Association between α4 integrin cytoplasmic tail and non-muscle myosin IIA regulates cell migration

Author:

Rosado Leslie A. Rivera1,Horn Troy A.1,McGrath Sara C.2,Cotter Robert J.2,Yang Joy T.1

Affiliation:

1. Department of Cell Biology, The Johns Hopkins University School of Medicine, Baltimore, MD 21205, USA

2. Middle Atlantic Mass Spectrometry Laboratory, The Johns Hopkins University School of Medicine, Baltimore, MD 21205, USA

Abstract

α4β1 integrin regulates cell migration via cytoplasmic interactions. Here, we report an association between the cytoplasmic tail of α4 integrin (α4 tail) and non-muscle myosin IIA (MIIA), demonstrated by co-immunoprecipitation of the MIIA heavy chain (HC) with anti-α4-integrin antibodies and pull-down of MIIA-HC with recombinant α4 tail from cell lysates. The association between the α4 tail and MIIA does not require paxillin binding or phosphorylation at Ser988 in the α4 tail. We found that substituting Glu982 in the α4 tail with alanine (E982A) disrupts the α4–MIIA association without interfering with the paxillin binding or Ser988 phosphorylation. By comparing stably transfected CHO cells, we show that the E982A mutation reduces the ability of α4β1 integrin to mediate cell spreading and to promote front–back polarization. In addition, we show that E982A impairs shear-flow-induced migration of the α4-integrin-expressing CHO cells by reducing their migration speed and directional persistence. The E982A mutation also leads to defects in the organization of MIIA filament bundles. Furthermore, when cells are plated on fibronectin and simulated with shear flow, α4β1 integrin forms filament-like patterns that co-align with MIIA filament bundles. These results provide a new mechanism for linking integrins to the actomyosin cytoskeleton and for regulating cell migration by integrins and non-muscle myosin II.

Publisher

The Company of Biologists

Subject

Cell Biology

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