schumacher Test., R. Trial Tr. at 896: 16-897: 10. HMR/ TKT argues that Dr. Eschbach testified that erythrocite mass change is a measure of therapeutic efficacy because increasing the number of red cells helps to heal or cure anemia. HMR/TKT’s Findings of Fact at 13. It omits, however, Dr. Esch-bach’s clear qualification that this is true only if “there’s significant mass changes.” Eschbach Test., R. Trial Tr. at 658: 13-15. He explained that when erythrocyte mass changes are of sufficient quantity, they elicit a therapeutic effect because they represent an increase in hematocrit. Id. at 660: 1-5.
Here, HMR/TKT does not produce any evidence that the red cell mass changes were significant or meaningful. Indeed, arguably it cannot prove such a thing. Dr. Eschbach’s testimony, undisputed by any of the expert witnesses, that a significant increase in erythrocyte mass is the same as an increase in hematocrit prevents HMR/TKT from so proving, because the Court has already found and the Federal Circuit has affirmed that there was no significant increase in hematocrit in any of the patients. Thus, there could be no significant increase in red cell mass.
For that matter, given that the red cell mass changes only occurred in one patient and were not shown to be significant, the evidence does not support a finding that Goldwasser’s EPO actually elicited red cell mass increases. 159
Further, HMR/TKT did not prove that a larger dose of Goldwasser’s EPO would have increased red cell mass, increased hematocrit, or elicited a therapeutic response. While there is some evidence in HMR/TKT’s favor, the bulk of it suggests the contrary.
First, Dr. Baron himself attempted to increase the dosage and the duration with patient # 3, and still there was no recorded increase in hematocrit above the baseline level at any time during or after the study. Indeed, the opposite occurred; as HMR/TKT’s expert attested, the patient’s red cell mass declined over the treatment period. Goldwasser Data, Ex. 242, at AM 47 038668 (patient # 3); Schumacher *333 Test., R. Trial Tr. 885: 14-886: 20; id. at 887: 1-5; Esehbaeh Test., R. Trial Tr. at 759: 6-17 (testifying that there was no significant increase in hematocrit for any of the three patients); 7/7/80 Baron Letter to FDA, Ex.2056, at A 193007 (explaining to the FDA that the third patient received a trial of the medication using an altered protocol that increased the dosage and length of time). 160
Second, although HMR/TKT presented evidence that the experimentors did not believe the EPO was toxic or impure, see, e.g., IND Application for EPO, Ex. 2489, at HMR 935380, 935344; 7/7/80 Baron Letter to FDA, Ex.2056, at A 193007, there is contrary evidence that Goldwasser’s EPO was unsuitable for increased dosages. Esehbaeh Test., R. Trial Tr. at 706: 1-16 (testifying that it was impure and toxic), IND Application for EPO, Ex. 2489, at HMR 935386. Dr. Esehbaeh even opined that, given these issues with the Goldwas-ser preparation, the international review boards likely would not have permitted Goldwasser to give more of his urinary EPO preparation to human subjects even had he wanted to, Esehbaeh Test., R. Trial Tr. at 705: 20-706: 16, and that skilled artisans would likely refrain from giving it to patients in larger dosages for longer duration. Id. at 704: 22-23, 705: 22-706: 16; IND Application for EPO, Ex. 2489, at HMR 935386.
Although HRM/TKT’s expert, Dr. Schu-macher testified that had Goldwasser’s EPO been continued in a larger does, an increase in hematocrit would have been seen, Schumacher Test., R. Trial Tr. at 894: 12-15, Dr. Esehbaeh testified that the results would not have been different had a larger dose been given to the patients over a longer period of time, because of the potential problems with the EPO. Esehbaeh Test., R. Trial Tr. at 770: 24-771: 6 (explaining that after he received the EPO T 1/2 values and became aware of the fragments and marked decrease in EPO clearance rate, he doubted whether giving more EPO would make any difference, and believed it might even be harmful); id. at 730-31 (same); id. at 704-706; of. 2/6/84 Baron Letter to National Center for Drugs and Biologies, Ex. 2058, at A 199034 (describing the increase in reticulo-cytes as only “mild to modest”).
Third, given the incentives to continue the study, the fact that the experimentors themselves chose to abandon it and considered it a failure indicates that an increase in dosage or length of administration would not have led to success. Goldwasser Dep. at 317: 14-321: 2;
161
cf. Fromson v.
*334
Advance Offset Plate, Inc.,
Thus, HMR/TKT failed to prove that Goldwasser’s EPO would have achieved therapeutic effectiveness had Goldwasser continued his experiment. The mere possibility of success is not enough to save HMR/TKT.
Cf. Continental Can Co. USA, Inc. v. Monsanto Co.,
(2) Conclusion
HMR/TKT contends that all three of the elicited responses discussed above are “surrogate markers of therapeutic efficacy of EPO because each of them represents a critical step in the development of eryth-roctyes.” HMR/TKT’s Proposed Findings of Fact ¶¶ 64-66. This specific contention, however, belies its argument. That these three responses are but surrogate markers or indicators that a therapeutic response is on the way necessarily indicates that they did not, in and of themselves, elicit a therapeutic response. This is consistent with this Court’s reading of Amgen’s specification (discussed in the claim construction part of this memorandum and opinion). These biological responses are critical steps, precursory responses, before a therapeutic result is achieved. Because Gold-wasser’s study did nothing more than elicit these biological effects or surrogate markers, experts from both sides agreed that there was no evidence that Goldwasser’s urinary EPO clinically improved the condition of any of the patients. See, e.g., Means Test., Trial Tr. at 1918: 16-1919: 12 (admitting that there is no evidence that the patients benefitted from any purported activity and labeling the activity as biologic effects); Eschbach Test., R. Trial Test, at 676: 7-18.
In sum, HMR/TKT failed to prove by clear and convincing evidence that Gold-wasser anticipates claim 1 of the ’422 patent.
b. Obviousness
HMR/TKT argues that Goldwasser alone renders claim 1 of the ’422 patent and claims 2-4 of the ’080 patent obvious.
(1) Claim 1 of the ’422 Patent and Claims 2-4 of the ’080 Patent
(a) Scope and Content of the Prior Art /Differences Between the Claimed Invention and the Prior Art
Goldwasser differs from claim 1 of the ’422 patent in that, as discussed above, it does not disclose EPO that is therapeutically effective or purified from mammalian cells grown in culture. Goldwasser differs from claims 2-4 of the ’080 patent in that it does not disclose the mature amino acid sequence of Figure 6 162 or EPO isolated *335 from a source other than human urine. 163 Moreover, claims 2-4 of the ’080 patent require production not just of reticulo-cytes, but also of red blood cells. Although one patient in Goldwasser showed an increase in red cell mass, the Court has found these increases neither significant nor meaningful — not only because the increases were not substantial enough to increase hematocrit, but also because the results occurred in only one patient. Thus, the Court found, as it did in Amgen I, that actual production of mature red blood cells was not evidenced. Lastly, claim 4 of the ’080 patent, like claim 1 of the ’422 patent, requires therapeutic effectiveness, but the Court has found Goldwas-ser’s EPO is not therapeutically effective.
(b) Level of Ordinary Skill in the Art and Reasonable Expectation of Success
In terms of claim 1 of the ’422 patent and claim 4 of the ’080 patent, HMR/TKT has not shown that one of ordinary skill in the art had a reasonable expectation of success in obtaining EPO compositions that achieved therapeutic effectiveness. Although HMR/TKT tried to show that it was simply a matter of increasing the length and amount of the dosage, it has not convinced the Court. 164 HMR/TKT provides no other support for its defense.
With respect to claims 2-3 of the ’080 patent, the evidence once again fails to show a reasonable expectation of success in achieving an increase in the production of red blood cells: The one patient that did receive the increased dosages showed a *336 decrease, not an increase, in red blood cell mass. HMR/TKT has produced no further evidence to support its contentions.
(c) Secondary Considerations
Even if HMR/TKT had shown a reasonable expectation of success on the part of one skilled in the art to practice the claimed invention, this Court would still conclude that HMR/TKT has failed to show by clear and convincing evidence that Goldwasser rendered the claims obvious. This is because the secondary considerations counsel strongly against a finding of obviousness, just as they did in the context of Sugimoto. The secondary considerations discussed above with respect to Sugimoto, and explicated in
Amgen I,
apply here.
Amgen I,
(2) Conclusion
Having considered the scope and content of the prior art, the differences between Goldwasser and the claimed invention, the level of skill in the art, and the objective secondary considerations, the Court holds that HMR/TKT has failed to show by clear and convincing evidence that Goldwasser renders claim 1 of the ’422 patent and claims 2-4 of the ’080 obvious.
VII. CONCLUSION, DECLARATION, AND ORDER FOR JUDGMENT
As with the first trial, it has been an honor to have presided over this case. The attorneys representing both parties litigated the case with dedication, skill, intelligence, integrity, and patience.
For the reasons set forth above, as a result of the remand trial the Court makes the further declaration:
Claim 1 of the ’422 patent is valid.
Claims 2-4 of the ’080 patent are valid.
Claims 4-9 of the ’698 patent are valid and literally infringed.
Claim 7 of the ’349 patent is valid and literally infringed.
SO ORDERED.
Notes
. "DNA” is short for "deoxyribonucleic acid.”
. This product is sold under the trademark EPOGEN®.
. Hoechst Marion Roussel, Inc. is now known as Aventis Pharmaceuticals, Inc.
