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调控蛋白 HrpG 和 HrpV 在丁香假单胞菌 pv. 番茄 DC3000 中的功能鉴定。

Functional Characterization of Key Residues in Regulatory Proteins HrpG and HrpV of Pseudomonas syringae pv. tomato DC3000.

机构信息

1 Imperial College London, Imperial College Road, London, SW7 2AZ, U.K.

2 Trio Medicines Ltd., Hammersmith Medicines Research, Cumberland Avenue, London, NW10 7EW, U.K.; and.

出版信息

Mol Plant Microbe Interact. 2017 Aug;30(8):656-665. doi: 10.1094/MPMI-03-17-0073-R. Epub 2017 Jun 7.

DOI:10.1094/MPMI-03-17-0073-R
PMID:28488468
Abstract

The plant pathogen Pseudomonas syringae pv. tomato DC3000 uses a type III secretion system (T3SS) to transfer effector proteins into the host. The expression of T3SS proteins is controlled by the HrpL σ factor. Transcription of hrpL is σ-dependent and bacterial enhancer-binding proteins HrpR and HrpS coactivate the hrpL promoter. The HrpV protein imposes negative control upon HrpR and HrpS through direct interaction with HrpS. HrpG interacts with HrpV and relieves such negative control. The sequence alignments across Hrp group I-type plant pathogens revealed conserved HrpV and HrpG amino acids. To establish structure-function relationships in HrpV and HrpG, either truncated or alanine substitution mutants were constructed. Key functional residues in HrpV and HrpG are found within their C-terminal regions. In HrpG, L101 and L105 are indispensable for the ability of HrpG to directly interact with HrpV and suppress HrpV-dependent negative regulation of HrpR and HrpS. In HrpV, L108 and G110 are major determinants for interactions with HrpS and HrpG. We propose that mutually exclusive binding of HrpS and HrpG to the same binding site of HrpV governs a transition from negative control to activation of the HrpRS complex leading to HrpL expression and pathogenicity of P. syringae.

摘要

植物病原菌丁香假单胞菌 pv. 番茄 DC3000 使用 III 型分泌系统(T3SS)将效应蛋白转移到宿主中。T3SS 蛋白的表达受 HrpL σ 因子控制。hrpL 的转录依赖于 σ,细菌增强子结合蛋白 HrpR 和 HrpS 共同激活 hrpL 启动子。HrpV 蛋白通过与 HrpS 的直接相互作用对 HrpR 和 HrpS 施加负调控。HrpG 与 HrpV 相互作用并通过这种负调控。在 Hrp 组 I 型植物病原菌中,序列比对揭示了保守的 HrpV 和 HrpG 氨基酸。为了在 HrpV 和 HrpG 中建立结构-功能关系,构建了截短或丙氨酸取代突变体。HrpV 和 HrpG 中的关键功能残基位于其 C 末端区域内。在 HrpG 中,L101 和 L105 对于 HrpG 直接与 HrpV 相互作用并抑制 HrpV 依赖的 HrpR 和 HrpS 负调控的能力是必不可少的。在 HrpV 中,L108 和 G110 是与 HrpS 和 HrpG 相互作用的主要决定因素。我们提出,HrpS 和 HrpG 对 HrpV 相同结合位点的排他性结合控制着从负调控到 HrpRS 复合物激活的转变,从而导致 hrpL 表达和丁香假单胞菌的致病性。

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