Ex Parte Saus et alDownload PDFPatent Trial and Appeal BoardMar 29, 201713400831 (P.T.A.B. Mar. 29, 2017) Copy Citation United States Patent and Trademark Office 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 APPLICATION NO. FILING DATE FIRST NAMED INVENTOR ATTORNEY DOCKET NO. CONFIRMATION NO. 13/400,831 02/21/2012 Juan Saus 11-365-US 1094 20306 7590 03/29/2017 MrnnNNFT T ROFFTNFN HT TT RFRT Rr RFRGROFF T T P EXAMINER 300 S. WACKER DRIVE HADDAD, MAHER M 3 2ND FLOOR CHICAGO, IL 60606 ART UNIT PAPER NUMBER 1644 MAIL DATE DELIVERY MODE 03/29/2017 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 Ex parte JUAN SAUS, FERNANDO REVERT, RAMON MERINO, JESUS MERINO, and FRANCISCO REVERT-ROS1 Appeal 2015-006665 Application 13/400,831 Technology Center 1600 Before RICHARD M. LEBOVITZ, JOHN G. NEW, and TIMOTHY G. MAJORS, Administrative Patent Judges. NEW, Administrative Patent Judge. DECISION ON APPEAL 1 Appellants state the real party-in-interest is FibroStatin S.L. App. Br. 3. Appeal 2015-006665 Application 13/400,831 SUMMARY Appellants file this appeal under 35 U.S.C. § 134(a) from the Examiner’s Non-Final Rejection of claims 4, 5 and 20—30 which stand rejected as unpatentable under 35 U.S.C. § 103(a) as being obvious over the combination of F. Revert et al., Increased Goodpasture Antigen-Binding Protein Expression Induces Type IV Collagen Disorganization and Deposit of Immunoglobulin A in Glomerular Basement Membrane, 171(5) Am. J. Pathol. 1419-30 (2007) (“Revert 2007”), F. Revert et al., Goodpasture Antigen-binding Protein Is a Soluble Exportable Protein That Interacts with Type IV Collagen: Identification of Novel Membrane-Bound Isoforms, 283(44) J. Biol. Chem. 30246-55 (2008) (“Revert 2008”), Saus et al. (US 2010/0021935 Al, January 28, 2010) (“Saus ’935”), and F. Bard et al., Peripherally Administered Antibodies against Amyloid B-Peptide Enter the Central Nervous System and Reduce Pathology in a Mouse Model of Alzheimer Disease, 6(5) Nature Medicine 916-19 (2000) (“Bard”).2 We have jurisdiction under 35 U.S.C. § 6(b). We AFFIRM. 2 The Examiner also rejected claims 4, 5 and 20—30 as unpatentable under 35 U.S.C. § 103(a) as being obvious over Saus ’935 and T. Miralem et al., Human Biliverdin Reductase Suppresses Goodpasture Antigen-binding Protein (GPBP) Kinase Activity: The Reductase Regulates Tumor Necrosis Factor-a-Nf-Kb-Dependent GPBP Expression, 285(17) J. BIOF. CHEM. 12551-58 (2010). Although Appellants argue this rejection in their Appeal Brief, the Examiner has withdrawn the rejection. See Non-Final Act. 11; Ans. 2. 2 Appeal 2015-006665 Application 13/400,831 NATURE OF THE CLAIMED INVENTION Appellants’ invention is directed to methods for the diagnosis and/or treatment of chronic kidney disease, immune complex-mediated glomeralamephritis (“IC-GN”), rheumatoid arthritis, and pulmonary fibrosis, and methods for identifying compounds for such therapeutic use. Abstract. GROUPING OF CLAIMS Appellants argue all claims together. Claim 4 is representative and recites: 4. A method for treating immune complex-mediated glomerulonephritis (GN), comprising administering to a subject in need thereof an amount effective of an antibody that binds to circulating 77 kD Goodpasture antigen binding protein (GPBP) to treat the immune complex-mediated GN. App. Br. 17. ISSUE AND ANALYSIS We agree with, and adopt, the Examiner’s findings of fact, reasoning, and conclusion that the claims would have been obvious over the cited prior art references. We address Appellants’ arguments below. 3 Appeal 2015-006665 Application 13/400,831 A. Rejection of the claims over Revert 2007, Revert 2008, Saus ’935, and Bard Issue Appellants argue the Examiner erred in finding the combined cited prior art references teach or suggest the limitations of claim 4 reciting: (1) “a method for treating immune complex-mediated glomerulonephritis (GN)”; (2) “administering to a subject... an antibody ... to treat the immune complex-mediated GN”; and (3) wherein the administered antibody “binds to circulating 77 kD Goodpasture antigen binding protein (GPBP).” App. Br. 6. Analysis Appellants argue the Examiner acknowledges that neither Revert 2007 nor Revert 2008 teaches or suggests any methods for treating immune complex-mediated GN (“IC-GN”), or any methods comprising administering antibodies of any kind to a subject, let alone antibodies that bind to circulating GPBP (“cGPBP”). App. Br. 6—7. Specifically, Appellants argue Revert 2007 neither teaches nor suggests methods of treating GN, nor does Revert 2007 disclose administration of antibodies to a subject, by which the antibodies bind circulating GPBP. Id. Rather, Appellants contend, the Examiner instead finds Revert 2007 teaches that “m vivo GPBP regulates type IV collagen organization and elevated expression of [ ] kinase induces immune complex-mediated