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枯草芽孢杆菌色氨酸操纵子转录本中的顺式作用位点调控该操纵子的表达。

cis-acting sites in the transcript of the Bacillus subtilis trp operon regulate expression of the operon.

作者信息

Kuroda M I, Henner D, Yanofsky C

机构信息

Department of Biological Sciences, Stanford University, California 94305-5020.

出版信息

J Bacteriol. 1988 Jul;170(7):3080-8. doi: 10.1128/jb.170.7.3080-3088.1988.

Abstract

Transcription of the trp operon of Bacillus subtilis is regulated by attenuation. A trpE'-'lacZ gene fusion preceded by the wild-type trp promoter-leader region was used to analyze regulation. Overproduction of the trp leader transcript in trans from a multicopy plasmid caused constitutive expression of the chromosomal trpE'-'lacZ fusion, presumably by titrating a negative regulatory factor encoded by the mtr locus. Subsegments of the trp leader region cloned onto the multicopy plasmid were examined for their abilities to elevate beta-galactosidase activity. An RNA segment spanning the portion of the leader transcript that forms the promoter-proximal strand of the proposed antiterminator structure was most active in this trans test. The data suggest that the mtr gene product, when activated by tryptophan, binds to this RNA segment and prevents formation of the antiterminator. In this manner, the trans-acting factor promotes formation of the RNA structure that causes transcription termination. Secondary-structure predictions for the leader segment of the trp operon transcript suggest that if the mtr factor bound this RNA segment in a nonterminated transcript, the ribosome-binding site for the first structural gene, trpE, could be sequestered in a stable RNA structure. We tested this possibility by comparing transcriptional and translational fusions containing the initial segments of the trp operon. Our findings suggest that the mtr product causes both transcription attenuation and inhibition of translation of trpE mRNA. Inhibition of translation initiation would reduce ribosome density on trpE mRNA, perhaps making it more labile. Consistent with this interpretation, the addition of tryptophan to mtr+ cultures increased the rate of trpE'-'lacZ mRNA decay.

摘要

枯草芽孢杆菌色氨酸操纵子的转录受衰减作用调控。利用位于野生型色氨酸启动子-前导区之前的色氨酸E'-乳糖Z基因融合体来分析调控情况。从多拷贝质粒反式过量产生色氨酸前导转录物会导致染色体上色氨酸E'-乳糖Z融合体的组成型表达,推测这是通过滴定由mtr位点编码的负调控因子实现的。对克隆到多拷贝质粒上的色氨酸前导区亚片段提升β-半乳糖苷酶活性的能力进行了检测。在这种反式检测中,跨越前导转录物中形成所提议抗终止子结构的启动子近端链部分的RNA片段最为活跃。数据表明,mtr基因产物在被色氨酸激活后,会与该RNA片段结合并阻止抗终止子的形成。通过这种方式,反式作用因子促进导致转录终止的RNA结构的形成。色氨酸操纵子转录物前导区的二级结构预测表明,如果mtr因子在未终止的转录物中结合该RNA片段,第一个结构基因色氨酸E的核糖体结合位点可能会被隔离在一个稳定的RNA结构中。我们通过比较包含色氨酸操纵子起始片段的转录融合体和平移融合体来检验这种可能性。我们的研究结果表明,mtr产物会导致色氨酸E mRNA的转录衰减和翻译抑制。翻译起始的抑制会降低色氨酸E mRNA上的核糖体密度,可能使其更不稳定。与这种解释一致的是,向mtr+培养物中添加色氨酸会增加色氨酸E'-乳糖Z mRNA的降解速率。

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