Actin cytoskeleton regulates functional anchorage-migration switch during T-cadherin-induced phenotype modulation of vascular smooth muscle cells

Agne Frismantiene; Emmanouil Kyriakakis; Boris Dasen; Paul Erne; Therese J Resink; Maria Philippova

doi:10.1080/19336918.2017.1319545

Actin cytoskeleton regulates functional anchorage-migration switch during T-cadherin-induced phenotype modulation of vascular smooth muscle cells

Cell Adh Migr. 2018 Jan 2;12(1):69-85. doi: 10.1080/19336918.2017.1319545. Epub 2017 May 25.

Authors

Agne Frismantiene¹, Emmanouil Kyriakakis¹, Boris Dasen¹, Paul Erne¹, Therese J Resink¹, Maria Philippova¹

Affiliation

¹ a Department of Biomedicine , Laboratory for Signal Transduction, University Hospital Basel and University of Basel , Basel , Switzerland.

Abstract

Vascular smooth muscle cell (SMC) switching between differentiated and dedifferentiated phenotypes is reversible and accompanied by morphological and functional alterations that require reconfiguration of cell-cell and cell-matrix adhesion networks. Studies attempting to explore changes in overall composition of the adhesion nexus during SMC phenotype transition are lacking. We have previously demonstrated that T-cadherin knockdown enforces SMC differentiation, whereas T-cadherin upregulation promotes SMC dedifferentiation. This study used human aortic SMCs ectopically modified with respect to T-cadherin expression to characterize phenotype-associated cell-matrix adhesion molecule expression, focal adhesions configuration and migration modes. Compared with dedifferentiated/migratory SMCs (expressing T-cadherin), the differentiated/contractile SMCs (T-cadherin-deficient) exhibited increased adhesion to several extracellular matrix substrata, decreased expression of several integrins, matrix metalloproteinases and collagens, and also distinct focal adhesion, adherens junction and intracellular tension network configurations. Differentiated and dedifferentiated phenotypes displayed distinct migrational velocity and directional persistence. The restricted migration efficiency of the differentiated phenotype was fully overcome by reducing actin polymerization with ROCK inhibitor Y-27632 whereas myosin II inhibitor blebbistatin was less effective. Migration efficiency of the dedifferentiated phenotype was diminished by promoting actin polymerization with lysophosphatidic acid. These findings held true in both 2D-monolayer and 3D-spheroid migration models. Thus, our data suggest that despite global differences in the cell adhesion nexus of the differentiated and dedifferentiated phenotypes, structural actin cytoskeleton characteristics per se play a crucial role in permissive regulation of cell-matrix adhesive interactions and cell migration behavior during T-cadherin-induced SMC phenotype transition.

Keywords: 2-D monolayer; 3-D spheroid; T-cadherin; actin cytoskeleton; adhesion; adhesion molecules; migration; phenotype modulation; vascular smooth muscle cell.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Actin Cytoskeleton / drug effects
Actin Cytoskeleton / metabolism*
Amides / pharmacology
Cadherins / metabolism*
Cell Adhesion / drug effects
Cell Adhesion / physiology
Cell Communication / drug effects
Cell Communication / physiology
Cell Differentiation / drug effects
Cell Differentiation / physiology
Cell Movement / drug effects
Cell Movement / physiology
Cells, Cultured
Humans
Integrins / metabolism
Muscle, Smooth, Vascular / drug effects
Muscle, Smooth, Vascular / metabolism*
Myocytes, Smooth Muscle / drug effects
Myocytes, Smooth Muscle / metabolism*
Pyridines / pharmacology

Substances

Amides
Cadherins
H-cadherin
Integrins
Pyridines
Y 27632

Grants and funding

This work was supported by the Swiss National Science Foundation (grant no. 310030_159589 to TJR), the Stiftung für Herz- und Kreislaufkrankheiten (grant to TJR), and a fellowship grant (to AF) “Förderung exzellenter Nachwuchsforschender," Forschungsfonds 2015, University of Basel.