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Efficient biosynthesis of 2-keto-D-gluconic acid by fed-batch culture of metabolically engineered Gluconobacter japonicus

机译:代谢工程改造的日本葡糖杆菌的分批补料培养有效合成2-酮-D-葡萄糖酸

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摘要

2-keto-d-gluconic acid (2-KGA) is a key precursor for synthesising vitamin C and isovitamin C. However, phage contamination is as constant problem in industrial production of 2-KGA using Pseudomonas fluorescens. Gluconobacter holds promise for producing 2-KGA due to impressive resistance to hypertonicity and acids, and high utilisation of glucose. In this study, the 2-KGA synthesis pathway was regulated to enhance production of 2-KGA and reduce accumulation of the by-products 5-keto-d-gluconic acid (5-KGA) and d-gluconic acid (D-GA) in the 2-KGA producer Gluconobacter japonicus CGMCC 1.49. Knocking out the ga5dh-1 gene from a competitive pathway and overexpressing the ga2dh-A gene from the 2-KGA synthesis pathway via homologous recombination increased the titre of 2-KGA by 63.81% in shake flasks. Additionally, accumulation of 5-KGA was decreased by 63.52% with the resulting G. japonicas-Δga5dh-1-ga2dh-A strain. Using an intermittent fed-batch mode in a 3 L fermenter, 2-KGA reached 235.3 g L−1 with a 91.1% glucose conversion rate. Scaling up in a 15 L fermenter led to stable 2-KGA titre with productivity of 2.99 g L−1 h−1, 11.99% higher than in the 3 L fermenter, and D-GA and 5-KGA by-products were completely converted to 2-KGA.
机译:2-酮-d-葡萄糖酸(2-KGA)是合成维生素C和异维生素C的关键前体。然而,噬菌体污染是使用荧光假单胞菌(Pseudomonasfluorescens)生产2-KGA的恒定问题。葡糖杆菌由于对高渗性和酸的出色耐受性以及葡萄糖的高利用率而有望生产2-KGA。在这项研究中,调节2-KGA合成途径以提高2-KGA的产量并减少副产物5-酮-d-葡萄糖酸(5-KGA)和d-葡萄糖酸(D-GA)的积累在2-KGA生产者日本葡糖杆菌CGMCC 1.49中。从竞争途径中剔除ga5dh-1基因,并通过同源重组从2-KGA合成途径中过表达ga2dh-A基因,使摇瓶中2-KGA的效价提高了63.81%。另外,得到的日本粳稻-Δga5dh-1-ga2dh-A菌株使5-KGA的积累减少了63.52%。在3 L的发酵罐中使用间歇补料分批模式,2-KGA达到235.3 g L -1 ,葡萄糖转化率为91.1%。在15 L的发酵罐中放大可产生稳定的2-KGA滴度,生产率为2.99 g L -1 h -1 ,比3 L发酵罐高11.99%, D-GA和5-KGA副产物完全转化为2-KGA。

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