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II类羊毛硫肽合成酶HalM2对底物的识别

Substrate Recognition by the Class II Lanthipeptide Synthetase HalM2.

作者信息

Rahman Imran R, Acedo Jeella Z, Liu Xiaoran Roger, Zhu Lingyang, Arrington Justine, Gross Michael L, van der Donk Wilfred A

机构信息

Department of Biochemistry, University of Illinois at Urbana-Champaign, Urbana, Illinois 61801, United States.

Department of Chemistry and Howard Hughes Medical Institute, University of Illinois at Urbana-Champaign, Urbana, Illinois 61801, United States.

出版信息

ACS Chem Biol. 2020 Jun 19;15(6):1473-1486. doi: 10.1021/acschembio.0c00127. Epub 2020 Apr 28.

DOI:10.1021/acschembio.0c00127
PMID:32293871
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC7305956/
Abstract

Class II lanthipeptides belong to a diverse group of natural products known as ribosomally synthesized and post-translationally modified peptides (RiPPs). Most RiPP precursor peptides contain an N-terminal recognition sequence known as the leader peptide, which is typically recognized by biosynthetic enzymes that catalyze modifications on the C-terminal core peptide. For class II lanthipeptides, these are carried out by a bifunctional lanthipeptide synthetase (LanM) that catalyzes dehydration and cyclization reactions on peptidic substrates to generate thioether-containing, macrocyclic molecules. Some lanthipeptide synthetases are extraordinarily substrate tolerant, making them promising candidates for biotechnological applications such as combinatorial biosynthesis and cyclic peptide library construction. In this study, we characterized the mode of leader peptide recognition by HalM2, the lanthipeptide synthetase responsible for the production of the antimicrobial peptide haloduracin β. Using NMR spectroscopic techniques, binding assays, and enzyme activity assays, we identified substrate residues that are important for binding to HalM2 and for post-translational modification of the peptide substrates. Additionally, we provide evidence of the binding site on the enzyme using binding assays with truncated enzyme variants, hydrogen-deuterium exchange mass spectrometry, and photoaffinity labeling. Understanding the mechanism by which lanthipeptide synthetases recognize their substrate will facilitate their use in biotechnology, as well as further our general understanding of how RiPP enzymes recognize their substrates.

摘要

II类羊毛硫肽属于一类多样的天然产物,称为核糖体合成及翻译后修饰肽(RiPPs)。大多数RiPP前体肽含有一个称为前导肽的N端识别序列,该序列通常被生物合成酶识别,这些酶催化C端核心肽上的修饰。对于II类羊毛硫肽,这些修饰由双功能羊毛硫肽合成酶(LanM)进行,该酶催化肽底物上的脱水和环化反应,以生成含硫醚的大环分子。一些羊毛硫肽合成酶具有极高的底物耐受性,使其成为组合生物合成和环肽库构建等生物技术应用的有前景的候选者。在本研究中,我们表征了负责抗菌肽嗜盐碱菌素β产生的羊毛硫肽合成酶HalM2识别前导肽的模式。使用核磁共振光谱技术、结合测定和酶活性测定,我们鉴定了对于与HalM2结合以及肽底物的翻译后修饰重要的底物残基。此外,我们使用截短的酶变体结合测定、氢-氘交换质谱和光亲和标记提供了酶上结合位点的证据。了解羊毛硫肽合成酶识别其底物的机制将促进其在生物技术中的应用,并进一步加深我们对RiPP酶如何识别其底物的总体理解。

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