glomerulonephritis.” Id. at 7 (quoting Non-Final Act. 3 (citing Revert 2007 1420)). Appellants argue that, similarly, the Examiner finds that Revert 2008 teaches “Goodpasture antigen-binding protein is a soluble exportable protein 4 Appeal 2015-006665 Application 13/400,831 that interacts with type IV collagen .... Revert et al teach that the 77-kDa GPBP is mainly found in the extracellular compartment both soluble (Fig. 5) or associated with glomerular basement membrane collagen.” Id. (quoting Non-Final Act. 3 (citing Revert 2008 30254). However, Appellants argue, Revert 2008 contains no teaching or suggestion regarding the treatment of IC-GN by administering anti-cGPBP antibodies, as recited in claim 4. Id. With respect to Saus ’935, Appellants contend the Examiner has mischaracterized the teachings of the reference. App. Br. 7. According to Appellants, Saus ’935 does not, in fact, teach that anti-GPBP antibodies would make useful therapeutics. Id. at 7—8. Appellants point to paragraph [0071] of Saus ’935, which recites: The polypeptides [91 kD GPBP and 77 kD GPBP] of this aspect of the invention can be used, for example, to produce antibodies against native GPBP forms, and as targets for identification of compounds that interfere with native GPBP activity, making them useful therapeutics for various disorders, including Goodpasture Syndrome. (emphases added by Appellants). Appellants contend that the pronoun “them,” when read in the context of the passage as a whole, refers back to “the polypeptides,” rather than to the “antibodies.” Id. at 8. Therefore, argue Appellants, Saus ’935 does not teach GPBP-binding antibodies that “mak[e] the antibodies useful therapeutics for various disorders,” as found by the Examiner. Id. Appellants next point to the Declaration of Dr. Juan Saus (the “Saus Declaration”), one of the co-inventors of the present application. App. Br. 8. Appellants point to paragraph 8 of the Saus Declaration as stating: The ’935 application teaches the existence of circulating GPBP (cGPBP) which is also referred to as circulating 77 kD GPBP, and 5 Appeal 2015-006665 Application 13/400,831 that cGPBP is a biomarker for diagnosing IC-GN. The ‘935 application does not disclose that cGPBP/77 kD GPBP, in addition to being a biomarker for the diagnosis of IC-GN, is also a therapeutic target for the treatment of IC-GN, as recited in the instant claims. Id. (emphasis added by Appellants). With respect to the teachings of Bard, Appellants contend Bard contains no teaching or suggestion of IC-GN, GPBP, or anti-GPBP antibodies. App. Br. 9. The Examiner responds that, first, Appellants are impermissibly attacking the references singly, when the Examiner relied upon the combined teachings and suggestions of the references. Ans. 6 (citing, e.g., In re Keller, 642 F.2d 413, 426 (C.C.P.A. 1981). The Examiner finds Appellants’ claimed invention differs from teachings and suggestions of Revert 2007 and Revert 2008 only in the recitation of a method for treating immune complex-mediated glomerulonephritis with administration of anti-cGPBP antibody. Non-Final Act. 4. Specifically, the Examiner finds Revert 2007 teaches that increased expression of GPBP, a protein that binds and phosphorylates basement membrane collagen in the renal glomerulus, has been associated with immune complex-mediated pathogenesis and that New Zealand White (“NZW”) mice develop age-dependent lupus-prone autoimmune response and IC-GM characterized by elevated GPBP, glomerular basement membrane (GBM) collagen disorganization and expansion and deposits of IgA on disrupted GBM. Non-Final Act. 2. The Examiner finds Revert 2007 provides in vivo evidence that GPBP regulates GBM collagen organization 6 Appeal 2015-006665 Application 13/400,831 and its elevated expression causes dissociation and subsequent accumulation of IgA on the GBM. Id. at 2—3. The Examiner also finds Revert 2007 teaches a previously unrecognized pathogenic mechanism that may be relevant in human primary immune complex-mediated glomerulonephritis. Id. at 3 (citing Revert 2007 Abstr., 1423 and 1426). The Examiner further finds Revert 2008 teaches GPBP is a soluble exportable protein that interacts with type IV collagen. Non-Final Act. 3. The Examiner finds cells express at least two GPBP isoforms resulting from canonical (77-kDa) and noncanonical (91-kDa) mRNA translation initiation: the 77-kDa polypeptide interacts with type IV collagen and localized as a soluble form in the extracellular compartment. Id. The Examiner also finds Revert 2008 teaches that the 77-kDa GPBP is mainly found in the extracellular compartment in soluble form or associated with glomerular basement membrane collagen. Id. at 4 (citing Revert 2008 30254). The Examiner also finds Revert 2008 teaches that various lines of evidence support that COL4A3BP (i.e., the