Ly depleted by transfecting previously characterized siRNAs [17]. Depletion resulted in a strong attenuation of the induction of double MLC phosphorylation at cell-cell contacts, but not along the leading edge (Fig. 1C). Co-immunoprecipitation indicated that wounding stimulated enhanced association of myosin IIA with ��-Sitosterol ��-D-glucoside biological activity p114RhoGEF (Fig. 1F). p114RhoGEF thus stimulates myosin activation during epithelial repair in a spatially controlled manner at cell-cell junctions. We next performed migration assays to KDM5A-IN-1 determine the functional importance of p114RhoGEF during epithelial wound repair. Cells transfected with control siRNAs closed wounds rapidly within 7 hours, reflecting the efficient migration behavior of corneal epithelial cells [33]. If p114RhoGEF had been depleted, the two opposing cell sheets moved slowly and a large gap between them remained even after 7 hours (Fig. 1D,E). p114RhoGEF is thus required for collective cell migration of HCE cells.Regulation of Single Tumor Cell Migration Cell Stiffness MeasurementsTo compare the stiffness of cells in different experimental conditions, we carried out AFM force spectroscopy measurements with a JPK Nanowizard-I (JPK instruments, Berlin, Germany) interfaced to an inverted optical microscope (IX-71, Olympus). AFM cantilevers with pyramidal tips (MLCT, Bruker, Karlsruhe, Germany) and nominal spring constants of 0.05 N.m-1 were modified by gluing 7.5 mm radius polystyrene beads (Invitrogen) to the cantilever underside with UV curing glue (UV curing, Loctite, UK). The spring constant of each cantilever was measured before affixing the bead using the thermal noise method implemented in the AFM software (JPK SPM). The sensitivity of the cantilever was set by measuring the slope of force-distance curves acquired on glass regions of the petri dish in which cells were plated (50 mm glass bottom Petri dishes, Willco wells, Amsterdam, The Netherlands). Prior to the experiment, the cell medium was replaced with Leibovitz L15 medium (Invitrogen) with 10 FBS. During AFM experiments, the tip of the cantilever was aligned over the centre of each cell and a force-distance curve acquired with an approach speed of 3 mm.s-1 and a target force of 1 nN. Stiffnesses were extracted from the force-distance curves by fitting the contact portion with a Hertzian contact model using custom-written Matlab routines as described in [29]. As p114RhoGEF regulates double MLC phosphorylation at cell-cell junctions, its role in cell locomotion might be limited to collective cell migration. To test this, we employed MDA-MB-231 cells, an invasive breast cancer cell line that expresses high levels of p114RhoGEF (Fig. S1). Transient transfections of siRNAs targeting p114RhoGEF led to efficient depletion of the protein in MDA-MB-231 cells (Fig. 2A). As positive controls, we depleted RhoA and an additional RhoA exchange factor, GEF-H1, known to stimulate RhoA close to the leading edge [34]. Depletion of both exchange factors, p114RhoGEF and GEF-H1, led to clear reductions in total RhoA activity (Fig. 2B). Time-lapse recordings followed by single cell tracking were then used to evaluate the importance of p114RhoGEF in single cell migration. Figure 2C,D shows that depletion of RhoA and GEF-H1 inhibited migration as expected, confirming that locomotion of MDA-MB-231 cells is RhoA dependent. Transfection of siRNAs targeting p114RhoGEF also strongly attenuated migration (Fig. 2C,D; Movies S1, S2, S3). Hence, p114RhoGEF also regulates singl.Ly depleted by transfecting previously characterized siRNAs [17]. Depletion resulted in a strong attenuation of the induction of double MLC phosphorylation at cell-cell contacts, but not along the leading edge (Fig. 1C). Co-immunoprecipitation indicated that wounding stimulated enhanced association of myosin IIA with p114RhoGEF (Fig. 1F). p114RhoGEF thus stimulates myosin activation during epithelial repair in a spatially controlled manner at cell-cell junctions. We next performed migration assays to determine the functional importance of p114RhoGEF during epithelial wound repair. Cells transfected with control siRNAs closed wounds rapidly within 7 hours, reflecting the efficient migration behavior of corneal epithelial cells [33]. If p114RhoGEF had been depleted, the two opposing cell sheets moved slowly and a large gap between them remained even after 7 hours (Fig. 1D,E). p114RhoGEF is thus required for collective cell migration of HCE cells.Regulation of Single Tumor Cell Migration Cell Stiffness MeasurementsTo compare the stiffness of cells in different experimental conditions, we carried out AFM force spectroscopy measurements with a JPK Nanowizard-I (JPK instruments, Berlin, Germany) interfaced to an inverted optical microscope (IX-71, Olympus). AFM cantilevers with pyramidal tips (MLCT, Bruker, Karlsruhe, Germany) and nominal spring constants of 0.05 N.m-1 were modified by gluing 7.5 mm radius polystyrene beads (Invitrogen) to the cantilever underside with UV curing glue (UV curing, Loctite, UK). The spring constant of each cantilever was measured before affixing the bead using the thermal noise method implemented in the AFM software (JPK SPM). The sensitivity of the cantilever was set by measuring the slope of force-distance curves acquired on glass regions of the petri dish in which cells were plated (50 mm glass bottom Petri dishes, Willco wells, Amsterdam, The Netherlands). Prior to the experiment, the cell medium was replaced with Leibovitz L15 medium (Invitrogen) with 10 FBS. During AFM experiments, the tip of the cantilever was aligned over the centre of each cell and a force-distance curve acquired with an approach speed of 3 mm.s-1 and a target force of 1 nN. Stiffnesses were extracted from the force-distance curves by fitting the contact portion with a Hertzian contact model using custom-written Matlab routines as described in [29]. As p114RhoGEF regulates double MLC phosphorylation at cell-cell junctions, its role in cell locomotion might be limited to collective cell migration. To test this, we employed MDA-MB-231 cells, an invasive breast cancer cell line that expresses high levels of p114RhoGEF (Fig. S1). Transient transfections of siRNAs targeting p114RhoGEF led to efficient depletion of the protein in MDA-MB-231 cells (Fig. 2A). As positive controls, we depleted RhoA and an additional RhoA exchange factor, GEF-H1, known to stimulate RhoA close to the leading edge [34]. Depletion of both exchange factors, p114RhoGEF and GEF-H1, led to clear reductions in total RhoA activity (Fig. 2B). Time-lapse recordings followed by single cell tracking were then used to evaluate the importance of p114RhoGEF in single cell migration. Figure 2C,D shows that depletion of RhoA and GEF-H1 inhibited migration as expected, confirming that locomotion of MDA-MB-231 cells is RhoA dependent. Transfection of siRNAs targeting p114RhoGEF also strongly attenuated migration (Fig. 2C,D; Movies S1, S2, S3). Hence, p114RhoGEF also regulates singl.