Cell motility was analysed using ECIS after being treated with different motility inhibitors and the motogen HGF. Following electrical wounding (5 V AC for 30 seconds) and treatment with HGF (50 ng/ml), MDApEF6 ± HGF, MDACl5exp ± HGF and MDACL5rib2 ± HGF showed an increase
in motility when compared to untreated cells. It was significantly enhanced after this website 5 hours of treatment (Figure 6a). Following experiments then examined the effect of motility inhibitors alone. When cells were treated with the Selleckchem Salubrinal N-WASP inhibitor (50 μM), the migration rate of MDApEF6 ± N-WASP, MDACl5exp ± N-WASP and MDACL5rib2 ± N-WASP was markedly reduced after 5 hours of treatment when compared to untreated cells (Figure 6b). The ROCK inhibitor (50nM)
was capable of altering the motility of MDApEF6 ± ROCK when compared to the untreated cells. However, no significant differences were found in the transfected cells, MDACl5exp ± ROCK and MDACl5rib2 ± ROCK, when compared to the untreated cells (Figure 6c). All these results were based on 3 repeat experiments that were combined and analysed using ANOVA. Figure 6 Effect of Claudin-5 on MDA-MB-231 cell migration following treatment with HGF, N-WASP inhibitor or ROCK inhibitor using ECIS. (a) Migration was significantly increased in MDApEF6 ± HGF, MDACl5exp ± HGF and MDACL5rib2 ± HGF when compared to untreated cells (p ≤ 0.001, p ≤ 0.001 and p = 0.003 PRN1371 concentration versus respective untreated controls) (n = 3). (b) Migration was significantly decreased in MDApEF6 ± N-WASP inhibitor, MDACl5exp ± N-WASP inhibitor and MDACL5rib2 ± N-WASP inhibitor when compared to untreated cells (p ≤ 0.001, p = 0.006 and p = 0.018 respectively) (n = 3). (c) Migration was significantly decreased in MDApEF6 ± ROCK inhibitor (p ≤ 0.001). MDACl5exp ± ROCK inhibitor and MDACL5rib2 ± ROCK inhibitor did not show significant differences when compared to untreated cells (p = 0.403 and p = 0.072 respectively) (n = 3).
In order to investigate any possible effect of Claudin-5 on protein level of N-WASP and ROCK 1, Western blot analysis was used to assess whether any direct effect was exerted at the Selleck Neratinib protein level in the control and transfected cells. MDA-MB-231Cl5exp and MDA-MB-231CL5rib2 Western blotting demonstrated very low levels of the N-WASP at protein level which was undetectable in MDA-MB-231pEF6 (Figure 7a). Protein levels of ROCK 1 showed a similar low level in all cells (Figure 7a). Thus, modulation of Claudin-5 appeared to cause an increase in N-WASP expression at the protein level. Figure 7 Western blot demonstrating levels of expression of N-WASP and ROCK 1 and protein-protein interactions. (a) Expression of N-WASP and ROCK 1 in transfected and control cells. (b) Co-immunoprecipitation of Claudin-5 with N-WASP and ROCK 1. (c) Co-immunoprecipitation of N-WASP with Claudin-5.