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WASP integrates substrate topology and cell polarity to guide neutrophil migration
Author(s) -
Rachel M. Brunetti,
Gabriele Kockelkoren,
Preethi Raghavan,
George R. R. Bell,
Derek Britain,
Natasha Puri,
Sean R. Collins,
Manuel D. Leonetti,
Dimitrios Stamou,
Orion D. Weiner
Publication year - 2021
Publication title -
the journal of cell biology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 5.414
H-Index - 380
eISSN - 1540-8140
pISSN - 0021-9525
DOI - 10.1083/jcb.202104046
Subject(s) - actin , biology , cell polarity , microbiology and biotechnology , cytoskeleton , cdc42 , regulator , actin cytoskeleton , cell migration , topology (electrical circuits) , substrate (aquarium) , cell , biophysics , gene , biochemistry , ecology , mathematics , combinatorics
To control their movement, cells need to coordinate actin assembly with the geometric features of their substrate. Here, we uncover a role for the actin regulator WASP in the 3D migration of neutrophils. We show that WASP responds to substrate topology by enriching to sites of inward, substrate-induced membrane deformation. Superresolution imaging reveals that WASP preferentially enriches to the necks of these substrate-induced invaginations, a distribution that could support substrate pinching. WASP facilitates recruitment of the Arp2/3 complex to these sites, stimulating local actin assembly that couples substrate features with the cytoskeleton. Surprisingly, WASP only enriches to membrane deformations in the front half of the cell, within a permissive zone set by WASP’s front-biased regulator Cdc42. While WASP KO cells exhibit relatively normal migration on flat substrates, they are defective at topology-directed migration. Our data suggest that WASP integrates substrate topology with cell polarity by selectively polymerizing actin around substrate-induced membrane deformations in the front half of the cell.

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