. The fifth patent involved in
Amgen I
was U.S. Patent No. 5,547,933 (issued Aug. 20, 1996) ("’933 patent”). Since this Court's
*214
ruling that the '933 patent was invalid for indefiniteness under 35 U.S.C. § 112, ¶ 2 was upheld on appeal,
Amgen II,
. Because many of the exhibits from the first trial were used in the second trial and the numbering system was simply continued in the second trial, the Court will not designate from which trial the exhibits came but instead simply refer to the trial exhibit number. When citing testimony, however, the Court will refer to the second trial as the "remand trial" and cite it as "R. Trial,” while the first trial will simply be cited as "Trial.”
. Amgen transfects CHO cells with a vector that contains both viral promoter DNA and the human EPO gene. ’933 Patent, Ex. 1, col. 25: 58-61;
Amgen I,
. The term "therapeutically effective” is found in claim 1 of the '422 patent and in claim 4 of the '080 patent.
. In its opinion, the Federal Circuit affirmed this Court's finding that Sugimoto did not anticipate the '080, '933, '349, and '698 patents.
Amgen II,
. The error was harmless because the Court, despite having concluded that Sugimoto was not enabled, "nevertheless conducted a full anticipation analysis” and found that " 'none of the cited references disclose[s] each and every limitation of any of Amgen’s individual claims' " of the '080, '933 and '349 patents.
Amgen II,
. It is clear from
Amgen II
that Amgen may on remand argue that the '422 patent is not anticipated because Sugimoto is not enabled.
See Amgen II,
. During the first trial, this Court found in favor of HMR/TKT on equivalent and literal infringement of the '698 patent after Amgen presented its case but before HMR/TKT had the opportunity to present its case on this issue.
. HMR/TKT also attempted to argue that the '698 patent should be declared unenforceable because it was obtained as a result of inequitable conduct. This Court, during the pretrial conference on September 24, 2003, ruled that HMR/TKT could not put on any evidence of inequitable conduct relating to the '698 patent because it was "satisfied that the pleadings, the pretrial documents early on as to ’698 did not frame that issue for trial.” 9/24/03 Pretrial Conf. Tr. at 26: 4-9.
.Therefore, these memos requested that the Court (1) construe "DNA encoding”; (2) decide whether HMR/TKT is allowed to make its step-plus-function arguments at this stage and if yes, determine whether the asserted claims *220 of the '349 and '698 patents are step-plus-function claims; and (3) determine whether HMR/TKT can argue the reverse doctrine of equivalents with respect to the '698 and '349 patents for the first time on remand and if so, whether this argument has merit.
. See generally Hon. Shira A. Scheindlin & Jonathan M. Redgrave, Revisions in Federal Ride 53 Provide New Options for Using Special Masters in Litigation, N.Y. St. B.A.J., Jan. 2004, at 10, reprinted sub. nom. The Evolution and Impact of the New Federal Rule Governing Special Masters, Fed. Law., Feb. 2004, at 35.
. While the reasoning need not be rehashed in this memorandum and opinion, the Court takes this opportunity to note a few typographical errors in the decision. At the following pages, the word "urinary” was inadvertently added where it should not have been: 154 (“urinary” is used five times in note 39 and should be deleted); 157 (the word "urinary” is used right before note 41 and should be deleted). As will be noted, the word "urinary” is used in many other places throughout the opinion. These uses of the word should remain. These errors do not in any way change the result of that opinion. Correction of them, however, makes the opinion more accurate.
.During the remanded trial, Amgen moved for Judgment Pursuant to Rule 52(c) that claims 4-9 of the '698 patent were infringed and not invalid under 35 U.S.C. § 112 [Doc. No. 778], The Court did not rule on this motion but instead deferred entering judgment until all of the evidence had been presented. See Fed.R.Civ.P. 52(c). The Court's final decisions regarding infringement and validity of the '698 patent will be explained in detail below.
. Previous decisions by the Court, such as claim constructions, will be explained in this memorandum.
. While the focus of the Markman hearing was on the patents, specification, and prosecution history, the Court writes now with the benefit of having presided over the entire second trial. Unsurprisingly, both parties continued to present arguments regarding construction throughout the trial, weaving in arguments regarding validity. The Court, however, construed the terms before the retrial and, therefore, the arguments and intrinsic evidence addressed in this memorandum regarding construction of these terms stem from these data provided before the retrial.
.The Federal Circuit refers to the term "therapeutically effective.” The Court notes, however, that claim 1 of the '422 patent and claim 4 of the '080 patent actually recite a “therapeutically effective amount" of either *223 "human erythropoietin” or "an erythropoei-tin glycoprotein product,” respectively. '422 and '080 Patents, Ex. 1 (emphasis added).
. The Court came to this conclusion because it found that the Goldwasser study was a failure.
. Although the Court did not receive evidence during the Markman hearing, for the sake of unity throughout this decision, citations to the patents are made to what was identified as Trial Exhibit 1 ("Ex. 1") (which contains the common specification and recitation of all the claims).
. HMR/TKT argues that Amgen’s position on this claim construction is inconsistent with its position on claim construction for all the other terms the Court has construed in the previous trial because Amgen here is seeking to limit the term’s definition via the specification and prosecution history. HMR/TKT’s Mem. in Opp'n re '422/’080 at 12. While it is true that Amgen has previously argued to the Court that the terms of the claims were entitled to their broadest possible scope, it also consistently argued that the words of the claim should prevail.
Amgen I,
Ultimately, how the issue has been framed will not change the analysis because it is clear from the principles of claim construction that claims are construed in light of the specification and prosecution history.
Southwall Techs., Inc. v. Cardinal IG Co.,
. At first glance, the extrinsic evidence rule in Vitronics appeal's to create somewhat of a conundrum, in that it discourages resort to extrinsic evidence while at the same time urging courts to begin claim construction by considering the plain and customary meaning of a term as understood hy one skilled in the art. How does a Court decipher the plain and customary meaning of a term as understood by one skilled in the art without resorting to extrinsic evidence about how one skilled in the art would construe the term?
The Federal Circuit is currently considering this question en banc. In granting a petition for rehearing en banc in Phillips v. AWH Corp., 03-1269, -1286, the Federal Circuit asked for briefing on the following questions:
1. Is the public notice function of patent claims better served by referencing primarily to technical and general purpose dictionaries and similar sources to interpret a claim term or by looking primarily to the patentee's use of the term in the specification? If both sources are to be consulted, in what order?
2. If dictionaries should serve as the primary source for claim interpretation, should the specification limit the full scope of the claim language (as defined by the dictionaries) only when the patentee has acted as his own lexicographer or when the specification reflects a clear disclaimer of claim scope? If so, what language in the *227 specification will satisfy those conditions? What use should be made of general as opposed to technical dictionaries? How does the concept of ordinary meaning apply if there are multiple dictionary definitions of the same term? If the dictionary provides multiple potentially applicable definitions for a term, is it appropriate to look to the specification to determine what definition or definitions should apply?
3. If the primary source for claim construction should be the specification, what use should be made of dictionaries? Should the range of the ordinary meaning of claim language be limited to the scope of the invention disclosed in the specification, for example, when only a single embodiment is disclosed and no other indications of breadth are disclosed?
4. Instead of viewing the claim construction methodologies in the majority and dissent of the now-vacated panel decision as alternative, conflicting approaches, should the two approaches be treated as complementary methodologies such that there is a dual restriction on claim scope, and a pat-entee must satisfy both limiting methodologies in order to establish the claim coverage it seeks?
5. When, if ever, should claim language be narrowly construed for the sole purpose of avoiding invalidity under, e.g., 35 U.S.C. §§ 102, 103 and 112?
6. What role should prosecution history and expert testimony by one of ordinary skill in the art play in determining the meaning of the disputed claim terms?
7. Consistent with the Supreme Court’s decision in Markman v. Westview Instruments, Inc.,517 U.S. 370 ,116 S.Ct. 1384 ,134 L.Ed.2d 577 (1996), and our en banc decision in Cybor Corp. v. FAS Technologies, Inc.,138 F.3d 1448 (Fed.Cir.1998), is it appropriate for this court to accord any deference to any aspect of trial court claim construction rulings? If so, in what circumstances, and to what extent?
Phillips, Order of July 21, 2004. Judge Rad-er, concurring in the granting of the petition, added the following:
Is claim construction amenable to resolution by resort to strictly algorithmic rules, e.g., specification first, dictionaries first, etc.? Or is claim construction better achieved by using the order or tools relevant in each case to discern the meaning of terms according to the understanding of one or ordinary skill in the art at the time of the invention, thus entrusting trial courts to interpret claims as a contract or statute?
Id. (Rader, J., concurring).
This Court’s approach is first to consider the plain and ordinary meaning as defined by dictionaries and technical treatises, and then to consider the file wrapper to determine what it communicates to the reader about the plain and customary definition of the term. It may provide clues as to how one skilled in the art would define the term or which dictionary or technical definition is adopted by those skilled in the art. Then again, it may clearly redefine the term and thus overrule the plain and ordinary meaning deciphered by the Court. Regardless, since the patent process is a public one, whatever definition is clearly supported in the file wrapper is the one that ought prevail, since this is the one on which the public relies. Thus, if a term supposedly has a specific technical meaning that cannot be gleaned from general dictionaries and treatises or the file wrapper, but can only be ascertained from expert testimony, this specific meaning will not be adopted, given the Vitronics rule against resort to extrinsic evidence.
