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A more recent version of this article appeared on December 23, 2005
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M509952200v1
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Papers In Press, published online ahead of print October 18, 2005
J. Biol. Chem, 10.1074/jbc.M509952200
Submitted on September 9, 2005
Revised on October 12, 2005
Accepted on October 18, 2005

H2-calponin is regulated by mechanical tension and modifies the function of actin cytoskeleton

M. Moazzem Hossain, James F. Crish, Richard L. Eckert, Jim J.-C. Lin, and Jian-Ping Jin

Medicine Dept., Section of Molecular Cardiology, Northwestern University, Evanston, IL 60201

Corresponding Author: jpjin{at}northwestern.edu

Calponin is an extensively studied actin-binding protein but its function is not well understood. Among three isoforms of calponin, h2-calponin is found in both smooth muscle and non-muscle cells. The present study demonstrates that epidermal keratinocytes and fibroblast cells express significant amounts of h2-calponin. The expression of h2-calponin is cell anchorage-dependent. The levels of h2-calponin decrease when cells are rounded up and remain low when cells are prevented from adherence to culture dish. H2-calponin expression resumes after the floating cells are allowed to form a monolayer in plastic dish. Cell cultures on polyacrylamide gels of different stiffness demonstrated that h2-calponin expression is affected by the mechanical properties of the culture matrix. When cells are cultured on soft gel that applies less traction force to the cell and, therefore, lower mechanical tension in the cytoskeleton, the level of h2-calponin is significantly lower than that in cells cultured on hard gel or rigid plastic dish. Force-expression of h2-calponin enhanced actin filaments’ resistance to cytochalasin B treatment. Keratinocyte differentiation is accompanied by a mechanical tension related up-regulation of h2-calponin. Lowering the tension of actin cytoskeleton by inhibiting non-muscle myosin II ATPase decreased h2-calponin expression. In contrast to the mechanical tension regulation of endogenous h2-calponin, the expression of h2-calponin using a cytomegalovirus promotor was independent of the stiffness of culture matrix. The results suggest that h2-calponin represents a novel manifestation of mechanical tension responsive gene regulation that may modify cytoskeleton function.


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