Matrix metalloproteinase 13 mediates nitric oxide activation of endothelial cell migration

Esther López-Rivera; Tania R. Lizarbe; Mónica Martínez‐Moreno; José M. López‐Novoa; Alicia Rodríguez‐Barbero; José Rodrigo; Ana Patricia Fernández; Alberto Álvarez; Santiago Lamas; Carlos Zaragoza

doi:10.1073/pnas.0408217102

Matrix metalloproteinase 13 mediates nitric oxide activation of endothelial cell migration

Esther López-Rivera(Instituto Cajal), Tania R. Lizarbe(Instituto Cajal), Mónica Martínez‐Moreno(Instituto Cajal), José M. López‐Novoa(Instituto Cajal), Alicia Rodríguez‐Barbero(Instituto Cajal), José Rodrigo(University of California, Los Angeles), Ana Patricia Fernández(University of California, Los Angeles), Alberto Álvarez(Instituto Cajal), Santiago Lamas(Instituto Cajal), Carlos Zaragoza(Instituto Cajal)

Proceedings of the National Academy of Sciences

February 22, 2005

10.1073/pnas.0408217102

Cited by 81Open Access

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Abstract

To explore the mechanisms by which NO elicits endothelial cell (EC) migration we used murine and bovine aortic ECs in an in vitro wound-healing model. We found that exogenous or endogenous NO stimulated EC migration. Moreover, migration was significantly delayed in ECs derived from endothelial NO synthase-deficient mice compared with WT murine aortic EC. To assess the contribution of matrix metalloproteinase (MMP)-13 to NO-mediated EC migration, we used RNA interference to silence MMP-13 expression in ECs. Migration was delayed in cells in which MMP-13 was silenced. In untreated cells MMP-13 was localized to caveolae, forming a complex with caveolin-1. Stimulation with NO disrupted this complex and significantly increased extracellular MMP-13 abundance, leading to collagen breakdown. Our findings show that MMP-13 is an important effector of NO-activated endothelial migration.

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