This Court's approach resolves the apparent conundrum by drawing a line between cognitive and investigative tasks. One can understand this process by analogizing claim construction to contract interpretation. When a judge interprets the meaning of a term in a run-of-the-mill contract, she is determining how an ordinary speaker of English would understand the term, in context, and she cannot look to extrinsic evidence unless there is some ambiguity. A dictionary constitutes extrinsic evidence of the "plain and customary” meanings that members of the relevant language community ascribe to various words, but it is also serves as a tool to enhance the judge's cognitive capacities, which capacities are then applied to the task of interpretation. In theory, at least, a judge interpreting a contract written in a foreign language would follow the same process, though she might want to gain some background understanding of the language from experts. Having acquired such background, she could then use foreign language dictionaries the same way she would use an English dictionary. Having acquired the additional cognitive capacity, the judge might find that a term's meaning is ambiguous, in which case the judge could turn to extrinsic evidence, say, of industry custom. In other words, the judge would then conduct an empirical investigation of the behavior of relevant actors.
*228 One could thus regard the task of judges in patent cases as one of learning a number of "difficult” words in the English language, or as one of entering a new community of language. In either case, seeking "fluency” is different from determining what customs prevail in a particular "art,” even if those customs involve the use of an otherwise ambiguous term. Having learned to "speak” the relevant "language” by consulting lay and technical dictionaries (and perhaps having acquired background understanding from experts), the judge can then apply these new cognitive capacities to determine whether, in context, the patent term is ambiguous. Finding that meaning, then, involves an application of the judge’s enhanced cognitive abilities, not an investigation of empirical facts.
In reality, construction of patent claims does not work the same way that interpretation of foreign-language contracts does. In practice, judges interpreting foreign language contracts rely on experts to interpret them. See, e.g., 1st Cir. R. 30(d) ("The court will not receive documents not in the English language unless translations are furnished.”); Ramos-Baez v. Bossolo-Lopez,240 F.3d 92 , 94 (1st Cir.2001) (similar); cf. 35 U.S.C. § 371(c)(2) (requiring that an applicant filing a national stage application submit a copy of the international application (with certain exceptions), as well as translation into the English language of the international application). Every foreign language contract is ■ treated as "ambiguous,” because learning a new language would involve too dramatic an expansion of a judge’s cognitive capacities, and an empirical investigation is the best that she can do (although once that investigation reveals which English translation is correct, the judge can then determine whether that translated document is ambiguous). The Federal Circuit has decided, however, that learning the meaning of technical terms in English, or mastering the language used by members of a community of English-speaking persons of ordinary skill in a particular art, does not reach that level. The task of claim construction falls on the "cognitive” side of the divide between expanding and applying cognitive capacities, on the one hand, and investigating empirical facts, on the other. Thus, only when application of the judge’s newly acquired cognitive capacities determines that a term's meaning is ambiguous does she then turn to empirical investigation of the behavior of persons skilled in the art. She then uses dictionaries, expert testimony, and so on not as a cognitive tool, but as evidence.
. To heal means "[t]o restore to health, or soundness; cure.” The American Heritage Dictionary, supra, at 599.
. This was the meaning of the term that this Court essentially adopted in its previous opinion. It was founded on expert testimony demonstrating that those skilled in the art would define "therapeutically effective” — as it relates to treating anemia- — as an increase in hematocrit. Again, however, resort to such extrinsic evidence ought be had only
"if necessary.” Vitronics,
. As will be noted infra, it appears that the patent examiner also believed that the patent needed to address for what disease states the product was "therapeutically effective.”
. Amgen argues, based on Altiris, that it can rely on expert testimony to confirm the plain and customary meaning of the word as understood by one skilled in the art. HMR/TKT argues that Amgen is using the expert testimony to change the ordinary meaning of a claim term. HMR/TKT’s Mem. in Opp'n re '422/'080 at 19. While the expert testimony does support the plain and ordinary meaning of the term since it defines what “cure” *231 means in the context of anemia patients, the Court will not rely on it to construe the claim, because even the Altiris court made clear that it was looking to expert testimony merely to understand the technology — not to construe the term itself.
. While the Court cannot rely on expert testimony to help construe the term "therapeutically effective” unless absolutely necessary, it may look to the expert testimony to better understand the technology.
Vitronics,
. Again, extrinsic evidence is being used to understand the technology — not to define the term.
. This is consistent with HMR/TKT's argument with respect to validity and Goldwasser that the biological effects are critical steps in the development of red blood cells, HMR/ TKT's Proposed Findings of Fact after Trial [Doc. No. 807] ¶¶ 64-66, and expert testimony. Experts on both sides agree that the biological effects are surrogate markers or early indicators that a therapeutic effect will follow. Foster Test., R. Trial Tr. at 946-47, 965; Schumacher Test., R. Trial Tr. at 807: 3-5, 813: 3-18; Eschbach Test., R. Trial Tr. at 660; 22 to 661: 8, 669: 10-670: 2, 766: 4-17; Christensen Test., R. Trial Tr. at 1185: 1-17, 1186: 9-24.
.This is not to suggest that the specification cannot provide guidance as to the scope of the claims absent a clear and deliberate act of lexicography by the patentee. Indeed, if the claim's scope cannot be ascertained from the ordinary and plain meaning of the words alone, the specification can assist and even limit the interpretation of the claims.
Teleflex, Inc. v. Ficosa N. Am. Corp.,
. If Amgen limited the invention to patients suffering from anemia, then by default the definition of "therapeutically effective” equates with an increase in hematocrit if only an increase in hematocrit heals or cures anemia.
. All of these patients are in many respects transfusion-dependent. Extrinsic evidence demonstrates that it is an increase in hemato-crit which eliminates the need for transfusions.
. If this were not the case, arguably, the patent would be invalid for indefiniteness. Issued patents are presumed to be valid, 35 U.S.C. § 282;
National Recovery Techs., Inc. v. Magnetic Separation Sys., Inc.,
. Amgen argues that the "minimization of the need for transfusion therapy” — which is used to increase the oxygen transport capacity of the blood — can only be achieved by raising an anemic patient's hematocrit for a sustained period. Amgen's Mem. in Support re ’422/'080 at 12. Therefore, it argues that this section supports its contention that the term "therapeutically effective” means an increase in hematocrit. Id. This section, however, is merely explicating one example of how the product is useful or advantageous— just as the section on the class of patients included patients suffering from anemias that can be cured by an increase in hematocrit but *237 also included patients in need of blood transfusions.
. As will be discussed infra, the extrinsic evidence shows that an increase in hematocrit is necessary to cure defective red blood cell production effectively.
. As will be discussed at great length infra, if the term “therapeutically effective” is properly construed only with reference to this class of patients, it is irrelevant whether Amgen actually refined the term to mean an "increase in hematocrit” as the evidence at trial confirmed that these types of patients are only healed or cured by an increase in hematocrit and not by any of the biological effects.
.Citing an unpublished opinion raises a number of difficult questions.
See Anastasoff v. United States,
. The specification at that time confirms this interpretation:
Novel glycoprotein products of the invention includes those having a primary structural conformation sufficiently duplicative of that of a naturally-occurring (e.g., human) erythropoietin to allow possession of one or more of the biological properties thereof and having an average carbohydrate composition which differs from that of naturally-occurring (e.g., human) eryth-ropoietin.
Amgen’s '422/'080 App., Tab G (Ex. 2), at Tab 6, at 180; see also id. at 181.
. This supports Amgen's contention that it defined “therapeutically effective” as an increase in hematocrit since, as will be discussed infra, the evidence shows that an increase in hematocrit — unlike the other biological effects listed in the specification— cures or heals the diseased states mentioned in the specification.
. These were the original claim numbers in the application 08/100,197 for what is now the ’422 patent. Also, the word "composition” was crossed out and handwritten above it was the word "preparation.”
. While "it is improper for a court to add extraneous limitations to a claim/'
Hoganas AB v. Dresser Indus., Inc.,
. As with the specification, these remarks make clear that any or all of the biological effects are part and parcel of therapeutic effectiveness, that is, that Amgen refined "therapeutically effective amount” to be one that, at the least, elicits one or more of the in vivo effects heretofore attributed to natural EPO.
. Although the Court does not read them as such, these sentences could be interpreted to support that "therapeutically effective” includes the biological effects. This ambiguity, however, does not establish HMR/TKT’s point. To the contrary, it demonstrates that the patentee did not clearly and deliberately redefine the term and that the plain and ordinary meaning should prevail.
.This ambiguity itself is helpful to Amgen, given that "claims should be construed to sustain their validity” and Amgen is not advancing a definition of the term that is contrary to the plain and ordinary meaning.
Rhine v. Casio, Inc.,
. Further support for the conclusion that Amgen was not redefining therapeutic effectiveness to include the biological effects regardless of whether they worked to heal or cure the patient is found in the prior art disclosed to the patent examiner.
Autogiro Co. of America
v.
United States,
. While the specification and prosecution history support Amgen's contention that it defined "therapeutically effective” to mean an increase in hematocrit, the intrinsic evidence does not show a clear and deliberate attempt to redefine the term this way. Even were this not the case, and the Court ruled there was a clear and deliberate intent to define "therapeutically effective” as an increase in hemato-crit — or for that matter had resorted to extrinsic evidence and ruled that this was how those skilled in the art defined the term — the end result regarding validity of these patents in view of prior art would not be different. As will be discussed further below, the evidence shows that the biologic effects of EPO do not elicit any meaningful health benefit to patients. Therefore, the only thing claimed in the patent that actually does heal or cure is an increase in hematocrit. Thus, by default the terms "therapeutically effective” and "increase in hematocrit” become synonymous.
