Synergistic activation of a human promoter in vivo by transcription factor Sp1.

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Mol Cell Biol. 1991 April; 11(4): 1935-1943

Synergistic activation of a human promoter in vivo by transcription factor Sp1.

G M Anderson and S O Freytag

Molecular Biology Research Program, Henry Ford Hospital, Detroit, Michigan 48202.

ABSTRACT

Many eucaryotic promoters contain multiple binding sites forsequence-specific DNA-binding proteins. In some cases, theseproteins have been shown to interact synergistically to activatetranscription. In this study, we address the possibility thatthe transcription factor Sp1 can synergistically activate anative human promoter in a cellular context that closely resemblesthat of a single-copy gene. Using DNase I footprinting withaffinity-purified Sp1, we show that the human argininosuccinatesynthetase (AS) promoter contains three sites that bind Sp1with different affinities. These binding sites were mutatedto abolish Sp1 binding, individually and in all possible combinations,to generate a series of AS promoter-chloramphenicol acetyltransferase(CAT) expression constructs. Mutations designed to increaseSp1 binding were also introduced at each site. The in vivo transcriptionalactivity of these mutant AS promoter-CAT constructs was thenmeasured in stably transfected human RPMI 2650 cell lines. Ourresults show that each of the three Sp1-binding sites contributesto full activation of the human AS promoter and that the relativecontribution of each site correlates well with its in vitroaffinity for Sp1. More importantly, we find that the three Sp1-bindingsites when present in the same promoter activate transcriptionto a level that is 8 times greater than would be expected giventheir individual activities in the absence of the other twosites. Thus, we provide direct evidence that Sp1-binding sitesin their native context in a human promoter can interact synergisticallyin vivo to activate transcription. The ability to activate transcriptionsynergistically may be the reason that many cellular promotershave multiple Sp1-binding sites arranged in tandem and in closeproximity.

Mol Cell Biol. 1991 April; 11(4): 1935-1943

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