SE142:/S1
From Metabolonote
Sample Set Information
ID | TSE1243 |
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Title | Physiological roles of the beta-substituted alanine synthase gene family in Arabidopsis. |
Description | The beta-substituted alanine (Ala) synthase (Bsas) family in the large superfamily of pyridoxal 5'-phosphate-dependent enzymes comprises cysteine (Cys) synthase (CSase) [O-acetyl-serine (thiol) lyase] and beta-cyano-Ala synthase (CASase) in plants. Nine genomic sequences encode putative Bsas proteins in Arabidopsis thaliana. The physiological roles of these Bsas isoforms in vivo were investigated by the characterization of T-DNA insertion mutants. Analyses of gene expression, activities of CSase and CASase, and levels of Cys and glutathione in the bsas mutants indicated that cytosolic Bsas1;1, plastidic Bsas2;1, and mitochondrial Bsas2;2 play major roles in Cys biosynthesis. Cytosolic Bsas1;1 has the most dominant contribution both in leaf and root, and mitochondrial Bsas2;2 plays a significant role in root. Mitochondrial Bsas3;1 is a genuine CASase. Nontargeted metabolome analyses of knockout mutants were carried out by a combination of gas chromatography time-of-flight mass spectrometry and capillary electrophoresis time-of-flight mass spectrometry. The level of gamma-glutamyl-beta-cyano-Ala decreased in the mutant bsas3;1, indicating the crucial role of Bsas3;1 in beta-cyano-Ala metabolism in vivo. |
Authors | Watanabe M, Kusano M, Oikawa A, Fukushima A, Noji M, Saito K. |
Reference | Plant Physiol. 2008 Jan;146(1):310-20. Epub 2007 Nov 16. |
Comment |
Sample Information
ID | S1 |
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Title | Plant Materials and Growth Conditions |
Organism - Scientific Name | Arabidopsis thaliana |
Organism - ID | NCBI taxonomy 3702 |
Compound - ID | |
Compound - Source | |
Preparation | Arabidopsis (Arabidopsis thaliana ecotype Col-0) plants were used as the wild type in this study. |
Sample Preparation Details ID | SS1 |
Comment |
Sample Preparation Details Information
ID | SS1 |
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Title | Sample Preparation |
Description | Plants were cultured on germination medium (GM)-agar medium containing 1% Suc (Valvekens et al., 1988) in a growth chamber at 22°C under 16-h-light (approximately 2,500 lux)/8-h-dark cycles for 2 weeks. The leaves and roots of the plants were harvested, immediately frozen with liquid nitrogen, and stored at −80°C until use. Identical plant materials were analyzed for their gene expression, enzyme activities, and metabolite profiles. |
Comment_of_details |