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本文引用的文献

1
Expression and assembly of a functional type IV secretion system elicit extracytoplasmic and cytoplasmic stress responses in Escherichia coli.功能性IV型分泌系统的表达与组装引发大肠杆菌的胞外和胞质应激反应。
J Bacteriol. 2006 Sep;188(18):6611-21. doi: 10.1128/JB.00632-06.
2
Synergistic effects in mixed Escherichia coli biofilms: conjugative plasmid transfer drives biofilm expansion.混合大肠杆菌生物膜中的协同效应:接合性质粒转移驱动生物膜扩张。
J Bacteriol. 2006 May;188(10):3582-8. doi: 10.1128/JB.188.10.3582-3588.2006.
3
Disarming pathogens--a new approach for antibiotic development.解除病原体武装——抗生素研发的新方法。
N Engl J Med. 2006 Jan 19;354(3):296-7. doi: 10.1056/NEJMcibr054591.
4
Hfq is a regulator of F-plasmid TraJ and TraM synthesis in Escherichia coli.Hfq是大肠杆菌中F质粒TraJ和TraM合成的调节因子。
J Bacteriol. 2006 Jan;188(1):124-31. doi: 10.1128/JB.188.1.124-131.2006.
5
Peptidoglycan degradation by specialized lytic transglycosylases associated with type III and type IV secretion systems.与III型和IV型分泌系统相关的特异性溶菌转糖基酶对肽聚糖的降解作用。
Microbiology (Reading). 2005 Nov;151(Pt 11):3455-3467. doi: 10.1099/mic.0.28141-0.
6
Biogenesis, architecture, and function of bacterial type IV secretion systems.细菌IV型分泌系统的生物发生、结构及功能
Annu Rev Microbiol. 2005;59:451-85. doi: 10.1146/annurev.micro.58.030603.123630.
7
Regulation of traJ transcription in the Salmonella virulence plasmid by strand-specific DNA adenine hemimethylation.沙门氏菌毒力质粒中traJ转录受链特异性DNA腺嘌呤半甲基化调控。
Mol Microbiol. 2005 Sep;57(6):1700-18. doi: 10.1111/j.1365-2958.2005.04788.x.
8
Regulation of finP transcription by DNA adenine methylation in the virulence plasmid of Salmonella enterica.肠炎沙门氏菌毒力质粒中DNA腺嘌呤甲基化对finP转录的调控
J Bacteriol. 2005 Aug;187(16):5691-9. doi: 10.1128/JB.187.16.5691-5699.2005.
9
Mutations in the C-terminal region of TraM provide evidence for in vivo TraM-TraD interactions during F-plasmid conjugation.TraM C 端区域的突变提供了 F 质粒接合过程中体内 TraM 与 TraD 相互作用的证据。
J Bacteriol. 2005 Jul;187(14):4767-73. doi: 10.1128/JB.187.14.4767-4773.2005.
10
The mating pair formation system of conjugative plasmids-A versatile secretion machinery for transfer of proteins and DNA.接合质粒的配对形成系统——用于蛋白质和DNA转移的多功能分泌机制。
Plasmid. 2005 Jul;54(1):1-25. doi: 10.1016/j.plasmid.2005.02.001.

GroEL通过促进激活蛋白TraJ的蛋白水解降解,在应激诱导的细菌接合负调控中起核心作用。

GroEL plays a central role in stress-induced negative regulation of bacterial conjugation by promoting proteolytic degradation of the activator protein TraJ.

作者信息

Zahrl Doris, Wagner Andrea, Tscherner Michael, Koraimann Günther

机构信息

Institut für Molekulare Biowissenschaften, Karl-Franzens-Universität Graz, Universitätsplatz 2, A-8010 Graz, Austria.

出版信息

J Bacteriol. 2007 Aug;189(16):5885-94. doi: 10.1128/JB.00005-07. Epub 2007 Jun 22.

DOI:10.1128/JB.00005-07
PMID:17586648
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1952051/
Abstract

Transcription of DNA transfer genes is a prerequisite for conjugative DNA transfer of F-like plasmids. Transfer gene expression is sensed by the donor cell and is regulated by a complex network of plasmid- and host-encoded factors. In this study we analyzed the effect of induction of the heat shock regulon on transfer gene expression and DNA transfer in Escherichia coli. Raising the growth temperature from 22 degrees C to 43 degrees C transiently reduced transfer gene expression to undetectable levels and reduced conjugative transfer by 2 to 3 orders of magnitude. In contrast, when host cells carried the temperature-sensitive groEL44 allele, heat shock-mediated repression was alleviated. These data implied that the chaperonin GroEL was involved in negative regulation after heat shock. Investigation of the role of GroEL in this regulatory process revealed that, in groEL(Ts) cells, TraJ, the plasmid-encoded master activator of type IV secretion (T4S) system genes, was less susceptible to proteolysis and had a prolonged half-life compared to isogenic wild-type E. coli cells. This result suggested a direct role for GroEL in proteolysis of TraJ, down-regulation of T4S system gene expression, and conjugation after heat shock. Strong support for this novel role for GroEL in regulation of bacterial conjugation was the finding that GroEL specifically interacted with TraJ in vivo. Our results further suggested that in wild-type cells this interaction was followed by rapid degradation of TraJ whereas in groEL(Ts) cells TraJ remained trapped in the temperature-sensitive GroEL protein and thus was not amenable to proteolysis.

摘要

DNA 转移基因的转录是 F 类质粒接合性 DNA 转移的前提条件。转移基因的表达由供体细胞感知,并受到质粒和宿主编码因子组成的复杂网络的调控。在本研究中,我们分析了热休克调节子的诱导对大肠杆菌中转移基因表达和 DNA 转移的影响。将生长温度从 22℃提高到 43℃会使转移基因表达短暂降低至检测不到的水平,并使接合转移减少 2 至 3 个数量级。相反,当宿主细胞携带温度敏感型 groEL44 等位基因时,热休克介导的抑制作用会得到缓解。这些数据表明伴侣蛋白 GroEL 参与了热休克后的负调控。对 GroEL 在这一调控过程中的作用进行研究发现,在 groEL(Ts)细胞中,与同基因野生型大肠杆菌细胞相比,质粒编码的 IV 型分泌(T4S)系统基因的主激活因子 TraJ 对蛋白水解的敏感性较低,半衰期延长。这一结果表明 GroEL 在热休克后对 TraJ 的蛋白水解、T4S 系统基因表达的下调以及接合过程中发挥直接作用。GroEL 在细菌接合调控中的这一新作用得到了有力支持,即发现 GroEL 在体内与 TraJ 特异性相互作用。我们的结果进一步表明,在野生型细胞中,这种相互作用之后 TraJ 会迅速降解,而在 groEL(Ts)细胞中,TraJ 仍被困在温度敏感型 GroEL 蛋白中,因此不易被蛋白水解。