gene which encodes GPBP) is an attractive target for strategies to treat antibody-mediated disorders which discriminate between different gene products (i.e., GPBP and GPBPA26/CERT), which are expressed at distinct cell compartments and are differentially regulated in response to stimuli. Id. at 3^4 (citing Revert 2008 30255). With respect to Saus ’935, the Examiner finds that, in paragraph [0071] of the reference quoted supra, the pronoun “them” refers to the antibodies and the compounds that interfere with native GPBP activities. Ans. 6—7. The Examiner points to paragraph [0003] of Saus ’935, which recites: “The identification of GPBP provided methods for identification of 7 Appeal 2015-006665 Application 13/400,831 compounds for the treatment of autoimmune disorders, cancer, protein misfolding-mediated disorders and aberrant apoptosis, and also provided potential therapeutics for these disorders.” Id. at 7. The Examiner also points to paragraph [0062] of Saus ’935, which recites: “The polypeptides of the invention can also be used, for example, as tools to identify candidate compounds for inhibiting various specific types of native GPBP isoforms and also to identify candidate compounds for treating, for example, autoimmunity and protein misfolding-mediated disorders, as discussed in more detail below.” Id. The Examiner also finds Saus ’935 teaches: “Various lines of evidence support that COL4A3BP is an attractive target for strategies to diagnose and treat antibody-mediated disorders.” Id. (citing Saus ’935 1 179). The Examiner also finds that Saus ’935 teaches: [B]y identifying circulating human 77-kDa GPBP, we provide compelling evidence that GPBP secretion is also biologically relevant in vivo. The finding that the levels of circulating 77-kDa GPBP correlate with GPBP glomerular expression and pathogenesis in mouse models of immune complex-mediated glomerulonephritis suggests that serological determination of GPBP is relevant in a clinical setting. Consistent with this, present studies demonstrating upregulation of circulating GPBP in Goodpasture patients support these conclusions and substantiate previous observations that GPBP is overexpressed in these patients. Ans. 9—10 (citing Saus ’935 1180). The Examiner consequently finds that a person of ordinary skill in the art would be motivated to target the circulating 77-kDa GPBP with an anti-77-kDa cGPBP antibody to combat IC-GN because the anti-cGPBP antibody suggested by Saus ’935 would 8 Appeal 2015-006665 Application 13/400,831 appear to be compatible with physiological use and is not incompatible with a therapeutic intention. Id. at 10. With respect to Appellants’ argument concerning the teachings of Bard, the Examiner finds Bard teaches: [TJransgenic overexpressing Ap (PDAPP mice) [sic] show many of the pathological features of Alzheimer disease, including extensive deposition of extracellular amyloid plaques, astrocytosis and neuritic dystrophy. Bard et al demonstrated that intraperitoneal administration of anti-Ap antibodies in transgenic mice overexpressing AB lead to brain Ap plaque clearance. Ans. 10 (quoting Non-Final Act. 5). The Examiner finds Bard thus teaches a “proof-of-concepf ’ for using antibodies against an elevated level of a specific protein in transgenic mice overexpressing that specific protein, which results in the development of, or predisposition to, various disease states, as an effective method to diminish the disease state. Ans. 11. Specifically, the Examiner finds Bard teaches a successful method of treatment of transgenic mice overexpressing a disease- linked protein by administering antibodies to that protein, and would lead a person of ordinary skill in the art made to combine the method taught by Bard with Revert 2007 and Revert 2008 to solve a similar problem with respect to IC-GN. Id. We are not persuaded by Appellants’ arguments. As an initial matter, we agree with the Examiner that Appellants “cannot show non-obviousness by attacking references individually where ... the rejections are based on combinations of references.” Keller, 642 F.2d 413. The gravamen of Appellants’ argument is that none of the references, Revert 2007, Revert 2008, and Saus ’935, teach the treatment of IC-GN by 9 Appeal 2015-006665 Application 13/400,831 administering anti-cGPBP antibodies, as recited in claim 4. App. Br. 7—9. Nevertheless, it is not disputed by Appellants that Revert 2007 and Revert 2008, as well as Saus ’935, teach that elevated levels of cGPBP are directly involved in the etiology of, and is a biomarker for, IC-GN. Id. With respect to whether, in paragraph [0071] of Saus ’935, the pronoun “them” refers to the GPBP polypeptides or antibodies directed against those polypeptides, we agree with Appellants that a plain reading of the passage reveals that “them” refers to the