沙眼衣原体rRNA P1启动子的突变分析确定了体外转录的四个重要区域。
Mutational analysis of the Chlamydia trachomatis rRNA P1 promoter defines four regions important for transcription in vitro.
作者信息
Tan M, Gaal T, Gourse R L, Engel J N
机构信息
Department of Medicine, University of California, San Francisco 94143-0654, USA.
出版信息
J Bacteriol. 1998 May;180(9):2359-66. doi: 10.1128/JB.180.9.2359-2366.1998.
Abstract
We have characterized the Chlamydia trachomatis ribosomal promoter, rRNA P1, by measuring the effect of substitutions and deletions on in vitro transcription with partially purified C. trachomatis RNA polymerase. Our analyses indicate that rRNA P1 contains potential -10 and -35 elements, analogous to Escherichia coli promoters recognized by E-sigma70. We identified a novel AT-rich region immediately downstream of the -35 region. The effect of this region was specific for C. trachomatis RNA polymerase and strongly attenuated by single G or C substitutions. Upstream of the -35 region was an AT-rich sequence that enhanced transcription by C. trachomatis and E. coli RNA polymerases. We propose that this region functions as an UP element.
摘要
我们通过测定部分纯化的沙眼衣原体RNA聚合酶对体外转录中替换和缺失的影响,对沙眼衣原体核糖体启动子rRNA P1进行了特性分析。我们的分析表明,rRNA P1含有类似于被E-sigma70识别的大肠杆菌启动子的潜在-10和-35元件。我们在-35区域下游立即鉴定出一个新的富含AT的区域。该区域的作用对沙眼衣原体RNA聚合酶具有特异性,并因单个G或C替换而强烈减弱。在-35区域上游是一个富含AT的序列,可增强沙眼衣原体和大肠杆菌RNA聚合酶的转录。我们认为该区域起着上游元件(UP元件)的作用。
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