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Fig. 5. Hsp90 is a component of the activated G ${alpha}$ 12 complex and is necessary for Src activation and ZO-2 phosphorylation. (A) Src activation in QL ${alpha}$ 12-MDCK cells +/–dox and +/–GA. Identical amounts of cell lysate were analyzed by western blotting with antibodies specific for pTyr-419 as described in the Materials and Methods. Membranes were stripped and reanalyzed for total Src and occludin. (B) Band intensity was quantified as described above and the pTyr-419 immunoreactivity normalized to total Src. The relative amount of pTyr419 for –dox and –dox +GA is shown in comparison to the +dox condition. (C) Phosphotyrosine content of immunoprecipitated ZO-2 from QL ${alpha}$ 12-MDCK cells +/–dox and +/–GA. ZO-2 was immunoprecipitated and analyzed with 4G10 anti-phosphotyrosine as described above. (D) Interaction of G ${alpha}$ 12 with ZO-1 in QL ${alpha}$ 12-MDCK cells +/–dox and +/–GA. ZO-1 was immunoprecipitated under the specified conditions and precipitates were analyzed for G ${alpha}$ 12 by western blotting. Control is lysate with beads alone. (E) Steady-state protein levels of TJ proteins and G ${alpha}$ 12 in QL ${alpha}$ 12-MDCK +/–dox and +/–GA (2 µM). (F) Validation of GST-TPR pull-down of activated G ${alpha}$ 12. QL ${alpha}$ 12- and G ${alpha}$ 12-MDCK cells were cultured in –dox, and lysates ( $~$ 800 µg) were pulled-down with 1 µg GST or GST-TPR, as described in the Materials and Methods, and analyzed by western blotting for G ${alpha}$ 12. 10% of the input of wild-type G ${alpha}$ 12 is shown in the lysate lane. (G) Hsp90 western blot of GST-TPR pull-downs from G ${alpha}$ 12- and QL ${alpha}$ 12-MDCK cells in –dox.

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