Cell Factory Design and Culture Process Optimization for Dehydroshikimate Biosynthesis in Escherichia coli

被引:28
|
作者
Choi, Si-Sun [1 ]
Seo, Seung-Yeul [2 ,3 ]
Park, Sun-Ok [2 ]
Lee, Han-Na [1 ,2 ]
Song, Ji-soo [1 ]
Kim, Ji-yeon [1 ]
Park, Ji-Hoon [1 ]
Kim, Sangyong [4 ,5 ]
Lee, Sang Joung [2 ]
Chun, Gie-Taek [3 ]
Kim, Eung-Soo [1 ]
机构
[1] Inha Univ, Dept Biol Engn, Incheon, South Korea
[2] STR Biotech Co Ltd, Chuncheon Si, South Korea
[3] Kangwon Natl Univ, Dept Mol Biosci, Chuncheon Si, South Korea
[4] Korea Inst Ind Technol, Green Chem & Mat Grp, Cheonan Si, South Korea
[5] Korea Univ Sci & Technol UST, Green Proc & Syst Engn Major, Daejeon, South Korea
关键词
dehydroshikimate; cell factory design; Escherichia coli; culture process; production optimization; MUCONIC ACID; 3-DEHYDROSHIKIMIC ACID; MICROBIAL-PRODUCTION; SHIKIMATE PATHWAY; ADIPIC ACID; CHEMICALS; STRAIN;
D O I
10.3389/fbioe.2019.00241
中图分类号
Q81 [生物工程学(生物技术)]; Q93 [微生物学];
学科分类号
071005 ; 0836 ; 090102 ; 100705 ;
摘要
3-Dehydroshikimate (DHS) is a useful starting metabolite for the biosynthesis of muconic acid (MA) and shikimic acid (SA), which are precursors of various valuable polymers and drugs. Although DHS biosynthesis has been previously reported in several bacteria, the engineered strains were far fromsatisfactory, due to their low DHS titers. Here, we created an engineered Escherichia coli cell factory to produce a high titer of DHS as well as an efficient system for the conversion DHS into MA. First, the genes showing negative effects on DHS accumulation in E. coli, such as tyrR (tyrosine dependent transcriptional regulator), ptsG (glucose specific sugar: phosphoenolpyruvate phosphotransferase), and pykA (pyruvate kinase 2), were disrupted. In addition, the genes involved in DHS biosynthesis, such as aroB (DHQ synthase), aroD (DHQ dehydratase), ppsA (phosphoenolpyruvate synthase), galP (D-galactose transporter), aroG (DAHP synthase), and aroF (DAHP synthase), were overexpressed to increase the glucose uptake and flux of intermediates. The redesigned DHS-overproducing E. coli strain grown in an optimized medium produced similar to 117 g/L DHS in 7-L fed-batch fermentation, which is the highest level of DHS production demonstrated in E. coli. To accomplish the DHS-to-MA conversion, which is originally absent in E. coli, a codon-optimized heterologous gene cassette containing asbF, aroY, and catA was expressed as a single operon under a strong promoter in a DHS-overproducing E. coli strain. This redesigned E. coli grown in an optimized medium produced about 64.5 g/L MA in 7-L fed-batch fermentation, suggesting that the rational cell factory design of DHS and MA biosynthesis could be a feasible way to complement petrochemical-based chemical processes.
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页数:11
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