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工程菌催化柠檬酸盐生成衣康酸盐的细胞催化作用。

Cell Catalysis of Citrate to Itaconate by Engineered .

机构信息

School of Chemical Engineering and Technology, Tianjin University, Tianjin 300350, China.

Frontier Science Center for Synthetic Biology and Key Laboratory of Systems Bioengineering (Ministry of Education), Tianjin 300072, China.

出版信息

ACS Synth Biol. 2021 Nov 19;10(11):3017-3027. doi: 10.1021/acssynbio.1c00320. Epub 2021 Oct 27.

DOI:10.1021/acssynbio.1c00320
PMID:34704752
Abstract

Itaconic acid (IA), an important five-carbon unsaturated dicarboxylic acid, is one of the top 12 renewable chemicals with an urgent need to reduce industrial production costs. which possesses the potential for cost-effective bioproduction of chemicals and organic acids due to its ability to grow under open nonsterile conditions and high tolerance to organic acid salts, was genetically engineered and used to produce IA from citrate by a cell catalytic strategy. Here, two essential genes (-aconitate decarboxylase encoding gene and aconitase (ACN) encoding gene ) were introduced into to construct an IA biosynthesis pathway. Further engineering modifications including coexpression of molecular chaperones GroESL, increasing the copy number of the gene encoding rate-limiting enzyme ACN, and weakening the competing pathway were implemented. Under the optimized condition for the cell catalytic system, the engineered strain TAZI-08 produced 451.45 mM (58.73 g/L) IA from 500 mM citrate, with 93.24% conversion in 36 h and a productivity of 1.63 g/(L h). An intermittent feeding strategy further increased the IA titer to 488.86 mM (63.60 g/L). The IA titer and citrate conversion in are the highest among heterologous hosts reported so far, demonstrating that this strain is a suitable chassis for hyperproduction of IA.

摘要

衣康酸(IA)是一种重要的五碳不饱和二羧酸,是 12 种急需降低工业生产成本的可再生化学品之一。由于其能够在开放非无菌条件下生长且对有机酸盐具有高耐受性,因此具有使化学品和有机酸实现经济高效的生物生产的潜力,被遗传工程改造,并通过细胞催化策略从柠檬酸盐生产 IA。在这里,两个必需基因(编码 - 乌头酸脱羧酶的基因和编码 aconitase (ACN) 的基因)被引入到 中,以构建 IA 生物合成途径。进一步进行了工程修饰,包括共表达分子伴侣 GroESL、增加限速酶 ACN 的编码基因的拷贝数以及削弱竞争途径。在细胞催化系统的优化条件下,工程菌株 TAZI-08 从 500mM 柠檬酸盐中生产了 451.45mM(58.73g/L)IA,在 36 小时内转化率为 93.24%,生产率为 1.63g/(L h)。间歇进料策略进一步将 IA 浓度提高到 488.86mM(63.60g/L)。到目前为止,在异源宿主中报告的 IA 浓度和柠檬酸盐转化率最高,表明该菌株是 IA 超生产的合适底盘。

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