Viscous drag as the source of active site perturbation during protease translocation: Insights into how inhibitory processes are controlled by serpin metastability

Authors
Shin, Jong-ShikYu, Myeong-Hee
Issue Date
2006-06-02
Publisher
ACADEMIC PRESS LTD ELSEVIER SCIENCE LTD
Citation
JOURNAL OF MOLECULAR BIOLOGY, v.359, no.2, pp.378 - 389
Abstract
The native form of serine protease inhibitors (serpins) is kinetically trapped in a metastable state, which is thought to play a central role in the inhibitory mechanism. The initial binding complex between a serpin and a target protease undergoes a conformational change that forces the protease to translocate toward the opposite pole. Although structural determination of the final stable complex revealed a detailed mechanism of keeping the bound protease in an inactive conformation, it has remained unknown how the serpin exquisitely translocates a target protease with an acyl-linkage unhydrolyzed. We previously suggested that the acyl-linkage hydrolysis is strongly suppressed by active site perturbation during the protease translocation. Here, we address what induces the transient perturbation and how the serpin metastability contributes to the perturbation. Inhibitory activity of alpha(1)-antitrypsin (alpha(1)AT) toward elastase showed negative correlations with medium viscosity and Stokes radius of elastase moiety, indicating that viscous drag directly affects the protease translocation. Stopped-flow measurements revealed that the change in the inhibitory activity is primarily caused by the change in the translocation rate. The native stability of alpha(1)AT cavity mutants showed a negative correlation with the translocation rate but a positive correlation with the acyl-linkage hydrolysis rate, suggesting that the two kinetic steps are not independent but closely related. The degree of active site perturbation was probed by amino acid nucleophiles, supporting the view that the changes in the acyl-linkage hydrolysis rate are due to different perturbation states. These results suggest that the active site perturbation is caused by local imbalance between a pulling force driving protease translocation and a counteracting viscous drag force. The structural architecture of serpin metastability seems to be designed to ensure the active site perturbation by providing a sufficient pulling force, so the undesirable hydrolytic activity of protease is strongly suppressed during the translocation. (c) 2006 Elsevier Ltd. All rights reserved.
Keywords
REACTIVE CENTER LOOP; CONFORMATIONAL CHANGE; HUMAN ALPHA(1)-ANTITRYPSIN; INFLUENZA HEMAGGLUTININ; PLASMINOGEN-ACTIVATOR; PROTEINASE COMPLEX; MICHAELIS COMPLEX; STRUCTURAL BASIS; NATIVE STRAIN; BETA-SHEET; REACTIVE CENTER LOOP; CONFORMATIONAL CHANGE; HUMAN ALPHA(1)-ANTITRYPSIN; INFLUENZA HEMAGGLUTININ; PLASMINOGEN-ACTIVATOR; PROTEINASE COMPLEX; MICHAELIS COMPLEX; STRUCTURAL BASIS; NATIVE STRAIN; BETA-SHEET; kinetic folding trap; metastability; alpha(1)-antitrypsin; acyl-linkage hydrolysis; conformational change
ISSN
0022-2836
URI
https://pubs.kist.re.kr/handle/201004/135409
DOI
10.1016/j.jmb.2006.03.045
Appears in Collections:
KIST Article > 2006
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