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一种催化立体选择性α-和β-酮还原的转酰基转移酶聚酮化合物装配线酶的结构与功能研究

Structural and functional studies of a trans-acyltransferase polyketide assembly line enzyme that catalyzes stereoselective α- and β-ketoreduction.

作者信息

Piasecki Shawn K, Zheng Jianting, Axelrod Abram J, Detelich Madeline E, Keatinge-Clay Adrian T

机构信息

Institute for Cellular and Molecular Biology, The University of Texas at Austin, Texas, 78712.

出版信息

Proteins. 2014 Sep;82(9):2067-77. doi: 10.1002/prot.24561. Epub 2014 Apr 16.

DOI:10.1002/prot.24561
PMID:24634061
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC4142079/
Abstract

While the cis-acyltransferase modular polyketide synthase assembly lines have largely been structurally dissected, enzymes from within the recently discovered trans-acyltransferase polyketide synthase assembly lines are just starting to be observed crystallographically. Here we examine the ketoreductase (KR) from the first polyketide synthase module of the bacillaene nonribosomal peptide synthetase/polyketide synthase at 2.35-Å resolution. This KR naturally reduces both α- and β-keto groups and is the only KR known to do so during the biosynthesis of a polyketide. The isolated KR not only reduced an N-acetylcysteamine-bound β-keto substrate to a D-β-hydroxy product, but also an N-acetylcysteamine-bound α-keto substrate to an L-α-hydroxy product. That the substrates must enter the active site from opposite directions to generate these stereochemistries suggests that the acyl-phosphopantetheine moiety is capable of accessing very different conformations despite being anchored to a serine residue of a docked acyl carrier protein. The features enabling stereocontrolled α-ketoreduction may not be extensive since a KR that naturally reduces a β-keto group within a cis-acyltransferase polyketide synthase was identified that performs a completely stereoselective reduction of the same α-keto substrate to generate the D-α-hydroxy product. A sequence analysis of trans-acyltransferase KRs reveals that a single residue, rather than a three-residue motif found in cis-acyltransferase KRs, is predictive of the orientation of the resulting β-hydroxyl group.

摘要

虽然顺式酰基转移酶模块化聚酮合酶装配线在很大程度上已从结构上进行了解析,但最近发现的反式酰基转移酶聚酮合酶装配线中的酶才刚刚开始通过晶体学进行观察。在此,我们以2.35埃的分辨率研究了杆菌烯非核糖体肽合成酶/聚酮合酶第一个聚酮合酶模块中的酮还原酶(KR)。这种KR能自然地还原α-酮基和β-酮基,是已知在聚酮生物合成过程中唯一能做到这一点的KR。分离出的KR不仅将与N-乙酰半胱胺结合的β-酮底物还原为D-β-羟基产物,还将与N-乙酰半胱胺结合的α-酮底物还原为L-α-羟基产物。底物必须从相反方向进入活性位点才能产生这些立体化学结构,这表明尽管酰基-磷酸泛酰巯基乙胺部分锚定在对接的酰基载体蛋白的丝氨酸残基上,但它仍能够呈现非常不同的构象。实现立体控制的α-酮还原的特征可能并不广泛,因为已鉴定出一种在顺式酰基转移酶聚酮合酶中自然还原β-酮基的KR,它对相同的α-酮底物进行完全立体选择性还原以生成D-α-羟基产物。对反式酰基转移酶KR的序列分析表明,与顺式酰基转移酶KR中发现的三残基基序不同,单个残基可预测所得β-羟基的取向。

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