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Comparison of proteins involved in pilus synthesis and mating pair stabilization from the related plasmids F and R100-1: insights into the mechanism of conjugation.来自相关质粒F和R100 - 1的菌毛合成及交配配对稳定化相关蛋白质的比较:对接合机制的见解
J Bacteriol. 1999 Sep;181(17):5149-59. doi: 10.1128/JB.181.17.5149-5159.1999.
2
Genetic analysis of the role of the transfer gene, traN, of the F and R100-1 plasmids in mating pair stabilization during conjugation.F质粒和R100 - 1质粒转移基因traN在接合过程中配对稳定作用的遗传分析。
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本文引用的文献

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Conjugal fertility associated with resistance factor R in Escherichia coli.大肠杆菌中与抗性因子R相关的接合生殖力
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2
Resistance transfer agents in Shigella.志贺氏菌中的抗性质粒转移因子
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Regulatory mechanisms in expression of the traY-I operon of sex factor plasmid R100: involvement of traJ and traY gene products.性因子质粒R100的traY-I操纵子表达中的调控机制:traJ和traY基因产物的作用。
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4
Genetic analysis of the role of the transfer gene, traN, of the F and R100-1 plasmids in mating pair stabilization during conjugation.F质粒和R100 - 1质粒转移基因traN在接合过程中配对稳定作用的遗传分析。
J Bacteriol. 1998 Aug;180(16):4036-43. doi: 10.1128/JB.180.16.4036-4043.1998.
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Epitopes fused to F-pilin are incorporated into functional recombinant pili.与F菌毛蛋白融合的表位被整合到功能性重组菌毛中。
J Mol Biol. 1998 Jun 12;279(3):589-603. doi: 10.1006/jmbi.1998.1773.
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Selective phage infection mediated by epitope expression on F pilus.由F菌毛上的表位表达介导的选择性噬菌体感染。
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Filamentous phage infection: required interactions with the TolA protein.丝状噬菌体感染:与TolA蛋白的必要相互作用。
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8
The cytoplasmic DNA-binding protein TraM binds to the inner membrane protein TraD in vitro.细胞质DNA结合蛋白TraM在体外与内膜蛋白TraD结合。
J Bacteriol. 1997 Oct;179(19):6133-7. doi: 10.1128/jb.179.19.6133-6137.1997.
9
TraM of plasmid R1 controls transfer gene expression as an integrated control element in a complex regulatory network.质粒R1的TraM作为复杂调控网络中的一个整合控制元件,控制转移基因的表达。
Mol Microbiol. 1997 Aug;25(3):495-507. doi: 10.1046/j.1365-2958.1997.4831853.x.
10
The C-terminal domain of TolA is the coreceptor for filamentous phage infection of E. coli.TolA的C末端结构域是丝状噬菌体感染大肠杆菌的共受体。
Cell. 1997 Jul 25;90(2):351-60. doi: 10.1016/s0092-8674(00)80342-6.

来自相关质粒F和R100 - 1的菌毛合成及交配配对稳定化相关蛋白质的比较:对接合机制的见解

Comparison of proteins involved in pilus synthesis and mating pair stabilization from the related plasmids F and R100-1: insights into the mechanism of conjugation.

作者信息

Anthony K G, Klimke W A, Manchak J, Frost L S

机构信息

Department of Biological Sciences, University of Alberta, Edmonton, Alberta, Canada T6G 2E9.

出版信息

J Bacteriol. 1999 Sep;181(17):5149-59. doi: 10.1128/JB.181.17.5149-5159.1999.

DOI:10.1128/JB.181.17.5149-5159.1999
PMID:10464182
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC94017/
Abstract

F and R100-1 are closely related, derepressed, conjugative plasmids from the IncFI and IncFII incompatibility groups, respectively. Heteroduplex mapping and genetic analyses have revealed that the transfer regions are extremely similar between the two plasmids. Plasmid specificity can occur at the level of relaxosome formation, regulation, and surface exclusion between the two transfer systems. There are also differences in pilus serology, pilus-specific phage sensitivity, and requirements for OmpA and lipopolysaccharide components in the recipient cell. These phenotypic differences were exploited in this study to yield new information about the mechanism of pilus synthesis, mating pair stabilization, and surface and/or entry exclusion, which are collectively involved in mating pair formation (Mpf). The sequence of the remainder of the transfer region of R100-1 (trbA to traS) has been completed, and the complete sequence is compared to that of F. The differences between the two transfer regions include insertions and deletions, gene duplications, and mosaicism within genes, although the genes essential for Mpf are conserved in both plasmids. F+ cells carrying defined mutations in each of the Mpf genes were complemented with the homologous genes from R100-1. Our results indicate that the specificity in recipient cell recognition and entry exclusion are mediated by TraN and TraG, respectively, and not by the pilus.

摘要

F和R100 - 1是密切相关的、去阻遏的接合质粒,分别来自IncFI和IncFII不相容群。异源双链图谱分析和遗传分析表明,这两种质粒的转移区域极为相似。质粒特异性可能出现在两种转移系统之间的松弛体形成、调控以及表面排斥水平上。在菌毛血清学、菌毛特异性噬菌体敏感性以及受体细胞中对OmpA和脂多糖成分的需求方面也存在差异。本研究利用了这些表型差异,以获取有关菌毛合成机制、交配配对稳定以及表面和/或进入排斥的新信息,这些过程共同参与交配配对形成(Mpf)。R100 - 1转移区域其余部分(trbA至traS)的序列已完成,并将完整序列与F的序列进行了比较。两个转移区域之间的差异包括插入和缺失、基因重复以及基因内的镶嵌现象,尽管对于Mpf至关重要的基因在两种质粒中都是保守的。携带每个Mpf基因特定突变的F + 细胞用来自R100 - 1的同源基因进行了互补。我们的结果表明,受体细胞识别和进入排斥中的特异性分别由TraN和TraG介导,而非由菌毛介导。