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3-hydroxy- and 3-keto-3-phenylpropionic acids: Novel metabolites of benzoic acid in horse urine
Authors:Mary Varwell Marsh  John Caldwell  Andrew J. Hutt  Robert L. Smith  Marian W. Horner  Edward Houghton  Michael S. Moss
Affiliation:2. Department of Pharmacology, St. Mary''s Hospital Medical School, London W2 1PG, U.K.;4. Racecourse Security Services Laboratories, P.O. Box 15, Snailwell Road, Newmarket, Suffolk CD8 7DT, U.K.
Abstract:The metabolism of benzoic acid has been examined in the horse, using 14C- and deuterium-labelled compounds. Chromatographic analysis of the urine showed the presence of hippuric acid, benzoyl glucuronide and benzoic acid and a discrete band which accounted for 2% of the dose administered. This material was isolated by solvent extraction and HPLC and, following treatment with diazomethane, examined by GC/MS.The major component of this fraction was 3-hydroxy-3-phenylpropionic acid methyl ester, which was accompanied by very much smaller amounts of cinnamic acid methyl ester and acetophenone. The two latter minor components have been shown to be artefacts produced during workup and analysis. Cinnamic acid methyl ester arises by the thermal decomposition of 3-hydroxy-3-phenylpropionic acid methyl ester on the GC column. It is proposed that acetophenone has formed, during workup, by decarboxylation of 3-keto-3-phenylpropionic acid.It is suggested that 3-hydroxy and 3-keto-3-phenylpropionic acids, which are also endogenous in horse urine, have arisen by an addition of a 2 carbon fragment to benzoyl CoA, in a sequence analogous to the reactions of fatty acid biosynthesis. Some implications of the metabolic interrelationships between xenobiotic acids and fatty acids are discussed.
Keywords:CoA  coenzyme A  NMR  nuclear magnetic resonance  MS  mass spectrometry  GC/MS  gas chromatography-mass spectrometry  TLC  thin layer chromatography  HPLC  high pressure liquid chromatography
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