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基于 Baeyer-Villiger 单加氧酶的大肠杆菌生物催化剂的工程改造,用于蓖麻油酸大规模生物转化为(Z)-11-(庚酰氧基)十一-9-烯酸。

Engineering of Baeyer-Villiger monooxygenase-based Escherichia coli biocatalyst for large scale biotransformation of ricinoleic acid into (Z)-11-(heptanoyloxy)undec-9-enoic acid.

机构信息

Department of Food Science and Engineering, Ewha Womans University, Seoul 120-750, Republic of Korea.

AP Technology, Suwon, Kyunggi 443-702, Republic of Korea.

出版信息

Sci Rep. 2016 Jun 17;6:28223. doi: 10.1038/srep28223.

DOI:10.1038/srep28223
PMID:27311560
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC4911592/
Abstract

Baeyer-Villiger monooxygenases (BVMOs) are able to catalyze regiospecific Baeyer-Villiger oxygenation of a variety of cyclic and linear ketones to generate the corresponding lactones and esters, respectively. However, the enzymes are usually difficult to express in a functional form in microbial cells and are rather unstable under process conditions hindering their large-scale applications. Thereby, we investigated engineering of the BVMO from Pseudomonas putida KT2440 and the gene expression system to improve its activity and stability for large-scale biotransformation of ricinoleic acid (1) into the ester (i.e., (Z)-11-(heptanoyloxy)undec-9-enoic acid) (3), which can be hydrolyzed into 11-hydroxyundec-9-enoic acid (5) (i.e., a precursor of polyamide-11) and n-heptanoic acid (4). The polyionic tag-based fusion engineering of the BVMO and the use of a synthetic promoter for constitutive enzyme expression allowed the recombinant Escherichia coli expressing the BVMO and the secondary alcohol dehydrogenase of Micrococcus luteus to produce the ester (3) to 85 mM (26.6 g/L) within 5 h. The 5 L scale biotransformation process was then successfully scaled up to a 70 L bioreactor; 3 was produced to over 70 mM (21.9 g/L) in the culture medium 6 h after biotransformation. This study demonstrated that the BVMO-based whole-cell reactions can be applied for large-scale biotransformations.

摘要

拜耶尔-维利格单加氧酶 (BVMO) 能够催化各种环状和线性酮的区域特异性拜耶尔-维利格氧化,分别生成相应的内酯和酯。然而,这些酶通常在微生物细胞中难以以功能性形式表达,并且在过程条件下相当不稳定,这阻碍了它们的大规模应用。因此,我们研究了恶臭假单胞菌 KT2440 的 BVMO 的工程改造和基因表达系统,以提高其活性和稳定性,用于蓖麻油酸(1)大规模生物转化为酯(即(Z)-11-(庚酰氧基)十一-9-烯酸)(3),可水解为 11-羟基十一-9-烯酸(5)(即聚酰胺-11 的前体)和正庚酸(4)。基于聚离子标签的 BVMO 融合工程和使用合成启动子进行组成型酶表达,使表达 BVMO 和微球菌黄色素的仲醇脱氢酶的重组大肠杆菌能够在 5 小时内将酯(3)生产到 85mM(26.6g/L)。然后,将 5L 规模的生物转化过程成功放大到 70L 生物反应器中;在生物转化 6 小时后,培养基中 3 的产量超过 70mM(21.9g/L)。本研究表明,基于 BVMO 的全细胞反应可用于大规模生物转化。

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Efficient Synthesis of Methyl 3-Acetoxypropionate by a Newly Identified Baeyer-Villiger Monooxygenase.新型 Baeyer-Villiger 单加氧酶高效合成 3-乙酰氧基丙酸甲酯。
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