Fig. 2.
Fig. 2. Contact with RAMOS-wt or RAMOS-4c increases phosphorylation of stromal cell ERK2. Stromal cells were incubated in medium alone (−) or in contact with RAMOS-wt (wt) or RAMOS-4c (4c) for 5 minutes at 37°C. Stromal cells and RAMOS cells were collected separately and lysed as detailed in the Materials and Methods. (A and B) Lysates were incubated with antibody-coated protein A sepharose overnight at 4°C. Sepharose beads were sedimented by centrifugation for 10 seconds. The supernatant lysate was removed from selected samples and then immunoprecipitates were washed, eluted, and electrophoresed. (A) Anti-ERK2 immunoprecipitates. RAMOS represents immunoprecipitation of a pool of equal amounts of RAMOS-wt and RAMOS-4c lysate. (B) Supernatant lysates removed from rabbit antimouse IgG (cont) or anti-ERK2 immunoprecipitations of stromal cells after RAMOS-wt contact. (Upper panels) Antiphosphotyrosine immunoblotting. (Lower panels) Anti-ERK2 immunoblotting. (C) Lane 1 (cont) represents control glutathione sepharose (lacking GST-Elk1) incubated with stromal cell lysate. Lanes 2 through 4 represent lysate from stromal cells, stromal cells in contact with RAMOS-wt, and stromal cells in contact with RAMOS-4c subjected to solid-phase kinase assay using GST-Elk1 as a substrate (upper panel) or immunostained with anti-ERK2 (lower panel). For lanes 5 and 6, lysates were precleared by immunoprecipitation with anti-ERK2 (*) before incubation with GST-Elk-1-sepharose. Lane 7 represents Elk1-GST sepharose not incubated with lysate. Autoradiography of γ32P-GST-Elk1 represents 10 minutes of exposure. Results are representative of three (A and B) and two (C) individual experiments.

Contact with RAMOS-wt or RAMOS-4c increases phosphorylation of stromal cell ERK2. Stromal cells were incubated in medium alone (−) or in contact with RAMOS-wt (wt) or RAMOS-4c (4c) for 5 minutes at 37°C. Stromal cells and RAMOS cells were collected separately and lysed as detailed in the Materials and Methods. (A and B) Lysates were incubated with antibody-coated protein A sepharose overnight at 4°C. Sepharose beads were sedimented by centrifugation for 10 seconds. The supernatant lysate was removed from selected samples and then immunoprecipitates were washed, eluted, and electrophoresed. (A) Anti-ERK2 immunoprecipitates. RAMOS represents immunoprecipitation of a pool of equal amounts of RAMOS-wt and RAMOS-4c lysate. (B) Supernatant lysates removed from rabbit antimouse IgG (cont) or anti-ERK2 immunoprecipitations of stromal cells after RAMOS-wt contact. (Upper panels) Antiphosphotyrosine immunoblotting. (Lower panels) Anti-ERK2 immunoblotting. (C) Lane 1 (cont) represents control glutathione sepharose (lacking GST-Elk1) incubated with stromal cell lysate. Lanes 2 through 4 represent lysate from stromal cells, stromal cells in contact with RAMOS-wt, and stromal cells in contact with RAMOS-4c subjected to solid-phase kinase assay using GST-Elk1 as a substrate (upper panel) or immunostained with anti-ERK2 (lower panel). For lanes 5 and 6, lysates were precleared by immunoprecipitation with anti-ERK2 (*) before incubation with GST-Elk-1-sepharose. Lane 7 represents Elk1-GST sepharose not incubated with lysate. Autoradiography of γ32P-GST-Elk1 represents 10 minutes of exposure. Results are representative of three (A and B) and two (C) individual experiments.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal