Cloning and characterization of a biotic-stress-inducible glutathione transferase from phaseolus vulgaris

dc.contributor.author	Chronopoulou, E	en
dc.contributor.author	Madesis, P	en
dc.contributor.author	Tsaftaris, A	en
dc.contributor.author	Labrou, NE	en
dc.date.accessioned	2014-06-06T06:52:59Z
dc.date.available	2014-06-06T06:52:59Z
dc.date.issued	2014	en
dc.identifier.issn	02732289	en
dc.identifier.uri	http://dx.doi.org/10.1007/s12010-013-0509-3	en
dc.identifier.uri	http://62.217.125.90/xmlui/handle/123456789/6293
dc.subject	Biotic stress	en
dc.subject	Glutathione transferase	en
dc.subject	Herbicide detoxification	en
dc.subject	Homology modeling	en
dc.title	Cloning and characterization of a biotic-stress-inducible glutathione transferase from phaseolus vulgaris	en
heal.type	journalArticle	en
heal.identifier.primary	10.1007/s12010-013-0509-3	en
heal.publicationDate	2014	en
heal.abstract	Glutathione transferases (GSTs, EC 2.5.1.18) are ubiquitous proteins in plants that play important roles in stress tolerance and in the detoxification of toxic chemicals and metabolites. In this study, we systematically examined the catalytic diversification of a GST isoenzyme from Phaseolus vulgaris (PvGST) which is induced under biotic stress treatment (Uromyces appendiculatus infection). The full-length cDNA of this GST isoenzyme (termed PvGSTU3-3) with complete open reading frame, was isolated using RACE-RT and showed that the deduced amino acid sequence shares high homology with the tau class plant GSTs. PvGSTU3-3 catalyzes several different reactions and exhibits wide substrate specificity. Of particular importance is the finding that the enzyme shows high antioxidant catalytic function and acts as hydroperoxidase, thioltransferase, and dehydroascorbate reductase. In addition, its K m for GSH is about five to ten times lower compared to other plant GSTs, suggesting that PvGSTU3-3 is able to perform efficient catalysis under conditions where the concentration of reduced glutathione is low (e.g.; oxidative stress). Its ability to conjugate GSH with isothiocyanates may provide an additional role for this enzyme to act as a regulator of the released isothiocyanates from glucosinolates as a response of biotic stress. Molecular modeling showed that PvGSTU3-3 shares the same overall fold and structural organization with other plant cytosolic GSTs, with major differences at their hydrophobic binding sites (H-sites) and some differences at the level of C-terminal domain and the linker between the C- and N-terminal domains. PvGSTU3-3, in general, exhibits restricted ability to bind xenobiotics in a nonsubstrate manner, suggesting that the biological role of PvGSTU3-3, is restricted mainly to the catalytic function. Our findings highlight the functional and catalytic diversity of plant GSTs and demonstrate their pivotal role for addressing biotic stresses in Phaseolus vulgaris. © 2013 Springer Science+Business Media New York.	en
heal.journalName	Applied Biochemistry and Biotechnology	en
dc.identifier.issue	2	en
dc.identifier.volume	172	en
dc.identifier.doi	10.1007/s12010-013-0509-3	en
dc.identifier.spage	595	en
dc.identifier.epage	609	en