Mechanism and Utility of the ATP-Grasp Enzyme BesA for the Synthesis of Non-natural Alkyne-Containing Dipeptides Applicable for Click Chemistry.

IF 3.8 2区生物学 Q2 BIOCHEMISTRY & MOLECULAR BIOLOGY

ACS Chemical Biology Pub Date : 2025-10-05 DOI:10.1021/acschembio.5c00676

Hono Otsuka, Takashi Fujishiro

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引用次数: 0

Abstract

Terminal alkyne-containing biomolecules are key compounds utilized in bioorthogonal chemistry via azide-alkyne cycloaddition click chemistry. Various synthetic strategies for the introduction of the terminal alkyne to biomolecules have been developed; however, an enzymatic terminal alkyne-modifying system is not well-explored because the biosynthetic systems for terminal alkynes are rare. Recently, BesA, a member of the ATP-grasp enzyme family, has been reported to exclusively utilize terminal alkyne-containing l-propargylglycine and l-glutamic acid as substrates in the synthesis of γ-l-glutamyl-l-propargylglycine. Because of its use of the terminal alkyne for click chemistry, a BesA-based catalytic system is regarded as a potentially attractive biocatalyst for the enrichment of terminal alkyne-containing biomolecules. Toward developing BesA-based biocatalysts, it is important to understand the structure-based mechanism of action of BesA, especially recognition of the terminal alkyne. Here, we elucidate the structural basis of BesA for synthesis of γ-l-glutamyl-l-propargylglycine. The X-ray crystal analysis of BesA unveiled a narrow substrate-binding cleft, beside Y33, R50, R365, and R404 as conserved residues among BesA enzymes from Streptomyces, as the active site for binding of two amino acids, l-propargylglycine and l-glutamic acid. In particular, the region beside Y33 is likely to accommodate the terminal alkyne of l-propargylglycine via CH-π interaction based on the dipeptide-docking simulation of BesA and the results of the activity assay of the BesA Y33A variant. Furthermore, we demonstrate a BesA-catalyzed conjugation system for the synthesis of non-natural alkyne-containing dipeptides. The BesA R50A variant showed a little activity for ligation between l-propargylglycine and 1-methyl-l-glutamate, affording 1-methyl-l-glutamyl-l-propargylglycine. Moreover, the BesA wild-type showed activity for ligation of l-homopropargylglycine and l-glutamic acid, yielding γ-l-glutamyl-l-homopropargylglycine. Structural comparison of BesA with proteins that possibly bind the alkynes shows the significance of Tyr in recognition of the alkynes. These findings highlight the usefulness of BesA-based biocatalytic systems in expanding the chemical space of alkyne-containing peptides applicable for click chemistry as well as understanding alkyne recognition by proteins.

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atp -抓取酶BesA合成非天然含炔二肽的机理及应用

末端含炔生物分子是叠氮化物-炔环加成键化学在生物正交化学中应用的关键化合物。将末端炔引入生物分子的各种合成策略已经被开发出来；然而，由于末端炔的生物合成系统很少，酶修饰末端炔的系统尚未得到很好的探索。最近，有报道称，作为atp抓附酶家族的一员，BesA专门利用末端含炔的l-丙氨酸和l-谷氨酸作为底物合成γ-l-谷氨酰基-l-丙氨酸。由于其使用末端炔进行点击化学，基于base的催化体系被认为是一种潜在的有吸引力的富集末端炔生物分子的生物催化剂。在开发BesA基生物催化剂的过程中，了解BesA的结构作用机理，特别是对末端炔的识别是十分重要的。在此，我们阐明了合成γ-l-谷氨酰胺-l-丙基甘氨酸的BesA的结构基础。x射线晶体分析发现，在链霉菌BesA酶的保守残基Y33、R50、R365和R404旁边，有一个狭窄的底物结合间隙，是结合l-丙基甘氨酸和l-谷氨酸两种氨基酸的活性位点。根据BesA的二肽对接模拟和BesA Y33A变体的活性测定结果，Y33旁边的区域可能通过CH-π相互作用容纳l-丙基甘氨酸的末端炔。此外，我们展示了一个besa催化的偶联体系，用于合成非天然含炔二肽。BesA R50A突变体对l-丙基甘氨酸和1-甲基-l-谷氨酸的连接表现出很小的活性，提供1-甲基-l-谷氨酰胺-l-丙基甘氨酸。此外，BesA野生型具有l-高异丙基甘氨酸和l-谷氨酸的结扎活性，生成γ-l-谷氨酰胺-l-高异丙基甘氨酸。BesA与可能结合炔烃的蛋白的结构比较表明Tyr对炔烃的识别具有重要意义。这些发现突出了基于besa的生物催化系统在扩展可用于点击化学的含炔肽的化学空间以及理解蛋白质对炔的识别方面的有效性。

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来源期刊

ACS Chemical Biology 生物-生化与分子生物学

CiteScore

7.50

自引率

5.00%

发文量

353

审稿时长

3.3 months

期刊介绍： ACS Chemical Biology provides an international forum for the rapid communication of research that broadly embraces the interface between chemistry and biology. The journal also serves as a forum to facilitate the communication between biologists and chemists that will translate into new research opportunities and discoveries. Results will be published in which molecular reasoning has been used to probe questions through in vitro investigations, cell biological methods, or organismic studies. We welcome mechanistic studies on proteins, nucleic acids, sugars, lipids, and nonbiological polymers. The journal serves a large scientific community, exploring cellular function from both chemical and biological perspectives. It is understood that submitted work is based upon original results and has not been published previously.