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NMR View: A computer program for the visualization and analysis of NMR data.NMR 视图:用于可视化和分析 NMR 数据的计算机程序。
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(1)H, (13)C and (15)N resonance assignments of the C-terminal domain of HasB, a specific TonB like protein, from Serratia marcescens.粘质沙雷氏菌中一种特定的类托敏B蛋白HasB的C末端结构域的氢、碳-13和氮-15共振归属
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Reactivation of the vanchrobactin siderophore system of Vibrio anguillarum by removal of a chromosomal insertion sequence originated in plasmid pJM1 encoding the anguibactin siderophore system.通过去除源自编码鳗弧菌素铁载体系统的质粒pJM1的染色体插入序列,鳗弧菌的钒弧菌素铁载体系统得以重新激活。
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Structural biology of bacterial iron uptake.细菌铁摄取的结构生物学
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Identification of amino acid residues required for ferric-anguibactin transport in the outer-membrane receptor FatA of Vibrio anguillarum.鉴定鳗弧菌外膜受体FatA中转运铁-鳗弧菌素所需的氨基酸残基。
Microbiology (Reading). 2007 Feb;153(Pt 2):570-584. doi: 10.1099/mic.0.2006/001735-0.
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Bioinformatic analysis of the TonB protein family.托恩B蛋白家族的生物信息学分析
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A novel protein, TtpC, is a required component of the TonB2 complex for specific iron transport in the pathogens Vibrio anguillarum and Vibrio cholerae.一种新型蛋白质TtpC是鳗弧菌和霍乱弧菌病原体中特定铁转运所需的TonB2复合物的组成成分。
J Bacteriol. 2007 Mar;189(5):1803-15. doi: 10.1128/JB.00451-06. Epub 2006 Dec 22.
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Interactions between TonB from Escherichia coli and the periplasmic protein FhuD.大肠杆菌的TonB与周质蛋白FhuD之间的相互作用。
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Structure of TonB in complex with FhuA, E. coli outer membrane receptor.与大肠杆菌外膜受体FhuA结合的TonB的结构
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Outer membrane active transport: structure of the BtuB:TonB complex.外膜主动运输:BtuB与TonB复合物的结构
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鱼类病原菌鳗弧菌中TonB2蛋白的分子特征分析

Molecular characterization of the TonB2 protein from the fish pathogen Vibrio anguillarum.

作者信息

López Claudia S, Peacock R Sean, Crosa Jorge H, Vogel Hans J

机构信息

Department of Molecular Microbiology and Immunology L-220, Oregon Health and Science University, Portland, OR 97239, USA.

出版信息

Biochem J. 2009 Feb 15;418(1):49-59. doi: 10.1042/BJ20081462.

DOI:10.1042/BJ20081462
PMID:18973471
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3032569/
Abstract

In the fish pathogen Vibrio anguillarum the TonB2 protein is essential for the uptake of the indigenous siderophore anguibactin. Here we describe deletion mutants and alanine replacements affecting the final six amino acids of TonB2. Deletions of more than two amino acids of the TonB2 C-terminus abolished ferric-anguibactin transport, whereas replacement of the last three residues resulted in a protein with wild-type transport properties. We have solved the high-resolution solution structure of the TonB2 C-terminal domain by NMR spectroscopy. The core of this domain (residues 121-206) has an alphabetabetaalphabeta structure, whereas residues 76-120 are flexible and extended. This overall folding topology is similar to the Escherichia coli TonB C-terminal domain, albeit with two differences: the beta4 strand found at the C-terminus of TonB is absent in TonB2, and loop 3 is extended by 9 A (0.9 nm) in TonB2. By examining several mutants, we determined that a complete loop 3 is not essential for TonB2 activity. Our results indicate that the beta4 strand of E. coli TonB is not required for activity of the TonB system across Gram-negative bacterial species. We have also determined, through NMR chemical-shift-perturbation experiments, that the E. coli TonB binds in vitro to the TonB box from the TonB2-dependent outer membrane transporter FatA; moreover, it can substitute in vivo for TonB2 during ferric-anguibactin transport in V. anguillarum. Unexpectedly, TonB2 did not bind in vitro to the FatA TonB-box region, suggesting that additional factors may be required to promote this interaction. Overall our results indicate that TonB2 is a representative of a different class of TonB proteins.

摘要

在鱼类病原菌鳗弧菌(Vibrio anguillarum)中,TonB2蛋白对于摄取内源性铁载体鳗弧菌素(anguibactin)至关重要。在此,我们描述了影响TonB2最后六个氨基酸的缺失突变体和丙氨酸替代。TonB2 C末端缺失超过两个氨基酸会消除高铁鳗弧菌素的转运,而替换最后三个残基则产生具有野生型转运特性的蛋白质。我们通过核磁共振光谱法解析了TonB2 C末端结构域的高分辨率溶液结构。该结构域的核心(残基121 - 206)具有αββαβ结构,而残基76 - 120是灵活且伸展的。这种整体折叠拓扑结构与大肠杆菌(Escherichia coli)的TonB C末端结构域相似,尽管存在两个差异:在TonB的C末端发现的β4链在TonB2中不存在,并且在TonB2中3环延伸了9埃(0.9纳米)。通过研究几个突变体,我们确定完整的3环对于TonB2活性并非必需。我们的结果表明,大肠杆菌TonB的β4链对于革兰氏阴性细菌物种中TonB系统的活性不是必需的。我们还通过核磁共振化学位移扰动实验确定,大肠杆菌TonB在体外与来自TonB2依赖性外膜转运蛋白FatA的TonB框结合;此外,在鳗弧菌高铁鳗弧菌素转运过程中,它在体内可以替代TonB2。出乎意料的是,TonB2在体外不与FatA的TonB框区域结合,这表明可能需要其他因素来促进这种相互作用。总体而言,我们的结果表明TonB2是一类不同的TonB蛋白的代表。