Literature DB >> 26759174

KIF17 regulates RhoA-dependent actin remodeling at epithelial cell-cell adhesions.

Bipul R Acharya1, Cedric Espenel1, Fotine Libanje2, Joel Raingeaud2, Jessica Morgan1, Fanny Jaulin3, Geri Kreitzer4.   

Abstract

The kinesin KIF17 localizes at microtubule plus-ends where it contributes to regulation of microtubule stabilization and epithelial polarization. We now show that KIF17 localizes at cell-cell adhesions and that KIF17 depletion inhibits accumulation of actin at the apical pole of cells grown in 3D organotypic cultures and alters the distribution of actin and E-cadherin in cells cultured in 2D on solid supports. Overexpression of full-length KIF17 constructs or truncation mutants containing the N-terminal motor domain resulted in accumulation of newly incorporated GFP-actin into junctional actin foci, cleared E-cadherin from cytoplasmic vesicles and stabilized cell-cell adhesions to challenge with calcium depletion. Expression of these KIF17 constructs also increased cellular levels of active RhoA, whereas active RhoA was diminished in KIF17-depleted cells. Inhibition of RhoA or its effector ROCK, or expression of LIMK1 kinase-dead or activated cofilin(S3A) inhibited KIF17-induced junctional actin accumulation. Interestingly, KIF17 activity toward actin depends on the motor domain but is independent of microtubule binding. Together, these data show that KIF17 can modify RhoA-GTPase signaling to influence junctional actin and the stability of the apical junctional complex of epithelial cells.
© 2016. Published by The Company of Biologists Ltd.

Entities:  

Keywords:  Actin; Cell–cell adhesion; Kinesin; Rho–GTPases

Mesh:

Substances:

Year:  2016        PMID: 26759174      PMCID: PMC4813313          DOI: 10.1242/jcs.173674

Source DB:  PubMed          Journal:  J Cell Sci        ISSN: 0021-9533            Impact factor:   5.285


  86 in total

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