Fig. 11.
Fig. 11. In vivo transcriptional activation mediated through the −93/−84 binding site correlates with Sp1 expression. Five micrograms of either the −124 promoter-reporter construct (WT) or the −124 XN2mt construct (mut) were cotransfected into SL2 cells in triplicate along with the indicated amounts of either the pPacSp1 expression plasmid or the empty pPacU expression vector. The pCMV βgal plasmid was also cotransfected to normalize for transfection efficiency. Relative reporter activity was calculated as in Fig 4, with the activity of the pGL2:SV40 promoter plasmid assigned a value of 1; error bars indicate ± SE.

In vivo transcriptional activation mediated through the −93/−84 binding site correlates with Sp1 expression. Five micrograms of either the −124 promoter-reporter construct (WT) or the −124 XN2mt construct (mut) were cotransfected into SL2 cells in triplicate along with the indicated amounts of either the pPacSp1 expression plasmid or the empty pPacU expression vector. The pCMV βgal plasmid was also cotransfected to normalize for transfection efficiency. Relative reporter activity was calculated as in Fig 4, with the activity of the pGL2:SV40 promoter plasmid assigned a value of 1; error bars indicate ± SE.

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