Figure 4
Figure 4. Defective hematopoiesis in Eng−/− embryos. (A) Whole E7.5 embryos derived from Eng+/− intercross were plated in M3434 and cultured in a low-oxygen incubator. The number of EryPs was reduced drastically in Eng−/− embryos (43.00 ± 18.2; n = 3) compared with Eng+/− (128.3 ± 31.52; n = 3) embryos (P = .0395 by 1-tailed Student t test). Definitive hematopoietic colonies do not show significant differences at this early time point. (B) YS from WT E9.5 embryos show normal vasculature, full of erythrocytes, whereas YS from Eng−/− embryos present primitive vasculature containing very few RBCs. Severe anemia was also observed in the AGM region of Eng−/− embryos (arrows in bottom panels). (C) The frequency of CD71+Ter119+ cells (erythroblasts) is severely decreased in Eng−/− YS compared with Eng+/− or Eng+/+ YS. **P < .05 and ***P < .01 by ANOVA. (D) qPCR gene-expression analyses in E9.5 YS from WT (+/+; n = 9), heterozygotes (+/−; n = 18), and knockout embryos (−/−; n = 15). Transcripts are normalized to GAPDH. Bars represent average gene expression for each genotype. Error bars indicate the SEM for each genotype. *P < .05 and **P < .01 by ANOVA. (E) E9.5 YS cells from Eng+/− intercrosses were assayed for hematopoietic colony formation. The frequency of GEMM and BFU-E progenitors was decreased significantly in the YS of knockout embryos (−/−; n = 7) compared with heterozygous (+/−; n = 25) or WT (+/+; n = 12). Horizontal bar represents the mean. *P < .05 and **P < .01 by ANOVA. (F) Representative GM, GEMM, and BFU-E colonies are shown at similar magnification (10× objective).

Defective hematopoiesis in Eng−/− embryos. (A) Whole E7.5 embryos derived from Eng+/− intercross were plated in M3434 and cultured in a low-oxygen incubator. The number of EryPs was reduced drastically in Eng−/− embryos (43.00 ± 18.2; n = 3) compared with Eng+/− (128.3 ± 31.52; n = 3) embryos (P = .0395 by 1-tailed Student t test). Definitive hematopoietic colonies do not show significant differences at this early time point. (B) YS from WT E9.5 embryos show normal vasculature, full of erythrocytes, whereas YS from Eng−/− embryos present primitive vasculature containing very few RBCs. Severe anemia was also observed in the AGM region of Eng−/− embryos (arrows in bottom panels). (C) The frequency of CD71+Ter119+ cells (erythroblasts) is severely decreased in Eng−/− YS compared with Eng+/− or Eng+/+ YS. **P < .05 and ***P < .01 by ANOVA. (D) qPCR gene-expression analyses in E9.5 YS from WT (+/+; n = 9), heterozygotes (+/−; n = 18), and knockout embryos (−/−; n = 15). Transcripts are normalized to GAPDH. Bars represent average gene expression for each genotype. Error bars indicate the SEM for each genotype. *P < .05 and **P < .01 by ANOVA. (E) E9.5 YS cells from Eng+/− intercrosses were assayed for hematopoietic colony formation. The frequency of GEMM and BFU-E progenitors was decreased significantly in the YS of knockout embryos (−/−; n = 7) compared with heterozygous (+/−; n = 25) or WT (+/+; n = 12). Horizontal bar represents the mean. *P < .05 and **P < .01 by ANOVA. (F) Representative GM, GEMM, and BFU-E colonies are shown at similar magnification (10× objective).

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