Part:BBa_K4759271

T7-RBS6-pntAB-RBS2-nadK

Design Notes

We cloned nadK and pntAB genes to construct the plasmid pACYCDuet-pntAB-nadK.

Usage and Biology

P450 enzyme catalysis required redox partners to transfer NADPH electrons to heme to catalyze the substrate. The content of NADPH in E. coli cells was low, which can only meet its own growth needs. By constructing a cofactor circulatory system, the effect of NADPH on whole-cell activity was investigated. However, the cost of exogenous NADPH addition is higher and the catalytic efficiency is low. NAD+ kinase (NadK) and membrane-bound hydrogenase (PntAB) can be used to enhance the circulation of NADPH. Thus, 3 recombinant strains are constructed. The recombinant plasmid pACYCDuet-nadK is expressed in E. coli C1 (C2 strain). The recombinant plasmid pACYCDuet-pntAB (BBa_K4759269) was expressed in E. coli C1 (C3 strain). The recombinant plasmid pACYCDuet-pntAB-nadK(BBa_K4759271) was expressed in E. coli C1 (C4 strain). Without the addition of NADPH, the conversion rate of whole-cell catalysts prepared by the C4 strain was as high as 99.1%.

Sequence and Features