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透过镜子:外消旋酶和差向异构酶活性部位对底物和产物的手性识别。

Through the Looking Glass: Chiral Recognition of Substrates and Products at the Active Sites of Racemases and Epimerases.

机构信息

Department of Biochemistry & Molecular Biology, Department of Chemistry, Dalhousie University, Halifax, Nova Scotia, B3H 4R2, Canada.

出版信息

Chemistry. 2020 Aug 17;26(46):10367-10390. doi: 10.1002/chem.201905826. Epub 2020 Jul 21.

Abstract

Unlike most enzymes, which exhibit stereospecific substrate binding, racemases and epimerases bind and catalyze the reversible interconversion of enantiomeric and epimeric pairs of substrates. Over the past 15 years, a growing number of racemase and epimerase structures have been solved, furnishing insights into the nature of chiral recognition of substrates by these enzymes. Those enzymes catalyzing stereoinversion of a carbon acid substrate through a direct 1,1-proton transfer mechanism all bind their substrates in a mirror-image packing orientation. This does not apply generally to racemases and epimerases that use other mechanisms, such as NADH-dependent epimerases that employ a "flipping" mechanism. In general, polar groups are bound and fixed at the three binding determinants on the protein defining a pseudo-mirror plane, while nonpolar groups may be mobile. The hydrogen atoms on each stereocenter are positioned antipodal with respect to the pseudo-mirror plane, making a two-base mechanism imperative. Recognition that mirror-image packing is the common binding mode for enantiomeric or epimeric substrates of these enzymes should inform modelling/docking studies and protein engineering.

摘要

与大多数表现出立体特异性底物结合的酶不同,消旋酶和差向异构酶结合并催化对映体和差向异构体底物对的可逆互变。在过去的 15 年中,越来越多的消旋酶和差向异构酶结构已被阐明,为这些酶对底物的手性识别的本质提供了深入了解。那些通过直接 1,1-质子转移机制催化碳酸底物立体反转的酶都以镜像包装取向结合其底物。这并不适用于使用其他机制(例如依赖 NADH 的差向异构酶使用的“翻转”机制)的消旋酶和差向异构酶。通常,极性基团结合并固定在蛋白质上的三个结合决定因素上,定义了一个拟似镜面,而非极性基团可能是可移动的。每个立体中心上的氢原子相对于拟似镜面呈对映关系,这使得双碱基机制成为必然。认识到这种酶的对映体或差向异构体底物的镜像包装是常见的结合模式,应该为建模/对接研究和蛋白质工程提供信息。

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