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dc.contributor.authorRashidi, MR
dc.contributor.authorAmini, K
dc.contributor.authorKhani, MY
dc.contributor.authorFaridi, A
dc.contributor.authorHanaee, J
dc.contributor.authorSorouraddin, MH
dc.date.accessioned2018-08-26T06:15:01Z
dc.date.available2018-08-26T06:15:01Z
dc.identifier.urihttp://dspace.tbzmed.ac.ir:8080/xmlui/handle/123456789/43071
dc.description.abstractAldehyde oxidase is a widely distributed enzyme that is involved in the metabolism of an extensive range of aldehydes and N-heterocyclic compounds with physiological, pharmacological, and toxicological relevance. In the present study, a highly sensitive RP-HPLC-fluorescence method based on the oxidation of phenanthridine to phenanthridinone has been developed and validated to assay aldehyde oxidase activity in biological samples. Determination of phenanthridinone was achieved on a C18 column using 10 mmol/L phosphate buffer (pH 5.0) containing 0.1 mmol/L EDTA-acetonitrile (40 + 60, v/v) as the mobile phase. The fluorescence intensity of phenanthridinone was measured at 364 nm with excitation at 236 nm. The proposed method was precise, accurate, specific and rapid (analysis time, approximately 8 min) with a mean RSD of 2.54%. Peak responses were linear from 0.5 to 100 nmol/L, with an LOD of 0.125 nmol/L. The applicability of the method was demonstrated by measurement of aldehyde oxidase activity in rat liver, kidney, ovary, and heart fractions.
dc.language.isoEnglish
dc.relation.ispartofJournal of AOAC International
dc.subjectAldehyde Oxidase
dc.subjectAnimals
dc.subjectChromatography, High Pressure Liquid
dc.subjectFemale
dc.subjectKidney
dc.subjectLiver
dc.subjectMale
dc.subjectMyocardium
dc.subjectOvary
dc.subjectPhenanthrenes
dc.subjectPhenanthridines
dc.subjectRats
dc.subjectRats, Sprague-Dawley
dc.titleA highly sensitive RP-HPLC-fluorescence method to study aldehyde oxidase activity.
dc.typearticle
dc.citation.volume94
dc.citation.issue2
dc.citation.spage550
dc.citation.epage4
dc.citation.indexPubmed


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