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Genomic organization and genomic structural rearrangements of Sphingobium japonicum UT26, an archetypal γ-hexachlorocyclohexane-degrading bacterium.苏云金芽胞杆菌 UT26 的基因组组织和基因组结构重排,这是一种典型的γ-六氯环己烷降解细菌。
Enzyme Microb Technol. 2011 Dec 10;49(6-7):499-508. doi: 10.1016/j.enzmictec.2011.10.005. Epub 2011 Nov 7.
2
Role of IncP-1β plasmids pWDL7::rfp and pNB8c in chloroaniline catabolism as determined by genomic and functional analyses.通过基因组和功能分析确定 IncP-1β 质粒 pWDL7::rfp 和 pNB8c 在氯苯胺代谢中的作用。
Appl Environ Microbiol. 2012 Feb;78(3):828-38. doi: 10.1128/AEM.07480-11. Epub 2011 Nov 18.
3
Opposing effects of DNA on proteolysis of a replication initiator.DNA 对复制起始因子蛋白水解的拮抗作用。
Nucleic Acids Res. 2012 Feb;40(3):1148-59. doi: 10.1093/nar/gkr813. Epub 2011 Oct 5.
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The IncP-1 plasmid backbone adapts to different host bacterial species and evolves through homologous recombination.IncP-1 质粒骨架能够适应不同的宿主细菌物种,并通过同源重组进行进化。
Nat Commun. 2011;2:268. doi: 10.1038/ncomms1267. Epub 2011 Apr 5.
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Replication and partitioning of the broad-host-range plasmid RK2.广泛宿主范围质粒 RK2 的复制和分配。
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6
Shifts in the host range of a promiscuous plasmid through parallel evolution of its replication initiation protein.通过复制起始蛋白的平行进化,使一个混杂质粒的宿主范围发生转变。
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PLoS One. 2010 Mar 22;5(3):e9729. doi: 10.1371/journal.pone.0009729.
9
Comparative genomics of pAKD4, the prototype IncP-1delta plasmid with a complete backbone.pAKD4 的比较基因组学,一个具有完整骨架的原型 IncP-1δ 质粒。
Plasmid. 2010 Mar;63(2):98-107. doi: 10.1016/j.plasmid.2009.11.005. Epub 2009 Dec 16.
10
Conformation of a plasmid replication initiator protein affects its proteolysis by ClpXP system.质粒复制起始蛋白的构象影响其被ClpXP系统的蛋白水解作用。
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长复制起始蛋白和短复制起始蛋白在 IncP-1 质粒命运中的作用。

Roles of long and short replication initiation proteins in the fate of IncP-1 plasmids.

机构信息

Institute for Bioinformatics and Evolutionary Studies, Department of Biological Sciences, University of Idaho, Moscow, Idaho, USA.

出版信息

J Bacteriol. 2012 Mar;194(6):1533-43. doi: 10.1128/JB.06395-11. Epub 2012 Jan 6.

DOI:10.1128/JB.06395-11
PMID:22228734
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3294859/
Abstract

Broad-host-range IncP-1 plasmids generally encode two replication initiation proteins, TrfA1 and TrfA2. TrfA2 is produced from an internal translational start site within trfA1. While TrfA1 was previously shown to be essential for replication in Pseudomonas aeruginosa, its role in other bacteria within its broad host range has not been established. To address the role of TrfA1 and TrfA2 in other hosts, efficiency of transformation, plasmid copy number (PCN), and plasmid stability were first compared between a mini-IncP-1β plasmid and its trfA1 frameshift variant in four phylogenetically distant hosts: Escherichia coli, Pseudomonas putida, Sphingobium japonicum, and Cupriavidus necator. TrfA2 was sufficient for replication in these hosts, but the presence of TrfA1 enhanced transformation efficiency and PCN. However, TrfA1 did not contribute to, and even negatively affected, long-term plasmid persistence. When trfA genes were cloned under a constitutive promoter in the chromosomes of the four hosts, strains expressing either both TrfA1 and TrfA2 or TrfA1 alone, again, generally elicited a higher PCN of an IncP1-β replicon than strains expressing TrfA2 alone. When a single species of TrfA was produced at different concentrations in E. coli cells, TrfA1 maintained a 3- to 4-fold higher PCN than TrfA2 at the same TrfA concentrations, indicating that replication mediated by TrfA1 is more efficient than that by TrfA2. These results suggest that the broad-host-range properties of IncP-1 plasmids are essentially conferred by TrfA2 and the intact replication origin alone but that TrfA1 is nonetheless important to efficiently establish plasmid replication upon transfer into a broad range of hosts.

摘要

广宿主范围的 IncP-1 质粒通常编码两种复制起始蛋白,TrfA1 和 TrfA2。TrfA2 是从 trfA1 内部翻译起始位点产生的。虽然 TrfA1 先前被证明对铜绿假单胞菌的复制是必需的,但它在其广宿主范围内的其他细菌中的作用尚未确定。为了确定 TrfA1 和 TrfA2 在其他宿主中的作用,首先比较了在四个系统发育上相距较远的宿主(大肠杆菌、恶臭假单胞菌、日本食酸菌和铜绿假单胞菌)中的一个小型 IncP-1β 质粒与其 trfA1 移框变体之间的转化效率、质粒拷贝数(PCN)和质粒稳定性。TrfA2 足以在这些宿主中进行复制,但 TrfA1 的存在增强了转化效率和 PCN。然而,TrfA1 并没有促进,甚至反而降低了质粒的长期稳定性。当 trfA 基因在四个宿主的染色体上通过组成型启动子克隆时,表达两种 TrfA1 和 TrfA2 或仅表达 TrfA1 的菌株,再次普遍引起 IncP1-β 复制子的 PCN 高于仅表达 TrfA2 的菌株。当在大肠杆菌细胞中以不同浓度产生单一的 TrfA 时,在相同的 TrfA 浓度下,TrfA1 维持比 TrfA2 高 3-4 倍的 PCN,表明 TrfA1 介导的复制比 TrfA2 更有效。这些结果表明,IncP-1 质粒的广宿主范围特性基本上仅由 TrfA2 和完整的复制起点赋予,但 TrfA1 对于在转移到广泛的宿主时有效地建立质粒复制仍然很重要。