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Biospeciation of tungsten in the serum of diabetic and healthy rats treated with the antidiabetic agent sodium tungstate

dc.contributor.authorGómez Gómez, María Milagros
dc.contributor.authorRodríguez Fariñas, Nuria
dc.contributor.authorCañas Montalvo, Benito
dc.contributor.authorDomínguez, Jorge
dc.contributor.authorGuinovart, Joan
dc.contributor.authorCámara Rica, Carmen
dc.date.accessioned2023-06-20T00:28:23Z
dc.date.available2023-06-20T00:28:23Z
dc.date.issued2011-05-30
dc.description.abstractIt is known that oral administration of sodium tungstate preserves the pancreatic beta cell function in diabetic rats. Healthy and streptozotocin-induced diabetic rats were treated with sodium tungstate for one, three or six weeks, after which the species of W in serum, were analysed. An increase in serum W with treatment time was observed. After six weeks, the serum W concentration in diabetic rats (70 mg L−1) was about 4.6 times higher than in healthy specimens. This different behaviour was also observed for Cu accumulation, while the Zn pattern follows the contrary. The patterns observed in the retention of Cu and Zn may be attributable to a normalization of glycaemia. The speciation analysis of W was performed using 2D separations, including an immunoaffinity packing and a SEC (Size Exclusion Chromatography) column coupled to an ICP-MS (Inductively Coupled Plasma Mass Spectrometry) for elemental detection. Ultrafiltration data together with SEC-ICP-MS results proved that around 80% of serum W was bound to proteins, the diabetic rats registering a higher W content than their healthy counterparts. Most of the proteinbound W was due to a complex with albumin. An unknown protein with a molecular weight higher tan 100 kDa was also found to bind a small amount of W (about 2%). MALDI-TOF (Matrix-Assisted Laser Desorption Ionization Time-of-Flight) analysis of the desalted and concentrated chromatographic fractions confirmed albumin as the main protein bound to tungstate in rat serum, while no binding to transferrin (Tf) was detected. The interaction between glutathione and W was also evaluated using standard solutions; however, the formation of complexes was not observed. The stability of the complexes between W and proteins when subjected to more stringent procedures, like those used in proteomic methodologies (denaturing with urea or SDS, boiling, sonication, acid media, reduction with -mercaptoethanol (BME) or DTT (dithiotreitol) and alkylation with iodoacetamide (IAA), was also evaluated. Our results indicate that the stability of the complexes between W and proteins is not too high enough to remain unaltered during protein separation by SDS–PAGE in denaturing and reducing conditions. However, the procedures for in-solution tryptic digestion and for ESI-MS analysis in MeOH/H2O/with 0.1% formic acid could be used for protein identification without large loss of binding between W and proteins.
dc.description.departmentDepto. de Química Analítica
dc.description.facultyFac. de Ciencias Químicas
dc.description.refereedTRUE
dc.description.sponsorshipSantander-Complutense
dc.description.statuspub
dc.eprint.idhttps://eprints.ucm.es/id/eprint/41814
dc.identifier.doidoi.org/10.1016/j.talanta.2011.02.050
dc.identifier.issn0039-9140
dc.identifier.officialurlhttp://www.sciencedirect.com/science/article/pii/S0039914011002037
dc.identifier.urihttps://hdl.handle.net/20.500.14352/42614
dc.issue.number4
dc.journal.titleTalanta
dc.language.isoeng
dc.page.final1018
dc.page.initial1011
dc.publisherElsevier
dc.relation.projectIDPR34/07-15829 and CTQ2008-01031
dc.rights.accessRightsopen access
dc.subject.cdu543
dc.subject.keywordTungsten biospeciation
dc.subject.keywordDiabetes
dc.subject.keywordRat serum
dc.subject.keywordSEC-ICP-MS
dc.subject.keywordMALDI-TOF
dc.subject.ucmQuímica analítica (Química)
dc.subject.unesco2301 Química Analítica
dc.titleBiospeciation of tungsten in the serum of diabetic and healthy rats treated with the antidiabetic agent sodium tungstate
dc.typejournal article
dc.volume.number84
dspace.entity.typePublication
relation.isAuthorOfPublication98fd9b6f-b112-42da-b0f7-b9ec1a9e748b
relation.isAuthorOfPublicationd44f01dd-fc33-4764-9cc9-4b0ac926f6f3
relation.isAuthorOfPublication47811cb6-7768-4f47-b356-c91b49efc7a2
relation.isAuthorOfPublication.latestForDiscoveryd44f01dd-fc33-4764-9cc9-4b0ac926f6f3

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