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Control of the ferric citrate transport system of Escherichia coli: mutations in region 2.1 of the FecI extracytoplasmic-function sigma factor suppress mutations in the FecR transmembrane regulatory protein.大肠杆菌柠檬酸铁转运系统的调控:FecI胞外功能sigma因子2.1区域的突变抑制FecR跨膜调节蛋白中的突变。
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Transcriptional regulation of ferric citrate transport in Escherichia coli K-12. Fecl belongs to a new subfamily of sigma 70-type factors that respond to extracytoplasmic stimuli.大肠杆菌K-12中柠檬酸铁转运的转录调控。Fecl属于响应胞外刺激的σ70型因子的一个新亚家族。
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Sites of interaction between the FecA and FecR signal transduction proteins of ferric citrate transport in Escherichia coli K-12.大肠杆菌K-12中柠檬酸铁转运的FecA和FecR信号转导蛋白之间的相互作用位点。
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Ferric citrate transport of Escherichia coli: functional regions of the FecR transmembrane regulatory protein.大肠杆菌的柠檬酸铁转运:FecR跨膜调节蛋白的功能区域
J Bacteriol. 1998 May;180(9):2387-94. doi: 10.1128/JB.180.9.2387-2394.1998.

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本文引用的文献

1
Surface signaling in ferric citrate transport gene induction: interaction of the FecA, FecR, and FecI regulatory proteins.柠檬酸铁转运基因诱导中的表面信号传导:FecA、FecR和FecI调节蛋白的相互作用。
J Bacteriol. 2000 Feb;182(3):637-46. doi: 10.1128/JB.182.3.637-646.2000.
2
The interface of sigma with core RNA polymerase is extensive, conserved, and functionally specialized.西格玛因子与核心RNA聚合酶的界面广泛、保守且功能特异。
Genes Dev. 1999 Nov 15;13(22):3015-26. doi: 10.1101/gad.13.22.3015.
3
The Escherichia coli sigma(E)-dependent extracytoplasmic stress response is controlled by the regulated proteolysis of an anti-sigma factor.大肠杆菌σ(E) 依赖性胞外应激反应由一种抗σ因子的调控性蛋白酶解作用控制。
Genes Dev. 1999 Sep 15;13(18):2449-61. doi: 10.1101/gad.13.18.2449.
4
Site-directed disulfide bonding reveals an interaction site between energy-coupling protein TonB and BtuB, the outer membrane cobalamin transporter.定点二硫键结合揭示了能量偶联蛋白托蛋白B(TonB)与外膜钴胺素转运蛋白BtuB之间的相互作用位点。
Proc Natl Acad Sci U S A. 1999 Sep 14;96(19):10673-8. doi: 10.1073/pnas.96.19.10673.
5
A mutation in region 1.1 of sigma70 affects promoter DNA binding by Escherichia coli RNA polymerase holoenzyme.σ70 区域 1.1 的突变影响大肠杆菌 RNA 聚合酶全酶与启动子 DNA 的结合。
EMBO J. 1999 Feb 1;18(3):709-16. doi: 10.1093/emboj/18.3.709.
6
Crystal structure of the outer membrane active transporter FepA from Escherichia coli.大肠杆菌外膜活性转运蛋白FepA的晶体结构
Nat Struct Biol. 1999 Jan;6(1):56-63. doi: 10.1038/4931.
7
Transmembrane signaling across the ligand-gated FhuA receptor: crystal structures of free and ferrichrome-bound states reveal allosteric changes.跨配体门控FhuA受体的跨膜信号传导:游离态和铁载体结合态的晶体结构揭示了变构变化。
Cell. 1998 Dec 11;95(6):771-8. doi: 10.1016/s0092-8674(00)81700-6.
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Siderophore-mediated iron transport: crystal structure of FhuA with bound lipopolysaccharide.铁载体介导的铁转运:结合脂多糖的FhuA晶体结构。
Science. 1998 Dec 18;282(5397):2215-20. doi: 10.1126/science.282.5397.2215.
9
Iron regulates transcription of the Escherichia coli ferric citrate transport genes directly and through the transcription initiation proteins.铁直接并通过转录起始蛋白来调节大肠杆菌柠檬酸铁转运基因的转录。
Arch Microbiol. 1998 Jun;169(6):483-90. doi: 10.1007/s002030050600.
10
Ferric citrate transport of Escherichia coli: functional regions of the FecR transmembrane regulatory protein.大肠杆菌的柠檬酸铁转运:FecR跨膜调节蛋白的功能区域
J Bacteriol. 1998 May;180(9):2387-94. doi: 10.1128/JB.180.9.2387-2394.1998.

