Ex Parte 5882856 et al

Patent Trial and Appeal BoardApr 28, 2016

90012837 (P.T.A.B. Apr. 28, 2016)

UNITED STA TES p A TENT AND TRADEMARK OFFICE APPLICATION NO. FILING DATE 90/012,837 04/12/2013 10769 7590 04/28/2016 Laboratory Corporation of America Holdings c/o Kilpatrick Townsend & Stockton LLP 1001 West Fourth Street Winston-Salem, NC 27101 FIRST NAMED INVENTOR 5882856 UNITED STATES DEPARTMENT OF COMMERCE United States Patent and Trademark Office Address: COMMISSIONER FOR PATENTS P.O. Box 1450 Alexandria, Virginia 22313-1450 www .uspto.gov ATTORNEY DOCKET NO. CONFIRMATION NO. LT00793 REX 2950 EXAMINER TURNER, SHARON L ART UNIT PAPER NUMBER 3991 MAILDATE DELIVERY MODE 04/28/2016 PAPER Please find below and/or attached an Office communication concerning this application or proceeding. The time period for reply, if any, is set in the attached communication. PTOL-90A (Rev. 04/07) UNITED STATES PATENT AND TRADEMARK OFFICE BEFORE THE PATENT TRIAL AND APPEAL BOARD ESOTERIX GENETIC LABORATORIES, LLC Patent Owner and Appellant Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 Technology Center 3900 Before RICHARD M. LEBOVITZ, JEFFREY N. FREDMAN, and JEFFREY B. ROBERTSON, Administrative Patent Judges. LEBOVITZ, Administrative Patent Judge. DECISION ON APPEAL Patent Owner, Esoterix Genetic Laboratories, LLC, 1 appeals from the Patent Examiner's final rejection of claims 1, 3, 4, 14--16, and 18 in the above-identified ex partes reexamination proceeding of 5,882,856. The Board's jurisdiction for this appeal is under 35 U.S.C. Â§Â§ 6(b ), 134(b ), and 306. We affirm-in-part and set forth a new ground of rejection under 37 C.F.R. Â§ 41.50(b). 1 Reel/Frame 25656-581. Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 I. STATEMENT OF CASE This appeal involves U.S. 5,882,856 ("the '856 patent") which issued March 16, 1999. A Request for Ex parte Reexamination under 35 U.S.C. Â§Â§ 301-307 and 37 C.F.R. Â§ 1.510 was filed on behalf of Life Technologies Corporation ("Requester") on April 12, 2013. Reexamination of the '856 patent was subsequently ordered and culminated in a Final Rejection ("Final Rej'n" mailed Aug. 25, 2014). Patent Owner appeals from the Final Rejection. An oral hearing in the appeal was held March 23, 2016. A transcript will be entered into the record in due course. A related appeal (Appeal No. 2015-007789) is pending before the Board and has been decided concurrently to this one. The related appeal is of U.S. Reexamination Control No. 90/012,838, which relates to U.S. Patent No, 6,207 ,372 ("the '372 patent"). The '372 patent is a continuation-in-part of the application that issued as the '856 patent. Claims 1, 3, 4, 14--16, and 18 stand finally rejected by the Examiner under 35 U.S.C. Â§ 102(e) (pre-AIA) as anticipated by Jeffreys (U.S. Pat. No. 5,811,235, issued Sept. 22, 1998). Final Rej'n 4. Independent claims 1 and 14 are reproduced below (brackets show deletions from original claim): 1. A multiplicity of single-stranded oligonucleotide DNA primers for simultaneous amplification of multiple target DNA sequences under a single set of reaction conditions in a single multiplex polymerase chain reaction (PCR), said primers having a 5'X domain and a 3'Y domain, wherein; a) each said 5'X domain comprises a common sequence that does not hybridize to and has no homology with any one of said multiple target DNA sequences or its complement, 2 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 whereby the synthesis of spurious amplification products are prevented; b) the melting temperature of a hybrid between X and its complement in the absence of other sequences is greater than about 60Â°C; c) each said 3 'Y domain comprises a unique sequence contained within or flanking one of said multiple target DNA sequences or its complement whereby the synthesis of spurious amplification products are prevented; and d) the melting temperature of a hybrid between at least one of said 3 '-Y domains and its complement, in the absence of other sequences, is different from the melting temperature of a hybrid between at least one other 3 '-Y domain and its complement present in said multiplex PCR; and e) each of said primers [being capable of] annealing specifically with it [sic?] cognate target sequence under uniform high stringency annealing conditions during said amplification. 14. A method of screening to simultaneously detect amplification products of multiple target DNA sequences in DNA sample(s), said method comprising the steps of: a) contacting said DNA sample(s) with a multiplicity of single-stranded oligonucleotide DNA primer pairs having a 5'X domain, and a 3 'Y domain, under single multiplex polymerase chain reaction conditions wherein coamplification of said multiple target DNA sequences occurs in one or more cycles of identical melting, annealing and extending temperatures and times, wherein each said X domain comprises a common sequence that is neither complementary to nor specific for said multiple target DNA sequences, whereby the synthesis of spurious amplification products are prevented; and each said Y domain comprises a unique sequence, wherein said unique sequence is complementary to and specific for one of said multiple target DNA sequences suspected to be present in said DNA sample(s), whereby the synthesis of spurious amplification products are prevented; and b) detecting said amplification products. 