Transcriptionally active immediate-early protein of pseudorabies virus binds to specific sites on class II gene promoters

Author:

Cromlish W A1,Abmayr S M1,Workman J L1,Horikoshi M1,Roeder R G1

Affiliation:

1. Laboratory of Biochemistry and Molecular Biology, Rockefeller University, New York, New York 10021-6399.

Abstract

In the presence of partially purified pseudorabies virus immediate-early protein, multiple sites of DNase I protection were observed on the adenovirus major late and human hsp 70 promoters. Southwestern (DNA-protein blot) analysis demonstrated that the immediate-early protein bound directly to the sequences contained in these sites. These sequences share only limited homology, differ in their affinities for the immediate-early protein, and are located at different positions on these two promoters. In addition, the site-specific binding of a temperature-sensitive immediate-early protein was eliminated by the same heat treatment which eliminates its transcriptional activating function, whereas the binding of the wild-type protein was unaffected by heat treatment. Thus, site-specific binding requires a functionally active immediate-early protein. Furthermore, immediate-early-protein-dependent in vitro transcription from the major late promoter was preferentially inhibited by oligonucleotides which are homologous to the high-affinity binding sites on the major late or hsp 70 promoters. These observations suggest that transcriptional stimulation by the immediate-early protein involves binding to cis-acting elements.

Publisher

American Society for Microbiology

Subject

Virology,Insect Science,Immunology,Microbiology

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