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http://dx.doi.org/10.4014/jmb.1711.11030

Modification of N-Terminal Amino Acids of Fungal Benzoate Hydroxylase (CYP53A15) for the Production of p-Hydroxybenzoate and Optimization of Bioproduction Conditions in Escherichia coli  

Tamaki, Shun (Division of Signal Responses, Biosignal Research Center, Kobe University)
Yagi, Mitsuhiko (Division of Signal Responses, Biosignal Research Center, Kobe University)
Nishihata, Yuki (Division of Signal Responses, Biosignal Research Center, Kobe University)
Yamaji, Hideki (Department of Chemical Science and Engineering, Graduate School of Engineering, Kobe University)
Shigeri, Yasushi (Health Research Institute, National Institute of Advanced Industrial Science and Technology (AIST))
Uno, Tomohide (Laboratory of Biochemistry, Graduate School of Agricultural Science, Kobe University)
Imaishi, Hiromasa (Division of Signal Responses, Biosignal Research Center, Kobe University)
Publication Information
Journal of Microbiology and Biotechnology / v.28, no.3, 2018 , pp. 439-447 More about this Journal
Abstract
The aromatic compound p-hydroxybenzoate (PHBA) is an important material with multiple applications, including as a building block of liquid crystal polymers in chemical industries. The cytochrome P450 (CYP) enzymes are beneficial monooxygenases for the synthesis of chemicals, and CYP53A15 from fungus Cochliobolus lunatus is capable of executing the hydroxylation from benzoate to PHBA. Here, we constructed a system for the bioconversion of benzoate to PHBA in Escherichia coli cells coexpressing CYP53A15 and human NADPH-P450 oxidoreductase (CPR) genes as a redox partner. For suitable coexpression of CYP53A15 and CPR, we originally constructed five plasmids in which we replaced the N-terminal transmembrane region of CYP53A15 with a portion of the N-terminus of various mammalian P450s. PHBA productivity was the greatest when CYP53A15 expression was induced at $20^{\circ}C$ in $2{\times}YT$ medium in host E. coli strain ${\Delta}gcvR$ transformed with an N-terminal transmembrane region of rabbit CYP2C3. By optimizing each reaction condition (reaction temperature, substrate concentration, reaction time, and E. coli cell concentration), we achieved 90% whole-cell conversion of benzoate. Our data demonstrate that the described novel E. coli bioconversion system is a more efficient tool for PHBA production from benzoate than the previously described yeast system.
Keywords
p-Hydroxybenzoate; cytochrome P450; CYP53A15; bioconversion;
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