Dynamic and balanced regulation of the thrABC operon gene for efficient synthesis of L-threonine

操纵子 苏氨酸 发酵 大肠杆菌 拉伤 生物化学 生物 基因 丝氨酸 磷酸化 解剖
作者
Ruxin Hao,Sumeng Wang,Xin Jin,Xiaoya Yang,Qingsheng Qi,Quanfeng Liang
出处
期刊:Frontiers in Bioengineering and Biotechnology [Frontiers Media SA]
卷期号:11 被引量:7
标识
DOI:10.3389/fbioe.2023.1118948
摘要

L-threonine is an essential amino acid used widely in food, cosmetics, animal feed and medicine. The thrABC operon plays an important role in regulating the biosynthesis of L-theronine. In this work, we systematically analyzed the effects of separating thrAB and thrC in different proportions on strain growth and L-threonine production in Escherichia coli firstly. The results showed that higher expression of thrC than thrAB enhanced cell growth and L-threonine production; however, L-threonine production decreased when the thrC proportion was too high. The highest L-threonine production was achieved when the expression intensity ratio of thrAB to thrC was 3:5. Secondly, a stationary phase promoter was also used to dynamically regulate the expression of engineered thrABC . This strategy improved cell growth and shortened the fermentation period from 36 h to 24 h. Finally, the acetate metabolic overflow was reduced by deleting the ptsG gene, leading to a further increase in L-threonine production. With these efforts, the final strain P 2.1 -2901Δ ptsG reached 40.06 g/L at 60 h fermentation, which was 96.85% higher than the initial control strain TH and the highest reported titer in shake flasks. The maximum L-threonine yield and productivity was obtained in reported fed-batch fermentation, and L-threonine production is close to the highest titer (127.30 g/L). In this work, the expression ratio of genes in the thrABC operon in E. coli was studied systematically, which provided a new approach to improve L-threonine production and its downstream products.
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