recited polypeptides rather than the antibodies. But we are not persuaded that this evidences that claim 4 would have been nonobvious. Rather, we find that a person of ordinary skill in this sophisticated art would understand that the identification of elevated levels of a circulating polypeptide directly implicated in the mechanism of IC-GN would be a natural target against which to direct immobilizing antibodies, as suggested both by paragraph [0071] of Saus (“this aspect of the invention can be used, for example, to produce antibodies against native GPBP forms”) as well as the teachings of Bard cited by the Examiner. We consequently agree with the Examiner that Saus ’935’s teaching of antibodies directed against the 77- kDacGPBP proteins in view of the known utility of antibodies in treating disease as taught by Bard would be an obvious, significant and promising direction in the development of therapies for the treatment of IC-GN. Finally, we agree with the Examiner that Bard, although not directed to IC-GN, would suggest to a person of ordinary skill in the art that antibodies directed against elevated levels of a circulating protein believed to be involved in the mechanism of a disease (Alzheimer’s disease, in the case of Bard) and would suggest that the use of antibodies directed against 10 Appeal 2015-006665 Application 13/400,831 circulating, disease-associated proteins as an effective mechanism of treating the polypeptide-associated disease by immobilizing the proteins. B. Reasonable Expectation of Success Issue Appellants next argue the Examiner erred because a person of ordinary skill at the time of filing would not have had a reasonable expectation of success in combining the references. App. Br. 9. Analysis Appellants point to the Saus Declaration, which opines: In fact one of skill in the art would expect that cGPBP-specific antibody treatment would not be effective to treat IC-GN. GPBP causes basement membrane collagen misfolding, which is expected to be accomplished inside the cell at the reticulum endoplasmic where basement membrane collagen assembles and antibodies cannot penetrate in this cellular compartment. The ’935 application discloses that increased cellular expression of GPBP is associated with increased levels of cGPBP and therefore extracellular cGPBP is a biomarker for monitoring what is occurring inside the cell. However, one of skill in the art would find it non-obvious and unexpected that blocking extracellular cGPBP would have consequences on any deleterious effects of intracellular GPBP, such as its basement membrane collagen misfolding and IC-GN, since there is no known positive feedback operating between extracellular (cGPBP) and intracellular (GPBP). App. Br. 10 (emphasis omitted) (quoting Saus Deck 19). Appellants therefore argue that there was nothing in the art at the time of filing to indicate that blocking circulating (extracellular) GPBP, as recited in 11 Appeal 2015-006665 Application 13/400,831 Applicants’ claims, would have any effect on intracellular GPBP, the latter of which is likely involved in IC-GN pathogenesis. Id. Therefore, Appellants contend, IC-GN is likely associated with the deleterious effects of intracellular GPBP, and the teachings of Revert 2008 — that circulating 77-kDa GPBP is mainly found extracellularly but not intracellularly — would have undermined a person of ordinary skill’s expectation of success in treating IC-GN by targeting extracellular GPBP. Id. at 11—12. Appellants next point to paragraph [0179] of Saus ’935 and Revert 2008 at page 30255, both of which recite: Various lines of evidence support that COL4A3BP is an attractive target for strategies to diagnose and treat antibody-mediated disorders, inflammation, ER stress-mediated diseases and drug resistant cancer. However, observations supporting these conclusions may now need to be re-interpreted since many have been obtained using tools (i.e. siRNA or antibodies) which failed to discriminate between different gene products (i.e. GPBP and GPBPA26/ACERT), that are expressed at distinct cell compartments, and are differentially regulated in response to stimuli. App. Br. 11 (emphases added by Appellants). Appellants assert this paragraph refers to antibody-mediated disorders, and not to antibody-based therapies. Id. Therefore, Appellants contend, this teaching provides no instruction whatsoever regarding using anti-COL4A3BP antibodies to treat IC-GN; a disease that is not even mentioned in paragraph [0179]. Id. Furthermore, Appellants note, the quoted paragraph states that “these conclusions may now need to be re-interpreted, suggesting that COL4A3BP may not, in fact, be an attractive target or suggest a reasonable expectation of success. App. Br. 11. 