10865623 (B.P.A.I. Apr. 12, 2010)

Ex Parte Fu

Board of Patent Appeals and InterferencesApr 12, 2010

10865623 (B.P.A.I. Apr. 12, 2010)

UNITED STATES PATENT AND TRADEMARK OFFICE __________ BEFORE THE BOARD OF PATENT APPEALS AND INTERFERENCES __________ Ex parte YANG-XIN FU __________ Appeal 2009-010614 Application 10/865,623 Technology Center 1600 __________ Decided: April 12, 2010 __________ Before TONI R. SCHEINER, RICHARD M. LEBOVITZ, and STEPHEN WALSH, Administrative Patent Judges. WALSH, Administrative Patent Judge. DECISION ON APPEAL This is an appeal under 35 U.S.C. § 134(a) involving claims for a method to induce T-cell anti-tumor activity. The Patent Examiner rejected the claims for failure to comply with the written description requirement. We have jurisdiction under 35 U.S.C. § 6(b). We reverse. Appeal 2009-010614 Application 10/865,623 2 STATEMENT OF THE CASE According to the Specification, the LIGHT protein has a role in T cell activation. (Spec. 2:[0009].) “Mutant LIGHT (LIGHTm) is generated to prevent protease digestion so LIGHT can be expressed on tumor cells.” (Id. at 3:[00012].) “Mutant light (designated LIGHTm), has the proteolytic site EKLI from positions 79-82 deleted from the amino acid sequence of normal LIGHT (FIG. 3A) (Tamada et al., 2000).”1 (Id. at 3:[00013].) Claims 7-9 and 17 are on appeal. (App. Br. 2.)2 Claim 7 is representative and reads as follows: 7. A protease resistant mutant LIGHT protein having the amino acid sequence of LIGHT with a protease site between the transmembrane domain and amino acid position 85 in the extracellular domain with a deletion in the protease site, wherein the mutant LIGHT protein is stably present on the surface of a tumor cell. The Examiner rejected claims 7-9 and 17 under 35 U.S.C. § 112, first paragraph, as failing to comply with the written description requirement. WRITTEN DESCRIPTION The Issue The Examiner’s position is that the Specification “provides no teaching on a mutant LIGHT protein as claimed including intracellular (amino acid position 1-46), transmembrane (amino acid position 47-77), and extracellular domain (amino acid position 78-240) with mutations or 1 Koji Tamada et al., Modulation of T-cell-mediated immunity in tumor and graft-versus-host disease models through the LIGHT co-stimulatory pathway, 6 NATURE MEDICINE 283-289 (2000). 2 Supplemental Appeal Brief dated Oct. 2, 2008. Appeal 2009-010614 Application 10/865,623 3 deletions at proteolytic site (amino acid position 79-82).” (Ans. 3.) According to the Examiner, “[t]he scope of the claims includes a genus having numerous structural variants.” (Id.) The Examiner finds the disclosure “insufficient to describe the genus.” (Id. at 6.) Appellant contends that the LIGHT protein’s amino acid and nucleotide sequences were well known in the art before the Application was filed. (App. Br. 11.) Appellant provides (1) a copy of a figure adapted from Tamada with underlining showing the LIGHT transmembrane domain and the protease site, and (2) a copy of Fig. 3A from the Application as filed, said to show the relative locations of the transmembrane domain, the extracellular domain and the protease site in the LIGHT protein. (Id. at 6.) Appellant further argues that “[t]he fact that the generated mutant LIGHT protein that has an inactivated protease site between the transmembrane domain and position 85 of the LIGHT protein I stably present on the surface of a tumor cell, demonstrates that if there are other protease sites, they are not functionally relevant for the purpose of stimulating an immune response within the tumor environment.” (Id. at 8.) The issue with respect to this rejection is whether the evidence supports a finding that a person of ordinary skill in the art would not credit Applicant with possession of the proteins defined by claim 7. Findings of Fact 1. Tamada disclosed the full length sequence of murine and human LIGHT proteins. (Tamada 284, Fig. 1a.) 2. According to Tamada, the name LIGHT is “derived from: homologous to lymphotoxins, shows inducible expression, and Appeal 2009-010614 Application 10/865,623 4 competes with herpes simplex virus glycoprotein D for herpes virus entry mediator;” and LIGHT has “Genome Database designation, TNFSF14.” (Tamada, 283, second paragraph.) 