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Metabolic engineering of an industrial bacterium Zymomonas mobilis for anaerobic l-serine production.


ABSTRACT: Due to the complicated metabolic and regulatory networks of l-serine biosynthesis and degradation, microbial cell factories for l-serine production using non-model microorganisms have not been reported. In this study, a combination of synthetic biology and process optimization were applied in an ethanologenic bacterium Zymomonas mobilis for l-serine production. By blocking the degradation pathway while introducing an exporter EceamA from E. coli, l-serine titer in recombinant Z. mobilis was increased from 15.30 mg/L to 62.67 mg/L. It was further increased to 260.33 mg/L after enhancing the l-serine biosynthesis pathway. Then, 536.70 mg/L l-serine was achieved by removing feedback inhibition with a SerA mutant, and an elevated titer of 687.67 mg/L was further obtained through increasing serB copies while enhancing the precursors. Finally, 855.66 mg/L l-serine can be accumulated with the supplementation of the glutamate precursor. This work thus not only constructed an l-serine producer to help understand the bottlenecks limiting l-serine production in Z. mobilis for further improvement, but also provides guidance on engineering non-model microbes to produce biochemicals with complicated pathways such as amino acids or terpenoids.

SUBMITTER: Wang Z 

PROVIDER: S-EPMC10972764 | biostudies-literature | 2024 Jun

REPOSITORIES: biostudies-literature

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Metabolic engineering of an industrial bacterium <i>Zymomonas mobilis</i> for anaerobic l-serine production.

Wang Zhen Z   Wang Xia X   Yan Xiongying X   Yi Haixia H   He Shuche S   Zhang Haoyu H   Zhou Xinli X   He Qiaoning Q   Yang Shihui S  

Synthetic and systems biotechnology 20240318 2


Due to the complicated metabolic and regulatory networks of l-serine biosynthesis and degradation, microbial cell factories for l-serine production using non-model microorganisms have not been reported. In this study, a combination of synthetic biology and process optimization were applied in an ethanologenic bacterium <i>Zymomonas mobilis</i> for l-serine production. By blocking the degradation pathway while introducing an exporter EceamA from <i>E. coli</i>, l-serine titer in recombinant <i>Z.  ...[more]

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