Figure 7
Figure 7. Transduction of CD34+ progenitors with the C/EBP-ϵ32/30 activator isoforms blocks expression of the C/EBP-ϵ14 repressor isoform. CD34+ cells were transduced for 72 hours with the C/EBP-ϵ32/30 (lane 1) or empty GFP (lane 2) retroviral vectors and grown in suspension cultures supplemented with IL-5 to drive eosinophil differentiation. Total protein and RNA was prepared at 14 days from 106 cells lysed in TRIzol (Invitrogen) and analyzed by Western blotting (A) for expression of the C/EBP-ϵ32/30 and ϵ14 isoforms, or semiquantitative RT-PCR (B) for expression of the C/EBP-ϵ14 repressor isoform. Western blotting for GAPDH was used to control for equal protein loading (A), and PCR for β2M was used for comparison of cDNA inputs (B). Vertical lines have been inserted in panel A to indicate repositioned gel lanes.

Transduction of CD34+ progenitors with the C/EBP-ϵ32/30 activator isoforms blocks expression of the C/EBP-ϵ14 repressor isoform. CD34+ cells were transduced for 72 hours with the C/EBP-ϵ32/30 (lane 1) or empty GFP (lane 2) retroviral vectors and grown in suspension cultures supplemented with IL-5 to drive eosinophil differentiation. Total protein and RNA was prepared at 14 days from 106 cells lysed in TRIzol (Invitrogen) and analyzed by Western blotting (A) for expression of the C/EBP-ϵ32/30 and ϵ14 isoforms, or semiquantitative RT-PCR (B) for expression of the C/EBP-ϵ14 repressor isoform. Western blotting for GAPDH was used to control for equal protein loading (A), and PCR for β2M was used for comparison of cDNA inputs (B). Vertical lines have been inserted in panel A to indicate repositioned gel lanes.

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