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dc.contributor.authorHorspool, L. J.
dc.contributor.authorMcKellar, Quintin
dc.date.accessioned2014-03-27T09:30:06Z
dc.date.available2014-03-27T09:30:06Z
dc.date.issued1991-09
dc.identifier.citationHorspool , L J & McKellar , Q 1991 , ' Determination of short-chain fatty acids in equine caecal liquor by ion exchange high performance liquid chromatography after solid phase extraction ' , Biomedical Chromatography , vol. 5 , no. 5 , pp. 202-6 . https://doi.org/10.1002/bmc.1130050505
dc.identifier.issn0269-3879
dc.identifier.otherPURE: 1444494
dc.identifier.otherPURE UUID: d4504350-6d6f-4efa-b055-662ef1a0f281
dc.identifier.otherPubMed: 1742550
dc.identifier.otherScopus: 0025740359
dc.identifier.urihttp://hdl.handle.net/2299/13208
dc.description.abstractA high performance liquid chromatography (HPLC) method was developed for the determination of seven short-chain fatty acids in equine caecal liquor. Samples were cleaned up on a Sep-pak (C18) cartridge, and the analyte was eluted from the extraction cartridge and filtered through a 0.45 micron cellulose nitrate filter. The analyte was chromatographed by ion exchange HPLC. Detection was by UV at 210 nm. Recovery from phosphate buffer (0.05 M, pH 7.0) and equine caecal liquor was 76.95% (lactic), 76.76% (valeric). The limit of (propionic), 89.35% (isobutyric), 88.73% (butyric), 80.33% (isovaleric) and 72.61% (valeric). The limit of detection of the short-chain fatty acids in phosphate buffer was 0.00006 M (lactic), 0.0001 M (acetic), 0.0002 M (propionic), 0.0001 M (isobutyric), 0.0002 M (butyric), 0.0002 M (isovaleric) and 0.0003 M (valeric). The specificity and sensitivity of this method was sufficiently high to allow the characterization of the pattern of these short-chain fatty acids in equine caecal liquor following intravenous administration of oxytetracycline at the recommended dose rate in a pony.en
dc.format.extent5
dc.language.isoeng
dc.relation.ispartofBiomedical Chromatography
dc.titleDetermination of short-chain fatty acids in equine caecal liquor by ion exchange high performance liquid chromatography after solid phase extractionen
dc.contributor.institutionOffice of the Vice-Chancellor
dc.contributor.institutionVeterinary Science
dc.contributor.institutionGeography, Environment and Agriculture
dc.description.statusPeer reviewed
rioxxterms.versionofrecordhttps://doi.org/10.1002/bmc.1130050505
rioxxterms.typeJournal Article/Review
herts.preservation.rarelyaccessedtrue


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