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https://scholarbank.nus.edu.sg/handle/10635/111804
Title: | Breakpoint cluster region gene product-related domain of n-chimaerin: Discrimination between Rac-binding and GTPase-activating residues by mutational analysis | Authors: | Ahmed, S. Lee, J. Wen, L.-P. Zhao, Z. Ho, J. Best, A. Kozma, R. Lim, L. |
Issue Date: | 1-Jul-1994 | Citation: | Ahmed, S.,Lee, J.,Wen, L.-P.,Zhao, Z.,Ho, J.,Best, A.,Kozma, R.,Lim, L. (1994-07-01). Breakpoint cluster region gene product-related domain of n-chimaerin: Discrimination between Rac-binding and GTPase-activating residues by mutational analysis. Journal of Biological Chemistry 269 (26) : 17642-17648. ScholarBank@NUS Repository. | Abstract: | The breakpoint cluster region gene product (Bcr) is a GTPase-activating protein (GAP) for members of the Rho family, Cdc42Hs, and Racl, as is the brain protein n-chimaerin. At least 15 proteins have sequence identity to the GAP domain (150 amino acid residues) of Bcr. The widespread occurrence of proteins that possess sequence identity to the Bcr-related GAP domain makes it especially important to understand its structure/ function relationships. Amino acid sequence alignment of these proteins reveals three blocks of conservation in the GAP domain. Here, we present a mutational analysis of this domain using n-chimaerin sequences. Ten mutations were constructed (at least two in each of the blocks of conservation), expressed as glutathione S-transferase fusion proteins in Escherichia coli, and purified. Seven of the mutants, including deletions, still possessed GAP activity for Rac1. Three of the mutants had no Rac1-GAP activity but were still able to bind Rac1. IC50 values obtained from competition experiments suggest that ra-chimaerin and the mutants with no GAP activity bound Rac1 with similar apparent binding constants. Thus, this mutant analysis allows discrimination between Rac1-binding and Rac1 GTPase- activating residues. | Source Title: | Journal of Biological Chemistry | URI: | http://scholarbank.nus.edu.sg/handle/10635/111804 | ISSN: | 00219258 |
Appears in Collections: | Staff Publications |
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