3 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 CLAIM INTERPRETATION Claim 1 Claim 1 is a composition of matter directed to a "multiplicity of single-stranded oligonucleotide DNA primers." The claim preamble recites that the single-stranded primers are "for simultaneous amplification of multiple target DNA sequences under a single set of reaction conditions in a single multiplex polymerase chain reaction (PCR)." The primers have 1) 5'X and 3 'Y domains and 2) the characteristics recited in limitations a) through e ). One of the key issues is this appeal is how the preamble and limitations a) through d) limit the scope of the claim. We begin with the legal principles. The "terms appearing in a [claim] preamble may be deemed limitations of a claim when they 'give meaning to the claim and properly define the invention."' In re Paulsen, 30 F.3d 1475, 1479 (Fed. Cir. 1994). "Conversely, where a patentee defines a structurally complete invention in the claim body and uses the preamble only to state a purpose or intended use for the invention, the preamble is not a claim limitation." Rowe v. Dror, 112 F.3d 473, 478 (Fed. Cir. 1997). In Rowe v. Dror, a claim to a "'balloon angioplasty catheter"' was interpreted in view of the application specification to mean a catheter that could be "inflated radially outward to dilate a narrowed region in a blood vessel," distinguishing it from the more general class of balloon catheters. Id. at 4 79--80. The phrase "'balloon angioplasty catheter"' breathed "life, meaning, and vitality" into the claim because it enabled the catheter to be used in the context of an angioplasty procedure. See Bell Comm. Res., v. Vitalink Com., 55 F.3d 615, 620 (Fed. Cir. 1995). 4 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 The intended use of the primers is for multiplex PCR "under a single set of reaction conditions," but the claim is not a method claim and does not require that multiplex PCR be carried out. For this reason, we construe the claim preamble to only impose the requirement that the primer structure be capable of being utilized in a multiplex PCR process. Limitations a) through e) recite additional characteristics of the primers. Limitation b) specifies that the melting temperature between X and its complement is greater than about 60Â°C. Limitation e) recites that each of the primers is "annealing specifically with it cognate target sequence under uniform high stringency annealing conditions during said amplification." Both requirements are functional limitations in that they define the structure of the primer by a function, i.e., the primer's function to melt and anneal at the recited conditions. See In re Schreiber, 128 F.3d 1473, 1478 (Fed. Cir. 1997) ("[a] patent applicant is free to recite features of an apparatus either structurally or functionally.") To satisfy these claim limitations, it has to be shown that primers possess the claimed functionality. However, because the claim is a composition, and not a method, it is not necessary that the primers were actually utilized in the prior art at the recited melting and annealing conditions. There are two phrases in the claim whose interpretation is in dispute: "multiplex" and "high stringency annealing conditions." During reexamination of an unexpired patent, the PTO must give claims their broadest reasonable construction consistent with the specification. In re Am. Acad. of Sci. Tech Ctr., 367 F.3d 1359, 1364 (Fed. Cir. 2004); In re Suitco 5 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 Surface, Inc., 603 F.3d 1255, 1259 (Fed. Cir. 2010); In re Abbott Diabetes Care Inc., 696 F.3d 1142, 1148 (Fed. Cir. 2012). Patent Owner contends that "a multiplex" PCR reaction as recited in the claim means the presence of three or more pairs of single-stranded primers, each pair targeting a different nucleic acid sequence. Appeal Br. 9- 10. We first look to the '856 patent to determine whether the words in the claim are defined. The '856 patent defines "'Multiplex PCR"' as a reference "to the simultaneous amplification of multiple DNA targets in a single polymerase chain reaction (PCR) mixture." '856 patent, col. 3, 11. 57-59. The ordinary meaning of "multiple" as defined in general purpose dictionary is "1: consisting of, including, or involving more than one ."2 Thus, by its ordinary definition, "multiplex" means more than one. The '856 patent describes problems with "employing more than a single pair of oligonucleotide primers" in a standard PCR reaction. '856 patent, col. 4, 11. 8-18. The patent states at the end of this description that "[ c ]learly, these problems are magnified when it is desired to use multiple primer pairs (>3-4) in a single reaction." Id. at col. 4, 11. 18-20. This statement indicates that more than three (">3") is at least an example of "multiple," and if read narrowly to define "multiple" as more than three (i.e., multiple is another word for "> 3 "), would be inconsistent with Patent Owner's position that "multiple" means three or more(= 3) and the examples in the '856 patent. Appeal Br. 10. 2 http://www.merriam-webster.com/dictionary/multiple 6 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 To support their position that "multiplex" means more than 2 (i.e., >2), Patent Owner cites the declaration of Anthony P. Shuber, 3 the sole inventor of the '372 patent, who states that it is his "belief that one of skill in the art would not consider the term multiplex to be a biplex assay, i.e., attempted amplification of two targets." Shuber Deel., p. 2. However, Mr. Shuber did not provide a factual basis for this opinion. Mr. Shuber's statement can also be seen to be inconsistent with the '856 patent which defines "multiplex" as meaning "multiple" targets, a term whose ordinary mean is more than one. Patent Owner also cites the Jeffreys patent which refers to "duplex or multiplex reactions" as if distinguishing between two (duplex) and more than two (multiplex). Jeffreys, col. 13, 1. 