作者
Jinli Chang, Jianping Jin, Pete Lollar, Wolfram Bode, Hans Brandstetter, Nobuko Hamaguchi, David L Straight, Darrel W Stafford
发表日期
1998/5/15
期刊
Journal of Biological Chemistry
卷号
273
期号
20
页码范围
12089-12094
出版商
Elsevier
简介
This study was designed to identify functionally important factor IX (FIX) residues. Using recombinant techniques and cell culture, we produced a mutant FIX with arginine at 338 changed to alanine (R338A-FIX). This molecule had approximately 3 times greater clotting activity than that of wild type FIX (wt-FIX) in the activated partial thromboplastin assay. R338A-FIX reacted normally with a panel of three FIX specific monoclonal antibodies and migrated on sodium dodecyl sulfate-polyacrylamide gels indistinguishably from wt-FIX. Using functional assays, we determined that R338A-FIXa'sK d for factor VIIIa (FVIIIa) was similar to that of wt-FIXa. Our kinetic analysis, using factor X as substrate, indicated that the mutation's major effects were a 3-fold increase ink cat and a 2-fold decrease inK m both manifested only in the presence of FVIIIa. R338A-FIXa's increased catalytic efficiency did not result from ablation of a …
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