12 Appeal 2015-006665 Application 13/400,831 The Examiner responds that Revert 2007 teaches that transgenic overexpression of human GPBP (hGPBP) in non-lupus-prone mice triggered similar glomerular abnormalities including deposits of IgA on a capillary glomerular basement membrane (“GBM”) that underwent dissociation, in the absence of an evident autoimmune response. Ans. 12. The Examiner finds Revert 2007 provides in vivo evidence that GPBP regulates GBM collagen organization, and elevated expression of GPBP causes dissociation and subsequent accumulation of IgA on the GBM. Id. The Examiner finds Revert 2007 describes a previously unrecognized pathogenic mechanism that may be relevant in human primary immune complex-mediated glomerulonephritis. Id. at 12—13 (citing Revert 2007 Abstr., 1423). The Examiner finds the teachings of Revert 2007 provide evidence that in vivo GPBP regulates type IV collagen organization and elevated expression of this kinase induces immune complex-mediated glomerulonephritis. Id. at 13 (citing Revert 2007 1420). The Examiner further finds Revert 2007 also teaches that their glomerulonephritis mouse models share the triad of elevated GPBP expression, type IV collagen alterations, and IgA deposit formation and autoimmune responses in Tg- hGPBP mice, including presence of anti-GBM autoantibodies, suggests that antibody binding to disrupted GBM occurs through an antigen-antibody- independent mechanism. Id. (citing Revert 2007 1429). The Examiner finds, however, that Revert 2007 teaches that Tg-hGPBP mice display less severe glomerular lesions than NZW mice, suggesting that autoantibodies are a contributing pathogenic factor in NZW mouse glomerulonephritis. Id. (citing Revert 2007 1429). 13 Appeal 2015-006665 Application 13/400,831 The Examiner further finds that Revert 2008 teaches that the cGPBP/77-kDa GPBP is mainly found in the extracellular compartment both as a soluble protein soluble and associated with glomerular basement membrane collagen. Ans. 14 (citing Revert 2008 30254). Importantly, the Examiner finds, Revert teaches that various lines of evidence support the conclusion that COL4A3BP (i.e., GPBP gene) is an attractive target for strategies to treat antibody-mediated disorders which discriminate between different gene products (i.e., GPBP and GPBPA26/CERT), which are expressed in distinct cell compartments and are differentially regulated in response to stimuli. Id. (citing Revert 2008 30255). The Examiner also finds Revert 2008 teaches that GPBP phosphorylates the NCI domain of the a3(IV))NCl which is a pivotal structure in the molecular and supramolecular organization of the glomerular basement membrane collagen and also the target of autoantibodies mediating glomerulonephritis in Goodpasture diseases. Id. The Examiner finds Revert 2008 thus teaches GPBP regulates glomerular basement membrane collagen organization and induces type IV collagen-based, antibody-mediated glomerulonephritis when its expression is abnormally elevated. Id. (citing Revert 2008 30246). The Examiner finds the Saus Declaration is insufficient to overcome the Examiner’s rejection because the anti-cGPBP antibodies would reach those 77-kDaGPBP associated with glomerular basement membrane collagen in the IC-GN treatment. Ans. 14—15. The Examiner further finds Saus ’935 provides an explicit suggestion that antibodies that binds to the native 77-kDaGPBP (cGPBP) polypeptide would be useful therapeutic agents for various disorders, including Goodpasture syndrome. Id. at 14—15 (citing Saus ’935 171). 14 Appeal 2015-006665 Application 13/400,831 With respect to Dr. Saus’ opinion regarding misfolding at the endoplasmic reticulum, and the antibodies’ lack of ability to penetrate the cellular compartment, the Examiner finds the opinion is not relevant because the anti-GPBP antibodies target the circulating/soluble 77-kDacGPBPs, and not the 91-kDa GPBPs present in the cellular compartments. Ans. 15. The Examiner finds a person of ordinary skill in the art would have been specifically motivated to target the cGPBP isoform in the treatment of IC- GN, because administering the anti-cGPBP antibody would discriminate between the different GPBP isoforms and would neutralize only the interaction between cGPBP and the type IV collagen complex and prevent the type IV collagen-based antibody-mediated glomerulonephritis. Id. Finally, the Examiner finds both Saus ’935 and Revert 2008 clarify the mechanisms by which various isoforms of GPBP are generated within the cells. Ans. 18. The Examiner finds Saus ’935 teaches that Identification of the circulating human 77-kDa GPBP provides compelling evidence that GPBP secretion is biologically relevant in vivo. Id. The Examiner finds Saus ’935 teaches that levels of circulating 77-kDa GPBP correlate with GPBP glomerular expression and pathogenesis in mouse models of immune complex-mediated glomerulonephritis, and suggests that