12103245 (P.T.A.B. Jun. 17, 2016)

Ex Parte Lewisch et al

Patent Trial and Appeal BoardJun 17, 2016

12103245 (P.T.A.B. Jun. 17, 2016)

UNITED STA TES p A TENT AND TRADEMARK OFFICE APPLICATION NO. FILING DATE 12/103,245 04/15/2008 28524 7590 06/21/2016 SIEMENS CORPORATION INTELLECTUAL PROPERTY DEPARTMENT 3501 Quadrangle Blvd Ste 230 Orlando, FL 32817 FIRST NAMED INVENTOR Sandra A. Lewisch 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. 2008P59106US 1591 EXAMINER YAKOVLEV A, GALINA M ART UNIT PAPER NUMBER 1678 NOTIFICATION DATE DELIVERY MODE 06/21/2016 ELECTRONIC 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. Notice of the Office communication was sent electronically on above-indicated "Notification Date" to the following e-mail address( es): ipdadmin.us@siemens.com PTOL-90A (Rev. 04/07) UNITED STATES PATENT AND TRADEMARK OFFICE BEFORE THE PATENT TRIAL AND APPEAL BOARD Ex parte SANDRA A. LEWISCH, PRATAP SINGH, VIRAL DESAI, KAREN L. KRAKOWSKI, and JAMES E. DUFFY Appeal2014-005132 Application 12/103,245 Technology Center 1600 Before RICHARD M. LEBOVITZ, FRANCISCO C. PRATS, and JOHN G. NEW, Administrative Patent Judges. LEBOVITZ, Administrative Patent Judge. DECISION ON APPEAL This appeal involves claims directed to a method for designing an antibody reagent for use in an assay for the detection of an analyte to obtain optimum assay sensitivity. Appellants appeal from the Examiner's final rejection of claims 1, 3-11, and 13-19 as obvious under 35 U.S.C. Â§ 103. We have jurisdiction under 35 U.S.C. Â§ 134. The rejection is affirmed. STATEMENT OF CASE Claims 1, 3-11, and 13-19 stand rejected under 35 U.S.C. Â§ 103(a) (pre-AIA) as obvious in view of Pierce (Applications Handbook and Catalog 200512006, pages 266-268, 277, 279-280, 282, 285) and Rong Appeal2014-005132 Application 12/103,245 ("Two-site imnmno-tluorometric assay of intact salmon calcitonin with improved sensitivity, Clinical Chem., 1997, vol. 43(1): 71-75). Claims 1 and 11 are independent claims. Appellants did not argue the claims separately. We select claim 1 as representative for deciding all issues. Claim 1 is reproduced below: 1. A method for designing an antibody reagent for use in an assay for the detection of an analyte to obtain an optimum assay sensitivity wherein the antibody reagent is a conjugate of a small molecule attached by a spacer group to an antibody for the analyte, the method comprising: preparing two or more of the conjugates by selecting a set of reaction parameters for each conjugate wherein the set of reaction parameters is different for each conjugate and wherein the set of reaction parameters is selected from the group consisting of the hydrophobicity or hydrophilicity of the spacer group, the length of the spacer group, the number of molecules of the small molecule attached to the antibody and the point of attachment of the small molecule to the antibody; conducting an assay for the analyte employing each conjugate; and selecting for use in the assay the conjugate that provides an optimum assay sensitivity in an assay for the detection of the analyte wherein assay sensitivity is monitored by monitoring a difference in the amount of signal obtained for calibrators spanning a suspected concentration range of interest of the analyte and wherein a difference in the signal detected between a calibrator of lowest concentration and next lowest concentration is at least about 50%, and signal detected for a calibrator of highest concentration is at least about 10 times greater than the signal detected for the calibrator of lowest concentration. 2 Appeal2014-005132 Application 12/103,245 REJECTION Rong describes an immunoassay for salmon calcitonin ("SCT") utilizing 1) a biotinylated capture antibody to "catch" the calcitonin and 2) an antibody labeled with a Eu chelate as signaling marker to detectably label the captured calcitonin. Rong 71 (Abstract; col. 2). The Examiner found that Rong tested various combinations of antibodies to determine the best combination with the highest sensitivity in detecting salmon calcitonin. Final Rej. 13. The Examiner found that Figure 1 of Rong summarizes the test results ofbiotinylated antibodies 309, 8A4, 5G9, and 3G4 (B-309, B-8A4, B-5G9, and B-3G4) and Eu-labeled antibodies 309 and 3G4 (Eu-309 and Eu-3G4) using salmon calcitonin as a calibrator in concentration ranges that read on the claimed calibrator concentrations. Id. The Examiner found that the combination of B-5G9/Eu- 309 resulted in the best sensitivity with low background. Id. Figure 1 of Rong is reproduced below: Salmon Ca!citonin (prnol/L) Â·Â·Â·<'.!