论文
In vitro oxidative decarboxylation of free fatty acids to terminal alkenes by two new P450 peroxygenases
发表年度: 2017
卷: 10
页: -
摘要: Background: P450 fatty acid decarboxylases represented by the unusual CYP152 peroxygenase family member OleT(JE) have been receiving great attention recently since these P450 enzymes are able to catalyze the simple and direct production of 1-alkenes for potential applications in biofuels and biomaterials. To gain more mechanistic insights, broader substrate spectra, and improved decarboxylative activities, it is demanded to discover and investigate more P450 fatty acid decarboxylases. Results: Here, we describe for the first time the expression, purification, and in vitro biochemical characterization of two new CYP152 peroxygenases, CYP-Aa162 and CYP-Sm46 Delta 29, that are capable of decarboxylating straight-chain saturated fatty acids. Both enzymes were found to catalyze the decarboxylation and hydroxylation of a broad range of free fatty acids (C-10-C-20) with overlapping substrate specificity, yet distinct chemoselectivity. CYP-Sm46 Delta 29 works primarily as a fatty (lauric) acid decarboxylase (66.1 +/- 3.9% 1-undecene production) while CYP-Aa162 more as a fatty (lauric) acid hydroxylase (72.2 +/- 0.9% hydroxy lauric acid production). Notably, the optical spectroscopic analysis of functional CYP-Sm46 Delta 29 revealed no characteristic P450 band, suggesting a unique heme coordination environment. Active-site mutagenesis analysis showed that substitution with the proposed key decarboxylation-modulating residues, His85 and Ile170, enhanced the decarboxylation activity of CYP-Aa162 and P450(BS beta), emphasizing the importance of these residues in directing the decarboxylation pathway. Furthermore, the steady-state kinetic analysis of CYP-Aa162 and CYP-Sm46 Delta 29 revealed both cooperative and substrate inhibition behaviors which are substrate carbon chain length dependent. Conclusions: Our data identify CYP-Sm46 Delta 29 as an efficient OleT(JE)-like fatty acid decarboxylase. Oxidative decarboxylation chemoselectivity of the CYP152 decarboxylases is largely dependent upon the carbon chain length of fatty acid substrates and their precise positioning in the enzyme active site. Finally, the kinetic mode analysis of the enzymes could provide important guidance for future process design.
刊物名称: BIOTECHNOLOGY FOR BIOFUELS
影响因子: 5.452