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哈维氏弧菌LuxN群体感应受体配体特异性的决定因素。

Determinants governing ligand specificity of the Vibrio harveyi LuxN quorum-sensing receptor.

作者信息

Ke Xiaobo, Miller Laura C, Bassler Bonnie L

机构信息

Department of Molecular Biology, Princeton University, Princeton, NJ, 08540, USA.

出版信息

Mol Microbiol. 2015 Jan;95(1):127-42. doi: 10.1111/mmi.12852. Epub 2014 Nov 27.

Abstract

Quorum sensing is a process of bacterial cell-cell communication that relies on the production, release and receptor-driven detection of extracellular signal molecules called autoinducers. The quorum-sensing bacterium Vibrio harveyi exclusively detects the autoinducer N-((R)-3-hydroxybutanoyl)-L-homoserine lactone (3OH-C4 HSL) via the two-component receptor LuxN. To discover the principles underlying the exquisite selectivity LuxN has for its ligand, we identified LuxN mutants with altered specificity. LuxN uses three mechanisms to verify that the bound molecule is the correct ligand: in the context of the overall ligand-binding site, His210 validates the C3 modification, Leu166 surveys the chain-length and a strong steady-state kinase bias imposes an energetic hurdle for inappropriate ligands to elicit signal transduction. Affinities for the LuxN kinase on and kinase off states underpin whether a ligand will act as an antagonist or an agonist. Mutations that bias LuxN to the agonized, kinase off, state are clustered in a region adjacent to the ligand-binding site, suggesting that this region acts as the switch that triggers signal transduction. Together, our analyses illuminate how a histidine sensor kinase differentiates between ligands and exploits those differences to regulate its signaling activity.

摘要

群体感应是细菌细胞间通讯的一个过程,它依赖于被称为自诱导物的细胞外信号分子的产生、释放以及受体驱动的检测。群体感应细菌哈氏弧菌仅通过双组分受体LuxN检测自诱导物N-((R)-3-羟基丁酰基)-L-高丝氨酸内酯(3OH-C4 HSL)。为了发现LuxN对其配体具有高度选择性的潜在原理,我们鉴定了具有改变特异性的LuxN突变体。LuxN使用三种机制来验证结合的分子是正确的配体:在整个配体结合位点的背景下,His210验证C3修饰,Leu166检测链长,并且强烈的稳态激酶偏向性为不适当的配体引发信号转导设置了能量障碍。LuxN激酶的开启状态和关闭状态的亲和力决定了配体将作为拮抗剂还是激动剂起作用。使LuxN偏向于激动的、激酶关闭状态的突变聚集在与配体结合位点相邻的区域,这表明该区域充当触发信号转导的开关。总之,我们的分析阐明了组氨酸传感器激酶如何区分配体并利用这些差异来调节其信号传导活性。

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