Srv2/cyclase-associated protein forms hexamericshurikensthat directly catalyze actin filament severing by cofilin

Author:

Chaudhry Faisal1,Breitsprecher Dennis1,Little Kristin1,Sharov Grigory2,Sokolova Olga2,Goode Bruce L.1

Affiliation:

1. Department of Biology, Rosenstiel Basic Medical Science Research Center, Brandeis University, Waltham MA, 02454

2. Faculty of Biology, Moscow State University, 119991, Moscow, Russia

Abstract

Actin filament severing is critical for the dynamic turnover of cellular actin networks. Cofilin severs filaments, but additional factors may be required to increase severing efficiency in vivo. Srv2/cyclase-associated protein (CAP) is a widely expressed protein with a role in binding and recycling actin monomers ascribed to domains in its C-terminus (C-Srv2). In this paper, we report a new biochemical and cellular function for Srv2/CAP in directly catalyzing cofilin-mediated severing of filaments. This function is mediated by its N-terminal half (N-Srv2), and is physically and genetically separable from C-Srv2 activities. Using dual-color total internal reflection fluorescence microscopy, we determined that N-Srv2 stimulates filament disassembly by increasing the frequency of cofilin-mediated severing without affecting cofilin binding to filaments. Structural analysis shows that N-Srv2 forms novel hexameric star-shaped structures, and disrupting oligomerization impairs N-Srv2 activities and in vivo function. Further, genetic analysis shows that the combined activities of N-Srv2 and Aip1 are essential in vivo. These observations define a novel mechanism by which the combined activities of cofilin and Srv2/CAP lead to enhanced filament severing and support an emerging view that actin disassembly is controlled not by cofilin alone, but by a more complex set of factors working in concert.

Publisher

American Society for Cell Biology (ASCB)

Subject

Cell Biology,Molecular Biology

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