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MBC in Press, published online ahead of print November 3, 2004
Mol. Biol. Cell 10.1091/mbc.E04-04-0277

A more recent version of this article appeared on January 1, 2005
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Submitted on April 1, 2004
Accepted on October 21, 2004

R-Ras Controls Membrane Protrusion and Cell Migration through the Spatial Regulation of Rac and Rho

Michele A. Wozniak,* Lina Kwong,* David Chodniewicz,{dagger} Richard L. Klemke,{dagger} and Patricia J. Keely*{ddagger}

*Department of Pharmacology, University of Wisconsin, Madison, WI 53706; {dagger}Department of Immunology, The Scripps Research Institute, La Jolla, CA 92037

Monitoring Editor: Mark Ginsberg

Although it is known that the spatial coordination of Rac and Rho activity is essential for cell migration, the molecular mechanisms regulating these GTPases during migration are unknown. We found that the expression of constitutively activated R-Ras (38V) blocked membrane protrusion and random migration. In contrast, expression of dominant negative R-Ras (41A) enhanced migrational persistence and membrane protrusion. Endogenous R-Ras is necessary for cell migration, as cells that were transfected with siRNA for R-Ras did not migrate. Expression of R-Ras (38V) decreased Rac activity and increased Rho activity around the entire cell periphery, while expression of dominant negative R-Ras (41A) showed the converse, suggesting that R-Ras can spatially activate Rho and inactivate Rac. Consistent with this role, endogenous R-Ras localized, and was preferentially activated at, the leading edge of migratory cells in response to adhesion. The effects of R-Ras on cell migration are mediated by PI3-Kinase, as an effector mutant that uncouples PI3-Kinase binding from R-Ras (38V) rescued migration. From these data, we hypothesize that R-Ras plays a key role in cell migration by locally regulating the switch from Rac to Rho activity after membrane protrusion and adhesion.


{ddagger}Corresponding author. E-mail: pjkeely{at}facstaff.wisc.edu




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