As mentioned earlier, an alternate route would have been to consider extrinsic evi *245 dence as to the meaning those skilled in the art would give the disputed term. Indeed, much evidence was presented at the first trial on the subject, the bulk of which supports Amgen’s contention that one skilled in the art would equate “therapeutically effective” with an increase in hematocrit when considering anemia. Two crucial witnesses for the defense conceded as much. Dr. Means testified that in the routine practice of medicine as it relates to EPO in treating anemia in patients, "an increase in hematocrit is how one defines a response.” Means Test., Trial Tr. at 1910: 9-13. Dr. Erslev agreed that the accepted standard by which physicians measure a therapeutic response to EPO is an increase in hematocrit. Erslev Test., Trial Tr. at 1675: 12-23. The only problem with relying on such evidence — other than the Federal Circuit’s ruling in Vitronics and the concern for public reliance on the record — is that this expert testimony was given in reference to anemic patients specifically and did not take into account the entire list of patients in the specification.
In hindsight, however, it appears that this distinction between anemia and the entire list of patients included in the specification is meaningless, for the evidence shows that only an increase in hematocrit provides a meaningful health benefit to the class of patients listed in the specification.
. Neither party objects to the Court now formally construing the term despite the fact that this issue was not raised during the first trial.
. "RNA” is short for "ribonucleic acid.”
. Dr. Kingston explained that the other "perfectly valid” way the word can be used, depending on the context, is to "describe all the instructions to make the mature protein.” Kingston Test., R. Trial Tr. at 163: 7-12. In other words, Dr. Kingston testified that the term can also mean that it provides all the instructions necessary to allow a certain protein to be made.
.Neither party directed the Court to the prosecution history. Therefore, the Court will not look to it to construe the disputed term.
. HMR/TKT believes it somehow bolsters its argument by pointing out that the Court construed the word "mature” to mean the
"fully realized
form of the amino acid sequence of Figure 6,”
Amgen I,
. Amgen's counsel provided a brief, undisputed, refresher for the Court as follows:
[T]he DNA encodes EPO. The DNA is transcribed to make a messenger RNA. That messenger RNA is then reprocessed in the cell. That messenger RNA is extruded from the nucleus. A ribosome binds to it, translates the messenger RNA into a protein. And a protein that is a copy of the entire DNA sequence of the messenger RNA, including both the leader sequence and the ... amino acid position 166, is made in the cell. The cell then ... further processes that protein cutting off ... the leader sequence of the protein and the amino acid at 166, and that is done before the cell then secretes the fully processed form of the hormone.... And as the protein is secreted from the cell, even though it's encoded by DNA that has 166 amino acid, the cell actually produces a protein that has 165 amino acid.
7/28/03 Hr’g Tr. at 45: 21-46: 12.
. It is true that the Court construed the term “mature erythropoietin amino acid sequence of FIG. 6” in the '080 patent to refer to the structure of the claimed EPO glycoprotein. In the '698 patent, however, the claims refer to the structure of the DNA, not of a protein.
. The Court noted that this construction applied any time DNA encoding was used throughout the various claims. 7/28/03 Hr’g Tr. at 56: 18-23.
. Dr. Lodish and Dr. Kingston appear to agree that there are two parts to genes. "One is the regulatory sequences that determine when and under what conditions the cells copy the gene into RNA; and the second is the coding sequence, the piece of DNA that actually specifies the amino acids in the encoded product." Lodish Test., R.. Trial Tr. at 1058: 20-25. They disagree about to what this claim is referring. Interestingly, at the same time that Dr. Kingston claims that this Court’s construction means the regulatory sequences — all the instructions for the protein— he admits that ”[t]he DNA that encodes each amino acid is the same” in both Amgen's and HMR/TKT’s cells. Kingston Test., R. Trial Tr. at 162: 18-19.
. For more background, see background discussion regarding construction of the term "DNA encoding.”
. The purpose of section 112, paragraph 6 was
to permit use of means expressions without recitation of all the possible means that might be used in a claimed apparatus.... The price that must be paid for use of that convenience is limitation of the claim to the means specified in the written description and equivalents thereof. Similarly, a step for accomplishing a particular function in a process claim may also be claimed without specificity subject to the same price.
O.I. Corp.,
. The Court compared the accused process to the preferred embodiment in the claim and concluded that "HMR/TKT's process for producing erythropoietin differs markedly from that disclosed by Amgen's specification” because it "utilizes the endogenous rather than exogenous EPO gene” and it "places it promoter upstream from rather than adjacent to the EPO gene.”
Amgen I,
.In other words, the Court went straight to a step-plus-function approach without first ruling that these were indeed step-plus-function claims. As will be discussed infra, the Court mentioned to the parties when giving a ruling of non-infringement of the '698 patent, that it was considering a means-plus-function type of analogy. When writing the opinion, however, the Court did not address whether step-plus-function claims were indeed involved and, despite any discussions to the contrary, did not base its ruling of non-infringement of the '698 patent on a finding that it involved step-plus-function claims.
. See the preceding section regarding "DNA encoding” for recitation of claims 4 and 6 of the '698 patent.
. The fact that Amgen’s counsel and the Court referred to "means-plus-function” as opposed to "step-plus-function” makes little difference in the Court's analysis here because the two concepts are very closely related, enough so that mention of one provides notice of the potential that the other may apply.
Seal-Flex,
. Thus definitive resolution of the procedural dispute is unnecessary.
. Expert testimony by one skilled in the art — extrinsic evidence which the Court need not to resort — implicitly supports defining "growing” as an act. Dr. Tlsty made clear that the term "growing” was one that was easily understood by one skilled in the art when he stated, without explanation, that he has "been growing and culturing cells since Die] was an undergraduate.” Tlsty Test., Trial Tr. at 832: 11-16;
cf. Greenberg v. Ethicon Endo-Surgery, Inc.,
The way in which HMR/TKT described the culturing and growing of its cells in Investiga-tional New Drug Application ("IND”) for HMR 4396 provides further evidence that the term has a reasonably well-understood meaning in the art. For example, it stated that "[Cjells grown as attached cultures in static flask were released by trypsination. The cells were resuspended in LONZA Biologies proprietary HM9 Serum-free medium .... Once a reliable pattern of growth was established, the serum supplement was progressively eliminated from the medium.” Amgen's App. to Mem. in Opp'n re '698 & '349, Tab T (Ex. 19, IND for HMR 4396) at 574.
. As will be discussed, HMR/TKT made a more detailed argument that claim 7 of the '349 patent is a step-plus-function claim. This argument fails, however, so it also fails when applied to the '698 patent.
. The issue was likely never brought to the Federal Circuit's attention since neither party, on appeal, had anything to gain in bringing it up.
. Importantly, however, neither is the converse true: the Federal Circuit in
O.I. Corp.,
which dealt with a claim very similar to the claim here, held that "a statement in a preamble of a result that necessarily follows from performing a series of steps does not convert each of those steps into step-plus-function clauses.”
O.I. Corp.,
. As discussed earlier, expert testimony by Dr. Tlsty and assertions in the IND by HMR/ TKT — extrinsic evidence to which the Court need not resort — also support that the terms "growing” and "culturing” have meanings reasonably well understood by those skilled in the art.
. Thus, as with the '698 patent, the procedural dispute and the Court's conclusion as to whether HMR/TKT should be allowed to raise this argument are moot.
. As remarked in
Amgen I,
. Generally, lire Court addresses each argument patent by patent. Where, as here, it makes sense to address more than one patent at once, due to their similarities, the Court will do so.
. The Court notes that it did not construe the term to include the splicing instructions for putting the codons together. That being said, the term does not occur in a vacuum. It is read with reference to "the mature eryth-ropoietin amino-acid sequence depicted in Figure 6 of the patent.” Thus, the claims themselves communicate that other steps are necessary to result in the correct order of amino acids.
. Amgen also argues that this Court stated during the 9/18/03 motion hearing that it was not going to address any issues that were not remanded to the Court by the Federal Circuit. Amgen's Reply to HMR/TKT’s Findings of Fact [Doc. No. 816] at 173. The issue of infringement, however, was remanded to this Court. A complete decision regarding infringement necessarily includes analysis of these defenses. Moreover, neither party contended that the Court ought not construe "DNA encoding.” To the contrary, both parties made it clear this term needed construction. As a result of that construction, a door to a new validity challenge was opened. Thus, to do its job adequately, the Court must address HMR/TKT's challenge.
Additionally, Amgen points out that this Court held that the cell claims (1, 3, 4, and 6) of the '349 patent are adequately described and enabled, and that these rulings are law of the case. Amgen's Reply to HMR/TKT's Opening Br. at n. 150. Claim 7 contains a "DNA encoding” limitation only through its dependence from claims 1 and 3. Id. As such, Amgen contends, any invalidity challenge to the '349 patent must address the only addition claim 7 makes, which is the "growing step.” Thus, Amgen reasons, HMR/TKT’s challenge regarding "DNA encoding” should fail. This procedural argument, however, need not be addressed, given the Court's ultimate finding, discussed below, that claim 7 of the '349 patent is not invalid for indefiniteness.
. For a discussion of the controversy within the Federal Circuit as to whether section 112 contains a separate written description requirement, or whether it only contains an enablement requirement, see Vernon M. Winters & Elizabeth Stotland Weiswasser, The Written Description Requirement: Ripe Enough? Or Is More Percolation Required, Fed. Law., Aug. 2004, at 20.
