Figure 6.
Figure 6. Mek1,2 inhibition reverses EpoR-HM erythroblast stage-specific differentiation defects. (A) Bone marrow–derived wt-EpoR, EpoR-HM, and EpoR-H erythroid progenitor cells were cultured for 72 hours in SP34-EX medium containing U0126 (± 10 μM). Expanded erythroblasts then were differentiated (in transferrin, BSA, and insulin-containing medium) with Epo at 2.5 U/mL and U0126 (± 10 μM). At 40 hours of culture, frequencies of high forward-angle light scatter erythroblasts were assayed. Note the reversal of differentiation defects in EpoR-HM erythroblasts as illustrated by U0126-induced decreases in forward scatter (cell size). (B) U0126 reversal of EpoR-HM erythroblast differentiation defects as analyzed by Ter119 and CD71 marker expression. At 40 hours of differentiation, EpoR-HM erythroblasts also exhibited significantly decreased frequencies of Ter119pos erythroblasts specifically within a subpopulation of maturing cells with decreased CD71 expression. U0126 reversed this defect (but had no significant effects on control wt-EpoR cells). (C) U0126 dose-dependent reversal of EpoR-HM erythroblast differentiation defects also was observed based on U0126-dependent increases in frequencies of Ter119pos erythroblasts. (D) U0126 inhibition of ERK1,2 activation in primary wt-EpoR, EpoR-HM, and EpoR-H erythroblasts. The capacity of U0126 to inhibit the Epo-stimulated activation of ERKs was confirmed directly by exposing expanded, Ter119-depleted erythroblast preparations to ± 10 μM U0126. In scatterplots, the numbers in quadrants (clockwise from bottom left) indicate the percentage of CD71negTer119neg, Ter119negCD71pos, CD71posTer119high, and Ter119highCD71neg cells among total live-gated cells. Boxes in each top right quadrant indicate the percentage of CD71highTer119high (top) and CD71lowTer119high (bottom) populations.

Mek1,2 inhibition reverses EpoR-HM erythroblast stage-specific differentiation defects. (A) Bone marrow–derived wt-EpoR, EpoR-HM, and EpoR-H erythroid progenitor cells were cultured for 72 hours in SP34-EX medium containing U0126 (± 10 μM). Expanded erythroblasts then were differentiated (in transferrin, BSA, and insulin-containing medium) with Epo at 2.5 U/mL and U0126 (± 10 μM). At 40 hours of culture, frequencies of high forward-angle light scatter erythroblasts were assayed. Note the reversal of differentiation defects in EpoR-HM erythroblasts as illustrated by U0126-induced decreases in forward scatter (cell size). (B) U0126 reversal of EpoR-HM erythroblast differentiation defects as analyzed by Ter119 and CD71 marker expression. At 40 hours of differentiation, EpoR-HM erythroblasts also exhibited significantly decreased frequencies of Ter119pos erythroblasts specifically within a subpopulation of maturing cells with decreased CD71 expression. U0126 reversed this defect (but had no significant effects on control wt-EpoR cells). (C) U0126 dose-dependent reversal of EpoR-HM erythroblast differentiation defects also was observed based on U0126-dependent increases in frequencies of Ter119pos erythroblasts. (D) U0126 inhibition of ERK1,2 activation in primary wt-EpoR, EpoR-HM, and EpoR-H erythroblasts. The capacity of U0126 to inhibit the Epo-stimulated activation of ERKs was confirmed directly by exposing expanded, Ter119-depleted erythroblast preparations to ± 10 μM U0126. In scatterplots, the numbers in quadrants (clockwise from bottom left) indicate the percentage of CD71negTer119neg, Ter119negCD71pos, CD71posTer119high, and Ter119highCD71neg cells among total live-gated cells. Boxes in each top right quadrant indicate the percentage of CD71highTer119high (top) and CD71lowTer119high (bottom) populations.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal