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一种将真菌效应蛋白递送入小麦的细菌 III 型分泌系统检测方法。

A bacterial type III secretion assay for delivery of fungal effector proteins into wheat.

出版信息

Mol Plant Microbe Interact. 2014 Mar;27(3):255-64. doi: 10.1094/MPMI-07-13-0187-FI.

DOI:10.1094/MPMI-07-13-0187-FI
PMID:24156769
Abstract

Large numbers of candidate effectors from fungal pathogens are being identified through whole-genome sequencing and in planta expression studies. Although Agrobacterium-mediated transient expression has enabled high-throughput functional analysis of effectors in dicot plants, this assay is not effective in cereal leaves. Here, we show that a nonpathogenic Pseudomonas fluorescens engineered to express the type III secretion system (T3SS) of P. syringae and the wheat pathogen Xanthomonas translucens can deliver fusion proteins containing T3SS signals from P. syringae (AvrRpm1) and X. campestris (AvrBs2) avirulence (Avr) proteins, respectively, into wheat leaf cells. A calmodulin-dependent adenylate cyclase reporter protein was delivered effectively into wheat and barley by both bacteria. Absence of any disease symptoms with P. fluorescens makes it more suitable than X. translucens for detecting a hypersensitive response (HR) induced by an effector protein with avirulence activity. We further modified the delivery system by removal of the myristoylation site from the AvrRpm1 fusion to prevent its localization to the plasma membrane which could inhibit recognition of an Avr protein. Delivery of the flax rust AvrM protein by the modified delivery system into transgenic tobacco leaves expressing the corresponding M resistance protein induced a strong HR, indicating that the system is capable of delivering a functional rust Avr protein. In a preliminary screen of effectors from the stem rust fungus Puccinia graminis f. sp. tritici, we identified one effector that induced a host genotype-specific HR in wheat. Thus, the modified AvrRpm1:effector-Pseudomonas fluorescens system is an effective tool for large-scale screening of pathogen effectors for recognition in wheat.

摘要

通过全基因组测序和体内表达研究,从真菌病原体中鉴定出大量候选效应子。虽然农杆菌介导的瞬时表达能够在双子叶植物中高通量地分析效应子的功能,但该方法在谷类叶片中并不有效。在这里,我们展示了一种经过工程改造的非致病性荧光假单胞菌,该菌能够表达丁香假单胞菌的 III 型分泌系统(T3SS)和小麦病原体黄单胞菌的 Xanthomonas translucens,能够将含有 T3SS 信号的融合蛋白递送到小麦叶片细胞中,分别来自丁香假单胞菌(AvrRpm1)和黄单胞菌(AvrBs2)的无毒(Avr)蛋白。一种钙调蛋白依赖性腺苷酸环化酶报告蛋白被这两种细菌有效地递送到小麦和大麦中。与黄单胞菌相比,荧光假单胞菌没有任何疾病症状,因此更适合检测具有无毒活性的效应蛋白诱导的过敏反应(HR)。我们进一步通过从 AvrRpm1 融合物中去除豆蔻酰化位点来修饰该递送系统,以防止其定位于质膜,这可能会抑制对 Avr 蛋白的识别。通过修饰后的递送系统将亚麻锈菌 AvrM 蛋白递送至表达相应 M 抗性蛋白的转基因烟草叶片中,诱导强烈的 HR,表明该系统能够递送功能性锈菌 Avr 蛋白。在初步筛选来自小麦条锈菌 Puccinia graminis f. sp. tritici 的效应子时,我们鉴定出一种在小麦中诱导宿主基因型特异性 HR 的效应子。因此,修饰后的 AvrRpm1:效应子-荧光假单胞菌系统是一种用于大规模筛选小麦识别的病原体效应子的有效工具。

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