大肠杆菌柠檬酸铁转运系统的调控:FecI胞外功能sigma因子2.1区域的突变抑制FecR跨膜调节蛋白中的突变。

Control of the ferric citrate transport system of Escherichia coli: mutations in region 2.1 of the FecI extracytoplasmic-function sigma factor suppress mutations in the FecR transmembrane regulatory protein.

作者信息

Stiefel A, Mahren S, Ochs M, Schindler P T, Enz S, Braun V

机构信息

Mikrobiologie/Membranphysiologie, Universität Tübingen, 72076 Tübingen, Germany.

出版信息

J Bacteriol. 2001 Jan;183(1):162-70. doi: 10.1128/JB.183.1.162-170.2001.

DOI:10.1128/JB.183.1.162-170.2001
PMID:11114913
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC94862/
Abstract

Transcription of the ferric citrate transport genes is initiated by binding of ferric citrate to the FecA protein in the outer membrane of Escherichia coli K-12. Bound ferric citrate does not have to be transported but initiates a signal that is transmitted by FecA across the outer membrane and by FecR across the cytoplasmic membrane into the cytoplasm, where the FecI extracytoplasmic-function (ECF) sigma factor becomes active. In this study, we isolated transcription initiation-negative missense mutants in the cytoplasmic region of FecR that were located at four sites, L13Q, W19R, W39R, and W50R, which are highly conserved in FecR-like open reading frames of the Pseudomonas aeruginosa, Pseudomonas putida, Bordetella pertussis, Bordetella bronchiseptica, and Caulobacter crescentus genomes. The cytoplasmic portion of the FecR mutant proteins, FecR(1-85), did not interact with wild-type FecI, in contrast to wild-type FecR(1-85), which induced FecI-mediated fecB transport gene transcription. Two missense mutations in region 2.1 of FecI, S15A and H20E, partially restored induction of ferric citrate transport gene induction of the fecR mutants by ferric citrate. Region 2.1 of sigma(70) is thought to bind RNA polymerase core enzyme; the residual activity of mutated FecI in the absence of FecR, however, was not higher than that of wild-type FecI. In addition, missense mutations in the fecI promoter region resulted in a twofold increased transcription in fecR wild-type cells and a partial restoration of fec transport gene transcription in the fecR mutants. The mutations reduced binding of the Fe(2+) Fur repressor and as a consequence enhanced fecI transcription. The data reveal properties of the FecI ECF factor distinct from those of sigma(70) and further support the novel transcription initiation model in which the cytoplasmic portion of FecR is important for FecI activity.

摘要

柠檬酸铁转运基因的转录是由柠檬酸铁与大肠杆菌K - 12外膜中的FecA蛋白结合启动的。结合的柠檬酸铁不一定被转运,但会启动一个信号,该信号由FecA穿过外膜,并由FecR穿过细胞质膜传递到细胞质中,在细胞质中FecI胞外功能(ECF)σ因子变得活跃。在本研究中,我们在FecR的细胞质区域分离出转录起始阴性错义突变体,这些突变体位于四个位点,即L13Q、W19R、W39R和W50R,它们在铜绿假单胞菌、恶臭假单胞菌、百日咳博德特氏菌、支气管败血博德特氏菌和新月柄杆菌基因组的FecR样开放阅读框中高度保守。与诱导FecI介导的fecB转运基因转录的野生型FecR(1 - 85)相比,FecR突变蛋白FecR(1 - 85)的细胞质部分不与野生型FecI相互作用。FecI第2.1区域的两个错义突变S15A和H20E部分恢复了柠檬酸铁对fecR突变体柠檬酸铁转运基因诱导的诱导作用。σ(70)的第2.1区域被认为与RNA聚合酶核心酶结合;然而,在没有FecR的情况下,突变的FecI的残余活性并不高于野生型FecI。此外,fecI启动子区域的错义突变导致fecR野生型细胞中的转录增加两倍,并使fecR突变体中fec转运基因转录部分恢复。这些突变减少了Fe(2+) Fur阻遏物的结合,从而增强了fecI转录。数据揭示了FecI ECF因子与σ(70)不同的特性,并进一步支持了新的转录起始模型,即FecR的细胞质部分对FecI活性很重要。