Figure 2.
Bone marrow-derived Lyn-/-erythroblasts falter in their development to Ter119pos erythroblasts. (A) Defects in Lyn-/- bone marrow-derived erythroblast development at a Ter119pos stage. Following 2.5 days of culture in SP34-EX medium, expanded Lyn+/+ and Lyn-/- erythroid progenitor cells were shifted to a transferrin, insulin, and Epo-containing differentiation medium. At day 1.5, frequencies of maturing erythroblasts were assayed based on Ter119 marker expression (i). Frequencies of CD71highTer119pos copositive cells also were assayed (bottom panels, circled populations). Overall frequencies of Ter119-positive and CD71+ erythroblasts from 3 independent experiments (n = 3 mice per experiment) are also graphed (i; mean ± SE). (B) CD71 and Ter119 marker expression among expanded erythroblasts also was assessed prior to differentiation. During this short-term expansion, marker profiles for Lyn+/+ and Lyn-/- populations were essentially equivalent. (C) Lyn-/- erythroblasts exhibit decreased survival at a Ter119pos stage. Bone marrow-derived erythroblasts from Lyn-/- and Lyn+/+ mice were expanded and shifted to differentiation conditions. At 24 hours of culture, frequencies of annexin V-positive cells among the maturing erythroblasts were assayed. Increased death among Lyn-/- erythroblasts also was confirmed by propidium iodide staining (data not shown). (D) In these cell populations (and at 24 hours of differentiation), levels of Bcl-xL and of activated PY416-p60-Src (p-Src) expression also were analyzed (by Western blotting) together with Lyn and GAPDH.