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二鸟苷酸环化酶应答调节因子WspR激活与自身抑制的决定因素

Determinants for the activation and autoinhibition of the diguanylate cyclase response regulator WspR.

作者信息

De Nabanita, Navarro Marcos V A S, Raghavan Rahul V, Sondermann Holger

机构信息

Department of Molecular Medicine, College of Veterinary Medicine, Cornell University, Ithaca, NY 14853, USA.

出版信息

J Mol Biol. 2009 Oct 30;393(3):619-33. doi: 10.1016/j.jmb.2009.08.030. Epub 2009 Aug 18.

Abstract

The bacterial second messenger bis-(3'-5')-cyclic dimeric guanosine monophosphate (c-di-GMP) controls secretion, cell adhesion, and motility, leading to biofilm formation and increased cytotoxicity. Diguanylate cyclases containing GGDEF and phosphodiesterases containing EAL or HD-GYP domains have been identified as the enzymes controlling cellular c-di-GMP levels, yet less is known regarding the molecular mechanisms governing regulation and signaling specificity. We recently determined a product-inhibition pathway for the diguanylate cyclase response regulator WspR from Pseudomonas, a potent molecular switch that controls biofilm formation. In WspR, catalytic activity is modulated by a helical stalk motif that connects its phospho-receiver and GGDEF domains. The stalks facilitate the formation of distinct oligomeric states that contribute to both activation and autoinhibition. Here, we provide novel insights into the regulation of diguanylate cyclase activity in WspR based on the crystal structures of full-length WspR, the isolated GGDEF domain, and an artificially dimerized catalytic domain. The structures highlight that inhibition is achieved by restricting the mobility of rigid GGDEF domains, mediated by c-di-GMP binding to an inhibitory site at the GGDEF domain. Kinetic measurements and biochemical characterization corroborate a model in which the activation of WspR requires the formation of a tetrameric species. Tetramerization occurs spontaneously at high protein concentration or upon addition of the phosphomimetic compound beryllium fluoride. Our analyses elucidate common and WspR-specific mechanisms for the fine-tuning of diguanylate cyclase activity.

摘要

细菌第二信使双(3'-5')-环二聚鸟苷单磷酸(c-di-GMP)控制分泌、细胞黏附及运动性,导致生物膜形成并增加细胞毒性。含有GGDEF结构域的二鸟苷酸环化酶和含有EAL或HD-GYP结构域的磷酸二酯酶已被鉴定为控制细胞内c-di-GMP水平的酶,但对于调控和信号特异性的分子机制了解较少。我们最近确定了来自铜绿假单胞菌的二鸟苷酸环化酶应答调节因子WspR的产物抑制途径,WspR是一种控制生物膜形成的有效分子开关。在WspR中,催化活性由连接其磷酸受体和GGDEF结构域的螺旋柄基序调节。柄促进形成不同的寡聚状态,这对激活和自抑制均有贡献。在此,我们基于全长WspR、分离的GGDEF结构域和人工二聚化催化结构域的晶体结构,对WspR中二鸟苷酸环化酶活性的调控提供了新见解。这些结构表明,抑制是通过限制刚性GGDEF结构域的移动性实现的,这由c-di-GMP与GGDEF结构域的抑制位点结合介导。动力学测量和生化特性证实了一个模型,其中WspR的激活需要形成四聚体物种。四聚化在高蛋白浓度下或添加拟磷酸化合物氟化铍后自发发生。我们的分析阐明了二鸟苷酸环化酶活性微调的共同机制和WspR特异性机制。

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