Allosteric communication in Dictyostelium myosin II

被引:0
|
作者
Piyali Guhathakurta
Ewa Prochniewicz
Joseph M. Muretta
Margaret A. Titus
David D. Thomas
机构
[1] University of Minnesota,Department of Biochemistry, Molecular Biology, and Biophysics
[2] University of Minnesota,Department of Genetics, Cell Biology, and Development
来源
Journal of Muscle Research and Cell Motility | 2012年 / 33卷
关键词
Actin; Cysteine; Lever arm; ADP; Fluorescence;
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中图分类号
学科分类号
摘要
Myosin’s affinities for nucleotides and actin are reciprocal. Actin-binding substantially reduces the affinity of ATP for myosin, but the effect of actin on myosin’s ADP affinity is quite variable among myosin isoforms, serving as the principal mechanism for tuning the actomyosin system to specific physiological purposes. To understand the structural basis of this variable relationship between actin and ADP binding, we studied several constructs of the catalytic domain of Dictyostelium myosin II, varying their length (from the N-terminal origin) and cysteine content. The constructs varied considerably in their actin-activated ATPase activity and in the effect of actin on ADP affinity. Actin had no significant effect on ADP affinity for a single-cysteine catalytic domain construct, a double-cysteine construct partially restored the actin-dependence of ADP binding, and restoration of all native Cys restored it further, but full restoration of function (similar to that of skeletal muscle myosin II) was obtained only by adding all native Cys and an artificial lever arm extension. Pyrene-actin fluorescence confirmed these effects on ADP binding to actomyosin. We conclude that myosin’s Cys content and lever arm both allosterically modulate the reciprocal affinities of myosin for ADP and actin, a key determinant of the biological functions of myosin isoforms.
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页码:305 / 312
页数:7
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