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a helix replacement mechanism directs metavinculin functions螺旋替代机制指导metavinculin功能
A Helix Replacement Mechanism Directs Metavinculin
Functions
Erumbi S. Rangarajan, Jun Hyuck Lee, S. D. Yogesha, Tina Izard*
Cell Adhesion Laboratory, Department of Cancer Biology, The Scripps Research Institute, Scripps Florida, Jupiter, Florida, United States of America
Abstract
Cells require distinct adhesion complexes to form contacts with their neighbors or the extracellular matrix, and vinculin links
these complexes to the actin cytoskeleton. Metavinculin, an isoform of vinculin that harbors a unique 68-residue insert in its
tail domain, has distinct actin bundling and oligomerization properties and plays essential roles in muscle development and
homeostasis. Moreover, patients with sporadic or familial mutations in the metavinculin-specific insert invariably develop
fatal cardiomyopathies. Here we report the high resolution crystal structure of the metavinculin tail domain, as well as the
crystal structures of full-length human native metavinculin (1,134 residues) and of the full-length cardiomyopathy-
associated DLeu954 metavinculin deletion mutant. These structures reveal that an a-helix (H1 9) and extended coil of the
metavinculin insert replace a-helix H1 and its preceding extended coil found in the N-terminal region of the vinculin tail
domain to form a new five-helix bundle tail domain. Further, biochemical analyses demonstrate that this helix replacement
directs the distinct actin bundling and oligomerization properties of metavinculin. Finally, the cardiomyopathy associated
DLeu954 and Arg975Trp metavinculin mutants reside on the replaced extended coil and the H19 a-helix, respectively. Thus,
a helix replacement mechanism directs metavinculin’s unique functions.
Citation: Rangarajan ES, Lee JH, Yogesha SD, Izard T (2010) A Helix Replacement Mechanis
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