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利用重组谷氨酸棒杆菌从α-酮酸前体生产非蛋白氨基酸。

Production of non-proteinogenic amino acids from α-keto acid precursors with recombinant Corynebacterium glutamicum.

机构信息

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

出版信息

Biotechnol Bioeng. 2013 Nov;110(11):2846-55. doi: 10.1002/bit.24962. Epub 2013 Jun 4.

DOI:10.1002/bit.24962
PMID:23737264
Abstract

In the present work, Corynebacterium glutamicum was metabolically engineered for the enantioselective synthesis of non-proteinogenic amino acids as valuable building blocks for pharmaceuticals and agrochemicals. The novel bio-catalytic activity of C. glutamicum was obtained by heterologous expression of the branched chain aminotransferase IlvE from Escherichia coli. Upon this modification, the recombinant cells converted the α-keto acid precursor 2-(3-hydroxy-1-adamantyl)-2-oxoethanoic acid (HOAE) into the corresponding amino acid 2-(3-hydroxy-1-adamantyl)-(2S)-amino ethanoic acid (HAAE). Similarly, also L-tert-leucine could be obtained from trimethyl pyruvate indicating a broader applicability of the novel strategy. In both cases, the amino group donor glutamate was supplied from the endogenous metabolism of the recombinant producer. Hereby, the uptake of the precursor and secretion of the product was supported by an enhanced cell permeability through treatment of ethambutol, which inhibits arabinosyl transferases involved in cell wall biosynthesis. The excretion of HAAE into the reaction medium was linked to the secretion of glutamate, indicating a similar mechanism for the export of both compounds. On the other hand, the efflux of L-tert-leucine appeared to be driven by active transport. Subsequent bioprocess engineering enabled HAAE and L-tert-leucine to be produced at a rate of 0.21 and 0.42 mmol (g dry cells)⁻¹  h⁻¹, respectively up to a final product titer of 40 mM. Beyond the given examples, integrated metabolic and cell envelop engineering might extend the production of a variety of other non-proteinogenic amino acids as well as chiral amines by C. glutamicum.

摘要

在本工作中,通过异源表达来自大肠杆菌的支链氨基酸转氨酶 IlvE,对谷氨酸棒杆菌进行了代谢工程改造,以用于非蛋白氨基酸的对映选择性合成,这些非蛋白氨基酸可用作药物和农用化学品的有价值的构建模块。经过这种修饰,重组细胞将 α-酮酸前体 2-(3-羟基-1-金刚烷基)-2-氧代乙 酸(HOAE)转化为相应的氨基酸 2-(3-羟基-1-金刚烷基)-(2S)-氨基乙 酸(HAAE)。同样,也可以从三甲基丙酮酸获得 L-叔亮氨酸,表明该新策略具有更广泛的适用性。在这两种情况下,氨基酸供体谷氨酸均来自重组生产菌的内源性代谢。通过乙 胺丁醇处理,增强了细胞通透性,从而支持前体的摄取和产物的分泌,乙 胺丁醇抑制参与细胞壁生物合成的阿拉伯糖基转移酶。HAAE 排泄到反应介质中与谷氨酸的分泌相关,表明这两种化合物的出口机制相似。另一方面,L-叔亮氨酸的外排似乎是由主动运输驱动的。随后的生物过程工程使 HAAE 和 L-叔亮氨酸的生产速率分别达到 0.21 和 0.42 mmol(g 干细胞)⁻¹  h⁻¹,最终产物终浓度达到 40 mM。除了给出的例子之外,综合代谢和细胞膜工程可能会扩展谷氨酸棒杆菌生产各种其他非蛋白氨基酸和手性胺的能力。

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