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Vanadium distribution, lipid peroxidation and oxidative stress markers upon decavanadate in vivo administration

dc.contributor.authorS. Soares, Sandra
dc.contributor.authorMartins, H.
dc.contributor.authorDuarte, Rui O.
dc.contributor.authorMoura, José J. G.
dc.contributor.authorCoucelo, Josefina
dc.contributor.authorGutiérrez-Merino, Carlos
dc.contributor.authorAureliano, M.
dc.date.accessioned2012-06-26T10:23:56Z
dc.date.available2012-06-26T10:23:56Z
dc.date.issued2007
dc.description.abstractThe contribution of decameric vanadate species to vanadate toxic effects in cardiac muscle was studied following an intravenous administration of a decavanadate solution (1 mM total vanadium) in Sparus aurata. Although decameric vanadate is unstable in the assay medium, it decomposes with a half-life time of 16 allowing studying its effects not only in vitro but also in vivo. After 1, 6 and 12 h upon decavanadate administration the increase of vanadium in blood plasma, red blood cells and in cardiac mitochondria and cytosol is not affected in comparison to the administration of a metavanadate solution containing labile oxovanadates. Cardiac tissue lipid peroxidation increases up to 20%, 1, 6 and 12 h after metavanadate administration, whilst for decavanadate no effects were observed except 1 h after treatment (+20%). Metavanadate administration clearly differs from decavanadate by enhancing, 12 h after exposure, mitochondrial superoxide dismutase (SOD) activity (+115%) and not affecting catalase (CAT) activity whereas decavanadate increases SOD activity by 20% and decreases ( 55%) mitochondrial CAT activity. At early times of exposure, 1 and 6 h, the only effect observed upon decavanadate administration was the increase by 20% of SOD activity. In conclusion, decavanadate has a different response pattern of lipid peroxidation and oxidative stress markers, in spite of the same vanadium distribution in cardiac cells observed after decavanadate and metavanadate administration. It is suggested that once formed decameric vanadate species has a different reactivity than vanadate, thus, pointing out that the differential contribution of vanadium oligomers should be taken into account to rationalize in vivo vanadate toxicity.por
dc.identifier.issn0162-0134
dc.identifier.urihttp://hdl.handle.net/10400.1/1296
dc.language.isoengpor
dc.peerreviewedyespor
dc.publisherElsevierpor
dc.subjectDecavanadatepor
dc.subjectOxifative stresspor
dc.titleVanadium distribution, lipid peroxidation and oxidative stress markers upon decavanadate in vivo administrationpor
dc.typejournal article
dspace.entity.typePublication
oaire.citation.endPage88por
oaire.citation.issue101por
oaire.citation.startPage80por
oaire.citation.titleJournal of Inorganic Biochemistrypor
person.familyNameSoares
person.familyNameGutierrez-Merino
person.familyNameAureliano
person.givenNameSandra
person.givenNameCarlos
person.givenNameManuel
person.identifier584146
person.identifier.ciencia-idAA14-3490-DC5E
person.identifier.orcid0000-0002-6562-2674
person.identifier.orcid0000-0003-3673-7007
person.identifier.orcid0000-0003-4858-3201
person.identifier.ridK-4574-2014
person.identifier.ridI-3283-2012
person.identifier.scopus-author-id10539327200
person.identifier.scopus-author-id6603412860
rcaap.rightsopenAccesspor
rcaap.typearticlepor
relation.isAuthorOfPublicationa98c149e-2a56-41b3-95fa-a45ae08599e6
relation.isAuthorOfPublication1edd3bda-28a9-4d7f-a404-f867f72ddefa
relation.isAuthorOfPublicationbb413661-7edd-4b57-8338-33889cfd05db
relation.isAuthorOfPublication.latestForDiscovery1edd3bda-28a9-4d7f-a404-f867f72ddefa

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