Figure 9. Inhibition of ERK and JNK MAPKs partially protects cells from apoptosis induced by the combination of IL-3 and TEL/PDGFβR signals. Cells were incubated in the presence (+ Tet) or absence (– Tet) of 2 μg/mL Tet for 24 hours, washed, and incubated for a further 24 or 48 hours (+ or – Tet) with (A) 20 pg/mL IL-3, (B) 20 pg/mL IL-3 with 10 μM U0126, or (C) 20 pg/mL IL-3 with 5 μM SP600125. Cells were stained for 15 minutes with 10 nM Di0C6 and 10 000 events analyzed per sample by FACS on channel FL1. (D) Bar chart summarizes the effects of TEL/PDGFβR expression on IL-3–induced survival in the presence of U0126 and SP600125. Data from 4 independent experiments using clones TP2 and TP15 were used. Mean and SEM are plotted for each treatment and 2-tailed paired Student t tests were applied to the data and values of significance indicated (P).
Figure 9.

Inhibition of ERK and JNK MAPKs partially protects cells from apoptosis induced by the combination of IL-3 and TEL/PDGFβR signals. Cells were incubated in the presence (+ Tet) or absence (– Tet) of 2 μg/mL Tet for 24 hours, washed, and incubated for a further 24 or 48 hours (+ or – Tet) with (A) 20 pg/mL IL-3, (B) 20 pg/mL IL-3 with 10 μM U0126, or (C) 20 pg/mL IL-3 with 5 μM SP600125. Cells were stained for 15 minutes with 10 nM Di0C6 and 10 000 events analyzed per sample by FACS on channel FL1. (D) Bar chart summarizes the effects of TEL/PDGFβR expression on IL-3–induced survival in the presence of U0126 and SP600125. Data from 4 independent experiments using clones TP2 and TP15 were used. Mean and SEM are plotted for each treatment and 2-tailed paired Student t tests were applied to the data and values of significance indicated (P).

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