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Lrp与大肠杆菌dadAX启动子区域的两个位点结合,直接抑制和激活转录。

Lrp binds to two regions in the dadAX promoter region of Escherichia coli to repress and activate transcription directly.

作者信息

Zhi J, Mathew E, Freundlich M

机构信息

Department of Biochemistry and Cell Biology, State University of New York at Stony Brook 11794, USA.

出版信息

Mol Microbiol. 1999 Apr;32(1):29-40. doi: 10.1046/j.1365-2958.1999.01314.x.

Abstract

The dadAX operon is expressed by multiple promoters that are repressed by leucine-responsive regulatory protein (Lrp) and activated by cyclic AMP-CRP. In previous work, we found that alanine or leucine acted as inducers to antagonize Lrp repression of the three major promoters directly. Here, we identify 11 Lrp binding sites located within 350 bp of dad DNA. A mutational analysis, coupled with in vivo and in vitro transcription experiments, indicated that Lrp sites that overlap the dad promoters were involved in repression. In contrast, sites upstream of the promoters did not appear to be necessary for repression, but were required for activation by Lrp plus alanine or leucine of one of the major dad promoters, P2. This activation by alanine or leucine was not simply relief of repression, as P2 transcription from a constitutive template was increased fivefold compared with the basal level of transcription found in the absence of Lrp and the co-activator cyclic AMP-CRP. Alanine or leucine decreased the affinity of Lrp to repressor sites, while having little or no effect on the binding of Lrp to activator sites. This differential effect of alanine and leucine on Lrp binding helps to explain how these modifiers influence both repression and activation of the dad operon.

摘要

dadAX操纵子由多个启动子表达,这些启动子受到亮氨酸响应调节蛋白(Lrp)的抑制,并被环磷酸腺苷 - CRP激活。在先前的研究中,我们发现丙氨酸或亮氨酸作为诱导剂直接拮抗Lrp对三个主要启动子的抑制作用。在此,我们在dad DNA的350 bp范围内鉴定出11个Lrp结合位点。通过突变分析以及体内和体外转录实验表明,与dad启动子重叠的Lrp位点参与抑制作用。相比之下,启动子上游的位点对于抑制作用似乎并非必需,但对于Lrp加丙氨酸或亮氨酸对主要dad启动子之一P2的激活作用是必需的。丙氨酸或亮氨酸的这种激活作用并非简单地解除抑制,因为与在没有Lrp和共激活剂环磷酸腺苷 - CRP时发现的基础转录水平相比,来自组成型模板的P2转录增加了五倍。丙氨酸或亮氨酸降低了Lrp与阻遏位点的亲和力,而对Lrp与激活位点的结合几乎没有影响。丙氨酸和亮氨酸对Lrp结合的这种差异效应有助于解释这些调节剂如何影响dad操纵子的抑制和激活作用。

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