首页> 美国卫生研究院文献>Proceedings of the National Academy of Sciences of the United States of America >Genetic disassembly and combinatorial reassembly identify a minimal functional repertoire of type III effectors in Pseudomonas syringae
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Genetic disassembly and combinatorial reassembly identify a minimal functional repertoire of type III effectors in Pseudomonas syringae

机译:遗传拆卸和组合重组确定丁香假单胞菌中III型效应子的最小功能库。

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摘要

The virulence of Pseudomonas syringae and many other proteobacterial pathogens is dependent on complex repertoires of effector proteins injected into host cells by type III secretion systems. The 28 well-expressed effector genes in the repertoire of the model pathogen P. syringae pv. tomato DC3000 were deleted to produce polymutant DC3000D28E. Growth of DC3000D28E in Nicotiana benthamiana was symptomless and 4 logs lower than that of DC3000ΔhopQ1-1, which causes disease in this model plant. DC3000D28E seemed functionally effectorless but otherwise WT in diagnostic phenotypes relevant to plant interactions (for example, ability to inject the AvrPto-Cya reporter into N. benthamiana). Various effector genes were integrated by homologous recombination into native loci or by a programmable or random in vivo assembly shuttle (PRIVAS) system into the exchangeable effector locus in the Hrp pathogenicity island of DC3000D28E. The latter method exploited dual adapters and recombination in yeast for efficient assembly of PCR products into programmed or random combinations of multiple effector genes. Native and PRIVAS-mediated integrations were combined to identify a minimal functional repertoire of eight effector genes that restored much of the virulence of DC3000ΔhopQ1-1 in N. benthamiana, revealing a hierarchy in effector function: AvrPtoB acts with priority in suppressing immunity, enabling other effectors to promote further growth (HopM1 and HopE1), chlorosis (HopG1), lesion formation (HopAM1-1), and near full growth and symptom production (AvrE, HopAA1-1, and/or HopN1 functioning synergistically with the previous effectors). DC3000D28E, the PRIVAS method, and minimal functional repertoires provide new resources for probing the plant immune system.
机译:丁香假单胞菌和许多其他变形杆菌病原体的毒力取决于通过III型分泌系统注入宿主细胞的效应蛋白的复杂组成。在模型病原体丁香假单胞菌(P. syringae pv)的库中28个表达良好的效应基因。删除番茄DC3000以产生多突变DC3000D28E。本生烟草中DC3000D28E的生长无症状,比DC3000ΔhopQ1-1的生长低4个对数,从而导致该模型植物的病害。 DC3000D28E似乎在功能上是无作用的,但在与植物相互作用有关的诊断表型方面却是野生型(例如,将AvrPto-Cya报告基因注入本塞姆氏烟草的能力)。通过同源重组将各种效应基因整合到天然基因座中,或通过可编程或随机体内组装穿梭系统(PRIVAS)将其整合到DC3000D28E的Hrp致病岛中的可交换效应基因座中。后一种方法利用双重衔接子并在酵母中重组,以将PCR产物有效组装成多个效应基因的程序或随机组合。结合了天然和PRIVAS介导的整合,以鉴定八个效应基因的最小功能库,这些基因恢复了本氏烟草中DC3000ΔhopQ1-1的大部分毒力,揭示了效应功能的层次:AvrPtoB在抑制免疫力方面具有优先作用,从而使其他促进进一步生长的效应子(HopM1和HopE1),萎黄病(HopG1),病灶形成(HopAM1-1)以及接近完全的生长和症状产生(AvrE,HopAA1-1和/或HopN1与以前的效应子协同作用)。 DC3000D28E,PRIVAS方法和最少的功能库为探索植物免疫系统提供了新资源。

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