Appeal No. 1999-2200 Application No. 08/896,063 GROUNDS OF REJECTION42 Claims 1, 2, 8-21 and 40 are rejected under 35 U.S.C. § 103 as being unpatentable over Bettler ‘92 in view of Puckett43. We reverse. Claim 1: The examiner states (Answer44, page 8) that: [I]t would have been prima facie obvious to the skilled artisan at the time the invention was made to isolate the cDNA encoding human GluR7 (EAA5) by using the nucleic acid of rat GluR7 of Bettler [‘92] as a probe to screen a human brain cDNA library, as taught by Puckett, in order to obtain large quantities of human GluR7 by subcloning the isolated nucleic acid into an expression vector and transfecting the expression vector into a host cell such as Hela cells or Xenopus oocytes. We emphasize the examiner’s statement to use the rat GluR7 nucleic acid as a probe to screen a human brain cDNA library as taught by Puckett. The screening method taught by Puckett uses reduced stringency conditions (Puckett, bridging paragraph, pages 7557-558, and page 7558, Results, column 1). Bettler ’92 teaches (page 259, column 1) that “[t]he coding region of the GluR5 cDNA clone was used as a probe to screen a rat cerebellum cDNA library under low stringency hybridization conditions … [o]ne cDNA clone encoding part 42 We note the examiner’s new ground of rejection of claims 1 and 2 under 35 U.S.C. § 112, first paragraph made in the Answer, was withdrawn by the examiner in the Supplemental Answer (Paper No. 37, mailed September 19, 1997. 43 We note the examiner withdrew her reliance on Heinemann that was applied in the Final Rejection (Paper No. 27, mailed June 6, 1996) in the alternative with Bettler ’92 in view of Puckett. 44 Paper No. 35, mailed May 13, 1997. 40Page: Previous 33 34 35 36 37 38 39 40 41 42 43 44 45 46 47 NextLast modified: November 3, 2007