3. Appellant’s Fig. 3A shows a schematic representation of the LIGHT protein, indicating where four amino acids were deleted. (Spec. 6:[00019].) 4. Appellant’s Fig. 9 “shows the nucleic acid sequence that encodes a LIGHT protein. . . . the region encoding a proteoloytic site that has been deleted in LIGHTm is underlined.” (Spec. 7:[00025].) 5. The record includes a Declaration of Yang-Xin Fu under 37 C.F.R. § 1.132. 6. Declarant Fu states: “[b]ased on the disclosure of a proteolytic site EKLI at positions 79-82 in a murine LIGHT sequence in the patent application, I identified a corresponding site EQLI at positions 81-84 near the transmembrane domain of the human LIGHT sequence by a computer alignment of the murine and the human LIGHT sequences.” (Decl. ¶ 5.) 7. Declarant Fu states: “based on the disclosure of a proteolytic site in murine LIGHT sequence and following methods disclosed in the present patent application, I was able to obtain a protease resistant mutant human LIGHT sequence.” (Id. at ¶ 7.) Principles of Law “[W]here . . . accessible literature sources clearly provided, as of the relevant date, genes and their nucleotide sequences . . . satisfaction of the written description requirement does not require either the recitation of … Appeal 2009-010614 Application 10/865,623 5 such genes and sequences.” Falko-Gunter Falkner v. Inglis, 448 F.3d 1357, 1363 (Fed. Cir. 2006). “It is not necessary that every permutation within a generally operable invention be effective in order for an inventor to obtain a generic claim, provided that the effect is sufficiently demonstrated to characterize a generic invention.” Capon v. Eshhar, 418 F.3d 1349, 1359 (Fed. Cir. 2005). Analysis The LIGHT protein was known in the art before Appellant filed the Application. (FF1, 2.) In the Specification, Appellant disclosed a protease site said to have been unrecognized in the art. Appellant claims to have discovered that when the protease site is mutated by deletion, the mutant LIGHT protein will have a stable presence on the surface of a tumor cell. The protease site is described as the four amino acid sequence EKLI in the murine sequence at about position 85. Declarant Fu states that there is a similar site in the human sequence. (FF6.) The Examiner finds no description of a “genus,” which the Examiner says has “numerous structural variants.” The claim is directed to “a protease resistant mutant LIGHT protein with . . . a deletion in the protease site.” We agree the claim is generic. However, we do not see evidence that a person of skill in the art would find the Specification’s description of the genus of deletion mutants within a four amino acid subsequence to be inadequate for the purpose of describing the invention defined in claim 7. In Amgen Inc. v. Hoechst Marion Roussel, Inc., 314 F.3d 1313, 1332 (Fed.Cir.2003) the court explained that the written description requirement may be satisfied “if in the knowledge of the art the disclosed function is Appeal 2009-010614 Application 10/865,623 6 sufficiently correlated to a particular, known structure.” We find that Appellant’s Specification establishes a correlation between deletions in the LIGHT protease site and the stable presence of protease resistant LIGHT on the surface of a tumor cell. Accordingly, we agree with Appellant that the evidence supports finding that a person of ordinary skill in the art would credit Appellant with possession of the mutant LIGHT protein defined in claim 7. CONCLUSION The evidence of record supports finding that a person of ordinary skill in the art would credit Applicant with possession of the protein defined by claim 7. SUMMARY We reverse the rejection of claims 7-9 and 17 under 35 U.S.C. § 112, first paragraph, as failing to comply with the written description requirement. REVERSED dm BARNES & THORNBURG LLP P.O. BOX 2786 CHICAGO, IL 60690-2786