34; col. 55, 11. 1-2. However, the term "multiplex" as used in the '856 patent claims is interpreted in view of the written description of the '856 patent, which does not necessarily use the term in the same way as in the Jeffreys patent. Moreover, Jeffreys also describes the "use of ARMS [Amplification Refractory Mutation System] to detect more than one suspected variant nucleotide in the same sample is conveniently referred to as multiplex ARMS." Id. at col. 14, 11. 5-7 (emphasis added). Thus, Jeffreys could also be read as consistent with the interpretation of multiplex as more than one. In sum, the preponderance of the evidence does not support Patent Owner's position that "multiplex" as utilized in the '856 patent means only 3 3 Declaration of Anthony P. Shuber, dated April 24, 2014. 7 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 or more, absent an express definition in the patent's written description or persuasive fact-based testimony of such meaning. The proper interpretation of the phrase "high stringency annealing conditions" is also disputed. Patent Owner contends that such conditions require an annealing temperature of 60Â°C, and would not include a temperature as low as 54Â°C. Appeal Br. 13-14. Patent Owner's support for this interpretation is that the '856 patent "disclose[s] testing of a range from 50-65Â°C (column 6, lines 52-55) in single amplifications and subsequent use of the optimized temperature 60Â°C in further multiplex reactions (column 7, lines 23-27)." Id. at 13. Patent Owner also relied on testimony by inventor Shuber that it is his "belief ... based upon reading the '856 and '372 patents, one of skill in the art would consider high stringency annealing conditions to be greater than 54Â°C, e.g., about 60Â°C." Shuber Deel., p. 2. The '856 patent does not provide a definition of "high stringency annealing conditions." The '856 patent discloses that "the annealing temperatures and primer concentrations may be calculated to some degree, conditions generally have to be empirically determined for each multiplex reaction." '856 patent, col. 1, 11. 54--56. The patent also discloses: each primer pair is evaluated independently to confirm that all primer pairs to be included in a single multiplex PCR reaction require the same amplification conditions (i.e., temperature, duration of annealing and extension steps). It was found (see example below) that all chimeric primers containing the M13 derived UPS as the 5' half of their sequence could be used at a broad range of annealing temperatures (i.e., 50Â°---60Â° C.). Id. at col. 5, 11. 53---60. The SS# 1 and SS#3 primers, for example, were noticeably inefficient at annealing temperatures above 60Â° C. The primer 8 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 pair designated SS#3-UPS, which corresponds to the SS#3 primers having the M13 UPS sequence on their 5' termini, was highly efficient in priming at all temperatures tested; furthermore, few spurious amplification products were detected in reactions containing SS#3-UPS primers. By contrast, SS#2 primers gave spurious amplification products at all three temperatures below 65Â° C [50Â°, 55Â°, and 60Â°]. Id. at col. 7, 11. 5-13. First, none of these disclosures characterize the annealing temperatures at "high stringency annealing conditions" as recited in the claims. Second, the temperature range, including the temperature of 60Â°C, is for UPS-tagged primers, which are specific universal primer sequences. Id. at col. 4, 1. 46-48. The claims, however, are not limited to the sequences. Further, the '856 patent specifically teaches that not all primers worked at 60Â°C (see above at col. 7, 11. 5-13, primer SS#2), inconsistent with Patent Owner's contention that 60Â°C is optimal and "high stringency annealing conditions." One of ordinary skill reading the '856 patent would not have discerned that 60Â°C constituted "high stringency annealing conditions" because a temperature range is disclosed and not all primers even worked in this range. Mr. Shuber's statements about the high-stringency temperature are not supported by evidence nor does he explain why "one of skill in the art would consider high stringency annealing conditions to be greater than 54Â°C, e.g., about 60Â°C." Shuber Deel., p. 2. On the other hand, another scientist with 14 years of research and development in the area of PCR assays testified that 9 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 an annealing step of 54 Â°C constitutes "'uniform high stringency annealing conditions."' Broomer Deel. 4 i-f 10. In sum, we do not find any persuasive factual support for limiting high stringency conditions to above 54 Â°C or 60Â°C. Claim 1 also recites that "spurious amplification products are prevented" when the multiplex PCR is carried out. We interpret "spurious" products to be "false-negative" products "which may be caused by annealing of the primers to sequences which are related to, but distinct from, the true recognition sequences." '856 patent, col. 1, 11. 46-50. Claim 14 Claim 14 is drawn to a "method of screening to simultaneously detect amplification products of multiple target DNA sequences in DNA sample( s ). The method comprises utilizing primer pairs with 5 'X and 3 'Y domains "under single multiplex polymerase chain reaction conditions." We construe the term "multiplex" as we did for claim 1. The X and Y domains are the same as they are in claim 1, i.e., to a common sequence "that is neither complementary to nor specific for said multiple target DNA sequences" and a unique sequence "complementary to and specific for one of said multiple target DNA sequences suspected." All of the primers in the screening method are required to have both domains. Claim 14 further requires that "spurious amplification products are prevented" when primer pairs are utilized to produce amplification products. 