serological determination of GPBP is relevant in a clinical setting. Id. The Examiner also finds Saus ’935 teaches that upregulation of circulating GPBP in Goodpasture patients support these conclusions and substantiate previous observations that GPBP is overexpressed in such patients. Id. (citing Saus ’935 1180). The Examiner finds Revert 2008 teaches that the 77-kDa cGPBP interacts with type IV collagen and can be localized in its soluble form in the 15 Appeal 2015-006665 Application 13/400,831 extracellular space. Id. (citing Revert 2008 Abstr.). The Examiner finds Revert 2008 teaches the 77-kDaGPBP phosphorylates the NCI domain of the a3(IV))NCl which is a pivotal structure in the molecular and supramolecular organization of the glomerular basement membrane collagen and also the target of autoantibodies mediating glomerulonephritis in Goodpasture diseases. Id. The Examiner finds Revert 2008 teaches 77-kDa cGPBP regulates glomerular basement membrane collagen organization and induces type IV collagen-based antibody-mediated glomerulonephritis when its expression is abnormally elevated and that an increased expression of the 77-kDa cGPBP perturbs the quaternary structure of type IV collagen, suggesting that the elevated cGPBP levels interfere with the conformational diversification program (tertiary structure) of the a3(IV)NCl domain. Id. (citing Revert 2008 30246, 30254—55). We are not persuaded by Appellants’ arguments. Appellants rely upon the Saus Declaration to argue that there would have been no reasonable expectation of success in combining the references. Dr. Saus opines, in relevant part: [0]ne of skill in the art would expect that cGPBP-specific antibody treatment would not be effective to treat IC-GN, GPBP causes basement membrane collagen misfolding, which is expected to be accomplished inside the cell at the reticulum endoplasmic [sic] where basement membrane collagen assembles and antibodies cannot penetrate in this cellular compartment. The ’935 application discloses that increased cellular expression of GPBP is associated with increased levels of cGPBP and therefore extracellular cGPBP is a biomarker for monitoring what is occurring inside the cell. However, one of skill in the art would find it nonobvious and unexpected that blocking extracellular cGPBP would have consequences on any deleterious effect of intracellular GPBP such as its basement membrane collagen 16 Appeal 2015-006665 Application 13/400,831 misfolding and IC-GN, since there is no known positive feedback operating between extracellular (cGPHP) and intracellular (GPBP). Saus Deck 19 (emphases in original). We have considered the opinions of Dr. Saus but are not persuaded they overcome the evidence of obviousness. Rather, we agree with the Examiner that Revert 2007 and Revert 2008, both of which list Dr. Saus as a coauthor, teach that the 77 kDa GBPB isoform is also involved in the etiology of IC-GN beyond acting as a mere biomarker. Revert 2008 teaches: Here we show that cells expressed at least two GPBP isoforms resulting from canonical (77-kDa) and noncanonical (91-kDa) mRNA translation initiation. The 77-kDa polypeptide interacted with type IV collagen and localized as a soluble form in the extracellular compartment. The 91-kDa polypeptide and its derived 120-kDa polypeptide associated with cellular membranes and regulated the extracellular levels of the 77-kDa polypeptide. Revert 2008 Abstr. Revert 2008 also teaches: “Here we demonstrate that the translation of the mRNA for GPBP generated several polypeptides, none of which were significantly expressed in the cytosol. On the contrary, the current study provides evidence that GPBP enters into the secretory pathway and interacts with type IV collagen.'1'’ Revert 2008 30247 (emphasis added). Revert 2008 also teaches: Several lines of evidence support the idea that GPBP regulates protein folding in the ER and supramolecular organization in the extracellular compartment rather than interorganelle ceramide traffic in the cytosol ...the 77-kDa GPBP is mainly found in the extracellular compartment both soluble (Fig. 5) or associated with glomerular basement membrane collagen (4) and is not expressed at significant levels in the cytosol of cultured cells... an increased expression of the 77-kDa GPBP perturbs the 17 Appeal 2015-006665 Application 13/400,831 quaternary structure of type IV collagen, suggesting that the elevated GPBP levels interfere with the conformational diversification program (tertiary structure) of the a3(IV)NCl domain. Revert 2008 30254—55. Although these teachings do not contradict the opinion of Dr. Saus that overexpression of GPBP within the cell, and particularly the 99-kDa intracellular isoform, play an important role in protein misfolding, the references also teach that the extracellular 77-kDa isoform, i.e., cGPBP