Fig. 5. An intact G-CRE is required for Gγ-globin promoter trans-activation.

A) Transient transfection assays were performed with wild type (Gγluc) and mutant Gγluc(m1), Gγluc(m2) and Gγluc(m3) reporter constructs in K562 cells (see Materials). B) Co-transfection studies were performed with the same reporter plasmids tested in Panel A and the pLen-cJun or pCMV-CREB1 expression vectors. The corresponding empty vectors pLen and pCMV were used as respective controls.