The cultures were then washed, fixed with 4% paraformaldehyde, and stained with an antibody that detects total YAP and with Hoechst 33342 to visualize the cell nuclei. epithelial cells. In turn, YAP and TAZ are necessary for the stimulation of the proliferative response of intestinal epithelial cells to GPCR agonists that act via PKD. The discovery of interaction between WZ3146 YAP and WZ3146 PKD pathways identifies a novel cross-talk in signal transduction and demonstrates, for the first time, that the PKDs feed into the YAP pathway. and (36, 38). Accordingly, multiple growth-promoting stimuli rapidly activate PKD1 catalytic activity in intestinal epithelial cells (23, 36, 38,C40) through activation loop phosphorylation (30, 35,C37). Furthermore, transgenic mice that express elevated PKD1 protein in intestinal epithelial cells display a marked increase in DNA-synthesizing cells in their intestinal crypts and a significant increase in the length and total number of cells per crypt (36). Collectively, these results support the notion that PKD1 signaling is a novel element in the pathway leading to proliferation of intestinal epithelial cells and confluent and quiescent cultures of IEC-18 cells were stimulated without (?) or with 10 nm ANG II for the indicated times. The cultures were then washed, fixed with 4% paraformaldehyde, and stained with an antibody that detects total YAP and with Hoechst 33342 to visualize the cell nuclei. quantification of WZ3146 the images shown in was determined with the CellProfiler software, as described under Experimental Procedures. The plot shown represents the mean nuclear/cytoplasmic ratios of YAP immunofluorescence S.E. = 8 fields (1400 cells were analyzed for each time point). Similar results were obtained in three independent experiments. represents the distribution of control and ANG II-stimulated cells (at 30 min) as a function of their nuclear/cytoplasmic ratio of YAP immunofluorescence based on the analysis of 1700 cells from one experiment. Similar results were obtained in 10 independent experiments. confluent cultures of IEC-18 cells were stimulated without (?) or with either 10% FBS (confluent cultures of IEC-18 cells were stimulated with ANG II at the indicated concentrations for 30 min. The cultures were then washed, fixed with 4% paraformaldehyde, and stained with an antibody that detects total YAP and with Hoechst 33342 to visualize the cell nuclei. quantification of nuclear/cytoplasmic ratio of YAP immunofluorescence shown in was determined with the CellProfiler software as described under Experimental Procedures. The plot shown are the mean ratios S.E. = 7 fields (1250 cells were analyzed for each concentration of ANG II). Similar results were obtained in a separate experiment. confluent cultures of IEC-18 cells were incubated without (and confluent cultures of IEC-18 cells were incubated without (?) or with ANG II (quantification of total YAP phosphorylated at Ser127 and Ser397 was performed using MultiGauge version 3.0. The results represent the mean S.E., = 3, and are expressed as percentage of the maximal level of YAP phosphorylated at Ser127 and Ser397. Similar results were obtained in three independent experiments. confluent cultures of IEC-18 cells Rabbit Polyclonal to GHITM were stimulated with 10 nm ANG II for 30 min. Then the cells were lysed, and YAP immunoprecipitates (cultures of IEC-18 cells were transfected with non-targeting siRNA (and and confluent cultures of IEC-18 cells were incubated in the absence (quantification of the nuclear/cytoplasmic ratio of YAP immunofluorescence shown in was determined with the CellProfiler software. The shown are the mean nuclear/cytoplasmic ratio S.E. = 6 fields (1,200 cells were analyzed for each condition). Similar results were obtained in three independent experiments. confluent cultures of IEC-18 cells were incubated in the absence (confluent cultures of IEC-18 cells were incubated in the absence (quantification of the nuclear/cytoplasmic ratio of YAP immunofluorescence shown in was WZ3146 determined with the CellProfiler software. The shown are the mean nuclear/cytoplasmic ratios S.E. = 6 fields (1,100 cells were analyzed for each condition). Similar results were obtained in four independent experiments. confluent cultures of IEC-18 WZ3146 cells were incubated in the absence (and image analysis in image analysis in quantification in.