. This is the same argument that HMR/TKT made during the first trial and on appeal with reference to the product claims of the '422 and '349 patents.
Amgen I,
. The term "operatively linked'' is not found in the '349 patent, so this argument only relates to the '698 patent.
. In
Amgen I,
the Court construed "opera-tively linked” to mean "the promoter DNA is linked to the EPO DNA in a way that maintains the capability of the promoter DNA to initiate transcription of the EPO DNA.”
Am-gen I,
. As stated in
Amgen I,
experts for both sides agreed that the specification did not explicitly show any examples of human EPO production whereby endogenous EPO DNA was expressed.
. HMR/TKT does not dispute Amgen’s contentions
(see
Amgen’s Reply to HMR/TKT’s Opening Brief After Trial at 34-35) that these are post-filing advancements. Moreover, in making its reverse doctrine of equivalents argument, HMR/TKT asserted that this difference contributed to the Court's finding that HMR 4396 was "technologically advanced.” HMR/TKT’s Mem. in Opp'n re '698 at 6;
see Amgen I, 126
F.Supp.2d at 104. Indeed, the Court found in
Amgen I,
and the Federal Circuit affirmed, that endogenous activation was a later-developed technology.
Amgen I, 126
F.Supp.2d at 160;
Amgen II,
. Professor John F.. Duffy has recently suggested an intriguing revision to the "prospect theory” of patents, which justifies "prospect patents”- — -"broad patents issued in the early stages of technical development” — on the ground that they create social benefit by encouraging investment in a technological prospect after the property right has been granted, rather than by encouraging the investment that led to the patent in the first place. John F. Duffy, Rethinking the Prospect Theory of Patents, 71 U. Chi. L.Rev. 439, 440 (2004). Professor Duffy agrees that "prospect patents” are socially beneficial in a forward-looking way, but for a different reason: they channel rivalry in such a way that the property right goes to the inventor who is willing to accept the least profit for it. See id. at 443-44. Because patents have fixed terms, obtaining a patent earlier in the technological development process means that the period between the date when the patentee can convert the invention into a marketable product and the date when the patent term ends (and hence the period when the property right will actually generate profit) will be shorter. See id.
.
See Amgen I,
. Amgen also argues that the Court's findings regarding proximity of the promoter concern the process for constructing cells (cells which been held to be adequately described and enabled) and are, therefore, irrelevant to the '698 and '349 claimed processes for producing EPO. Amgen's Reply to HMR/TKT's Opening Br. After Trial at 35; Amgen’s Reply to HMR/TKT's Findings of Fact at 41. This argument fails. Just because the cells themselves and the EPO product were found to be adequately described and enabled by the product claims does not mean that the method by which the cells are constructed or the EPO is made is necessarily adequately described and enabled in the process claims.
*268
As this Court pointed out in
Amgen I,
"[a] product patent claims a structural entity that, though some process must be undertaken in order to create it, is in no way defined or limited by how it is made.”
. While the Court found in the first trial that HMR/TKT's promoter placement was a "technological advance” over Amgen’s process, the Court notes that it did so in a different context under a different burden of proof and that the ultimate holding of the Court was reversed. In
Amgen I,
the Court held that HMR/TKT had shown by a preponderance of
*269
the evidence that its process was substantially different from the process identified in Am-gen's '698 patent and claim 7 of the '349 patent.
Amgen I,
. In any case, even if the Court were to conclude, as HMR/TKT urges, that no one then had the courage to use the splice sites as HMR/TKT later did, HMR/TKT's written description challenge would still fail; if the courage and knowledge had been missing and HMR/TKT's placement of the promoter had been truly innovative and new, then this technique would have constituted a post-filing technological advance — something Amgen need not have described in order to satisfy section 112, paragraph 1.
. Although the Court intimated in
Amgen I
that the written description requirement may be different for process claims as opposed to product claims,
. Dr. Lodish also conceded that placement of the promoter can indeed affect expression, Lodish Test., Trial Tr. at 421; cf. Kingston Test., R. Trial Tr. at 44; 20-45: 1-5. He clarified, however, that the difference in expression is determined not by the number of pairs between the promoter and the EPO gene necessarily but by other factors concerning the general area of the chromosome in which it finds itself. Lodish Test., Trial Tr. at 420-421.
. The Court refers to HMR 4396 — as an example of a process that places the promoter further upstream — to support the conclusion that the specification communicates to those skilled in the art a process that incorporates such upstream placement.
. While there was much debate about this subject, as discussed in more detail infra (parts V.A.3-4, V.B.4), the Court credits Dr. Lodish's testimony explaining that the exons are not' included when one skilled in the art refers to the splice donor and acceptor sites. Lodish Test., R. Trial Tr. at 1107-1110; id. at 1132-33 (explaining that it is the splice donor sequence, not the splice junction, that will determine where downstream and with what corresponding DNA downstream a splice junction will splice, and stating that “the splice donor is the sequence ... that is removed during the splicing process,” the splice acceptor is the sequence that is removed downstream, and "it's the regions on either side that aré linked together.”). There is testimony by Dr. Kingston and evidence from the HMR/TKT's IND that supports this conclusion. As a result, the Court concludes that HMR 4396 uses the same splice donor site as that disclosed in Amgen’s specification. Kingston Test., Trial Tr. at 1431: 10-19, •1432: 14-24, 1433: 1-22, 1440: 19-25 (admitting that absent the exons, the splice donor sites were the same and that the intended effect was to splice out what is in between, including intervening sequences and the deleterious ATGs).
. HMR/TKT also relies on
PIN/NIP, Inc. v. Platte Chemical Co.,
. In
Genentech,
the patentee was "attempting to bootstrap a vague statement of a problem into an enabling disclosure sufficient to dominate someone else's solution of the problem.”
Genentech,
. In
Enzo,
the Federal Circuit declared that the minimal disclosure constituted "no more than a plan or invitation to practice” the invention in cells other than E. coli.
Enzo,
. HMR/TKT asserts in its Opening Brief after Trial that the reason that the skilled worker would not have expected that linkages further upstream would produce EPO is that "the expression process would be interrupted or misdirected by sequences, such as other start codons or stop codons, that intervened between the promoter and the EPO DNA.” While this information about the difficulties of upstream promoter placement might work to support a finding of undue experimentation, HMR/TKT does not even argue that this is what it shows. Moreover, the only support it provides for this statement is the Court’s previous finding in Amgen I, which was implicitly rejected by the Federal Circuit. Tellingly, HMR/TKT offers no concrete evidence or expert testimony addressing how it would have been difficult for the skilled artisan to make and use the invention as it is claimed or what type of experimentation would be necessary. Id. at 49.
. It is true that in
Texas Instruments Inc. v. United States International Trade Commission,
. As Amgen points out (and HMR/TKT does not dispute), “DNA and protein are two distinct types of biological molecules,” and, therefore, "the claim limitation must be carefully construed in light of the relevant claim language.” Amgen's Reply to HMR/TKT's Findings of Fact at 36.
. Dr. Lodish based his opinion on a comparison between the sequence of complementary DNA (“cDNA”) made by HMR/TKT’s contract manufacturer from the EPO DNA in R223 cells and the codons for amino acids at positions +1 to +166 of Figure 6. Lodish Test., R. Trial Tr. at 1066: 23-1067: 18; Lodish Test., Trial Tr. 245: 16-247: 18. It is undisputed that a cDNA is simply a DNA copy of a messenger RNA. In other words, the DNA is transcribed into an RNA transcript first. Then the RNA transcript is spliced into a messenger RNA. The cDNA is made as a direct DNA copy of the messenger RNA using reverse transcriptase so the sequence of the cDNA will be that of the messenger RNA. Lodish Test., R. Trial Tr. at 1066.
. HMR/TKT neither claims nor cites to any authority claiming that the antecedent for a claim limitation must be found in the meat of the claim and not in the preamble.
. The Federal Circuit made clear in
SRI International,
that after the patentee has proved literal infringement,
“the accused in-fringer
may undertake the burden of going forward to establish the fact of non-infringement under the reverse doctrine of equivalents.”
Thus, here — notwithstanding its unpersuasive arguments to the contrary — HMR/TKT has the burden of making a prima facie showing that "the accused device is outside the fair and equitable scope of the invention.” Siril-la, Feddo & Antone, supra, at 101.
. If it were based solely on the claim language itself, the analysis would not differ from basic literal infringement and section 112 analysis.
. Although the Federal Circuit may never have upheld a decision based on the reverse doctrine of equivalents, some appellate courts, before the Federal Circuit was created, applied the doctrine of equivalents defensively without expressly identifying it as the reverse doctrine.
See, e.g., Leesona Corp. v. United States,
.District Courts also appear to be reluctant to apply the reverse doctrine of equivalents.
But see Marvin Glass & Assocs. v. Sears, Roebuck & Co.,
. If the claims are broader than the “spirit and intent” of the invention, this will most likely be apparent by a close reading of the specification. At this point, a section 112 challenge may be initiated in lieu of a reverse doctrine of equivalents argument. As discussed immediately infra, however, this challenge may not always be successful. This is where the reverse doctrine of equivalents comes in.
. Despite not relying on it, the Federal Circuit has affirmed the viability of the reverse doctrine of equivalents many times, see, e.g., Sirilla, Feddo & Antone, supra, at 87-97 and app. A (identifying many cases that applied the principals of the reverse doctrine and that supported its viability).
