Downstream deletion analysis of the lac promoter

Author:

Xiong X F1,de la Cruz N1,Reznikoff W S1

Affiliation:

1. Department of Biochemistry, College of Agricultural and Life Science, University of Wisconsin-Madison 53706.

Abstract

We have generated a series of deletions in the downstream region of the lac promoter. The promoter activities of these mutations were compared by measuring the levels of beta-galactosidase gene expression in vivo. Our results show that deletion of downstream lac promoter sequences changes the promoter strength only two- to threefold. The effects of these deletions on transcription initiation site location were studied through primer extension assay of in vivo mRNAs. We found that the transcription start sites are primarily chosen as an approximate distance from the -10 region of the lac promoter; however, starts are sometimes manifested at a GAATT(C) sequence, which is identical to the wild-type preferred start site. lac promoter P2 and a newly identified promoter, P3, are transcribed in vivo at low levels. Catabolite activator protein complexed with cyclic AMP represses P2 and P3 expression in vivo. The secondary catabolite activator protein binding site plays at most a modest role in catabolite repression in vivo.

Publisher

American Society for Microbiology

Subject

Molecular Biology,Microbiology

Reference21 articles.

1. Cyclic AMP receptor protein: role in transcription activation;Crombrugghe B.;Science,1985

2. Mutations in the lac P2 promoter;Donnelly C. E.;J. Bacteriol.,1987

3. Edright R. H. 1982. Sequence homologies in the DNA of six sites known to bind to the catabolite gene activator protein of Escherichia coli p. 91-100. In W. L. Duax and J. F. Griffin (ed.) Molecular structure and biological activity. Elsevier New York.

4. Complication analysis of Escherichia coli promoter DNA sequence;HaIwley D. K.;Nucleic Acids Res.,1983

5. Unidirection digestion with exonuclease III in DNA sequence analysis;Henikoff S.;Methods Enzymol.,1987

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