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苏氨酸醛缩酶:工程改造及筛选具有增强底物和立体特异性的酶的研究进展

Threonine aldolases: perspectives in engineering and screening the enzymes with enhanced substrate and stereo specificities.

作者信息

Fesko Kateryna

机构信息

Institute of Organic Chemistry, Graz University of Technology, Stremayrgasse 9, A-8010, Graz, Austria.

出版信息

Appl Microbiol Biotechnol. 2016 Mar;100(6):2579-90. doi: 10.1007/s00253-015-7218-5. Epub 2016 Jan 26.

Abstract

Threonine aldolases have emerged as a powerful tool for asymmetric carbon-carbon bond formation. These enzymes catalyse the unnatural aldol condensation of different aldehydes and glycine to produce highly valuable β-hydroxy-α-amino acids with complete stereocontrol at the α-carbon and moderate specificity at the β-carbon. A range of microbial threonine aldolases has been recently recombinantly produced by several groups and their biochemical properties were characterized. Numerous studies have been conducted to improve the reaction protocols to enable higher conversions and investigate the substrate scope of enzymes. However, the application of threonine aldolases in organic synthesis is still limited due to often moderate yields and low diastereoselectivities obtained in the aldol reaction. This review briefly summarizes the screening techniques recently applied to discover novel threonine aldolases as well as enzyme engineering and mutagenesis studies which were accomplished to improve the catalytic activity and substrate specificity. Additionally, the results from new investigations on threonine aldolases including crystal structure determinations and structural-functional characterization are reviewed.

摘要

苏氨酸醛缩酶已成为不对称碳-碳键形成的有力工具。这些酶催化不同醛与甘氨酸的非天然醛醇缩合反应,以产生具有高价值的β-羟基-α-氨基酸,在α-碳上具有完全的立体控制,在β-碳上具有适度的特异性。最近,几个研究小组已经通过重组方式生产了一系列微生物苏氨酸醛缩酶,并对其生化特性进行了表征。已经进行了大量研究来改进反应方案,以实现更高的转化率,并研究酶的底物范围。然而,由于在醛醇反应中常常获得中等产率和低非对映选择性,苏氨酸醛缩酶在有机合成中的应用仍然有限。本文简要总结了最近用于发现新型苏氨酸醛缩酶的筛选技术,以及为提高催化活性和底物特异性而进行的酶工程和诱变研究。此外,还综述了关于苏氨酸醛缩酶的新研究结果,包括晶体结构测定和结构-功能表征。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/ddf0/4761611/a984674a767b/253_2015_7218_Sch1_HTML.jpg

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