Fig. 3.
Fig. 3. KL, as well as FL, are required for optimal proB-cell development from flt3− candidate murine stem cells. Lin−/loSca1+c-kit+ cells were sorted into flt3+ and flt3− populations and cultured in the presence of the indicated cytokines at a density of 1 cell per well. Fifteen to 25 days after initiation of culture, individual colonies were picked and analyzed by flow cytometry to verify the presence of proB-cells, as defined by combined B220 and CD19 expression. No proB-colonies were found in response to KL + IL-7. Results represent the mean (+SEM) of 4 individual experiments. Cells stimulated with an optimal combination of cytokines (KL + FL + MGDF + IL-3 + G-CSF + GM-CSF + Epo) served as a control for total number of in vitro clonogenic progenitors. Three independent single-cell experiments with flt3+ and flt3− cells showed a high cloning frequency, 98 (1)% and 97 (1)%, respectively. Thus, the data are presented as percent B-lymphoid colonies of the total number of clonogenic progenitors.

KL, as well as FL, are required for optimal proB-cell development from flt3 candidate murine stem cells. Lin−/loSca1+c-kit+ cells were sorted into flt3+ and flt3 populations and cultured in the presence of the indicated cytokines at a density of 1 cell per well. Fifteen to 25 days after initiation of culture, individual colonies were picked and analyzed by flow cytometry to verify the presence of proB-cells, as defined by combined B220 and CD19 expression. No proB-colonies were found in response to KL + IL-7. Results represent the mean (+SEM) of 4 individual experiments. Cells stimulated with an optimal combination of cytokines (KL + FL + MGDF + IL-3 + G-CSF + GM-CSF + Epo) served as a control for total number of in vitro clonogenic progenitors. Three independent single-cell experiments with flt3+ and flt3 cells showed a high cloning frequency, 98 (1)% and 97 (1)%, respectively. Thus, the data are presented as percent B-lymphoid colonies of the total number of clonogenic progenitors.

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