4 Declaration of Adam Broomer, dated April 11, 2013. 10 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 Because claim 14 is a method claim, the claim requires the primers pairs to have been utilized in such a way that spurious amplification is prevented. ANTICIPATION BY JEFFREYS A. Claims 1, 3, and 4 The Examiner found that Example 15, col. 35, 1. 45 to col. 36, 1. 30, of Jeffreys anticipates claim 1. Final Rej 'n 4--5. The example utilizes two pairs of tagged gene-specific primers, one pair to the normal CFTR gene and the second pair to a mutant APC gene sequence. Jeffreys, col. 35, 1. 45 to col. 36, 1. 30. Each of the primers has a TAG sequence. The Examiner found that the CFTR and APC sequences meet the limitation of the "3 'Y domain," where "c) said 3 'Y domain comprises a unique sequence contained within or flanking one of said multiple target DNA sequences or its complement." Final Rej'n 4--6. The Examiner found that the TAG sequence meets the limitation of "a) each said 5' X domain comprises a common sequence that does not hybridize to and has no homology with any one of said multiple target DNA sequences or its complement." Id. Consequently, each of the primers has "a 5'X domain and a 3 'Y domain" as required by the claim. For limitation "b) the melting temperature of a hybrid between X and its complement in the absence of other sequences is greater than about 60Â° C," the Examiner calculated the TAG's melting temperature and determined it to be above 60Â°C (72Â°C and 66.1Â°C, depending on the formula utilized). Id. at 6. 11 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 The claim also requires that "spurious amplification products are prevented" when the multiple primer pairs are used "for simultaneous amplification of multiple target DNA sequences under a single set of reaction conditions in a single multiplex polymerase chain reaction (PCR)." Limitation ( e) requires "each of said primers [being capable of] annealing specifically with it cognate target sequence under uniform high stringency annealing conditions during said amplification." Example 15 of Jeffreys does not disclose a temperature at which annealing is accomplished. The Examiner found the declaration by Adam Broomer reproduced Jeffreys's multiplex PCR and demonstrated that specific amplification products occurred under a single set of art standard high stringency annealing conditions. Final Rej 'n. 6. The PCR assay carried out by Mr. Broomer performed annealing at 54 Â°C (Broomer Deel. i-f 1 O; Answer 10), which is within the effective PCR range mentioned in the '856 patent for multiplex PCR ('856 patent, col. 5, 11. 59--60; col. 7, 11. 2-3). Patent Owner contends that the Examiner erred in finding that Jeffreys anticipates claim 1. Specifically, Patent Owner contends that Jeffreys fails to disclose ( 1) a multiplicity of primers for multiplex PCR; and (2) primers that anneal specifically with their cognate target "under uniform high stringency annealing conditions." Appeal Br. 26. "multiplex" Patent Owner contends that Jeffreys does not anticipate the claim because it only describes two primer pairs, where one is for detecting a control sequence (CFTR) and the other is for detecting a target sequence 12 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 (APC). Appeal Br. 27. Patent Owner states that the primers are "designed, at best, for use in a biplex reaction." Id. Patent Owner also argues that Jeffreys needed to use a two-step method, because no PCR products would be detected in the first step. Id. at 28. According to Patent Owner, "detectable products are not observed after step 1 because it is a primer extension reaction and amplification is not carried out for a sufficient number of rounds to produce detectable products." Id. Based on the Declaration by Parker, 5 Patent Owner further argues that "when step 1 is carried out for a sufficient number of rounds of amplification, only the APC primer product is detectable given the high concentration of primers used." Id. To begin with, we have interpreted "multiplex" PCR to read on PCR assay utilizing two primer pairs, each to a target sequence. Since Jeffreys describes two primer pairs - one to the CFTR target gene and the other to the APC gene - we conclude that the claim limitation of"[ a] multiplicity of single-stranded oligonucleotide DNA primers for simultaneous amplification of multiple target DNA sequences under a single set of reaction conditions in a multiplex polymerase chain reaction (PCR)" is met. While one primer set is utilized as a "control," it still satisfies the claim because it comprises a "sequence contained within or flanking said target sequence," where the target is the CFTR gene. Patent Owner's argument that the first step of Jeffreys's two-step assay would not produce PCR product improperly focuses on Jeffreys' s 5 Declaration of Scott Parker, dated December 17, 2014. 13 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 method steps. Claim 1 is a composition of matter claim. As discussed already, the claim has several functional requirements, including: â€¢ "simultaneous amplification of multiple target DNA sequences under a single set of reaction conditions in a single multiplex polymerase chain reaction (PCR)" â€¢ "each of said primers annealing specifically with it [sic?] cognate target sequence under uniform high stringency annealing conditions during said amplification" Along with the initial Request for Reexamination, a declaration under 37 C.F.R. Â§ 1.132 by Adam Broomer was filed as evidence that Jeffreys's primers possess the recited functional properties. Request 17. Mr. Broomer, a staff scientist at Life Technologies - the Third Party Requester - performed a multiplex PCR reaction using the two primer pairs in Jeffreys's Example 15 directed to the CFTR and APC genes. Broomer Deel. i-f 6. Mr. Broomer used final concentrations of the CFTR and APC primers of 200 nM and 250 nM, respectively (id. at i-f 7), and genomic DNA for the CFTR gene and a synthetic gene fragment for the APC gene (id. at i-f 8). Mr. Broomer stated that he used standard PCR concentrations for the PCR reagents. Id. at i-f 9. The annealing step was carried out at 54 Â°C for thirty seconds, which Mr. Broomer stated were "'uniform high stringency annealing conditions"' based on his experience and disclosure in the patent. Id. at i-f 10. Mr. Broomer performed multiplex PCR with both primer pairs and template DNA. Gel electrophoresis was used to detect the PCR reaction products. Id. at i-f 11. Mr. Broomer described the presence of reaction products corresponding to the CFTR and APC genes. Id. at i-f 15. Mr. Broomer 14 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 concluded that "the PCR reactions with Jeffreys' primers . . . yielded PCR amplification products of the expected size(s) and were virtually free of any spurious products, and that each primer annealed specifically with its cognate target sequence under uniform stringency annealing conditions." Id. at i-f 16 (footnote omitted). The Examiner found that Mr. Broomer's experiment established that Jeffreys's primers meet the functional limitations of claim 1. Patent Owner argues that step 1 of Jeffreys's Example 15 does not produce detectable PCR product and therefore cannot anticipate the claim. This argument is not persuasive since Broomer's declaration shows that there are conventional PCR conditions in which the primers amplify "multiple target DNA sequences under a single set of reaction conditions" as required by claim 1. Claim 1 is not a method claim so it is not necessary that the primers be utilized in the same way and concentrations as they are in Example 15 as long as the primers have the properties recited in the claim, which Mr. Broomer established they do. See Appeal Br. 20 attempting to distinguish Broomer based on the differences in concentration between the Broomer experiment and Jeffreys' Example 15. To rebut Mr. Broomer's declaration, Patent Owner provided a declaration by their own technical expert, Scott Parker ("Parker Deel."). Mr. Parker performed PCR reactions using Jeffreys' s CFTR and APC primer pairs. Parker Deel. i-f 7. Two PCR reactions were carried out, at annealing temperatures of 60Â°C (Figs. 1 and 2) and 54Â°C (Fig. 3), respectively. Id. at i-fi-15---6. For the PCR reaction as 60Â°C (Figs. 1 and 2), the concentrations of primers were the same as those in Broomer's experiment; for the reaction at 15 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 54Â°C (Fig. 3), primer concentrations were those described in Jeffreys's Example 15. Id. at i-f 9. The PCR products for each reaction were analyzed by gel electrophoresis and fluorescent dye staining. Id. at i-f 11. Mr. Parker found that at an annealing temperature of 60Â°C, and using the primer concentrations in the Broomer experiment, CFTR control primers did not produce an amplification product and non-specific amplification was observed. Id. at i-f 13. At an annealing temperature of 54Â°C, and using the primer concentrations in Example 15 of Jeffreys, Mr. Parker found that the PCR reaction failed "to produce a detectable amplification product for CFTR and may result in non-specific amplification of the wild-type APC gene." Id. at i-f 14. Patent Owner contends that the Parker Declaration shows that the primer pairs of Jeffreys are distinguishable from the claimed primers (Appeal Br. 21-23) because simultaneous amplification of both primer pairs were not observed at either temperature and thus each of Jeffreys's primers are not "e) ... annealing specifically with it cognate target sequence under uniform high stringency annealing conditions during said amplification" as required by claim 1. Patent Owner concludes: The Parker Declaration demonstrates that the Jeffreys primers are structurally different from the primers of claim 1 because spurious amplification products and a lack of CFTR primer product are observed using the Jeffreys primers under high stringency annealing conditions. Furthermore, Parker used primer concentrations disclosed by Jeffreys whereas Broomer did not. The difference in outcome in the Parker experiments versus Broomer [experiments] in fact proves the very point the Appellants seek to make: the Jeffreys primers do not inherently have the characteristics of the claimed primers, even in a biplex PCR instead of a multiplex PCR. 16 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 Id. at 23. We do not agree that the weight of the evidence supports the conclusion that Jeffreys' s primers do not meet the properties of the claimed primers. The three experiments described in the declarations are summarized in the table below: Annealing CFTR APC temperature concentration concentration Broomer 54Â°C for 30 sec 200nM 250nM Parker (Fig 3) 54Â°C for 30 sec lOnM 1 ÂµM Parker (Figs 1 60Â°C for 30 sec 200nM 250nM and2) Broomer's