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肠球菌素 II 型聚酮合酶由 II 型硫酯酶 EncL 引发单元选择的 policing。

Policing starter unit selection of the enterocin type II polyketide synthase by the type II thioesterase EncL.

机构信息

Scripps Institution of Oceanography, University of California San Diego, La Jolla, CA 92093, USA.

出版信息

Bioorg Med Chem. 2011 Nov 15;19(22):6633-8. doi: 10.1016/j.bmc.2011.04.024. Epub 2011 Apr 16.

DOI:10.1016/j.bmc.2011.04.024
PMID:21531566
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3162089/
Abstract

Enterocin is an atypical type II polyketide synthase (PKS) product from the marine actinomycete 'Streptomyces maritimus'. The enterocin biosynthesis gene cluster (enc) codes for proteins involved in the assembly and attachment of the rare benzoate primer that initiates polyketide assembly with the addition of seven malonate molecules and culminates in a Favorskii-like rearrangement of the linear poly-β-ketone to give its distinctive non-aromatic, caged core structure. Fundamental to enterocin biosynthesis, which utilizes a single acyl carrier protein (ACP), EncC, for both priming with benzoate and elongating with malonate, involves maintaining the correct balance of acyl-EncC substrates for efficient polyketide assembly. Here, we report the characterization of EncL as a type II thioesterase that functions to edit starter unit (mis)priming of EncC. We performed a series of in vivo mutational studies, heterologous expression experiments, in vitro reconstitution studies, and Fourier-transform mass spectrometry-monitored competitive enzyme assays that together support the proposed selective hydrolase activity of EncL toward misprimed acetyl-ACP over benzoyl-ACP to facilitate benzoyl priming of the enterocin PKS complex. While this system resembles the R1128 PKS that also utilizes an editing thioesterase (ZhuC) to purge acetate molecules from its initiation module ACP in favor of alkylacyl groups, the enterocin system is distinct in its usage of a single ACP for both priming and elongating reactions with different substrates.

摘要

肠球菌素是一种来自海洋放线菌 '海洋链霉菌' 的非典型 II 型聚酮合酶 (PKS) 产物。肠球菌素生物合成基因簇 (enc) 编码参与组装和附着罕见苯甲酸启动子的蛋白,该启动子通过添加七个丙二酸盐分子引发聚酮体组装,并最终导致线性聚-β-酮发生类似于 Favorskii 的重排,形成其独特的非芳香、笼状核心结构。肠球菌素生物合成的基础是利用单个酰基载体蛋白 (ACP) EncC 进行苯甲酸的初始和丙二酸盐的延伸,这涉及到维持酰基-EncC 底物的正确平衡,以实现有效的聚酮体组装。在这里,我们报告了 EncL 作为 II 型硫酯酶的特性,它可以编辑 EncC 的起始单元(错误)启动。我们进行了一系列体内突变研究、异源表达实验、体外重组研究和傅里叶变换质谱监测的竞争性酶测定,这些研究共同支持了 EncL 对错误启动的乙酰-ACP 相对于苯甲酰-ACP 的选择性水解酶活性,以促进肠球菌素 PKS 复合物的苯甲酰基启动。虽然该系统类似于也利用编辑硫酯酶 (ZhuC) 将乙酸盐分子从其起始模块 ACP 中清除以有利于烷基酰基基团的 R1128 PKS,但肠球菌素系统的独特之处在于它使用单个 ACP 进行不同底物的起始和延伸反应。

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