Figure 5
Figure 5. Tyrosine 719 in KIT receptor is sufficient for recruiting protein complex involving p85α, SHP2, and Gab2 to KITD814V. (A) The 32D cells bearing WT KIT or KITD814V were starved for 8 hours in serum- and growth factor-free medium followed by incubation with or without II-B08 (20μM) for 1 hour. After incubation, equal amounts of protein lysates were subjected to immunoprecipitation with anti-SHP2 or anti-p85α antibodies followed by Western blot analysis using anti-p85α, anti-SHP2, or anti-Gab2 antibodies. Similar results were observed in 2 independent experiments. (B) Primary BM-derived cells expressing WT KIT or KITD814V from WT or Gab2−/− mice were starved and subjected to proliferation assay in the absence of growth factors by thymidine incorporation. Bars represent the mean (± SD) thymidine incorporation from 1 of 3 independent ex-eriments performed in quadruplicate. *P < .01, WT-KITD814V vs Gab2−/−-KITD814V. (C) The 32D cells bearing WT KIT, KITD814V, KITD814V-Y719, or KITD814V-F7 were starved of serum and growth factors for 8 hours, and equal amounts of protein lysates were subjected to immunoprecipitation with an anti-KIT antibody, anti-p85α antibody, or anti-SHP2 antibody followed by Western blot analysis using anti-KIT, anti-p85α, anti-SHP2, or anti-Gab2 antibodies as indicated. Similar results were observed in 2 or 3 independent experiments.

Tyrosine 719 in KIT receptor is sufficient for recruiting protein complex involving p85α, SHP2, and Gab2 to KITD814V. (A) The 32D cells bearing WT KIT or KITD814V were starved for 8 hours in serum- and growth factor-free medium followed by incubation with or without II-B08 (20μM) for 1 hour. After incubation, equal amounts of protein lysates were subjected to immunoprecipitation with anti-SHP2 or anti-p85α antibodies followed by Western blot analysis using anti-p85α, anti-SHP2, or anti-Gab2 antibodies. Similar results were observed in 2 independent experiments. (B) Primary BM-derived cells expressing WT KIT or KITD814V from WT or Gab2−/− mice were starved and subjected to proliferation assay in the absence of growth factors by thymidine incorporation. Bars represent the mean (± SD) thymidine incorporation from 1 of 3 independent ex-eriments performed in quadruplicate. *P < .01, WT-KITD814V vs Gab2−/−-KITD814V. (C) The 32D cells bearing WT KIT, KITD814V, KITD814V-Y719, or KITD814V-F7 were starved of serum and growth factors for 8 hours, and equal amounts of protein lysates were subjected to immunoprecipitation with an anti-KIT antibody, anti-p85α antibody, or anti-SHP2 antibody followed by Western blot analysis using anti-KIT, anti-p85α, anti-SHP2, or anti-Gab2 antibodies as indicated. Similar results were observed in 2 or 3 independent experiments.

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