Â·Â·Â· SCT v 8"'309#/Eu.'.3G4 Â·Â·Â·OÂ·Â·Â· SCT v B-5G9!Eu<3G4 ... 41.... SCT v 8-5G9!Eu-Â·309# i Â·Â·Â·VÂ·Â·Â· SCT v 8-3G4/EUÂ·Â·3iJ9# Â·Â·Â·Â¢Â·Â·Â· SGT v B-309#iE.u~309# . Â·"-Â¢-"Â· SCT v B-8.A.4/Eu-:~O':i# 3 Appeal2014-005132 Application 12/103,245 Figure 1 is a graph showing different conjugates tested at a range of calcitonin concentrations ("calibrators"). The combination of B-5G9/Eu-309 (represented by a triangle in the figure) resulted in the best sensitivity. With respect to the claimed limitation that a "signal detected for a calibrator of highest concentration is at least about 10 times greater than the signal detected for the calibrator of lowest concentration" as recited in claim 1, the Examiner found that it would have been obvious to have chosen the calibrators for optimal assay sensitivity and calcitonin range to be detected. Final Rej. 15, 20. The Examiner acknowledged that Figure 1 does not show the signal being 10-fold different between the lowest and highest calibrator concentrations, but found that Figures 3 and 4 of Rong show linearity using biotinylated 5G9 and Eu-labeled 309# with over an 18-fold signal difference. Id. at 16-17; 18-19. The Examiner further found that Rong teaches linearity until at least 300 pmol/L and that linearity over a wide calibrator concentration range is desirable to improve accuracy when it is desired to detect the analyte calcitonin over a broad range. Answer 9. Appellants contend that Figure 1 of Rong shows a signal difference of about 7.9, which is only about 7 times greater than that for the lowest calibrator. Appeal Br. 7. Appellants also contend that Figures 3 and 4 show "only the conjugate B-5G9 (biotinylated 5G9 antibody) and its separate use in an assay for salmon calcitonin." Id. Appellants state that only Figure 1 shows a "side by side comparison of conjugates," and in this experiment the calibrator concentrations do not meet the claimed requirement for a signal of 10 times great between the lowest and highest concentrations. Id. at 7-8. Appellants also state: 4 Appeal2014-005132 Application 12/103,245 [The] results depicted in Figs. 3 and 4 of Rong represent the use of a single conjugate in the determinations of salmon calcitonin concentrations and have no relationship to the results of assays on several conjugates, the results of which are summarized in Fig. 1 of Rong. Id. at 8. In the Reply Brief, Appellants state that Figure 1 shows results of calibrator concentrations between 0 and 10 pmol/L. Reply Br. 6. Appellants conclude: "To impute more into the disclosure of Fig. 1 is speculation. Appellant submits that the Office's interpretation of the above teaching of Rong is based on Appellant's disclosure and does not represent what a person of ordinary skill in the art would have been fairly taught by Rong." Id. Appellants also argue that the spacer in Rong was the same for all conjugates, while the claims require different reaction parameters which include using different spacers. Id. DISCUSSION The main dispute in this Appeal is whether Rong teaches or suggests that the signal detected for the highest concentration of calibrator is "at least about 10 times greater" than the signal detected for the lowest concentration of calibrator as required by independent by claims 1 and 11, and all the claims which depend from them. The Examiner cited Figs. 1, 3, and 4 of Rong as making this signal range obvious to one of ordinary skill in the art. Final Rej. 13-14. Claim 1 requires "preparing two or more of the conjugates by selecting a set of reaction parameters for each conjugate," "conducting an assay for the analyte employing each conjugate," and "selecting for use in 5 Appeal2014-005132 Application 12/103,245 the assay the conjugate that provides an optimum assay sensitivity." Fig. 1 of Rong shows "two or more conjugates" being tested, as required by the claims, to determine which combination of capture and labeling antibody gave the best sensitivity. Rong 72 ("Tests of Antibody Combinations."). Calcitonin serves as the calibrator. As explained in the Specification, a calibrator is a known amount of analyte. Spec i-f 8. Calibrators are tested over a range of concentrations, as shown in Rong' s Fig. 1 (0 to 10 pmol/L calcitonin), to monitor and calibrate the performance of the