. Indeed, many scholars and judges have noted the similarity in operation between applying section 112, ¶6 and the reverse doctrine of equivalents. Both restrict the coverage of literal claim language.
See,
e.g.,
Valmont v. Reinke,
. A blocking patent situation occurs when an improvement is patented but the improvement patent infringes on the original patent. Lemley, Economics, at 1009-1010. The original patent owner is entitled to damages from past infringement and an injunction against future use of the infringing invention. Id. At the same time, however, the original patent owner cannot use the patented improvement without risking liability for damages and a potential injunction. Id. Thus, "the original patent owner can prevent the improver from *288 using his patented technology but the improver can prevent the original patent owner from using the improvement. Unless the parties bargain, no one gets the benefit of the improvement.'' Id.
. Merges argues that it should be used by judges to "releas[e] pressure that builds up when pioneers and improvers fail to agree to a license.'' Merges; Blocking Patents, at 75-76.
. In
Westinghouse,
the device described by the original patentee could not produce the result achieved by the accused device, that is, it could not quickly and smoothly stop a moving train.
Westinghouse,
. Even if HMR/TKT had made out a prima facie case, Amgen has successfully rebutted the defense, as will be made clear in the discussion below.
. HMR/TKT groups and labels its reasons for applying the reverse doctrine of equivalents differently in its various submissions. See, e.g., HMR/TKT's Opening Br. After Trial 11-19; HMR/TKT’s Proposed Findings of Fact at 25-41. For ease of analysis, based on the parties’ arguments at trial and submissions after trial, and the overlap among the arguments, the Court groups HMR/TKT's reasons into four areas. While the Court has considered each of HMR/TKT's contentions, and concluded that each fails for the primary reasons explained above, not every contention need be addressed specifically in this section.
. The Court first addresses homologous recombination and endogenous EPO DNA because HMR/TKT seems to assert that these points, in their own right — aside from the neighborhood theory' — work to justify evocation of the reverse doctrine of equivalents. HMR/TKT’s reliance on these differences appears to stem from the Court’s prior factual findings and legal conclusions. Indeed, the Court previously found that HMR/TKT did not equivalently infringe the '698 patent because HMR/TKT’s process performs the same function in a substantially different way, based, in part, on the fact that HMR used homologous recombination and endogenous EPO DNA while the embodiments in Amgen's specification only addressed heterologous recombination and exogenous EPO DNA.
Amgen I,
.As discussed earlier, it is undisputed that endogenous activation technology and homologous recombination were unknown to those skilled in the art when Amgen filed its patent application in 1983-84. HMR/TKT's Findings of Fact ¶ 488; Amgen’s Reply to HMR/ TKT’s Opening Br. After Trial [Doc. No. 815] at 34-35. As a result, exogenous EPO DNA expression systems and heterologous recombination techniques were not depicted in Am-gen's examples in the patent. Trial Tr. at 375: 19-25; 376-381;
see also Amgen I,
. It is clear that HMR/TKT claims its construct has a more efficient expression system' — expressing more EPO per gene copy than the cells made following example 10 in Amgen’s patent. See, e.g., HMR/TKT’s Reply Br. After Trial at 29-30. It is unclear, however, whether it is truly claiming that its process makes more EPO, as it appears from some of its submissions. Regardless, HMR/TKT never provides any support for such a contention, as will be discussed further below.
. Dr. Lodish pointed out that both cell types contain the same expression construct; the R223 cells simply contain more copies of it. Lodish Test., Trial Tr. at 163: 16-18. This, however, does not amount to a functional difference in the cells' ability to produce EPO. Id. at 178: 4-12.
. Even if it was material, HMR/TKT has still not met its burden because, as discussed immediately above, much evidence was presented that factors other than the neighborhood could cause the differences in EPO production efficiency and Dr. Kingston did not control for these factors.
. To be clear, none of the examples requires that the EPO coding sequences be “cut away” from their native regulatory sequences. To the contrary, according to Dr. Wall, Exam-pie 10 retains a downstream native EPO regulatory sequence — the hyposix inducible element ("HIE”). Wall Test., R. Trial Tr. at 1128: 10-1129: 1.
. As noted earlier, HMR/TKT offers no support — except previous statements by this Court — for its assertion that no one skilled in the art could have or would have in 1984 dared to place the promoter so far upstream from the coding sequence.
. HMR/TKT argues that its upstream promoter placement and the difference in the type of promoter optimize its process, and it cites testimony by Dr. Lodish and Dr. Wall admitting that the location and strength of the promoter affect the promoter's activity. See, e.g., HMR/TKTs Findings of Fact ¶¶ 117, 119. These arguments, however, fail to justify evocation of the doctrine for the same reasons discussed earlier. First, mere improvement or superiority is not enough. Second, it is unclear that HMR/TKT has shown any relevant optimization, since increased EPO production or quality is not claimed. Third, the location of the promoter or type of strong viral promoter are not specifically claimed or defined by the specification.
. This involves the step of translation. When the messenger RNA is translated, the result is a polypeptide which has a leader sequence. Kingston Test., R. Trial Tr. at 53: 2-4. During HMR/TKT’s translation, the leader sequence contains both the hGH and human EPO amino acids. Id.
. That this other type of culturing is described during the preparatory stage does not change the analysis because, according to HMR/TKT's expert, the cells are ''growing” and producing EPO in the preparatory stage. Hancock Test., R. Trial Tr. at 263: 3-264: 11. Therefore, this culturing method can be deemed part of the "growing” step described in the claims.
. This trial, as indeed all civil trials in this session of the Court, was conducted pursuant to strict overall time limits established by the parties pre-trial and confirmed by order of the Court. Reasonable time limits have been confirmed by the nation’s most thoughtful commentators as a trial technique that enhances the quality of justice and improves the administrative aspects of any civil trial. The Vanishing Trial, Discussion at the ABA Section on Litigation Symposium (Dec. 12-14, 2003). The Court has long followed this salutary practice.
Lareau v. Page,
. The Court’s conclusion that HMR/TKT’s mode of culturing is not "so far changed in principle” or "substantially different” finds further support in the fact that HMR/TKT’s expert stated that HMR/TKT itself employs roller bottle culturing in an early stage of its manufacturing process. Hancock Test., R. Trial Tr. at 265: 13-266: 13; HMR/TKT’s IND, Ex. 19, at 566, 574.
. As discussed earlier, the Court held and the Federal Circuit affirmed that HMR/TKT literally infringed claims 1, 3, 4, and 6.
Amgen I,
. In one of its claim construction submissions, HMR/TKT proffered that “culturing under suitable nutrient conditions” means the same things as "growing in vitro, under suitable nutrient conditions.” 10/18/99 Amgen’s Claim Construction Submission, Ex. A, at 5. In its memorandum in support of its step-plus-function arguments regarding the ’349 and '698 patent, HMR/TKT asserted the exact same arguments with regard to the step of growing and the step of culturing.
Experts also used the two words interchangeably. Dr. Tlsty stated that he had been "growing and culturing cells since [he] was an undergraduate.” Amgen’s Opp’n at 13; Tlsty Test., Trial Tr. at 832: 1-16; see also HMR/TKT's IND, Ex. 19, at 574 (describing the culturing of HMR/TKT's R223 cells).
. Indeed, it is even less appropriate to apply the reverse doctrine of equivalents with respect to the ’349 patent than with respect to the '698 patent, since these same reverse doctrine arguments were made and rejected by the Federal Circuit with respect to the product claims of the ’349 patent, and, as mentioned earlier, HMR/TKT has not adduced, nor has the Court found, any case law sug *304 gesting that process patents should be analyzed differently than product patents.
. As is so frequently the case in the patent area, this is not a true presumption at all,
see
Fed.R.Evid. 301, but rather a burden shifting mechanism that places the burden of proving nonenablement on the patentee. For criticism of this recurrent imprecision in language, see
Amgen III,
. HMR/TKT argues that Amgen’s burden of proof is higher than proof by a fair preponderance of the evidence. See HMR/TKT's Reply Br. After Trial at 4 n.* (claiming it is one of "persuasive evidence”). The Court disagrees. First, it is unclear to what standard HMR/TKT believes Amgen should be held, since proof by a fair preponderance is by its very nature "persuasive.” Second, the Federal Circuit indicated in Amgen II that the burden should be commensurate with that required of an applicant, before the PTO, to overcome a rejection for anticipation by proving non-enablement of the prior art. The Federal Circuit held that:
an accused infringer should be similarly entitled to have the district court presume the enablement of unclaimed (and claimed) material in a prior art patent defendant asserts against a plaintiff.... Like the applicant in ex parte prosecution, ... the pat-entee may argue that the relevant claimed or unclaimed disclosures of a prior art patent are not enabled and therefore are not pertinent prior art.
Amgen II,
As applied to this case, the conclusion that Sugimoto is enabled may be rebutted by Am-gen if it shows by a fair preponderance of the evidence that it is not.
But see Halliburton
v.
Weatherford,
No. 302CV1347-N,
. Evidently, Amgen even tried to purchase the starting materials and the hybrid cells directly from Sugimoto’s assignee, Hayashi-bara Company, Ltd. See Rathmann Test., R. Trial Tr. at 599: 8-13. While it may be, as HMR/TKT asserts, that Amgen simply did not offer a large enough incentive to retrieve the starting materials, the fact remains that no one skilled in the art was able to obtain them in any manner, i.e., via deposit, financial incentive, or experimentation.
