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Fig. 9. Rac inhibition reduces integrin β1 expression in PKC ${epsilon}$ ^+/+ fibroblasts. (A) As described in the Materials and Methods, western blot analysis was used to detect integrin β1 expression in PKC ${epsilon}$ ^+/+ and PKC ${epsilon}$ ^-/- fibroblasts. Cells were incubated in the presence or absence of the Rac inhibitor NSC23766 (100 µM, 1 hour). Rac inhibition reduced integrin β1 expression in PKC ${epsilon}$ ^+/+, but not in PKC ${epsilon}$ ^-/-, cells, indicating Rac operates upstream of integrin β1 expression and, in this context, in a PKC ${epsilon}$ -dependent fashion. Rac inhibition also reduced ${alpha}$ -SMA protein expression in PKC ${epsilon}$ ^+/+, but not PKC ${epsilon}$ ^-/-, cells. (B) As described in the Materials and Methods, a floating collagen gel contraction assay was used to detect ECM contraction by PKC ${epsilon}$ ^+/+ and PKC ${epsilon}$ ^-/- fibroblasts over a 24-hour period. Cells were incubated in the presence or absence of the Rac inhibitor NSC23766 (100 µM). Contraction was observed only in untreated PKC ${epsilon}$ ^+/+ cells (^*P<0.05). (C) As described in the Materials and Methods, a cell migration assay was performed on PKC ${epsilon}$ ^+/+ and PKC ${epsilon}$ ^-/- fibroblasts over a 72-hour period in the presence or absence of the Rac inhibitor NSC23766 (100 µM). Gap size expressed as a percentage of the original wound is shown (average±s.d.). The presence of the Rac inhibitor reduced migration of PKC ${epsilon}$ ^+/+ cells (^*P<0.05).

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