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构建一条在大肠杆菌中高效生物合成水杨苷的新途径。

Engineering a novel pathway for efficient biosynthesis of salicin in Escherichia coli.

作者信息

Wang Jingyan, Zhao Qianjing, Chen Xin, Lu Yichen, Sun Xinxiao, Yuan Qipeng, Wang Jia, Shen Xiaolin

机构信息

State Key Laboratory of Chemical Resource Engineering, Beijing University of Chemical Technology, Beijing, 100029, China.

State Key Laboratory of Chemical Resource Engineering, Beijing University of Chemical Technology, Beijing, 100029, China.

出版信息

Metab Eng. 2024 Nov;86:172-180. doi: 10.1016/j.ymben.2024.10.003. Epub 2024 Oct 9.

DOI:10.1016/j.ymben.2024.10.003
PMID:39389256
Abstract

Salicin is a natural glycoside compound widely used to treat fever, inflammation, and analgesia. Currently, salicin is primarily extracted from willow bark, which is not only cumbersome in terms of extraction and separate steps, but also subject to seasonal and geographic limitations. In this study, a highly efficient biosynthetic pathway for salicin synthesis was designed and constructed in E. coli. The most important precursor in the synthetic pathway of salicin designed in this study is salicyl alcohol. Building on a previously constructed biosynthetic salicylic acid metabolic pathway, the production of salicyl alcohol in shake flask fermentation reached 1.7 g/L by increasing the supply of shikimic acid pathway precursor PEP and salicyl alcohol precursor chorismate. According to the principle of substrate similarity, this study identified the key enzyme OsSGT1 from Oryza sativa, which uses E. coli endogenous UDP-glucose as a glycosyl donor to glycosylate salicyl alcohol into salicin. By redefining the optimal substrate of OsSGT1, and balancing metabolic flux along with increasing the supply of UDP-glucose, salicin production in shake flasks reached 4 g/L. Finally, culturing the high-yield strain in a 3-L fermenter resulted in the synthesis of 14.62 g/L of salicin. To the best of our knowledge, this achievement marks the highest salicin production through microbial fermentation to date.

摘要

水杨苷是一种天然糖苷化合物,广泛用于治疗发热、炎症和镇痛。目前,水杨苷主要从柳树皮中提取,这不仅在提取和分离步骤上繁琐,而且受到季节和地理限制。在本研究中,设计并在大肠杆菌中构建了一条用于水杨苷合成的高效生物合成途径。本研究设计的水杨苷合成途径中最重要的前体是水杨醇。基于先前构建的生物合成水杨酸代谢途径,通过增加莽草酸途径前体PEP和水杨醇前体分支酸的供应,摇瓶发酵中水杨醇的产量达到了1.7 g/L。根据底物相似性原理,本研究从水稻中鉴定出关键酶OsSGT1,它利用大肠杆菌内源性UDP-葡萄糖作为糖基供体,将水杨醇糖基化为水杨苷。通过重新定义OsSGT1的最佳底物,并平衡代谢通量以及增加UDP-葡萄糖的供应,摇瓶中的水杨苷产量达到了4 g/L。最后,在3-L发酵罐中培养高产菌株,水杨苷的合成量达到了14.62 g/L。据我们所知,这一成果标志着迄今为止通过微生物发酵生产水杨苷的最高产量。

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