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Pyruvate production using engineered Escherichia coli

机译:使用工程化大肠杆菌生产丙酮酸

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摘要

Pyruvate plays an essential role in the central carbon metabolism of multiple organisms and is used as a raw material in the chemical, biochemical and pharmaceutical industries. To meet demand, large amounts of pyruvate are produced through fermentation processes. Here we describe a simple and efficient method for producing pyruvate in Escherichia coli. To stop carbon flux from pyruvate to fatty acids, the accBC genes, which encode the enzyme that catalyzes the first step of fatty acid biosynthesis and is essential for vegetative growth, were manipulated within the genome; its native promoter was replaced with the tetracycline (or doxycycline)-regulated promoter and the corresponding transcriptional regulator genes. The resulting strain grew normally in the presence of doxycycline, but showed poor growth upon withdrawal of doxycycline. Using this strain, we developed a high pyruvate producing strain (strain LAFCPCPt-accBC-aceE), in which the tetracycline-regulated promoter was also introduced upstream of aceE, and the ackA-pta, adhE, cra, ldhA, pflB and poxB genes were deleted. After determining the optimal culture conditions for this strain, the final pyruvate concentration reached 26.1 g L−1 after 72 h with a theoretical yield of 55.6 %. These levels are high enough to indicate that the developed strain has the potential for application to industrial production of pyruvate.
机译:丙酮酸在多种生物的碳代谢中起着至关重要的作用,并被用作化学,生化和制药行业的原料。为了满足需求,通过发酵过程产生了大量的丙酮酸。在这里,我们描述了一种在大肠杆菌中生产丙酮酸的简单有效的方法。为了阻止从丙酮酸到脂肪酸的碳通量,在基因组内操纵了accBC基因,该基因编码催化脂肪酸生物合成第一步的酶,对营养生长至关重要。其天然启动子被四环素(或强力霉素)调节的启动子和相应的转录调节基因取代。所得菌株在强力霉素存在下正常生长,但在强力霉素停药后生长缓慢。使用该菌株,我们开发了高丙酮酸生产菌株(菌株LAFCPCPt-accBC-aceE),其中四环素调节的启动子也被引入aceE的上游,以及ackA-pta,adhE,cra,ldhA,pflB和poxB基因被删除。在确定了该菌株的最佳培养条件后,丙酮酸的终浓度在72 h后达到26.1 g L -1 ,理论收率为55.6%。这些水平足够高,表明所开发的菌株具有用于丙酮酸工业生产的潜力。

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