Ent correlated with activation of cortactin [28]. On the other hand, Rac1-dependent translocation of cortactin to the cell periphery could be observed by confocal microscope in single cellsCav-1 Mirin price Regulates Rac1 Activation and PermeabilityFigure 7. Down-regulation of caveolin-1 expression enhanced Rac1 activity, which was abolished by NSC-23766. A.Primary PMVECs transfected with control or caveolin-1 shRNA were challenged with TNF-a(100 ng/ml) for 2 hours. Rac1 activity in the cell lysates was evaluated using GTPase pull-down assays and normalized to the total GTPase content in cell lysates. Caveolin-1 deficient cells showed a significant increase in GTPbound Rac1 compared with control shRNA cells in the resting state (2.560.2-fold increase, P.0.001) and after TNF-a stimulation (2.760.4-fold increase, P.0.01).B. Measurement of Rac1 activity by GTPase pulldown assays. Down-regulation of caveolin-1 expression resulted in increased activity of Rac1 to 250620 of controls shRNA. Incubation with NSC-23766(200 mM, 30 min) abolished this effect. Co-treated with NSC-23766 and TNF-a, the activity of Rac1 decreased more than that treated with TNF-a alone. Each data point represents the mean6SD. derived from six independent experiments, *P,0.05, **P,0.01, ***P,0.001. doi:10.1371/journal.pone.0055213.gso that we could assess endothelial function by 76932-56-4 web changes in cell shape. We provide evidence that increased Rac1 activity leads to cortactin redistribution from the cytoplasm into membrane [30], which triggers peripheral actin polymerization [30] and formation of the peripheral actin rim, and thus EC barrier enhancement [17]. Moreover, our data demonstrate that Rac1 activity is negatively controlled by caveolin-1 and down-regulation of caveolin-1 can protect barrier function in the primary RPMVEC undergoing TNF-a stimulation. Our experiments demonstrate that TNF-a induced barrier breakdown in cultured primary RPMVEC was a direct result of impaired Rac1 signaling. We observed an increase of central actin stress fibers and the disappearance of cortactin from the cell periphery when exposured to TNF-a. This cellular change was accompanied by decreased Rac1 activity. All these changes were associated with hyperpermeablilty of the endothelial cell monolayer. However, activation of Rac1 could enhance cortical actin rim formation resulting in the protection of endothelial barrier from injury due to TNF-a. In our study, activation of Rac1 induced lamellipodia formation [31], cortactin localization to the cell periphery and activated cell spreading, which is important to inhibit cell collapse and prevent gap formation [32]. Many reportshave revealed that Sphingosine-1-phosphate (S1P) induced strong Rac1 activation and promoted the translocation of cortactin to the cell periphery and augmentation of the cortical actin ring. These events may account for its barrier-enhancing properties [33,34]. Moreover, S1P signaling, via the Rac1 pathway [35] regulates the cortactin-Arp2/3 complex formation, which ultimately results in the formation of lamellipodia and endothelial spreading [36,37]. Previous studies have shown that Rac1 associates with the scaffolding domain of Cav-1 through its hypervariable C-terminal domain and that Cav-1 is part of a negative-feedback loop that controls cell polarity, spreading and migration by regulating the degradation of activated Rac1 [38]. Cav-1-deficient cells lose normal cell polarity [39,40], exhibit impaired wound healing [41], and ha.Ent correlated with activation of cortactin [28]. On the other hand, Rac1-dependent translocation of cortactin to the cell periphery could be observed by confocal microscope in single cellsCav-1 Regulates Rac1 Activation and PermeabilityFigure 7. Down-regulation of caveolin-1 expression enhanced Rac1 activity, which was abolished by NSC-23766. A.Primary PMVECs transfected with control or caveolin-1 shRNA were challenged with TNF-a(100 ng/ml) for 2 hours. Rac1 activity in the cell lysates was evaluated using GTPase pull-down assays and normalized to the total GTPase content in cell lysates. Caveolin-1 deficient cells showed a significant increase in GTPbound Rac1 compared with control shRNA cells in the resting state (2.560.2-fold increase, P.0.001) and after TNF-a stimulation (2.760.4-fold increase, P.0.01).B. Measurement of Rac1 activity by GTPase pulldown assays. Down-regulation of caveolin-1 expression resulted in increased activity of Rac1 to 250620 of controls shRNA. Incubation with NSC-23766(200 mM, 30 min) abolished this effect. Co-treated with NSC-23766 and TNF-a, the activity of Rac1 decreased more than that treated with TNF-a alone. Each data point represents the mean6SD. derived from six independent experiments, *P,0.05, **P,0.01, ***P,0.001. doi:10.1371/journal.pone.0055213.gso that we could assess endothelial function by changes in cell shape. We provide evidence that increased Rac1 activity leads to cortactin redistribution from the cytoplasm into membrane [30], which triggers peripheral actin polymerization [30] and formation of the peripheral actin rim, and thus EC barrier enhancement [17]. Moreover, our data demonstrate that Rac1 activity is negatively controlled by caveolin-1 and down-regulation of caveolin-1 can protect barrier function in the primary RPMVEC undergoing TNF-a stimulation. Our experiments demonstrate that TNF-a induced barrier breakdown in cultured primary RPMVEC was a direct result of impaired Rac1 signaling. We observed an increase of central actin stress fibers and the disappearance of cortactin from the cell periphery when exposured to TNF-a. This cellular change was accompanied by decreased Rac1 activity. All these changes were associated with hyperpermeablilty of the endothelial cell monolayer. However, activation of Rac1 could enhance cortical actin rim formation resulting in the protection of endothelial barrier from injury due to TNF-a. In our study, activation of Rac1 induced lamellipodia formation [31], cortactin localization to the cell periphery and activated cell spreading, which is important to inhibit cell collapse and prevent gap formation [32]. Many reportshave revealed that Sphingosine-1-phosphate (S1P) induced strong Rac1 activation and promoted the translocation of cortactin to the cell periphery and augmentation of the cortical actin ring. These events may account for its barrier-enhancing properties [33,34]. Moreover, S1P signaling, via the Rac1 pathway [35] regulates the cortactin-Arp2/3 complex formation, which ultimately results in the formation of lamellipodia and endothelial spreading [36,37]. Previous studies have shown that Rac1 associates with the scaffolding domain of Cav-1 through its hypervariable C-terminal domain and that Cav-1 is part of a negative-feedback loop that controls cell polarity, spreading and migration by regulating the degradation of activated Rac1 [38]. Cav-1-deficient cells lose normal cell polarity [39,40], exhibit impaired wound healing [41], and ha.