5' flanking and first intron sequences of the human β-actin gene required for efficient promoter activity

Abstract

We have identified a CCAAT box element that is required for the efficient transcription of the human β-actin gene. Both in vivo transient transfection assays in cultured HeLa cells and in vitro run-off transcription assays in HeLa whole cell extracts demonstrated the requirement of this element for efficient promoter activity. A gel mobility shift assay revealed a Hela nuclear factor that specifically interacted with the β-actin CCAAT element in vitro; mutation of the first three base pairs of the CCAAT pentanucleotide abolished binding of this factor. Competition gel shift experiments revealed that three sequence elements located within the β-actin promoter, each containing a CC(A/T)₆GG motif similar to that contained within the c-fos serum response element, were able to bind a different nuclear factor, serum response factor (SRF). One of these CC(A/T)₆GG motifs is contained within a first intron fragment that enhanced transcription from a heterologous promoter in vivo.