experiment was said to show that Jeffreys's primers meet all the claimed limitations. Parker's experiments were said to show the primers do not have all the characteristics of the claimed primers. However, as the table shows, Parker did not reproduce Broomer's experiment since the primer concentrations at 54 Â°C were different. The data, taken together, show that different PCR conditions can produce different results. Nonetheless, Broomer's conditions show that Jeffreys's primers meet the claimed limitation of "simultaneous amplification of multiple target DNA sequences under a single set of reaction conditions in a single multiplex polymerase chain reaction (PCR)." Contrary to Patent Owner's contention (Appeal Br. 31 ), Mr. Broomer did not have to carry out the same primers concentrations as in step 1 of Example 15 because claim 1 does not require it. 17 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 "uniform high stringency annealing conditions" Patent Owner contends that 54 Â°C is not "uniform high stringency annealing conditions." We have already determined that Patent Owner did not provide adequate evidence to establish that 54Â°C is excluded from the scope of the claim. Consequently, the argument made by Mr. Shuber that the loss of signal at 54 Â°C in the Broomer experiments is evidence that specific annealing at 60Â°C would not occur is moot. Appeal Br. 21, 32. Patent Owner also argues that Jeffreys teaches that the primer pairs do not anneal at high stringency conditions. Jeffreys's primers contain a TAG sequence (the 5'X domain of claim 1 which does not hybridize to target sequences) and gene-specific sequence (the 3 'Y domain of claim 1 which contains the target sequences). Jeffreys describes a two-step process. In the Step 1, a "multiplex PCR reaction" containing the CFTR and APC primers is carried out. Jeffreys, col. 35, 11. 59---65. No temperatures are disclosed. In Step 2, the products of the PCR reaction are used to seed a second PCR reaction. Id. at col. 35, 11. 66---67. The reaction contains only the TAG primer-the 5 'X domain of claim 1. Jeffreys states: This second PCR reaction is performed at a high annealing temper[ a ]ture which prevents the action of any carried-over control PCR primers. The TAG primers, however, are able to efficiently amplify the control and ARMS PCR products at the elevated annealing temper[ a ]ture. Therefore, the presence of the somatic mutation will lead to the formation of an ARMS and a control PCR product after step 2 PCR whereas in its absence only the control PCR product will be detected. Id. at col. 36, 11. 4--10. 18 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 Patent Owner contends that Jeffreys's statements establish that "the control PCR primers are unable to work at a high annealing temperature." Appeal Br. 19. Jeffreys's example appears to be prophetic. There is no disclosure at what temperatures the PCR reactions is conducted. Jeffreys also does not disclose the "high annealing" temperature mentioned in the second PCR reaction. Mr. Broomer provides evidence that carrying out step 1 with both primer pairs at 54 Â°C in standard PCR conditions resulted in amplification of the CFTR and APC targets. While this temperature may not be the "high annealing" temperature contemplated by Jeffreys, we have not been directed to sufficient evidence that 54 Â°C is disqualified as a "high stringency annealing" temperature within the scope of the claim. Consequently, Jeffreys teaching has not been established to be inconsistent with Mr. Broomer' s experiment. 5 'X and 3 'Y domains Patent Owner contends that primers described in Jeffreys's Example 15 do not meet the requirements of the X and Y domains (Appeal Br. 34), but provides no substantive argument as to why the TAG sequence and CFTR and APC gene sequences in the table that spans columns 3 5-3 6 are deficient. For the foregoing reasons, we affirm the rejection of claim 1. The same arguments were made for Claims 3 and 4. These claims therefore fall with claim 1. 19 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 B. Claims 14--16 and 18 Claim 14 is a method claim. Claims 15 and 16 depend from it. Claim 14 requires detecting multiple amplification products, where the amplification products are produced "under single multiplex polymerase chain reaction conditions ... in one or more cycles of identical melting, annealing and extending temperatures and times," "whereby the synthesis of spurious amplification products are prevented." Example 15 of Jeffreys does not disclose the conditions at which the multiplex PCR was accomplished. Since the PCR conditions are unstated by Jeffreys, for anticipation to be established, it must be shown Example 15 "inherently," as an inseparable attribute of it, would result in the claimed requirement of detecting amplification products multiple target DNA sequences without spurious amplification products. "[A ]nticipation by inherent disclosure is appropriate only when the reference discloses prior art that must necessarily include the unstated limitation .... " Transclean Corp. v. Bridgewood Servs., Inc., 290 F.3d 1364, 1373 (Fed. Cir. 2002). "Inherency, however, may not be established by probabilities or possibilities. The mere fact that a certain thing may result from a given set of circumstances is not sufficient." Cont'! Can Co. USA, Inc. v. Monsanto Co., 948 F.2d 1264, 1269 (Fed. Cir. 1991). "Inherent anticipation requires that the missing descriptive material is 'necessarily present,' not merely probably or possibly present, in the prior art." Trintec Indus., Inc. v. Top- US.A. Corp., 295 F.3d 1292, 1295 (Fed. Cir. 2002). Mr. Broomer's experiment establishes PCR conditions which "simultaneously detect amplification products of multiple target DNA sequences." The experiments 20 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 carried out by Mr. Parker, however, show that not all PCR conditions result in the amplification of both target sequences without the synthesis of spurious amplification product. See supra at p. 17. Appeal Br. 37-38. Because not all PCR conditions meet the claim limitations, Jeffreys does not "necessarily" result in the claimed limitations. Consequently, we are compelled to reverse the anticipation rejection of claim 14, and claims 15 and 16 which depend from it. We also reverse the rejection of claim 18 for similar reasons. In reaching this decision, however, we do not agree with Patent Owner that Jeffreys fails to describe multiplex PCR using two pairs of primers to different target sequences, where the primers comprise X and Y domains as recited in claim 14. Our reasoning is the same as it is for claim 1, and therefore it is unnecessary to repeat here. In addition to this, Patent Owner contends Jeffreys doesn't anticipate since no amplification product is detected in step 1, but requires a further amplification step using primers to the TAG. Appeal Br. 36. We do not agree because the claim is open-ended and step "b) detecting said amplification products" does not require the amplification products of step "a)" to be detected. The claim does not exclude a second step corresponding to Jeffreys's step 2 in which amplification products are produced after step (a) and then detected in step (b). 21 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 NEW GROUND OF REJECTION Claim 14--16 While we agree with Patent Owner that Claim 14 is not anticipated by Jeffreys, there is sufficient evidence of record that the claimed subject matter would have been obvious to one of ordinary skill in the art. As discussed under the anticipation rejection, Jeffreys describes two different sets of primers, one to the CFTR gene and the other to the APC gene. Jeffreys, cols. 35-36 (table). The primers have X and Y domains which correspond to the recited common ("TAG") and unique (CFTR and APC) sequences, respectively. Patent Owner inconsistently argued that such domains were not present in Jeffreys's primers while admitting at the same time that the X domain primers could be used to amplify the products of Jeffreys's step 1. Appeal Br. 36. Because there is no evidentiary support or substantive arguments to support Patent Owner's contention, we find this argument to be without merit. Example 15 of Jeffreys describes two steps. In the first step, gene specific primers are utilized in a multiplex PCR reaction. Jeffreys, col. 35, 11. 59---65. In step 2, the "products of the PCR reaction (step 1 above) are used to seed the second PCR reaction." Id. at col. 35, 11. 66----67. The primer used in the second step is the TAG sequence, which corresponds to the claimed "common sequence" of the X domain. Id. at col. 36, 11. 1--4. "This second PCR reaction is performed at a high annealing temper[ a ]ture which prevents the action of any carried-over control PCR primers." Id. at col. 36, 11. 4--6. The PCR reaction products are detected in the second step. Id. at col. 36, 11. 5-15. 22 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 Step a) of claim 14 comprises contacting a DNA sample with multiple primer pairs and subjecting the sample to one or more PCR cycles. This step is met by step 1 of Jeffreys. Jeffreys, col. 35, 11. 59---65. Patent Owner attempts to distinguish claim 14 from Jeffreys by arguing that the detecting step b) of claim 14 ("detecting said amplification products") is performed on the PCR products of step a), while Jeffreys detects amplification products only after step 2) has been carried out using the TAG sequences. Appeal Br. 36-37. In other words, Patent Owner contends that Jeffreys describes an additional step which is excluded by the claim. This argument is not persuasive. Step b) of claim 14 recites "detecting said amplification products." The term "amplification products" appears in the claim preamble. However, step a) only refers to "spurious amplification products" whose detection is not desired. Thus, antecedent basis for the "amplification products" of step b) is in the claim preamble not in step a). Claim 14, therefore, does not require the amplification products of step a) to be detected in claim b ). Rather, the claim is open to detecting the amplification products of another step, such as step 2 of Jeffreys. Moreover, even if we read the claim as Patent Owner does, claim 14 would still have been obvious to one of ordinary skill in the art. Jeffreys describes using a "tail" sequence primer which does not hybridize to target region. The first time Jeffreys describes the "tail" primer it is in the context of detecting tandem repeats. Jeffreys, col. 3, 1. 50 to col. 4, 1. 14. Jeffreys explains that the tail primer overcomes a problem of progressively shortening amplification products. Id. Jeffreys teaches amplification with both tail and sequence specific primers in the same reaction: "The method 23 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 of the present invention is conveniently effected in a single reaction using the type specific and common primers in combination with the tail specific primer." Id. at col. 4, 11. 24--27. Jeffreys discloses that the principle of using tail primers "may be applied to any convenient detection method involving amplification by primer extension." Id. at col. 12, 11. 