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Discovery of an Escherichia coli Esterase with High Activity and Enantioselectivity toward 12-O-Isopropylideneglycerol Esters

机译:发现对12-O-异亚丙基甘油酯具有高活性和对映选择性的大肠杆菌酯酶

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摘要

Escherichia coli has been widely used as an expression host for the identification of desired biocatalysts through screening or selection assays. We have previously used E. coli in growth selection and screening assays for identification of Bacillus subtilis lipase variants (located in the periplasm) with improved activity and enantioselectivity toward 1,2-O-isopropylideneglycerol (IPG) esters. In the course of these studies, we discovered that E. coli itself exhibits significant cytoplasmic esterase activity toward IPG esters. In order to identify the enzyme (or enzymes) responsible for this esterase activity, we analyzed eight E. coli knockout strains, in which single esterase genes were deleted, for their ability to hydrolyze IPG butyrate. This approach led to the identification of esterase YbfF as the major E. coli enzyme responsible for the hydrolytic activity toward IPG esters. The gene coding for YbfF was cloned and overexpressed in E. coli, and the corresponding protein was purified and characterized for its biocatalytic performance. YbfF displays a high level of activity toward IPG butyrate and IPG caprylate and prefers the R-enantiomer of these substrates, producing the S-enantiomer of the IPG product with high enantiomeric excess (72 to 94% ee). The enantioselectivity of YbfF for IPG caprylate (E = 40) could be significantly enhanced when using dimethylformamide (DMF) or dimethyl sulfoxide (DMSO) as cosolvents in kinetic resolution experiments. The enzyme also shows high enantioselectivity toward 1-phenylethyl acetate (E ≥ 200), giving the chiral product (R)-1-phenylethanol with >99% ee. The high activity and enantioselectivity of YbfF make it an attractive enzyme for organic synthesis.
机译:大肠杆菌已广泛用作表达宿主,用于通过筛选或选择测定法鉴定所需的生物催化剂。我们以前曾在生长选择和筛选试验中使用大肠杆菌来鉴定枯草芽孢杆菌脂肪酶变体(位于周质中),并具有增强的活性和对1,2-O-异亚丙基甘油(IPG)酯的对映选择性。在这些研究过程中,我们发现大肠杆菌本身对IPG酯表现出显着的细胞质酯酶活性。为了鉴定负责这种酯酶活性的一种或多种酶,我们分析了八种大肠杆菌敲除菌株的水解IPG丁酸酯的能力,其中删除了单个酯酶基因。这种方法导致酯酶YbfF被鉴定为主要的大肠杆菌酶,负责对IPG酯的水解活性。克隆了编码YbfF的基因并在大肠杆菌中过表达,并纯化了相应的蛋白质并对其生物催化性能进行了表征。 YbfF对IPG丁酸酯和IPG辛酸酯显示出高水平的活性,并且偏爱这些底物的R-对映体,从而产生IPG产品的S-对映体,其对映体过量较高(ee为72至94%)。当在动力学拆分实验中使用二甲基甲酰胺(DMF)或二甲基亚砜(DMSO)作为助溶剂时,YbfF对IPG辛酸酯(E = 40)的对映选择性可以大大提高。该酶还显示出对乙酸1-苯乙酯(E≥200)的高对映选择性,从而使手性产物(R)-1-苯乙醇的ee大于99%。 YbfF的高活性和对映选择性使其成为有机合成的诱人酶。

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