Fig. 3.
Fig. 3. MAPK phosphorylation is not fully dependent on Shc phosphorylation. Cell lysates were prepared either before (−) or after (+) stimulation with exogenous TPO (14 ng/mL for 10 minutes). Parental BAF3 cells were used as well as clones engineered to express the full-length murine Mpl receptor (mMpl) or mutated receptors, which were truncated after either 111 or 69 cytoplasmic amino acids (T-111 and T-69, respectively).11 (A) One hundred micrograms of each lysate was evaluated by Western blotting and probed to detect double-phosphorylated ERK1 and ERK2. The blot was stripped and reprobed with ERK2 antibody to confirm equal loading in all lanes. (B) Shc was immunoprecipitated from 1 mg of each cell lysate. The immunoprecipitated protein was evaluated by Western blotting and probed with a phosphotyrosine-specific antibody (4G10). The blot was stripped and reprobed to verify the presence of Shc in all lanes.

MAPK phosphorylation is not fully dependent on Shc phosphorylation. Cell lysates were prepared either before (−) or after (+) stimulation with exogenous TPO (14 ng/mL for 10 minutes). Parental BAF3 cells were used as well as clones engineered to express the full-length murine Mpl receptor (mMpl) or mutated receptors, which were truncated after either 111 or 69 cytoplasmic amino acids (T-111 and T-69, respectively).11 (A) One hundred micrograms of each lysate was evaluated by Western blotting and probed to detect double-phosphorylated ERK1 and ERK2. The blot was stripped and reprobed with ERK2 antibody to confirm equal loading in all lanes. (B) Shc was immunoprecipitated from 1 mg of each cell lysate. The immunoprecipitated protein was evaluated by Western blotting and probed with a phosphotyrosine-specific antibody (4G10). The blot was stripped and reprobed to verify the presence of Shc in all lanes.

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