4.3 Article

Systems Biology Engineering of the Pantothenate Pathway to Enhance 3HB Productivity in Escherichia coli

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BIOTECHNOLOGY AND BIOPROCESS ENGINEERING
卷 26, 期 4, 页码 621-629

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KOREAN SOC BIOTECHNOLOGY & BIOENGINEERING
DOI: 10.1007/s12257-021-0033-1

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3-hydroxybutyrate; pantothenate kinase; Escherichia coli; bioplastics; CoA; acetyl-CoA

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By upregulating the expression of pantothenate kinase (PanK) genes, the CoA titer in Escherichia coli was increased, leading to higher 3-hydroxybutyrate (3HB) production. Eukaryotic PanK genes, from fungal and mammalian origins, were found to be effective in enhancing 3HB titers in bacterial cells, offering a promising strategy for biotechnological production improvement. Overexpressing exogenous PanKs provided several advantages over endogenous counterparts, with PanKII specifically showing potential for sustained metabolic sink through only being inhibited by acetyl-CoA.
The monomer, 3-hydroxybutyrate (3HB), plays an interesting role as a precursor for antibiotics, vitamins, and bioplastics such as polyhydroxybutyrates (PHB). The biotechnological production of both compounds in Escherichia coli has seen increased interest in the last decade. The central metabolite in the 3HB production pathway is acetyl-CoA, the derivative of coenzyme A (CoA). Enriching the intracellular pool of these cofactors could improve 3HB titers. In our study, we opted to increase CoA titers by upregulating pantothenate kinase (PanK), the rate limiting step in CoA biosynthetic pathway. To this end, 4 PanKs genes of different taxonomic origins (mammalian, fungal, and bacterial) were individually expressed and evaluated in 3HB producing E. coli cells. In shake flask studies, strains expressing Aspergillus nidulans PankII and Mus musculus PanK1 beta achieved the highest 3HB titers. In a bioreactor fermentation, the strain harboring murine PanK1 beta resulted in 7.6 g/L compared to 5.4 g/L of 3HB in the control strain. Although structurally different from the bacterial PankI, our study showed that eukaryotic Panks can supplement the kinase activity in prokaryotes. Expressing the exogenous PanKs offer several advantages over the host's enzyme; PanKII is only inhibited by acetyl-CoA, for which the 3HB-production system would provide a constant metabolic sink. Additionally, PanK1 beta is weakly regulated by acetyl-CoA, and its activity is stimulated by free CoA. Overexpressing eukaryotic PanKs constitutes a suitable strategy for improving 3HB titers in E. coli.

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