plays an external role in generating the autoimmune response and GBM disruption characteristic of IC-GN. This latter isoform would be understood by a person of ordinary skill to be predictably susceptible to treatment with anti-cGPBP antibodies because since it has been identified as interfering with the collagen structure, neutralizing it would be reasonably expected to have at least some beneficial effect on the disease. Finally, Saus ’935 teaches: Immunohistochemical evidence suggests that GPBP is primarily extracellular, although with the potential to localize to various intracellular sites (3,4). Protein distribution is highly informative with respect to protein function; therefore additional studies were needed to understand the biological function of GPBP. Here we demonstrate that the translation of the mRNA for GPBP generated several polypeptides, none of which were significantly expressed in the cytosol. On the contrary, the current study provides evidence that [the 77-kD isoform of] GPBP enters into the secretory pathway and interacts with type IV collagen. Saus ’935 1134 (emphasis added). The same reference teaches: “An increased expression of the 77-kDa GPBP perturbs the quaternary structure of type IV collagen, suggesting that the elevated GPBP levels interferes with 18 Appeal 2015-006665 Application 13/400,831 the conformational diversification program (tertiary structure) of the a3(IV)NCl domain .... Increased serum levels of GPBP correlates with type IV-collagen based glomerulonephritis.” Saus ’935 1177. Moreover, we have explained our reasoning with respect to paragraph [0071] of Saus ’935. Taken together, we find that these teachings outweigh the opinion of Dr. Saus that GPBP acts via an intracellular mechanism unavailable to circulating antibodies. We consequently agree with the Examiner’s findings and conclusion that a person of ordinary skill in the art would have a reasonable expectation of success in combining the references to arrive at Appellants’ claimed method. 19 Appeal 2015-006665 Application 13/400,831 C. Unpredictability of the prior art Issue Appellants next argue that the Examiner erred because a person of ordinary skill in the art would not have had a reasonable expectation of success in arriving at Applicants’ claimed invention merely from the combination of Bard with the other cited references at least because (1) when considered in its totality, the art was unpredictable, and (2) Bard’s teachings relate to an entirely different disease with an entirely different pathology. App. Br. 12. Analysis Appellants argue that, at the time of filing, Bard was but one example in the art of attempted treatment of a disease linked to overexpression of a protein by administering an antibody specific for that protein. App. Br. 13. Appellants point to another piece of prior art, S. Higa et al., Administration of Anti-interleukin 18 Antibody Fails to Inhibit Development of Dermatitis in Atopic Dermatitis-Model Mice NC/Nga, 149 British Journal of Dermatology 39-45 (2003) (“Higa”). According to the Saus Declaration: Higa, et al., teaches that increased IL-18 serum levels (e.g., a circulating cytokine protein) were found to correlate with onset and development of dermatitis [....] However, when the authors investigated whether administration of anti-IL-18 antibody could be used to treat dermatitis, they found that continuous injections of anti-IL-18 antibody failed to inhibit the onset and development of dermatitis. To the contrary, the treatment tended to lead to an exacerbation of dermatitis and scratching behavior. Higa, et al., demonstrates that the effects on a disease of administration of an antibody to a protein whose over-expression 20 Appeal 2015-006665 Application 13/400,831 is associated with that disease cannot be reasonably predicted by one of ordinary skill in the art. App. Br. 13 (quoting Saus Decl. Tflf 13—14) (emphasis added by Appellants). Appellants therefore argue that the Saus Declaration makes clear that to one of skill in the art, the results of administration of an antibody to a protein, the overexpression of which is correlated with a disease state, are unpredictable. Id. Appellants assert that the Examiner’s findings failed to consider the teachings of Higa in their entirety. App. Br. 14. According to Appellants, at the time of filing, both the rationale and the results of Higa were in the prior art, and one of ordinary skill considering Higa as a whole, would have understood that the art was unpredictable, and that there was no reasonable expectation of success in treating a condition characterized by overexpression of a protein using an antibody to that protein. Id. Appellants argue further that, setting aside the teachings of Higa, even the art within the field of Alzheimer’s disease, addressed by Bard, was and