. Amgen also tried to argue that Sugimo-to's failure to confirm hybrid formation or identify what confirmation method was used suggests that Sugimoto is not enabled. Dr. Green, however, agreed with Dr. Kingston that procedures for characterizing the selected cells were well known to those of skill in the art as of 1980-1984. See, e.g., Green Test., R. Trial Tr. at 392: 23-393: 4,413: 23-416: 22,507: 11-13; Kingston Test., R. Trial Tr. at 92: 24-93: 16. While the failure to confirm hybridization leads to skepticism *310 about Sugimoto’s claims, there was, by contrast with selection methods, no suggestion that carrying out these well-known confirmation techniques was difficult or posed additional problems.
For similar reasons, Amgen’s argument that Sugimoto is not enabled because he did not teach how to grow his cells in
in vitro
cell culture fails.
See, e.g.,
Amgen’s Post-Trial Br. at 11, 12. Although Dr. Lodish testified on remand that some types of kidney cells are not capable of growth in culture with only routine experimentation, Lodish Test., R. Trial Tr. at 337: 24-341: 10, he had testified during the first trial that one of ordinary skill in the art as of 1984 could adapt a vertebrate cell line to continuous growth in culture with only routine experimentation, Lodish Test., Trial Tr. at 535-36. Moreover, Amgen points to no evidence or experiments, other than Dr. Lodish's unsubstantiated and contradictory testimony, that undue experimentation would be required to adapt the cells in Sugimoto’s patent to grow in culture.
See Burning v. Hirose,
That Dr. Green did not believe that Sugimo-to actually achieved growth in culture as reported does not prove that Sugimoto did not enable the process. As discussed earlier in the context of the enablement of Amgen’s patents, it is not necessary that a disclosed invention have actually been made or even actually attempted.
See Donohue,
. Dr. Kingston defined a person of ordinary skill in the field of molecular and cell biology as someone who had a relevant PhD and roughly two years of experience working in the area. Kingston Test., R. Trial Tr. at 128: 12-14. Sugimoto filed his patent application in 1980.
Id.
at 17-24. Dr. Kingston himself was in the second year of his postdoctoral work in 1983, having received his PhD in 1981. At the time Sugimoto’s patent application was filed — the relevant time period for determining whether Sugimoto was enabled — Dr. Kingston was not even considered one skilled in the art.
Plant Genetic Systems,
. Although the Federal Circuit made clear that this fact alone is not sufficient to prove non-enablement,
Amgen II,
. While this memorandum contains inadmissible hearsay, Fed.R.Evid. 801, it was admitted without objection, see R. Trial Tr. at 604-06, and is thus entitled to full probative weight. The confirming testimony to which objection was properly raised, Rathmann Test., R. Trial Tr. at 599: 8-13 (testifying that the assignee had said that the project had been discontinued); id. at 602: 8-14 (explaining that the assignee had abandoned the program so he attempted to offer money to try to retrieve some cells), was admitted only for the fact of communication (relevant on the issue of Amgen's ability to obtain the cells) and plays no part in this aspect of the analysis.
.In addition, Amgen argues strenuously that there is no evidence that Sugimoto actually accomplished what he claimed, that is, there is no evidence that he purified the EPO or for that matter that the lysate produced from the cells actually contained human EPO — let alone EPO that would have been therapeutically effective. See, e.g., Amgen's Proposed Findings of Fact and Conclusions of Law ¶37; Amgen’s Post Trial Br. at 12-13; Amgen’s Reply to HMR/TKT’s Opening Br. at *313 8; Amgen’s Reply to HMR/TKT’s Proposed Findings of Fact ¶ 220. In support, Amgen points out that Sugimoto never claims in the specification actually to have purified the EPO, to have made an EPO pharmaceutical composition, or to have administered it to any patient in need of EPO treatment. Sugimoto Patent, Ex. 2229, col. 3: 51-65; Green Test., R. Trial Tr. at 492: 5-12. Indeed, even HMR/ TKT's Dr. Heartlein conceded that Sugimoto did not purify what he called EPO and that there was no evidence that Sugimoto’s protein was ever formulated into a pharmaceutical composition or that the protein actually would be suitable as a pharmaceutical. Heartlein Test., Trial Tr. at 1820: 22-25; 1821: 7-11; 1824: 20-1825: 3.
The Court agrees that, given the lack of sufficient controls (attested to by various experts) and the reliance only on the Cotes Assay, Sugimoto’s entire patent lacks reliable confirmation that he did what he claimed. As discussed earlier in the context of the enablement of Amgen's patent, however, it is not necessary that a disclosed invention actually have been made or even actually attempted.
See Donohue,
. HMR/TKT makes one last effort to show enablement by arguing that Amgen itself recognized Sugimoto’s enablement by identifying Sugimoto as an EPO-producing cell line in its patents. See, e.g., HMR/TKT’s Response to Amgen’s Proposed Conclusions of Law and Findings of Fact at 10. This argument is baseless. In Amgen’s patents and the prosecution history, Amgen merely repeats what Sugimoto reported to have done. See, e.g., '933 Patent, Ex. 1, col. 7: 24-35; '933 Patent File History, Ex. 2034, at 237. This type of reporting is part of an inventor’s duty to recount assertions in prior art as Dr. Lin testified. Lin Test., R. Trial Tr. at 587: 18-588: 23. Further, that Amgen tried to procure the cells from Sugimoto does not show that Amgen believed Sugimoto’s experiments to be successful, but instead that it was trying to obtain the starting materials — if indeed they were obtainable — so that it could attempt to verify that which Sugimoto claims. Lastly, Amgen told the PTO that Sugimoto did not suggest or teach recombinant procedures involving cloning the EPO gene. 10/3/86 Amendment, Ex. 2001, at 250. This last argument therefore fails.
. The Federal Circuit has stressed the importance of this showing:
[V]irtually all [inventions] are combinations of old elements.... Therefore, an examiner may often find eveiy element of a claimed invention in the prior art. If identification of each claimed element in the prior art were sufficient to negate patentability, very few patents would ever issue.... To counter this potential weakness in the obviousness construct, the suggestion to combine requirement stands as a critical safeguard against hindsight analysis and rote application of the legal test for obviousness.
Rouffet,
. HMR/TKT contends and Amgen does not dispute that in this action, "a person of ordinarily skill in the art of the patents-in-suit in 1983-84 would have been a scientist with a Ph.D. or M.D. in the biological, biochemical or medical sciences, working in research at *318 ■ the time and having at least two years of postdoctoral research experience in protein production, glycoslyation, and purification, and in the preparation and clinical evaluation of protein-based pharmaceutical compositions for use in human therapy.” HMR/TKT's Proposed Conclusions of Law ¶ 80; Amgen's Responsive Conclusions of Law (accepting by not refuting this assertion); see also Kingston Test., R. Trial Tr. at 128: 12-14 (agreeing that one skilled in the filed of molecular and cell biology "would be somebody who has a PhD and roughly two years of experience working in the area”).
. Although both parties agree that the Federal Circuit in
Amgen II
stated that a reference need not be enabling to be considered prior art when analyzing obviousness, they disagree as to the extent that a non-enabled prior art may be considered. Amgen argues that it is only that which the non-enabled art actually teaches that can be considered.
See, e.g.,
Amgen’s Reply to HMR/TKT's Proposed Findings of Fact ¶¶ 215, 216 (arguing that "to render obvious the asserted prior art must enable ordinarily skilled artisans to make and use the claimed invention” and citing
Beckman Instruments,
A review of the case law does not provide a definitive answer but indicates that although a reference need not be enabled to be prior art, the reference when combined with other references or common knowledge of ordinarily skilled artisans at the time of the obviousness inquiry should enable the claimed invention, that is, place it in possession of the public. "If not, every otherwise anticipating reference that is proved to be non-enabling would automatically render the claim obvious, despite not teaching ordinarily skilled artisans how to make and use the invention.” Amgen's Reply to HMR/TKT's Proposed Findings of Fact ¶216. Arguably, if the non-enabled reference can be combined with other references or knowledge of those skilled in the art such that the combination teaches how to make and use the now claimed invention then it should render the claim obvious. In other words, if by the time the claimed invention is patented, the skill in the art or other references that have been suggested have filled in the missing blanks from the non-enabled reference, then the claimed invention should be rendered obvious. On 'the other hand, if the missing blanks are still missing (or the non-enabled reference does not suggest the right combination of other references) then the non-enabled reference should not be able to render the claimed invention obvious. In sum, although a prior art refer *319 ence need not be enabled to render a claimed invention obvious, enablement is not wholly irrelevant. As discussed above, here, the missing blanks were still missing when Am-gen filed its patents, and HMR/TKT has not shown a reasonable expectation of success on the part of skilled artisans.
. This Court interpreted "purified from mammalian cells grown in culture” to mean purified to substantial homogeneity. '
Amgen I,
. See discussion supra regarding Figure 6 and obviousness of the '080 and '422 patents.
. HMR/TKT argues that the "non-human” or "other than human” limitations of the asserted patent claims cannot save them from invalidation, because they are source or process limitations. HMR/TKT's Opening Br. After Trial at 42. As HMR/TKT admits, however, there are other "missing elements” from Sugimoto's patent, like transcription control sequences, the amino acid sequence found in Figure 6, amplified marker DNA, the DHFR gene, and operative linkage to the EPO gene. These differences, as will be discussed further below, are determinative notwithstanding the "non-human” or "other than human” limitations. Therefore, the Court declines to address this argument as it relates to these patents. That being said, it is not altogether clear that source or process limitations are irrelevant when considering process claims, as opposed to product claims.
