Cofilin is a marker of myofibroblast differentiation in cells from porcine aortic cardiac valves

doi:10.1152/ajpheart.01305.2007

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Am J Physiol Heart Circ Physiol 294: H1767-H1778, 2008. First published February 8, 2008; doi:10.1152/ajpheart.01305.2007
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Cofilin is a marker of myofibroblast differentiation in cells from porcine aortic cardiac valves

M. Pho,¹ W. Lee,¹ D. R. Watt,² C. Laschinger,¹ C. A. Simmons,² and C. A. McCulloch¹

¹Canadian Institutes of Health Research Group in Matrix Dynamics and ²Institute of Biomaterials and Biomedical Engineering, University of Toronto, Toronto, Canada

Submitted 6 November 2007 ; accepted in final form 2 February 2008

The formation of myofibroblasts in valve interstitial cell (VIC)populations contributes to fibrotic valvular disease. We examinedmyofibroblast differentiation in VICs from porcine aortic valves.In normal valves, cells immunostained for ${alpha}$ -smooth muscle actin( ${alpha}$ -SMA, a myofibroblast marker) were rare (0.69 ± 0.48%),but in sclerotic valves of animals fed an atherogenic diet,myofibroblasts were spatially clustered and abundant (31.2 ±6.3%). In cultured VIC populations from normal valves, SMA-positivemyofibroblasts were also spatially clustered, abundant (21%positive cells after 1 passage), and stained for collagen typeI and vimentin but not desmin. For an analysis of stem cells,two-color flow cytometry of isolated cells stained with Hoechst33342 demonstrated that 0.5% of VICs were side population cells;none stained for SMA. Upon culture, sorted side population cellsgenerated $~$ 85% SMA-positive cells, indicating that some myofibroblastsoriginate from a rare population with stem cell characteristics.Plating cells on rigid collagen substrates enabled the formationof myofibroblasts after 5 days in culture, which was completelyblocked by culture of cells on compliant collagen substrates.Exogenous tensile force also significantly increased SMA expressionin VICs. Isotope-coded affinity tags and mass spectrometry wereused to identify differentially expressed proteins in myofibroblastdifferentiation of VICs. Of the nine proteins that were identified,cofilin expression and phospho-cofilin were strongly increasedby conditions favoring myofibroblast differentiation. Knockdownof cofilin with small-interfering RNA inhibited collagen gelcontraction and reduced myofibroblast differentiation as assessedby the SMA incorporation into stress fibers. When compared withnormal valves, diseased valves showed strong immunostainingfor cofilin that colocalized with SMA in clustered cells. Weconclude that in VICs, cofilin is a marker for myofibroblastsin vivo and in vitro that arise from a rare population of stemcells and require a rigid matrix for formation.

actin; fibroblasts; isotope-coded affinity tags; ${alpha}$ -smooth muscle actin

Address for reprint requests and other correspondence: C. A. McCulloch, Univ. of Toronto, 150 College St., Rm. 244, Fitzgerald Bldg., Toronto, ON, Canada M5S 3E2 (e-mail: christopher.mcculloch{at}utoronto.ca)