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谷氨酸棒杆菌腺苷酸化和非腺苷酸化 P 蛋白 GlnK 的晶体结构。

Crystal structures of adenylylated and unadenylylated P protein GlnK from Corynebacterium glutamicum.

机构信息

Division of Biotechnology, Department of Biology, Friedrich-Alexander-Universität Erlangen-Nürnberg, Henkestrasse 91, 91052 Erlangen, Germany.

Division of Microbiology, Department of Biology, Friedrich-Alexander-Universität Erlangen-Nürnberg, Staudtstrasse 5, 91058 Erlangen, Germany.

出版信息

Acta Crystallogr D Struct Biol. 2021 Mar 1;77(Pt 3):325-335. doi: 10.1107/S2059798321000735. Epub 2021 Feb 19.

Abstract

P proteins are ubiquitous signaling proteins that are involved in the regulation of the nitrogen/carbon balance in bacteria, archaea, and some plants and algae. Signal transduction via P proteins is modulated by effector molecules and post-translational modifications in the P T-loop. Whereas the binding of ADP, ATP and the concomitant binding of ATP and 2-oxoglutarate (2OG) engender two distinct conformations of the T-loop that either favor or disfavor the interaction with partner proteins, the structural consequences of post-translational modifications such as phosphorylation, uridylylation and adenylylation are far less well understood. In the present study, crystal structures of the P protein GlnK from Corynebacterium glutamicum have been determined, namely of adenylylated GlnK (adGlnK) and unmodified unadenylylated GlnK (unGlnK). AdGlnK has been proposed to act as an inducer of the transcription repressor AmtR, and the adenylylation of Tyr51 in GlnK has been proposed to be a prerequisite for this function. The structures of unGlnK and adGlnK allow the first atomic insights into the structural implications of the covalent attachment of an AMP moiety to the T-loop. The overall GlnK fold remains unaltered upon adenylylation, and T-loop adenylylation does not appear to interfere with the formation of the two major functionally important T-loop conformations, namely the extended T-loop in the canonical ADP-bound state and the compacted T-loop that is adopted upon the simultaneous binding of Mg-ATP and 2OG. Thus, the P-typical conformational switching mechanism appears to be preserved in GlnK from C. glutamicum, while at the same time the functional repertoire becomes expanded through the accommodation of a peculiar post-translational modification.

摘要

P 蛋白是普遍存在的信号蛋白,参与调节细菌、古菌以及一些植物和藻类中的氮/碳平衡。P 蛋白的信号转导受效应分子和 P T 环中的翻译后修饰调节。ADP、ATP 的结合以及 ATP 和 2-氧戊二酸(2OG)的同时结合导致 T 环的两种不同构象,这两种构象有利于或不利于与伴侣蛋白相互作用,而翻译后修饰(如磷酸化、尿苷酰化和腺苷酰化)的结构后果则知之甚少。在本研究中,已确定来自谷氨酸棒杆菌的 P 蛋白 GlnK 的晶体结构,即腺苷酸化的 GlnK(adGlnK)和未修饰的非腺苷酸化的 GlnK(unGlnK)。adGlnK 被提议作为转录阻遏物 AmtR 的诱导物,并且 GlnK 中的 Tyr51 的腺苷酸化被提议是该功能的先决条件。unGlnK 和 adGlnK 的结构首次提供了有关 T 环共价连接 AMP 部分的结构影响的原子见解。腺苷酸化后整体 GlnK 折叠保持不变,并且 T 环腺苷酸化似乎不会干扰两种主要功能上重要的 T 环构象的形成,即典型的 ADP 结合的延伸 T 环和同时结合 Mg-ATP 和 2OG 时采用的紧凑 T 环。因此,在来自 C. glutamicum 的 GlnK 中,P 型典型的构象转换机制似乎被保留,而同时通过容纳特殊的翻译后修饰,功能范围得到扩展。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/c981/7919409/c78d8455187f/d-77-00325-fig1.jpg

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