Figure 3
Figure 3. Abnormally accelerated apoptosis of Eμ-myc/bcl-2−/− B cells in culture. Survival assays were performed on purified populations of preneoplastic bone marrow–derived pro-B (Ly5.2+ B220+ sIg− c-Kit+) or pre-B cells (Ly5.2+ B220+ sIg− c-Kit−) and splenic immature (Ly5.2+ B220+ sIgMhi sIgDlo) or mature B lymphocytes (Ly5.2+ B220+ sIgMlo sIgDhi) from mice 8 to 12 weeks following reconstitution with fetal liver cells from wt (▴), bcl-2−/− (▵), Eμ-myc (■), and Eμ-myc/bcl-2−/− (□) E14.5 embryos. The purified donor-derived B-cell populations were cultured in the absence of cytokines for the indicated time periods, and cell viability was measured by staining with PI plus annexin V and FACS analysis. Data represent means ± SEM from 4 to 8 independent experiments for each cell subset and genotype.

Abnormally accelerated apoptosis of Eμ-myc/bcl-2−/− B cells in culture. Survival assays were performed on purified populations of preneoplastic bone marrow–derived pro-B (Ly5.2+ B220+ sIg c-Kit+) or pre-B cells (Ly5.2+ B220+ sIg c-Kit) and splenic immature (Ly5.2+ B220+ sIgMhi sIgDlo) or mature B lymphocytes (Ly5.2+ B220+ sIgMlo sIgDhi) from mice 8 to 12 weeks following reconstitution with fetal liver cells from wt (▴), bcl-2−/− (▵), Eμ-myc (■), and Eμ-myc/bcl-2−/− (□) E14.5 embryos. The purified donor-derived B-cell populations were cultured in the absence of cytokines for the indicated time periods, and cell viability was measured by staining with PI plus annexin V and FACS analysis. Data represent means ± SEM from 4 to 8 independent experiments for each cell subset and genotype.

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