Identificador persistente para citar o vincular este elemento: http://hdl.handle.net/10553/43017
Campo DC Valoridioma
dc.contributor.authorGarcía-Arencibia, Moisésen_US
dc.contributor.authorDávila, Normaen_US
dc.contributor.authorCampión, Javieren_US
dc.contributor.authorCarranza, M. Carmenen_US
dc.contributor.authorCalle, Consueloen_US
dc.contributor.otherGarcia-Arencibia, Moises-
dc.contributor.otherGarcia-Arencibia, Moises-
dc.contributor.otherGarcia-Arencibia, Moises-
dc.date.accessioned2018-11-21T12:06:31Z-
dc.date.available2018-11-21T12:06:31Z-
dc.date.issued2005en_US
dc.identifier.issn0960-0760en_US
dc.identifier.urihttp://hdl.handle.net/10553/43017-
dc.description.abstractThis study was designed to explore the possible existence and location of estrogen response elements (EREs) in the human insulin receptor (hIR) gene promoter. Transfections of U-937 cells with the reported plasmids phIR(−1819)-GL2, phIR(−1473)-GL2, and phIR(−876)-GL2, that contain the −1819 to −271 bp fragment of the hIR promoter (wild-type promoter) and progressive 5 deletions of this promoter, revealed that while the activity of the wild-type promoter, was repressed 36% by treatment with 17 -estradiol (E2), the activities of progressive 5 deletions of this promoter were reduced by 26% and by 0%, by this hormone. This suggests that E2 needs the wild-type promoter for full transcriptional repression of this gene and it also suggests the presence of putative EREs in the region between −1819/−877 bp of this promoter. To identify these EREs we performed a computer search, using the SEQFIND programme developed in our laboratory, by homology with the consensus vit-ERE (5 GGTCAnnnTGACC3) of the Xenopus vitellogenin A2 gene promoter. The results of our search indicated no sequence identical to this consensus ERE, and neither was any sequence found to show 9 or 8 of the 10 bases of this consensusin this promoter. Nevertheless, a putative hIR ERE1 (5 AGTGAaacTGGCC3 ) showing 7 bases of the consensus vit-ERE, and 10 bases of the optimal binding sequence ERE (5 CA/GGGTCAnnnTGACCT/CG3 ), was identified between −1430/−1418 bp of the hIR promoter. An AP-1-like site was covering the 3 half-element of this ERE; another AP-1-like site was overlapping the first AP-1-like site, and finally a third AP-1-like site was located beside to the 5 half-element. In addition, another putative hIR ERE2 (5 GCTCCtagCAAAC3 ) showing 5 bases of the consensus vit-ERE, and 9 bases of the optimal binding sequence ERE, was located upstream of the hIR promoter, between −1567/−1555 bp. An AP-1-like site was located downstream of the 3 half-element of this ERE, and another AP-1-like site was beside the 5 half-element. EMSA analysis using nuclear extracts of E2-treated cells and natural sequences, including these putative EREs, indicated that ER – the only isoform expressed in U-937 cells – specifically recognized both EREs because ERb –DNA complexes were efficiently competed by the corresponding unlabelled probe and supershifted by the anti-human ERb (L-20) antibody. These data provide the first identification of EREs complexed with AP-1-like sites in the hIR promoter, which account for the transcriptional repression of the hIR gene mediated by ERb in U-937 cellsen_US
dc.languageengen_US
dc.publisher0960-0760
dc.relation.ispartofJournal of Steroid Biochemistry and Molecular Biologyen_US
dc.sourceJournal of Steroid Biochemistry and Molecular Biology[ISSN 0960-0760],v. 94, p. 1-14en_US
dc.subject2302 Bioquímicaen_US
dc.subject320507 Neurologíaen_US
dc.subject.other17b -Estradiolen_US
dc.subject.otherEstrogen receptor betaen_US
dc.subject.otherEstrogen response elementen_US
dc.subject.otherAP-1 siteen_US
dc.subject.otherHuman insulin receptor gene promoteren_US
dc.subject.otherXenopus vitellogenin A2 gene promoteren_US
dc.subject.otherTranscriptional regulationen_US
dc.subject.otherEstrogen-induced insulin resistanceen_US
dc.subject.otherU-937 human promonocytic cellsen_US
dc.titleIdentification of two functional estrogen response elements complexed with AP-1-like sites in the human insulin receptor gene promoteren_US
dc.typeinfo:eu-repo/semantics/articleen_US
dc.typeArticleen_US
dc.identifier.doi10.1016/j.jsbmb.2004.12.020en_US
dc.identifier.scopus18144375206-
dc.identifier.isi000229445500001-
dcterms.isPartOfJournal Of Steroid Biochemistry And Molecular Biology
dcterms.sourceJournal Of Steroid Biochemistry And Molecular Biology[ISSN 0960-0760],v. 94 (1-3), p. 1-14
dc.contributor.authorscopusid15821889300-
dc.contributor.authorscopusid6603832510-
dc.contributor.authorscopusid8771597400-
dc.contributor.authorscopusid7003707347-
dc.contributor.authorscopusid6507623704-
dc.description.lastpage14en_US
dc.description.firstpage1en_US
dc.relation.volume94en_US
dc.investigacionCiencias de la Saluden_US
dc.type2Artículoen_US
dc.identifier.wosWOS:000229445500001-
dc.contributor.daisngid1760567-
dc.contributor.daisngid1542970-
dc.contributor.daisngid155790-
dc.contributor.daisngid2372378-
dc.contributor.daisngid28200538-
dc.identifier.investigatorRIDK-9920-2013-
dc.identifier.investigatorRIDB-5538-2012-
dc.identifier.investigatorRIDB-5538-2012-
dc.utils.revisionen_US
dc.identifier.ulpgcen_US
dc.description.jcr2,866
dc.description.jcrqQ2
dc.description.scieSCIE
item.grantfulltextnone-
item.fulltextSin texto completo-
crisitem.author.orcid0000-0002-1618-4487-
crisitem.author.fullNameGarcía Arencibia, Moisés-
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