d-Aspartyl residue in a peptide can be liberated and metabolized by pig kidney enzymes |
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| Authors: | Y. Kera K. Funabashi T. Matsumoto T. Watanabe H. Nagasaki R. Yamada |
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| Affiliation: | (1) Department of BioEngineering, Nagaoka University of Technology, 940-21 Nagaoka, Niigata, Japan;(2) Department of Food Science and Nutrition, Doshisha Women's College of Liberal Arts, Kyoto, Japan |
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| Abstract: | ![]()
Summary The presence of an enzyme activity which hydrolyzes glycyl-d-aspartate was found in the homogenates of pig kidney cortex. The activity was inhibited by metal chelating agents and cilastatin, suggesting that the enzyme was a cilastatin-sensitive metallo-peptidase. Of the two hydrolysis products,d-aspartate was found to be less accumulated than glycine. The fate ofd-aspartate was, therefore, examined and the amino acid was found to be converted tol-aspartate,l-alanine and pyruvate, in the presence ofl-glutamate. Experiments with enzyme inhibitors suggested that the conversion involvedd-aspartate oxidase, aspartate aminotransferase and alanine aminotransferase as well as decarboxylation of oxaloacetate produced fromd-aspartate. All the results indicate that the enzymes in the pig kidney can liberate thed-aspartyl residue in the peptide and convert it to the compounds readily utilizable. The finding suggests a probable metabolic pathway of thed-aspartate-containing peptide. |
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| Keywords: | Amino acids Hydrolysis of glycyl-d-aspartate d-Aspartyl residue in peptides Metallo-enzyme Conversion ofd-aspartate tol-amino acids d-Aspartate oxidase Aspartate aminotransferase Alanine aminotransferase |
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