Figure 1
Figure 1. Cbfb-MYH11 causes Cbfb/Runx1 repression–independent defects during primitive hematopoiesis. (A) Representative FACS plots of Ter119 and c-Kit staining of the primitive blood from embryos of the indicated ages and genotypes. Percentage of cells in each gate is given. Line graphs of the percentage (%) of (B) BrdU-positive (+) and (C) annexin V+, 7AAD-low cells in the peripheral blood of littermate embryos of the indicated genotypes and ages. Bar graphs of the percentage of (D) BrdU+ and (E) annexin V+, 7AAD-low cells in the peripheral blood of Cbfb+/+ and Cbfb−/− littermate embryos of the indicated ages. Data from age-matched Cbfb+/MYH1 embryos was included for comparison. *Statistically significant difference (P < .05) compared with Cbfb+/+ embryos; **statistically significant difference (P < .05) compared with Cbfb+/+ and Cbfb−/− embryos. N ≥ 3 for all genotypes and ages. Error bars indicate SD within each genotype.

Cbfb-MYH11 causes Cbfb/Runx1 repression–independent defects during primitive hematopoiesis. (A) Representative FACS plots of Ter119 and c-Kit staining of the primitive blood from embryos of the indicated ages and genotypes. Percentage of cells in each gate is given. Line graphs of the percentage (%) of (B) BrdU-positive (+) and (C) annexin V+, 7AAD-low cells in the peripheral blood of littermate embryos of the indicated genotypes and ages. Bar graphs of the percentage of (D) BrdU+ and (E) annexin V+, 7AAD-low cells in the peripheral blood of Cbfb+/+ and Cbfb−/− littermate embryos of the indicated ages. Data from age-matched Cbfb+/MYH1 embryos was included for comparison. *Statistically significant difference (P < .05) compared with Cbfb+/+ embryos; **statistically significant difference (P < .05) compared with Cbfb+/+ and Cbfb−/− embryos. N ≥ 3 for all genotypes and ages. Error bars indicate SD within each genotype.

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