Figure 1.
Figure 1. NK cell and BL differentiation potential of UCB CD34+ HPC populations. Purified UCB CD34+ cells were sorted into CD45RAintCD7- (R1), CD45RAhiCD7- (R2), CD45RAhiCD7+ (R3), CD45RAintCD7+ (R4), and CD45RA-CD7+ (R5) populations and cultured for 21 days with SCF, FL, IL-2, IL-7, and IL-15 (NK condition without MS5). Alternatively, cells were seeded onto MS5 cells with SCF, TPO, and IL-7 and cultured for 14 days (B condition). At the end of the cultures, cells were harvested and labeled with CD56-PE and CD19-FITC mAbs before FACS analysis: histograms and the indicated percentages of specifically labeled cells are based on control mAb labeling. In vitro-generated NK cells were homogeneously CD8+CD56+, whereas a minority of CD10+CD19+ BLs coexpressed CD20. At culture initiation none of the populations tested contained CD56+ cells; CD34+CD19+ pre-B cells represented 6% ± 2% (n = 3) of sorted CD45RAhiCD7- (R2) cells. Data are from 1 of 2 experiments.

NK cell and BL differentiation potential of UCB CD34+ HPC populations. Purified UCB CD34+ cells were sorted into CD45RAintCD7- (R1), CD45RAhiCD7- (R2), CD45RAhiCD7+ (R3), CD45RAintCD7+ (R4), and CD45RA-CD7+ (R5) populations and cultured for 21 days with SCF, FL, IL-2, IL-7, and IL-15 (NK condition without MS5). Alternatively, cells were seeded onto MS5 cells with SCF, TPO, and IL-7 and cultured for 14 days (B condition). At the end of the cultures, cells were harvested and labeled with CD56-PE and CD19-FITC mAbs before FACS analysis: histograms and the indicated percentages of specifically labeled cells are based on control mAb labeling. In vitro-generated NK cells were homogeneously CD8+CD56+, whereas a minority of CD10+CD19+ BLs coexpressed CD20. At culture initiation none of the populations tested contained CD56+ cells; CD34+CD19+ pre-B cells represented 6% ± 2% (n = 3) of sorted CD45RAhiCD7- (R2) cells. Data are from 1 of 2 experiments.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal