![Fig. 2. SDF-1 counteracts apoptosis-associated nuclear DNA degradation in PB Inc+CD34+ cells. / PB CD34+ cells purified immediately after density gradient separation (Inc−) or after incubation on a plastic support (Inc+) were incubated (1 × 105 cells/mL) under apoptosis-inducing culture conditions (serum- and cytokine-free medium [IMDM]). Freshly isolated cells (A) or cells harvested after a 4-day incubation (B) were processed for apoptosis assessment by “sub-G1 peak” detection as indicated in “Materials and methods.” The biologic effect of SDF-1 on apoptosis was evaluated by adding rhSDF-1α at various concentrations (0.01, 0.05, 0.1, 0.5 ng/mL) to the culture medium. The percentages of sub-G1apoptotic cells shown for each histogram are for one experiment representative of the 3 performed. The logarithm fluorescence of PI is expressed in channel numbers. Maximal effect of SDF-1 was obtained for 0.5 ng/mL in Inc− cells and for 0.05 ng/mL in Inc+ cells.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/99/4/10.1182_blood.v99.4.1117/6/h80422156002.jpeg?Expires=1723232067&Signature=OfJhIArl83tOfSq-at5eVoEqgoiWOXdb2o7~etus3q7TrRSa6oIiIbnc5SZW5YZc5arjgMpnsUt4vOMi12ZIYap42oVLPlZEZix~J2cBMoTbD2CStZjIQJFC~WdVmE9oAtonR-1JOPVY98nihOYb35a9VwAzPj1mlWOc1CLtNvu8ZbgTZX5CZJv3HM1~tidxdGrVAtvJGzOkmiC99INc8~ECnU1sBG878ftMBS5k2By-c8H5Z09So-F1oj6AOsiBIEDTuRcR54IoPtFkf8reEjpiFGwPVAMq5Mtrx73-c7Ae5hYXuHbjl6u6d2zrK8e5SzbmRdGttfmd29vp7HLTmg__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
SDF-1 counteracts apoptosis-associated nuclear DNA degradation in PB Inc+CD34+ cells.
PB CD34+ cells purified immediately after density gradient separation (Inc−) or after incubation on a plastic support (Inc+) were incubated (1 × 105 cells/mL) under apoptosis-inducing culture conditions (serum- and cytokine-free medium [IMDM]). Freshly isolated cells (A) or cells harvested after a 4-day incubation (B) were processed for apoptosis assessment by “sub-G1 peak” detection as indicated in “Materials and methods.” The biologic effect of SDF-1 on apoptosis was evaluated by adding rhSDF-1α at various concentrations (0.01, 0.05, 0.1, 0.5 ng/mL) to the culture medium. The percentages of sub-G1apoptotic cells shown for each histogram are for one experiment representative of the 3 performed. The logarithm fluorescence of PI is expressed in channel numbers. Maximal effect of SDF-1 was obtained for 0.5 ng/mL in Inc− cells and for 0.05 ng/mL in Inc+ cells.