See, e.g., In re Luck,
, Indeed, the only experimental evidence on record attempting to do what Dr. Kingston described by way of Sugimoto and the prior art failed. As HMR/TKT put it in its 5/10/00 trial brief, "Amgen's Dr. Browne failed completely when he attempted to transfect cells with viral promoters to increase their production of EPO.” Amgen's App. to Mot. for Judgment re '349, Tab E (HMR/TKT’s 5/10/00 Trial Br.), at 22.
. Importantly, the Weis et al. article, discussed above, studied a gene that had already been cloned, and therefore the researchers were able to confirm the structure of the mouse DNA that had been inserted into hamster cells, using Southern blotting techniques. Weis et al., supra, Ex. 2477, at 4881-82, Fig. 3.
. This reasoning also applies to claims 5, 7, 8, and 9, as they are dependant on the other claims.
Cf. Fine,
. HMR/TKT argues as it did with the '080 and '422 patents that the cloning and isolation of EPO is the subject of Lin's original '008 patent, and thus cannot save the patents in issue here. In other words, HMR/ TKT argues that because Amgen first reported os discovery of the genetic sequence of EPO in the '008 patent, reference to the genetic sequence can simply be ignored in the obviousness inquiry concerning all other patents. The Court disagrees. First, HMR/TKT offers no legal support for this contention. Second, the genetic sequence of EPO is at the heart of these patents. Simply because the sequence specifically is not a novel addition as compared to Amgen's other patents does not render it obvious in light of Sugimoto's patent.
.HMR/TKT does not contend that Gold-wasser anticipates the asserted claims of the '080, ’349, or '698 patents or renders obvious any of the asserted claims of the '698 or '349 patents. See, e.g., HMR/TKT’s Opening Br. After Trial [Doc. No. 808] at i.-iii.
. Dr. Goldwasser's work does not pertain to cells that have been altered by recombinant means.
Amgen I,
. The history of patents that are no longer at issue is not included below. For that information, see
Amgen I,
. As the Court has discussed above, this procedure promotes comity and collegiality among the Federal Circuit and the district courts.
. HMR/TKT does not contend that Gold-wasser anticipates the asserted claims of the '080, ’349, and '698 patents or renders obvious any of the asserted claims of the '698 or '349 patents. See, e.g., HMR/TKT’s Opening Br. After Trial at i.-iii.
. Amgen also argues that Goldwasser does not disclose the limitation "purified from mammalian cells grown in culture.” HMR/ TKT argues that this is a source or process limitation that the Federal Circuit specifically pointed out could not save claim 1 from invalidation in an anticipation analysis. The Court need not address the issue since, as will be shown below, the evidence shows that Gold-wasser did not disclose EPO that is "therapeutically effective.”
.HMR/TKT did not argue specifically that an increase in erythroid cells in the marrow signifies a therapeutic response. HMR/TKT's Proposed Findings of Fact at 6-14 (contending that reticulocytes, ferokinetics and erythrocyte mass change (i.e., red cell mass change) are measures of therapeutic efficacy). Presumably, this is because erythroid marrow stimulation means the marrow is stimulated to raise the reticulocytes. Schumacher Test., R. Trial Tr. at 17-25. Therefore, any argument about erythroid cells in the marrow would necessarily be included in an argument about reticulocytes.
. The Court also notes that HMR/TKT produced no evidence that heart attack or stroke were risks associated with the diseases listed in the specification or that a reduction in the risk of stroke or heart attacks helps to heal or cure the diseased states listed in the specification.
. This is consistent with the Court's findings in
Amgen I,
that "[b]y increasing and maintaining the patient's hematocrit to normal or near normal levels, the ability of the patient’s blood to provide a steady supply of sufficient oxygen to body tissues can be restored.”
. Dr. Eschbach illustrated his point with an analogy to a bathtub. Eschbach Test., R. Trial Tr. at 662-64. The Court borrows the analogy to provide background here. Consider a bathtub: the water is the level of hemato-crit, the spigot spits out reticulocytes (the early red blood cells), and the drain is the cell destruction or loss. Hematocrit is measured by the amount of red cells produced and by the number of red cells destroyed. In a patient suffering from renal failure, many times the hematocrit drops because red cell destruction exceeds the rate at which red cells are being produced. When EPO stimulation is started, it is as if the spigot has been turned on, increasing the amount of reticulocytes flowing into the tub. Eventually, the tub may start to fill, but there is no guarantee that it will, because the drain is not completely *329 plugged. Iron deficiency, infection, inflammation, or blood loss could prevent the reti-culocytes from maturing or could destroy red blood cells. Therefore, simply measuring what is coming out of the spigot and not taking into account what is going down the drain is not sufficient.
. Hematocrit is the ratio of the red-cell mass to the total blood volume.
. For an explanatory depiction, see Ohls' Demonstrative Ex. 4.
. Indeed, in the cited studies regarding anemia of prematurity, hematocrit was always measured. Darlene A. Calhoun et al., Consistent Approaches to Procedures and Practices in Neonatal Hematology, 27 Clinics in Perinatology 733 (2000), Ex. 252, at 734-35 (basing decision to use transfusions solely on hematocrit); Robin K. Ohls et al., Effects of Early Erythropoietin Therapy on the Transfusion Requirements of Preterm Infants Below 1250 Grams Birth Weight: A Multicenter, Randomized, Controlled Trial, 108 Pediatrics 934 (2001), Ex. 253, at 934 (abstract) (measuring hematocrit and concluding that EPO should not be used in infants under 1250 grams birth weight, because it did not prevent use of transfusions); Robin K. Ohls & Robert D. Christensen, Recombinant Erythropoietin Compared with Erythrocyte Transfusion in the Treatment of Anemia of Prematurity, 119 J. Pediatrics 781 (1991), Ex. 2507, at 781 (measuring hematocrit and concluding that EPO offers promise as an alternative to transfusion in neonates with anemia of prematurity).
. Both Dr. Christensen and Dr. Ohls agreed that the goal of using EPO in infants with anemia prematurity is to avoid transfusions. Ohls Test., R. Trial Tr. at 1027: 7-10; Christensen Test., R. Trial Tr. at 1200: 7-21.
. When red blood cells are produced, iron in the blood plasma clears into the bone marrow. Schumacher Test., R. Trial Tr. at 805. The rate of clearance of iron from the plasma is known as the plasma iron clearance rate. Id.; Eschbach Test., R. Trial Tr. at 693: 4-11. For further explanation, see Eschbach Test., R. Trial Tr. at 689-91.
. HMR/TKT has made other arguments in support of its contention, most of which center on the literature. The Court, however, has not found any of these arguments persuasive, given Amgen’s more than adequate counter-arguments. See, e.g., HMR/TKT's Proposed Findings of Fact ¶¶ 52-60; Amgen’s Response to HMR/TKT's Proposed Findings of Fact ¶¶ 24-29.
. This is consistent with the Court's finding in
Amgen I
that “actual production of mature red blood cells was not achieved.”
Amgen I,
. HMR/TKT argues that Dr. Baron did not extend the duration long enough, since he only administered the medicine for three weeks. See, e.g., Schmumacher Test., R. Trial Tr. at 894: 13-15. It points to Dr. Baron's letter to the FDA, which stated that "one ■ needs to give larger doses than initially anticipated and for more prolonged periods of time to achieve the substantial and lasting stimulation of red cell production.” 7/7/80 Baron Letter to FDA, Ex.2056, at A 193007. It also points to testimony by Drs. Schumacher and Esehbaeh and to Amgen’s product literature, which claim that a rise in hematocrit usually occurs within two to six weeks. Schumacher Test., R. Trial Tr. at 894: 12-16; Esehbaeh Test., R. Trial Tr. at 725: 12-21; Physicians’ Desk Reference (56th ed.2002), Ex. 2497, at 582. Notwithstanding this, Dr. Esehbaeh testified that an effective EPO therapy would have produced immediate and dramatic increases in hematocrit. Esehbaeh Test., R. Trial Tr. at 679: 8-680: 14. Further, even if the Court agreed with HMR/TKT on this specific issue, as discussed above, the evidence simply does not show that an increased dosage would necessarily have lead to therapeutic effectiveness. Here, the red cell mass of the patient that received the altered protocol actually decreased.
. HMR/TKT tries to soften the impact of this testimony by arguing that Goldwasser was hired as a consultant by Amgen in 1981. The study, however, was not discontinued un *334 til 1988. IND Application for EPO, Ex. 2489, at HMR 935313. Therefore, HMR/TKT has not shown a causal link between the consultancy and the discontinuation.
. For the significance of this difference, see the discussion of whether Sugimoto renders these claims obviousness.
. With respect to "purified from mammalian cells grown in culture” and "not isolated from human urine,” the Federal Circuit made clear that a finding of non-obviousness cannot be rendered solely on source or process limitations.
Amgen II,
. Indeed, there is evidence suggesting that it would not have been possible to give increased amounts of the Goldwasser EPO to patients. In a letter to the FDA, Goldwasser made clear that the supply was limited and that preparing more was a painstaking task. 7/7/80 Baron Letter to FDA, Ex.2056, at A 193007; see also S/n/19 Application for Continuation Grant, Ex. 250, at A 196293 (explaining that the supply of EPO is small and the study was contingent on obtaining more); IND Application for EPO, Ex. 2489, at HMR 935313 (requesting in 1988 that the IND be put on inactive status, as the researchers "do not have sufficient supplies of the drug available to carry on anticipated studies at this time and for the immediate foreseeable future”).