Figure 6
Figure 6. Primitive erythroid progenitors in murine yolk sac cultures and murine ESC cultures are inhibited after treatment with RA and are increased by DEAB. All statistical analyses used 1-way Student t tests to calculate P values comparing treated groups with the normalized control; *P < .01, **P < .001. (A) Pooled, stage-matched yolk sac explants were cultured in vehicle control, 10−5M AGN193109, 10−5M DEAB, or 10−6M RA, and plated in methylcellulose for colony-forming assays. The data are depicted as mean fold change in comparison to the vehicle control cultures ± SEM. After DEAB treatment, P = .1 for Ery-CFC and P = .08 for BFU-E colonies. For AGN193109 treatment, P = .06 for EryP-CFC and P = .08 for BFU-E colonies. There was no statistical difference in the total number of cells for each treatment. (B) EBs from ESC cultures were incubated in the presence of various concentrations of RA, 10−4M DEAB, or DMSO control, then plated for colony-forming assays as described in “Methods.” (C) 10−6M RA, DEAB, or DMSO was added to EB shaking cultures at various time points between days 2 and 6 of ESC differentiation and washed out after 24 hours of incubation. After the sixth day of ESC differentiation, cells were counted and plated for colony assays.

Primitive erythroid progenitors in murine yolk sac cultures and murine ESC cultures are inhibited after treatment with RA and are increased by DEAB. All statistical analyses used 1-way Student t tests to calculate P values comparing treated groups with the normalized control; *P < .01, **P < .001. (A) Pooled, stage-matched yolk sac explants were cultured in vehicle control, 10−5M AGN193109, 10−5M DEAB, or 10−6M RA, and plated in methylcellulose for colony-forming assays. The data are depicted as mean fold change in comparison to the vehicle control cultures ± SEM. After DEAB treatment, P = .1 for Ery-CFC and P = .08 for BFU-E colonies. For AGN193109 treatment, P = .06 for EryP-CFC and P = .08 for BFU-E colonies. There was no statistical difference in the total number of cells for each treatment. (B) EBs from ESC cultures were incubated in the presence of various concentrations of RA, 10−4M DEAB, or DMSO control, then plated for colony-forming assays as described in “Methods.” (C) 10−6M RA, DEAB, or DMSO was added to EB shaking cultures at various time points between days 2 and 6 of ESC differentiation and washed out after 24 hours of incubation. After the sixth day of ESC differentiation, cells were counted and plated for colony assays.

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