1-12. In extending this principle to detecting diagnostic mutations, Jeffreys describes the two step procedure of Example 15. Id. at col. 12, 11. 15-65 (the tail specific primer is referred to as the "TAG"). However, Jeffreys specifically teaches that a one-step process can be used, making it obvious to have collapsed steps 1 and 2 of Example 15 into a single step. Because step a) of claim 14 is open- ended, it can comprise additional primers, such as a tail-specific primer to the common sequence of the X domain. The reaction conditions, including annealing at 54 Â°C, under which no spurious amplification products are described by Mr. Broomer as conventional PCR conditions in the art. Innis provides evidentiary support. Innis teaches utilizing an annealing temperature of 55Â°C which is a "high- stringency annealing temperature." Innis 382 (PCR Protocols, edited by M.A. Innis et al., Academic Press, 1990). It would have been routine optimization to choose the specific PCR conditions necessary for detection of specific amplification products. Claim 15 depends on claim 14, and further recites that said "multiple target DNA sequences are located within different regions of a gene present in said DNA sample(s)." Jeffreys teaches primers specific to different mutations within different regions of the CFTR gene. Jeffreys, col. 35-38. 24 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 Claim 16 depends from claim 14 and further recites "wherein said multiple target DNA sequences are located within multiple genes present in said DNA sample(s)." Jeffreys teaches primers specific to different genes, i.e., the APC and CFTR genes. Id. at cols. 35-36:40-41. In sum, claims 14--16 are rejected under 35 U.S.C. Â§ 103(a) as obvious in view of Jeffreys and Innis. The declaration by Mr. Broomer is relied upon as evidence that standard PCR conditions as described in Innis would specifically amplify the CFTR and APC sequences without the synthesis of spurious amplification products. We designate this a new ground of rejection under 37 C.F.R. Â§ 41.50(b). Claim 18 Claim 18 is a product by process claim directed to a "multiplicity of amplified target DNA free of spurious amplification products." Step 1 carried out by Jeffreys would have the recited amplification products of claim 18 because the primers are the same as those recited in the claim as discussed in the rejection of claim 1. Where, as here, the claimed and prior art products are identical or substantially identical, or are produced by identical or substantially identical processes, the PTO can require an applicant to prove that the prior art products do not necessarily or inherently possess the characteristics of his claimed product. ... Whether the rejection is based on "inherency" under 35 U.S.C. Â§ 102, on "prima facie obviousness" under 35 U.S.C. Â§ 103, jointly or alternatively, the burden of proof is the same, and its fairness is evidenced by the PTO' s inability to manufacture products or to obtain and compare prior art products. 25 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 In re Best, 562 F.2d 1252, 1255 (CCPA 1977) (footnote omitted). Patent Owner's attempt to distinguish the products of claim 18 from Jeffreys and the Broomer declaration does not identify a single structural difference between what is claimed and what would be produced by Jeffreys's step 1 utilizing standard PCR conditions. Appeal Br. 40-42. Patent Owner's argument is unpersuasive because it focuses on the method steps, rather than the product which is claimed. It appears that all the inventors have recognized is that using Jeffreys's primers, without a second amplification step, achieves efficient amplification. '856 patent, col. 4, 11. 4-- 55. However, we designate this as a new ground of rejection because Jeffreys does not describe the amplification conditions. In sum, claim 18 is rejected under 35 U.S.C. Â§ 103(a) as obvious in view of Jeffreys and Innis. The declaration by Mr. Broomer is relied upon as evidence that standard PCR conditions as described in Innis would specifically amplify the CFTR and APC sequences without the synthesis of spurious amplification products. We designate this a new ground of rejection under 37 C.F.R. Â§ 41.50(b). NEW GROUND OF REJECTION This decision contains a new ground of rejection pursuant to 37 C.F.R. Â§ 41.50(b ). This section provides that "[a] new ground of rejection ... shall not be considered final for judicial review." Section 41.50(b) also provides that Appellant, WITHIN TWO MONTHS FROM THE DATE OF THE DECISION, must exercise one of the following two options with 26 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 respect to the new ground of rejection to avoid termination of the appeal as to the rejected claims: ( 1) Reopen prosecution. Submit an appropriate amendment of the claims so rejected or new evidence relating to the claims so rejected, or both, and have the matter reconsidered by the examiner, in which event the proceeding will be remanded to the examiner .... (2) Request rehearing. Request that the proceeding be reheard under Â§ 41.52 by the Board upon the same record .... Requests for extensions of time in this ex parte reexamination proceeding are governed by 37 C.F.R. Â§ 1.550(c). See 37 C.F.R. Â§ 41.50(f). AFFIRMED-IN-PART 37 C.F.R. Â§ 41.50(b) 27 Appeal2015-008320 Reexamination Control 90/012,837 U.S. Patent 5,882,856 PATENT OWNER: LABORATORY CORPORATION OF AMERICA HOLDINGS C/O KILPATRICK TOWNSEND & STOCKTON LLP 1001 West Fourth Street Winston-Salem, NC 27101 THIRD PARTY REQUESTER: LIFE TECHNOLOGIES CORPORATION ATTN: IP DEPARTMENT 5791 Van Allen Way Carlsbad, CA 92008 28