A Medicago truncatula homoglutathione synthetase is derived from glutathione synthetase by gene duplication |
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Authors: | Frendo P Jiménez M J Mathieu C Duret L Gallesi D Van de Sype G Hérouart D Puppo A |
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Affiliation: | Laboratoire de Biologie Végétale et Microbiologie, Centre National de la Recherche Scientifique, Formation de Recherche en Evolution 2294, Université de Nice-Sophia Antipolis, Parc Valrose, 06108 Nice cedex 2, France. frendo@unice.fr |
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Abstract: | Glutathione (GSH) and homo-GSH (hGSH) are the major low-molecular weight thiols synthesized in Medicago truncatula. Two M. truncatula cDNAs (gshs1 and gshs2) corresponding to a putative GSH synthetase (GSHS) and a putative hGSH synthetase (hGSHS) were characterized. Heterologous expression of gshs1 and gshs2 cDNAs in an Escherichia coli strain deficient in GSHS activity showed that GSHS1 and GSHS2 are a GSHS and an hGSHS, respectively. Leucine-534 and proline-535 present in hGSHS were substituted by alanines that are conserved in plant GSHS. These substitutions resulted in a strongly stimulated GSH accumulation in the transformed E. coli strain showing that these residues play a crucial role in the differential recognition of beta-alanine and glycine by hGSHS. Phylogenetic analysis of GSHS2 and GSHS1 with other eukaryotic GSHS sequences indicated that gshs2 and gshs1 are the result of a gene duplication that occurred after the divergence between Fabales, Solanales, and Brassicales. Analysis of the structure of gshs1 and gshs2 genes shows they are both present in a cluster and in the same orientation in the M. truncatula genome, suggesting that the duplication of gshs1 and gshs2 occurred via a tandem duplication. |
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