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通过转录起始位点的UTP敏感选择与UTP依赖的重复转录来调控大肠杆菌中upp基因的表达。

Regulation of upp expression in Escherichia coli by UTP-sensitive selection of transcriptional start sites coupled with UTP-dependent reiterative transcription.

作者信息

Tu A H, Turnbough C L

机构信息

Department of Microbiology, University of Alabama at Birmingham, 35294, USA.

出版信息

J Bacteriol. 1997 Nov;179(21):6665-73. doi: 10.1128/jb.179.21.6665-6673.1997.

DOI:10.1128/jb.179.21.6665-6673.1997
PMID:9352914
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC179593/
Abstract

Expression of the upp gene of Escherichia coli, which encodes the pyrimidine salvage enzyme uracil phosphoribosyltransferase, is negatively regulated by pyrimidine availability. In this study, we demonstrate that this regulation occurs mainly by UTP-sensitive selection of alternative transcriptional start sites, which produces transcripts that differ in the ability to be productively elongated. The upp initially transcribed region contains the sequence GATTTTTTTTG (nontemplate strand). Transcription is initiated primarily at the first two bases in this sequence, designated G6 and A7 (counting from the promoter -10 region). High intracellular levels of UTP favor initiation at position A7; however, the resulting transcripts are subject to reiterative transcription (i.e., repetitive nucleotide addition) within the run of T residues in the initially transcribed region. The resulting AUUUUn (where n = 1 to >50) transcripts are not extended to include downstream upp sequences. In contrast, low intracellular levels of UTP strongly favor initiation at position G6, which results in transcripts that generally do not engage in reiterative transcription and thus can be normally elongated. This mechanism ensures that high levels of uracil phosphoribosyltransferase are produced only under conditions of pyrimidine limitation. The mechanisms that account for UTP-sensitive start site selection and different fates of upp transcripts, as well as the general use of UTP-dependent reiterative transcription in gene regulation, are discussed in detail.

摘要

大肠杆菌upp基因编码嘧啶补救酶尿嘧啶磷酸核糖基转移酶,其表达受嘧啶可用性的负调控。在本研究中,我们证明这种调控主要通过对替代转录起始位点的UTP敏感性选择来实现,这会产生在有效延伸能力上存在差异的转录本。upp最初转录区域包含序列GATTTTTTTTG(非模板链)。转录主要在该序列的前两个碱基处起始,分别命名为G6和A7(从启动子-10区域开始计数)。细胞内高浓度的UTP有利于在A7位置起始转录;然而,所产生的转录本在最初转录区域的T残基序列内会经历重复转录(即重复添加核苷酸)。所产生的AUUUUn(其中n = 1至>50)转录本不会延伸以包含下游的upp序列。相反,细胞内低浓度的UTP强烈有利于在G6位置起始转录,这会产生通常不会进行重复转录从而能够正常延伸的转录本。这种机制确保只有在嘧啶限制条件下才会产生高水平的尿嘧啶磷酸核糖基转移酶。本文详细讨论了导致UTP敏感性起始位点选择和upp转录本不同命运的机制,以及UTP依赖性重复转录在基因调控中的普遍应用。

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