CHARACTERIZATION OF AN R-BINDING SITE MEDIATING THE R-INDUCED ACTIVATION OF THE EPSTEIN-BARR-VIRUS BMLF1 PROMOTER

被引:71
作者
GRUFFAT, H
DURAN, N
BUISSON, M
WILD, F
BUCKLAND, R
SERGEANT, A
机构
[1] ECOLE NORMALE SUPER LYON,VIROL MOLEC LAB,CNRS,UMR 49,46 ALLEE DITALIE,F-69364 LYONS 07,FRANCE
[2] FAC MED ALEXIS CARREL,CNRS,UMR30,LYONS 8,FRANCE
关键词
D O I
10.1128/JVI.66.1.46-52.1992
中图分类号
Q93 [微生物学];
学科分类号
071005 ; 100705 ;
摘要
In cells latently infected with Epstein-Barr virus, the switch from latency to productive infection is linked to the expression of two Epstein-Barr virus transcription factors called EB1 and R. R is an enhancer factor, and an R-responsive element (RRE) has been identified in the BMLF1 promoter. In this study, we have used bidirectional deletion mutagenesis to delineate the BMLF1 RRE (RRE-M) to a 44-bp sequence. We also show that R expressed from a recombinant vaccinia virus protects RRE-M against digestion by DNase I. Using mobility shift assays and dimethyl sulfate interferences, we have characterized the contact points between in vitro-translated R and the DNA. R binds in vitro to one site by simultaneously contacting two sequences within the site, which are separated by 8 bp: 5'-catGTCCCtctatcatGGCGCagac-3'. Site-directed mutagenesis of this sequence completely impaired the binding of R in vitro and rendered the BMLF1 promoter nonresponsive to R. The results suggest that the R-inducible BMLF1 enhancer is composed of a single R-binding site, called RRE-M.
引用
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页码:46 / 52
页数:7
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