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Double function hydroperoxide lyases/epoxyalcohol synthases (CYP74C) of higher plants: identification and conversion into allene oxide synthases by site-directed mutagenesis
Authors:Yana Y. Toporkova  Svetlana S. Gorina  Elena K. Bessolitsyna  Elena O. Smirnova  Valeria S. Fatykhova  Fredi Brühlmann  Tatiana M. Ilyina  Lucia S. Mukhtarova  Alexander N. Grechkin
Affiliation:1. Kazan Institute of Biochemistry and Biophysics, Russian Academy of Sciences, P.O. Box 30, Kazan 420111, Russia;2. Firmenich SA, Corporate R&D, Route des Jeunes 1, CH-1211, Geneva 8, Switzerland
Abstract:The CYP74C subfamily of fatty acid hydroperoxide transforming enzymes includes hydroperoxide lyases (HPLs) and allene oxide synthases (AOSs). This work reports a new facet of the putative CYP74C HPLs. Initially, we found that the recombinant CYP74C13_MT (Medicago truncatula) behaved predominantly as the epoxyalcohol synthase (EAS) towards the 9(S)-hydroperoxide of linoleic acid. At the same time, the CYP74C13_MT mostly possessed the HPL activity towards the 13(S)-hydroperoxides of linoleic and α-linolenic acids. To verify whether this dualistic behaviour of CYP74C13_MT is occasional or typical, we also examined five similar putative HPLs (CYP74C). These were CYP74C4_ST (Solanum tuberosum), CYP74C2 (Cucumis melo), CYP74C1_CS and CYP74C31 (both of Cucumis sativus), and CYP74C13_GM (Glycine max). All tested enzymes behaved predominantly as EAS toward 9-hydroperoxide of linoleic acid. Oxiranyl carbinols such as (9S,10S,11S,12Z)-9,10-epoxy-11-hydroxy-12-octadecenoic acids were the major EAS products. Besides, the CYP74C31 possessed an additional minor 9-AOS activity. The mutant forms of CYP74C13_MT, CYP74C1_CS, and CYP74C31 with substitutions at the catalytically essential domains, namely the “hydroperoxide-binding domain” (I-helix), or the SRS-1 domain near the N-terminus, showed strong AOS activity. These HPLs to AOSs conversions were observed for the first time. Until now a large part of CYP74C enzymes has been considered as 9/13-HPLs. Notwithstanding, these results show that all studied putative CYP74C HPLs are in fact the versatile HPL/EASs that can be effortlessly mutated into specific AOSs.
Keywords:EAS  epoxyalcohol synthase  DES  divinyl ether synthase  AOS  allene oxide synthase  HPL  hydroperoxide lyase  9-H(P)OD  9-H(P)OT  13-H(P)OD  13-H(P)OT  IMAC  immobilised metal affinity chromatography  Me  methyl  TMS  trimethylsilyl  TIC  total ion current  SIM  selected ion monitoring  COSY  correlation spectroscopy  HSQC  heteronuclear single quantum coherence spectroscopy  HMBC  heteronuclear multiple-bond correlation spectroscopy  Oxylipins  Cytochrome P450  CYP74C subfamily enzymes  Epoxyalcohol synthase  Hydroperoxide lyase  Site-directed mutagenesis
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