Figure 6
Figure 6. Suppression of FANCL expression in human CD34+ cord blood stem and progenitor cells leads to diminished β-catenin activity and multilineage progenitor expansion. (A) Approximately 3000 to 6000 CD34+ cord blood stem and progenitor cells were transduced with scrambled (Scr) or FANCL shRNA and the LEF-TCF-eGFP reporter. Cells were analyzed for eGFP expression after 3 days of puromycin selection (7 days total in culture). Remaining eGFP-positive cells were calculated by multiplying the starting CD34+ cells by the proportion of viable cells and the proportion of eGFP-positive cells. Each data point is expressed relative to the Scr condition. Shown are from 3 independent experiments (except FANCL shRNA construct B) with replicates plotted separately on the graph. The average of the 3 experiments is shown as a horizontal line within the graph. (B) Methylcellulose colony-forming assays were carried out as described. Colony count and type were scored; CFUs, GEMM colonies, and GM colonies. Summarized data are shown for 4 independent experiments (mean ± SEM). There were very few erythroid burst-forming units in these experiments. *Not statistically significant; **P < .04, Student t test. For these studies, transduced CD34+ cells were selected for puromycin resistance. In the colony-forming assays, unselected (no puromycin) cells were also grown to control for any potential effects of viral transduction on cell viability and colony formation that are independent of FANCL suppression.

Suppression of FANCL expression in human CD34+ cord blood stem and progenitor cells leads to diminished β-catenin activity and multilineage progenitor expansion. (A) Approximately 3000 to 6000 CD34+ cord blood stem and progenitor cells were transduced with scrambled (Scr) or FANCL shRNA and the LEF-TCF-eGFP reporter. Cells were analyzed for eGFP expression after 3 days of puromycin selection (7 days total in culture). Remaining eGFP-positive cells were calculated by multiplying the starting CD34+ cells by the proportion of viable cells and the proportion of eGFP-positive cells. Each data point is expressed relative to the Scr condition. Shown are from 3 independent experiments (except FANCL shRNA construct B) with replicates plotted separately on the graph. The average of the 3 experiments is shown as a horizontal line within the graph. (B) Methylcellulose colony-forming assays were carried out as described. Colony count and type were scored; CFUs, GEMM colonies, and GM colonies. Summarized data are shown for 4 independent experiments (mean ± SEM). There were very few erythroid burst-forming units in these experiments. *Not statistically significant; **P < .04, Student t test. For these studies, transduced CD34+ cells were selected for puromycin resistance. In the colony-forming assays, unselected (no puromycin) cells were also grown to control for any potential effects of viral transduction on cell viability and colony formation that are independent of FANCL suppression.

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