Metabolic engineering of Escherichia coli for efficient production of L-arginine

Hai-De Wang; Jian-Zhong Xu; Wei-Guo Zhang

doi:10.1007/s00253-022-12109-4

Metabolic engineering of Escherichia coli for efficient production of L-arginine

Appl Microbiol Biotechnol. 2022 Sep;106(17):5603-5613. doi: 10.1007/s00253-022-12109-4. Epub 2022 Aug 6.

Authors

Hai-De Wang¹, Jian-Zhong Xu², Wei-Guo Zhang³

Affiliations

¹ The Key Laboratory of Industrial Biotechnology, Ministry of Education, School of Biotechnology, Jiangnan University, 1,800# Lihu Road, 214122, WuXi, People's Republic of China.
² The Key Laboratory of Industrial Biotechnology, Ministry of Education, School of Biotechnology, Jiangnan University, 1,800# Lihu Road, 214122, WuXi, People's Republic of China. xujianzhong@jiangnan.edu.cn.
³ The Key Laboratory of Industrial Biotechnology, Ministry of Education, School of Biotechnology, Jiangnan University, 1,800# Lihu Road, 214122, WuXi, People's Republic of China. zhangweiguojn@163.com.

PMID: 35931894
DOI: 10.1007/s00253-022-12109-4

Abstract

As an important semi-essential amino acid, L-arginine (L-Arg) has important application prospects in medicine and health care. However, it remains a challenge to efficiently produce L-Arg by Escherichia coli (E. coli). In the present study, we obtained an E. coli A1 with L-Arg accumulation ability, and carried out a series of metabolic engineering on it, and finally obtained an E. coli strain A7 with high L-Arg production ability. First, genome analysis of strain A1 was performed to explore the related genes affecting L-Arg accumulation. We found that gene speC and gene speF played an important role in the accumulation of L-Arg. Second, we used two strategies to solve the feedback inhibition of the L-Arg pathway in E. coli. One was the combination of a mutation of the gene argA and the deletion of the gene argR, and the other was the combination of a heterologous insertion of the gene argJ and the deletion of the gene argR. The combination of exogenous argJ gene insertion and argR gene deletion achieved higher titer accumulation with less impact on strain growth. Finally, we inserted the gene cluster argCJBDF of Corynebacterium glutamicum (C. glutamicum) to enhance the metabolic flux of the L-Arg pathway in E. coli. The final strain obtained 70.1 g/L L-Arg in a 5-L bioreactor, with a yield of 0.326 g/g glucose and a productivity of 1.17 g/(L· h). This was the highest level of L-Arg production by E. coli ever reported. Collectively, our findings provided valuable insights into the possibility of the industrial production of L-Arg by E. coli. KEY POINTS: • Genetic background of E. coli A1 genome analysis. • Heterologous argJ substitution of argA mutation promoted excessive accumulation of L-Arg in E. coli A1. • The overexpression of L-Arg synthesis gene cluster argCJBDF of Corynebacterium glutamicum (C. glutamate) promoted the accumulation of L-Arg, and 70.1 g/L L-Arg was finally obtained in fed-batch fermentation.

Keywords: Escherichia coli; Fermentation; L-arginine; Metabolic engineering; argJ.

MeSH terms

Arginine
Corynebacterium glutamicum*
Escherichia coli
Fermentation
Metabolic Engineering*

Substances

Arginine

Grants and funding

111-2-06/Overseas Expertise Introduction Project for Discipline Innovation