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Am J Physiol Cell Physiol 285: C674-C685, 2003. First published May 21, 2003; doi:10.1152/ajpcell.00608.2002
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VASCULAR BIOLOGY

LPP, a LIM protein highly expressed in smooth muscle

Isabelle Gorenne,1 Robert K. Nakamoto,1 Clayton P. Phelps,1 Mary C. Beckerle,2 Avril V. Somlyo,1 and Andrew P. Somlyo1

1Department of Molecular Physiology and Biological Physics, University of Virginia, Charlottesville, Virginia 22908; and 2Huntsman Cancer Institute and Department of Biology, University of Utah, Salt Lake City, Utah 84112

Submitted 31 December 2002 ; accepted in final form 16 May 2003

An 80-kDa protein, prominently expressed in smooth muscle, was microsequenced and identified as LPP, the product of the lipoma-preferred partner gene (Petit MMR, Mols R, Schoenmakers EFPM, Mandahl N, and Van de Ven WJM. Genomics 36: 118–129, 1996). Using a specific anti-LPP antibody, we showed, in Western blots and with immunofluorescence microscopy, the selective expression of LPP in vascular and visceral smooth muscles (~0.5–1 ng/µg total protein). In other mature (noncultured) tissues, including heart and skeletal muscle, the protein is present only in trace amounts and is closely correlated with the levels of the smooth muscle marker {alpha}-actin. In freshly isolated guinea pig bladder smooth muscle cells, immunofluorescence images showed LPP as linear arrays of punctate, longitudinally oriented staining superimposed with vinculin staining on the plasma membrane surface. A corresponding pattern of periodic labeling at the membrane in transverse sections of bladder smooth muscle suggested an association of LPP with peripheral dense bodies. In cultured rat aortic smooth muscle cells, LPP colocalized with vinculin at focal adhesions but not with p120 catenin or {alpha}-actinin. Overexpression of the protein increased EGF-stimulated migration of vascular smooth muscle cells in Transwell assays, suggesting the participation of LPP in cell motility. The Rho-kinase inhibitor Y-27632 dissociated focal adhesions and LPP staining at the cell periphery and enhanced the nuclear accumulation of LPP induced by leptomycin B, indicating that LPP has a potential for relocating to the nucleus through a shuttling mechanism that is sensitive to inhibition of Rho-kinase.

LIM protein; dense plaque; Rho-kinase; nuclear transport; cell migration



Address for reprint requests and other correspondence: A. P. Somlyo, PO Box 800736, Charlottesville, VA 22908 (E-mail: aps2n{at}virginia.edu).




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