Figure 4.
Figure 4. Faltered Epo-induced reticulocyte formation in EpoR-HM mice and attenuated maturation of EpoR-HM erythroblasts in vitro. (A) Deficient reticulocyte production in Epo-treated EpoR-HM mice. At 1 and 24 hours, Epo was administered to wt-EpoR, EpoR-HM, and EpoR-H mice (2.5 U/g). On day 5, induced levels of reticulocytes were assayed. Illustrated are representative flow cytometric profiles of thiazole orange staining, together with mean reticulocyte values (± SE) (n = 4 wt-EpoR, EpoR-HM, and EpoR-H mice per group). (B) Attenuated formation of low FALS CD71pos Ter119pos EpoR-HM erythroblasts in vitro. Bone marrow–derived erythroid progenitor cells were expanded for 3 days in SP34-EX medium and were then transferred to differentiation medium (containing Epo, insulin, and transferrin). At 40 hours of culture, frequencies of maturing CD71highTer119pos erythroblasts were analyzed by flow cytometry (Bi, left panels). Maturation was also assessed based on transitions to low side-angle and forward-angle light scatter populations (Bi, right panels). In panel Bii, defects in this transition for EpoR-HM erythroblasts are graphically summarized. The numbers in quadrants (clockwise from bottom left) indicate the percentage of CD71negTer119neg, Ter119negCD71pos, and CD71posTer119high cells among total live-gated cells. Plotted values are mean values plus or minus SE; n = 3 wt-EpoR, EpoR-HM, and EpoR-H mice per group, representative of 3 experiments.

Faltered Epo-induced reticulocyte formation in EpoR-HM mice and attenuated maturation of EpoR-HM erythroblasts in vitro. (A) Deficient reticulocyte production in Epo-treated EpoR-HM mice. At 1 and 24 hours, Epo was administered to wt-EpoR, EpoR-HM, and EpoR-H mice (2.5 U/g). On day 5, induced levels of reticulocytes were assayed. Illustrated are representative flow cytometric profiles of thiazole orange staining, together with mean reticulocyte values (± SE) (n = 4 wt-EpoR, EpoR-HM, and EpoR-H mice per group). (B) Attenuated formation of low FALS CD71pos Ter119pos EpoR-HM erythroblasts in vitro. Bone marrow–derived erythroid progenitor cells were expanded for 3 days in SP34-EX medium and were then transferred to differentiation medium (containing Epo, insulin, and transferrin). At 40 hours of culture, frequencies of maturing CD71highTer119pos erythroblasts were analyzed by flow cytometry (Bi, left panels). Maturation was also assessed based on transitions to low side-angle and forward-angle light scatter populations (Bi, right panels). In panel Bii, defects in this transition for EpoR-HM erythroblasts are graphically summarized. The numbers in quadrants (clockwise from bottom left) indicate the percentage of CD71negTer119neg, Ter119negCD71pos, and CD71posTer119high cells among total live-gated cells. Plotted values are mean values plus or minus SE; n = 3 wt-EpoR, EpoR-HM, and EpoR-H mice per group, representative of 3 experiments.

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