Regulation of collagen synthesis by inhibitory Smad7 in cardiac myofibroblasts

doi:10.1152/ajpheart.00910.2006

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Am J Physiol Heart Circ Physiol 293: H1282-H1290, 2007. First published May 18, 2007; doi:10.1152/ajpheart.00910.2006
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Regulation of collagen synthesis by inhibitory Smad7 in cardiac myofibroblasts

Baiqiu Wang, Amer Omar, Tatjana Angelovska, Vanja Drobic, Sunil G. Rattan, Stephen C. Jones, and Ian M. C. Dixon

Institute of Cardiovascular Science, St. Boniface General Hospital Research Centre and Department of Physiology, University of Manitoba, Winnipeg, Canada

Submitted 23 August 2006 ; accepted in final form 17 May 2007

Transforming growth factor- $beta$ ₁ (TGF- $beta$ ₁) signal and downstream Smadsplay an important role in tissue fibrosis and matrix remodelingin various etiologies of heart failure. Inhibitory Smad7 (I-Smad7)is an inducible regulatory Smad protein that antagonizes TGF- $beta$ ₁signal mediated via direct abrogation of R-Smad phosphorylation.The effect of ectopic I-Smad7 on net collagen production wasinvestigated using hydroxyproline assay. Adenovirus-mediatedI-Smad7 gene (at 100 multiplicity of infection) transfer wasassociated with significant decrease of collagen synthesis inthe presence and absence of TGF- $beta$ ₁ in primary rat cardiac myofibroblasts.In I-Smad7-infected cells, we also observed the ablation ofTGF- $beta$ ₁-induced R-Smad2 phosphorylation vs. LacZ controls. OverdrivenI-Smad7 was associated with significantly increased expressionof immunoreactive 65-kDa matrix metalloproteinase-2 (MMP-2)protein in culture medium of myofibroblast compared with LacZ-infectedcells. Expression of the 72-kDa MMP-2 variant, e.g., the inactiveform, was not altered by exogenous I-Smad7 transfection/overexpression.Furthermore, I-Smad7 overexpression was associated with a significantincrease and decrease in expression of p27 and phospho-Rb protein,respectively, as well as reduced [³H]thymidine incorporationvs. Ad-LacZ-infected controls. We suggest that negative modulationof R-Smad phosphorylation by ectopic I-Smad7 may contributeto the downregulation of collagen in cardiac myofibroblastsand may suppress the proliferation of these cells. Thus treatmentstargeting the collagen deposition by overexpression of I-Smad7may provide a new therapeutic strategy for cardiac fibrosis.

myofibroblast; cardiac remodeling; matrix metalloproteinase; p27; fibroblast proliferation; cardiac fibrosis

Address for reprint requests and other correspondence: I. M. C. Dixon, Institute of Cardiovascular Science, St. Boniface General Hospital Research Centre, 351 Tache Ave., Winnipeg, MB, Canada R2H 2A6 (e-mail: idixon{at}sbrc.ca)