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pubmed-article:1651407pubmed:abstractTextA detailed mutational analysis of the regulatory DNA sequence elements that control expression of the hepatitis B virus major surface antigen gene was performed in the human hepatoma cell lines HepG2.1 and Huh7, using transient transfection assays. Seven regions (A to G) of the major surface antigen promoter located within 200 nucleotides of the RNA initiation site have been identified which influence the level of transcription from this promoter. The three distal regions (A to C), located between -188 and -68, appear to possess a level of redundancy in their ability to influence the transcriptional activity from the major surface antigen promoter. The simultaneous deletion of regions A, B, and C resulted in an approximately fourfold reduction in transcription from the major surface antigen promoter. Region D, located between -67 and -49, is an essential element of the major surface antigen promoter. The three proximal regions (E to G) are located within 45 nucleotides of the major transcription initiation site. Region E prevents the negative influence of region F and can compensate for the effect of mutation of region G on transcription from the major surface antigen promoter. Region G can compensate for the effect of the loss of a functional region E sequence on the transcriptional activity of the major surface antigen promoter only in the absence of a functional region F sequence. These results imply that the level of expression of the major surface antigen gene is controlled by the complex interplay between a minimum of six transcription factors which activate and one transcription factor which represses transcription from this gene.lld:pubmed
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pubmed-article:1651407pubmed:articleTitleComplex regulation of transcription from the hepatitis B virus major surface antigen promoter in human hepatoma cell lines.lld:pubmed
pubmed-article:1651407pubmed:affiliationDepartment of Molecular and Experimental Medicine, Research Institute of Scripps Clinic, La Jolla, California 92037.lld:pubmed
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pubmed-article:1651407pubmed:publicationTypeResearch Support, U.S. Gov't, P.H.S.lld:pubmed
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