assay. Id. The dispute arises because Fig. 1 does not show a signal difference of 10-fold between the lowest and highest concentrations, but rather the difference is less than 8-fold. The Examiner found it would have been obvious to optimize the assay to achieve high sensitivity (Final Rej. 15, 20) and pointed to Figs. 3 and 4 of Rong where an about 18-fold difference in detected signal was observed between the lowest and highest concentrations of calibrator, providing evidence that a signal difference of greater than 10 is described by Rong (id. at 17). Appellants argue that Figs. 3 and 4 only look at one conjugate, not two or more as required by the claim, and state the skilled worker would not have imputed the information from Figs. 3 and 4 into Fig. 1. Appeal Br. 7- 8. Appellants' arguments are not supported by adequate evidence. Fig. 1 of Rong is a "calibration curve." Rong 72 ("Tests of Antibody Combinations"). The calibration curve, as reproduced above, shows that as the calibrator is increased for the combination of B-5G9/Eu-309 (represented by a triangle in the figure), the fluorescence increased linearly. Such a curve allows unknown amounts of calcitonin in samples to be determined by 6 Appeal2014-005132 Application 12/103,245 matching the measured fluorescence of an unknown sample to a point on the calibration curve. Rong teaches that its assay can be used to monitor calcitonin levels in patients. Our studies (Fig. 5) demonstrate that the assay has clinical applications. We can readily monitor the serum concentrations of SCT in patients who have received the drug. Since the assay is linear over the wide range of 0.3 to 300 pmol/L, high and low concentrations can be measured in the same assay and without the need for sample dilution. Both of these assay characteristics improve its accuracy. Id. at 74. Thus, while Fig. 1 is conducted over a limited range of 0 to 10 pmol/L with a less than 10 fold difference in signal between the lowest and highest concentrations, Rong teaches that for clinical applications it is desirable to test for low and high concentrations in the same assay, providing a reason to have used a broader range of calibrator which would be reasonably expected to result in a greater difference in fluorescent signal than depicted in Fig. 1. Figs. 3 and 4 of Rong show that a greater than 10-fold difference in signal can be achieved. When the assay is to be designed for high and low analyte concentrations as taught by Rong (id. at 74), it would have been obvious to have optimized different conjugates, as Rong did in Fig. 1, but over the broader concentration range to identify the antibody conjugate pair with the best sensitivity. Appellants' arguments focus on Fig. 1, but do not adequately address the obviousness of performing Fig. 1 over a broader concentration as motivated by Rong's teachings. Appellants in the Reply Brief argue that the spacers are the same in Rong, while the claim requires them to be different. Reply Br. 6. We have not been pointed to where this argument was made in the Appeal Brief. 7 Appeal2014-005132 Application 12/103,245 Nonetheless, Appellants have not identified language in the claim which requires the spacers to be different. The limitation in claim 1 at issue reads (underlining added): selecting a set of reaction parameters for each conjugate wherein the set of reaction parameters is different for each conjugate and wherein the set of reaction parameters is selected from the group consisting of the hydrophobicity or hydrophilicity of the spacer group, the length of the spacer group, the number of molecules of the small molecule attached to the antibody and the point of attachment of the small molecule to the antibody The limitation only requires that one parameter is different, and such parameter could be something other than the spacer, e.g., "the number of molecules of the small molecule attached to the antibody and the point of attachment of the small molecule to the antibody." The Examiner addressed these differences on, e.g., page 14 of the Final Rejection. For the foregoing reasons, we affirm the rejection of claims 1 and 11. Dependent claims 3-10 and 13-19 fall with claims 1 and 11 because separate reasons for their patentability were not provided. 37 C.F.R. Â§ 41.37(c)(l)(iv). TIME PERIOD No time period for taking any subsequent action in connection with this appeal may be extended under 37 C.F.R. Â§ 1.136(a)(l )(iv). AFFIRMED 8