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dc.contributorUniversitat de Vic - Universitat Central de Catalunya. Facultat de Ciències i Tecnologia
dc.contributorUniversitat de Vic - Universitat Central de Catalunya. Departament de Biociències
dc.contributorHIV Controllers Consortium of the AIDS Spanish Network
dc.contributor.authorEgaña-Gorroño, Lander
dc.contributor.authorGuardo, Alberto C.
dc.contributor.authorBargalló, Manel E.
dc.contributor.authorPlanet, Evarist
dc.contributor.authorVilaplana, Elisenda
dc.contributor.authorEscribà, Tuixent
dc.contributor.authorPérez, Iñaki
dc.contributor.authorGatell, J.M.
dc.contributor.authorGarcia, Felipe
dc.contributor.authorArnedo, Mireia
dc.contributor.authorPlana, Montserrat
dc.date.accessioned2018-06-27T17:58:36Z
dc.date.available2018-06-27T17:58:36Z
dc.date.created2016
dc.date.issued2016
dc.identifier.citationEgana-Gorrono, L., Guardo, A. C., Bargallo, M. E., Planet, E., Vilaplana, E., Escriba, T., et al. (2016). MicroRNA profile in CD8+T-lymphocytes from HIV-infected individuals: Relationship with antiviral immune response and disease progression. Plo s One, 11(5), e0155245.es
dc.identifier.issn1932-6203
dc.identifier.urihttp://hdl.handle.net/10854/5481
dc.description.abstractBackground The relationship between host microRNAs (miRNA), viral control and immune response has not yet been elucidated in the field of HIV. The aim of this study was to assess the differential miRNA profile in CD8+ T-cells between HIV-infected individuals who differ in terms of viral replication control and immune response. Methods miRNA profile from resting and CD3/CD28-stimulated CD8+ T-cells from uninfected individuals (HIV-, n = 11), Elite Controllers (EC, n = 15), Viremic Controllers (VC, n = 15), Viremic Progressors (VP, n = 13) and HIV-infected patients on therapy (ART, n = 14) was assessed using Affymetrix miRNA 3.1 arrays. After background correction, quantile normalization and median polish summarization, normalized data were fit to a linear model. The analysis comprised: resting samples between groups; stimulated samples between groups; and stimulated versus resting samples within each group. Enrichment analyses of the putative target genes were perfomed using bioinformatic algorithms. Results A downregulated miRNA pattern was observed when resting samples from all infected groups were compared to HIV-. A miRNA downregulation was also observed when stimulated samples from EC, ART and HIV- groups were compared to VP, being hsa-miR-4492 the most downregulated. Although a preferential miRNA downregulation was observed when stimulated samples were compared to the respective resting samples, VP presented a differential miRNA expression pattern. In fact, hsa-miR-155 and hsa-miR-181a were downregulated in VP whereas in the other groups, either an upregulation or no differences were observed after stimulation, respectively. Overall, functional enrichment analysis revealed that the predicted target genes were involved in signal transduction pathways, metabolic regulation, apoptosis, and immune response. Conclusions Resting CD8+ T-cells do not exhibit a differential miRNA expression between HIV-infected individuals but they do differ from non-infected individuals. Moreover, a specific miRNA pattern is present in stimulated CD8+ T-cells from VP which could reflect a detrimental pattern in terms of CD8+ T-cell immune response.es
dc.formatapplication/pdfes
dc.format.extent19 p.es
dc.language.isoenges
dc.publisherPublic Library of Sciencees
dc.rightsAquest document està subjecte a aquesta llicència Creative Commonses
dc.rights.urihttp://creativecommons.org/licenses/by/4.0/es/es
dc.subject.otherADNes
dc.subject.otherMalaltieses
dc.subject.otherRNAes
dc.subject.otherResposta immunitàriaes
dc.titleMicroRNA Profile in CD8+ T-Lymphocytes from HIV-Infected Individuals: Relationship with Antiviral Immune Response and Disease Progressiones
dc.typeinfo:eu-repo/semantics/articlees
dc.identifier.doihttp://dx.doi.org/10.1371/journal.pone.0155245
dc.rights.accessRightsinfo:eu-repo/semantics/openAccesses
dc.type.versioninfo:eu-repo/publishedVersiones
dc.indexacioIndexat a WOS/JCRes
dc.indexacioIndexat a SCOPUSes


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