Figure 6
Figure 6. Increased caspase activation and apoptosis in Fnip1−/− B cells. (A) Bar graph showing the frequency of dead cells within pro-B (B220lowIgM−CD25−) and pre-B (B220lowIgM−CD25+) populations from Fnip1+/+ and Fnip1−/− mice as measured by DAPI staining. Mean ± SD from 4 independent experiments, (pro-B) P = .1, (pre-B) P < .02, Student t test. (B) Flow cytometric measurement of caspase activity in Fnip1+/+ and Fnip1−/− pre-B cells from interleukin 7 ex vivo cultures. Twenty-four hours after interleukin 7 removal cells were stained with DAPI and FAM, a carboxyfluorescein moiety that becomes covalently linked to the active site of caspases. (C) Flow cytometric analysis of BM and (D) spleen cells from Fnip1−/− mice reconstituted with an Eμ-Bcl2 transgene. BM cells were stained with anti-B220 and anti-IgM antibodies; staining for splenocytes was with anti-CD4 and anti-CD19. Each FACS analysis is representative of 3 independent experiments.

Increased caspase activation and apoptosis in Fnip1−/− B cells. (A) Bar graph showing the frequency of dead cells within pro-B (B220lowIgMCD25) and pre-B (B220lowIgMCD25+) populations from Fnip1+/+ and Fnip1−/− mice as measured by DAPI staining. Mean ± SD from 4 independent experiments, (pro-B) P = .1, (pre-B) P < .02, Student t test. (B) Flow cytometric measurement of caspase activity in Fnip1+/+ and Fnip1−/− pre-B cells from interleukin 7 ex vivo cultures. Twenty-four hours after interleukin 7 removal cells were stained with DAPI and FAM, a carboxyfluorescein moiety that becomes covalently linked to the active site of caspases. (C) Flow cytometric analysis of BM and (D) spleen cells from Fnip1−/− mice reconstituted with an Eμ-Bcl2 transgene. BM cells were stained with anti-B220 and anti-IgM antibodies; staining for splenocytes was with anti-CD4 and anti-CD19. Each FACS analysis is representative of 3 independent experiments.

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