Literature DB >> 24806962

Cellular microenvironments reveal defective mechanosensing responses and elevated YAP signaling in LMNA-mutated muscle precursors.

Anne T Bertrand1, Simindokht Ziaei1, Camille Ehret1, Hélène Duchemin1, Kamel Mamchaoui1, Anne Bigot1, Michèle Mayer2, Susana Quijano-Roy3, Isabelle Desguerre4, Jeanne Lainé1, Rabah Ben Yaou1, Gisèle Bonne5, Catherine Coirault6.   

Abstract

The mechanisms underlying the cell response to mechanical forces are crucial for muscle development and functionality. We aim to determine whether mutations of the LMNA gene (which encodes lamin A/C) causing congenital muscular dystrophy impair the ability of muscle precursors to sense tissue stiffness and to respond to mechanical challenge. We found that LMNA-mutated myoblasts embedded in soft matrix did not align along the gel axis, whereas control myoblasts did. LMNA-mutated myoblasts were unable to tune their cytoskeletal tension to the tissue stiffness as attested by inappropriate cell-matrix adhesion sites and cytoskeletal tension in soft versus rigid substrates or after mechanical challenge. Importantly, in soft two-dimensional (2D) and/or static three-dimensional (3D) conditions, LMNA-mutated myoblasts showed enhanced activation of the yes-associated protein (YAP) signaling pathway that was paradoxically reduced after cyclic stretch. siRNA-mediated downregulation of YAP reduced adhesion and actin stress fibers in LMNA myoblasts. This is the first demonstration that human myoblasts with LMNA mutations have mechanosensing defects through a YAP-dependent pathway. In addition, our data emphasize the crucial role of biophysical attributes of cellular microenvironment to the response of mechanosensing pathways in LMNA-mutated myoblasts.
© 2014. Published by The Company of Biologists Ltd.

Entities:  

Keywords:  Cell microenvironment; LMNA; Mechanosensitivity; Muscular dystrophy; Yes-associated protein

Mesh:

Substances:

Year:  2014        PMID: 24806962     DOI: 10.1242/jcs.144907

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


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