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质粒编码的RepA起始蛋白对pPS10宿主范围的调控

Modulation of pPS10 host range by plasmid-encoded RepA initiator protein.

作者信息

Maestro Beatriz, Sanz Jesús M, Díaz-Orejas Ramón, Fernández-Tresguerres Elena

机构信息

Departamento de Microbiología Molecular, Centro de Investigaciones Biológicas, Consejo Superior de Investigaciones Científicas, Madrid, Spain.

出版信息

J Bacteriol. 2003 Feb;185(4):1367-75. doi: 10.1128/JB.185.4.1367-1375.2003.

Abstract

We report here the isolation and analysis of novel repA host range mutants of pPS10, a plasmid originally found in Pseudomonas savastanoi. Upon hydroxylamine treatment, five plasmid mutants were selected for their establishment in Escherichia coli at 37 degrees C, a temperature at which the wild-type form cannot be established. The mutations were located in different functional regions of the plasmid RepA initiation protein, and the mutants differ in their stable maintenance, copy number, and ability to interact with sequences of the basic replicon. Four of them have broadened their host range, and one of them, unable to replicate in Pseudomonas, has therefore changed its host range. Moreover, the mutants also have increased their replication efficiency in strains other than E. coli such as Pseudomonas putida and Alcaligenes faecalis. None of these mutations drastically changed the structure or thermal stability of the wild-type RepA protein, but in all cases an enhanced interaction with host-encoded DnaA protein was detected by gel filtration chromatography. The effects of the mutations on the functionality of RepA protein are discussed in the framework of a three-dimensional model of the protein. We propose possible explanations for the host range effect of the different repA mutants, including the enhancement of limiting interactions of RepA with specific host replication factors such as DnaA.

摘要

我们在此报告了pPS10新型repA宿主范围突变体的分离与分析,pPS10是一种最初在野油菜黄单胞菌中发现的质粒。经羟胺处理后,选择了五个质粒突变体,因为它们能在37℃的大肠杆菌中稳定存在,而野生型在此温度下无法稳定存在。这些突变位于质粒RepA起始蛋白的不同功能区域,突变体在稳定维持、拷贝数以及与基本复制子序列相互作用的能力方面存在差异。其中四个拓宽了宿主范围,还有一个无法在假单胞菌中复制,因此改变了宿主范围。此外,这些突变体在除大肠杆菌外的其他菌株(如恶臭假单胞菌和粪产碱菌)中复制效率也有所提高。这些突变均未显著改变野生型RepA蛋白的结构或热稳定性,但在所有情况下,通过凝胶过滤色谱法均检测到与宿主编码的DnaA蛋白的相互作用增强。在该蛋白的三维模型框架内讨论了这些突变对RepA蛋白功能的影响。我们为不同repA突变体的宿主范围效应提出了可能的解释,包括增强RepA与特定宿主复制因子(如DnaA)的有限相互作用。

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