is unpredictable. Appellants point to B. Spencer and E. Masliah, Immunotherapy for Alzheimer’s disease: Past, Present and Future, 6(114) Frontiers in Aging Neuroscience, 1-7 (2014) (“Spencer”). App. Br. 14. Appellants assert Spencer reviews anti-Ap immunotherapies for the treatment of Alzheimer’s disease, many of which failed. Id. Appellants quote Spencer as teaching: “Although many of these immunotherapeutic approaches have failed to affect significant improvements in the mild to moderate AD patients being treated, the exact cause of failure is not known.” Id. (quoting Spencer 4). Appellants contend that these failures, and the lack of understanding regarding their causes, indicate confusion and 21 Appeal 2015-006665 Application 13/400,831 unpredictability in the art—even within the same disease addressed by Bard. Id. According to Appellants, the predictability and expectation of success is even lower in applying the Alzheimer’s disease-based teachings of Bard to IC-GN: an entirely different disease with a different pathology, using different antibodies against a different protein target. Id. Appellants argue that, in applying Bard to arrive at Appellants’ claimed methods of treating IC-GN, one of skill would have had to make a number of substantial and scientifically baseless assumptions regarding similarities between Alzheimer’s disease and IC-GN. Id. The Examiner responds that, in their arguments, Appellants do not provide persuasive evidence that one skilled in the art would not have accepted that the anti-Ap antibodies taught by Bard could be used to treat Alzheimer’s. Ans. 21. Also, according to the Examiner, the issue shared in the teachings of Bard, Revert 2007, and Revert 2008 is the overexpression of a polypeptide with pathological features that can be treated with anti polypeptide antibodies, as long as the antibody is accessible to the polypeptide. Id. The Examiner finds that, in the instant application, studies involving passive immunization have suggested that the primary mechanism for Ap clearance is peripheral and is not due to antibodies entering the CNS. Id. The Examiner finds that it has been shown that, following intraperitoneal injection of anti-Ap antibodies in the PDAPP mouse, there is a rapid 1,000- fold increase in circulating plasma Ap, suggesting that circulating ant-Ap antibodies bind to plasma Ap and thus cause a disruption in the equilibrium between the brain and plasma removing Ap from the brain. Id. (citing R.B. DeMattos et al., Peripheral Anti-A/l Antibody Alters CNS and Plasma A ft 22 Appeal 2015-006665 Application 13/400,831 Clearance and Decreases Brain Afi burden in a Mouse Model of Alzheimer’s Disease, 98(15) Proc. Nat’l Acad. Sci. USA 8850-55 (2001). The Examiner finds further that Higa supports the Examiner’s position that those skilled in the contemporary art would have a reasonable expectation of success that the antibody targeting of a protein whose overexpression correlates with a specific disorder would be effective to treat the disorder, because if there had been no such expectation, the study would not have been attempted. Ans. 21. We are not persuaded by Appellants’ arguments. As an initial matter, the Spencer reference was published in 2014 and is therefore does not reflect evidence the state of the art at the time of invention. The obviousness analysis, rather, is determined by what the combined teachings of the prior art references would have suggested [at the time of Appellants’ claimed invention] to those of ordinary skill in the art. In re Keller, 642 F.2d 413, 425 (CCPA. 1981). We therefore do not reach Appellants’ arguments with respect to the teachings of Spencer. Although we acknowledge that Higa teaches a different outcome from that of Bard, only a reasonable expectation of success, not absolute predictability, is necessary for a conclusion of obviousness. See In re Longi, 795 F.2d 887, 897 (Fed. Cir. 1985). Inasmuch as Higa teaches that “[sjurprisingly” the administration of its antibodies did not inhibit the disorder, Higa evidences that skilled persons would have reasonably expected the opposite result. (Higa 41.) We agree with the Examiner that the teachings of Bard would provide a reasonable basis for a person of ordinary skill in the art to expect success in attempting to apply the method, as suggested by Saus ’935, of directing antibodies against the circulating 77- 23 Appeal 2015-006665 Application 13/400,831 kDa isoform of GPBP as a means of treating IC-GN. We consequently affirm the Examiner’s rejection of the claims. DECISION The Examiner’s rejection of claims 4—5 and 20—30 under 35 U.S.C. § 103(a) is affirmed. No time period for taking any subsequent action in connection with this appeal may be extended under 37 C.F.R. § 1.136(a)(1). AFFIRMED 24 Copy with citationCopy as parenthetical citation
