Combinatorial promoter engineering of glucokinase and phosphoglucoisomerase for improved N-acetylglucosamine production in Bacillus subtilis

被引:31
|
作者
Ling, Meixi [1 ,2 ]
Liu, Yanfeng [1 ,2 ]
Li, Jianghua [1 ,2 ]
Shin, Hyun-dong [3 ]
Chen, Jian [2 ]
Du, Guocheng [1 ,2 ]
Liu, Long [1 ,2 ]
机构
[1] Jiangnan Univ, Key Lab Carbohydrate Chem & Biotechnol, Minist Educ, Wuxi 214122, Peoples R China
[2] Jiangnan Univ, Key Lab Ind Biotechnol, Minist Educ, Wuxi 214122, Peoples R China
[3] Georgia Inst Technol, Sch Chem & Biomol Engn, Atlanta, GA 30332 USA
基金
中国国家自然科学基金;
关键词
N-acetylglucosamine; Bacillus subtilis; Promoter engineering; Metabolic engineering; ESCHERICHIA-COLI; ENHANCED GLUCOSAMINE; EXPRESSION; LEVEL; OPTIMIZATION; PROTEINS; KINETICS;
D O I
10.1016/j.biortech.2017.09.063
中图分类号
S2 [农业工程];
学科分类号
0828 ;
摘要
In previous work, a recombinant Bacillus subtilis strain was successfully constructed for microbial production of N-acetylglucosamine (GlcNAc). In this study, GlcNAc titer was further improved by combinatorial promoter engineering of key genes glck encoding glucokinase and pgi encoding phosphoglucoisomerase. First, three promoters including constitutive promoter P-43, xylose inducible promoter P-xylA, and isopropyl-beta-d-thiogalactoside inducible P-grac were used to replace the native promoters of glcK and pgi, yielding 12 recombinant strains. It was found that when glcK and pgi were both under the control of promoter PxylA, the highest GlcNAc titer in 3-L fedbatch bioreactor reached 35.12 g/L, which was 52.6% higher than that of the initial host. Next, the transcriptional levels of the related genes in glycolysis, GlcNAc synthesis pathway, peptidoglycan synthesis pathway, and pentose phosphate pathway were investigated by quantitative real-time PCR analysis. Fine-tuning upper GlcNAc synthesis pathway by combinatorial promoter substitution significantly enhanced GlcNAc production in engineered B. subtilis.
引用
收藏
页码:1093 / 1102
页数:10
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