Fig. 7.
Fig. 7. Endogenous SDF-1 improves PB Inc−CD34+ autonomous cell survival. / (A) PB CD34+ cells purified immediately after density gradient separation (Inc−) or (B) after incubation on a plastic support (Inc+) were incubated (1 × 105 cells/mL) for 48 hours under apoptosis-inducing culture conditions (serum- and cytokine-free medium [IMDM]). The role of endogenous SDF-1 was evaluated by adding an anti–SDF-1 neutralizing antibody (10 ng/mL) to the culture. Freshly isolated cells and cells harvested after a 48-hour incubation were processed for apoptosis assessment by using the annexin-V apoptosis detection kit as indicated in “Materials and methods.” The percentages of annexin-V+ PI− apoptotic cells and annexin-V+ PI+ necrotic cells shown for each histogram are for one experiment representative of the 3 performed.

Endogenous SDF-1 improves PB IncCD34+ autonomous cell survival.

(A) PB CD34+ cells purified immediately after density gradient separation (Inc) or (B) after incubation on a plastic support (Inc+) were incubated (1 × 105 cells/mL) for 48 hours under apoptosis-inducing culture conditions (serum- and cytokine-free medium [IMDM]). The role of endogenous SDF-1 was evaluated by adding an anti–SDF-1 neutralizing antibody (10 ng/mL) to the culture. Freshly isolated cells and cells harvested after a 48-hour incubation were processed for apoptosis assessment by using the annexin-V apoptosis detection kit as indicated in “Materials and methods.” The percentages of annexin-V+ PI apoptotic cells and annexin-V+ PI+ necrotic cells shown for each histogram are for one experiment representative of the 3 performed.

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