Cryopreservation effect on proliferative and chondrogenic potential of human chondrocytes isolated from superficial and deep cartilage

UDC.coleccionInvestigaciónes_ES
UDC.departamentoFisioterapia, Medicina e Ciencias Biomédicases_ES
UDC.grupoInvReumatoloxía (INIBIC)es_ES
UDC.grupoInvGrupo de Investigación en Terapia Celular e Medicina Rexenerativa (TCMR)es_ES
UDC.grupoInvTerapia Celular e Medicina Rexenerativa (INIBIC)es_ES
UDC.grupoInvGrupo de Investigación en Reumatoloxía e Saúde (GIR-S)es_ES
UDC.institutoCentroINIBIC - Instituto de Investigacións Biomédicas de A Coruñaes_ES
dc.contributor.authorMuiños-López, Emma
dc.contributor.authorRendal-Vázquez, Esther
dc.contributor.authorHermida Gómez, Tamara
dc.contributor.authorFuentes Boquete, Isaac Manuel
dc.contributor.authorDíaz-Prado, Silvia
dc.contributor.authorBlanco García, Francisco J
dc.date.accessioned2015-06-15T12:02:54Z
dc.date.available2015-06-15T12:02:54Z
dc.date.issued2012-04-06
dc.description.abstract[Abstract] Objectives: To compare the proliferative and chondrogenic potential of fresh and frozen chondrocytes isolated from superficial and deep articular cartilage biopsies. Materials and Methodology: The study included 12 samples of fresh and frozen healthy human knee articular cartilage. Cell proliferation was tested at 3, 6 and 9 days. Studies of mRNA quantification, protein expression and immunofluorescence for proliferation and chondrogenic markers were performed. Results: Stimulation of fresh and frozen chondrocytes from both superficial and deep cartilage with fetal bovine serum produced an increase in the proliferative capacity compared to the non-stimulated control group. In the stimulated fresh cells group, the proliferative capacity of cells from the deep biopsy was greater than that from cells from the superficial biopsy (0.046 vs 0.028, respectively, p<0.05). There was also a significant difference between the proliferative capacity of superficial zone fresh (0.028) and frozen (0.051) chondrocytes (p<0.05). CCND1 mRNA and protein expression levels, and immunopositivity for Ki67 revealed a higher proliferative capacity for fresh articular chondrocytes from deep cartilage. Regarding the chondrogenic potential, stimulated fresh cells showed higher SOX9 and Col II expression in chondrocytes from deep than from superficial zone (p<0.05, T student test). Conclusions: The highest rate of cell proliferation and chondrogenic potential of fresh chondrocytes was found in cells obtained from deep cartilage biopsies, whereas there were no statistically significant differences in proliferative and chondrogenic capacity between biopsy origins with frozen chondrocytes. These results indicate that both origin and cryopreservation affect the proliferative and chondrogenic potential of chondrocytes.es_ES
dc.description.sponsorshipServizo Galego de Saúde; PS07/84es_ES
dc.description.sponsorshipInstituto de Salud Carlos III; CIBER BBN CB06-01-0040
dc.description.sponsorshipMinisterio Ciencia e Innovacion; PLE2009-0144
dc.description.sponsorshipMinisterio Ciencia e Innovación; PI 08/2028
dc.identifier.citationMuíños-López E, Rendal-Vázquez ME, Hermida-Gómez T. Cryopreservation effect on proliferative and chondrogenic potential of human chondrocytes isolated from superficial and deep cartilage. Open Orthopedics J. 2012;6:150-159es_ES
dc.identifier.urihttp://hdl.handle.net/2183/14679
dc.language.isoenges_ES
dc.publisherBentham Openes_ES
dc.relation.urihttp://dx.doi.org/10.2174/1874325001206010150es_ES
dc.rightsCreative Commons Licencees_ES
dc.rightsReconocimiento-NoComercial 4.0 Internacional
dc.rights.accessRightsopen accesses_ES
dc.rights.urihttp://creativecommons.org/licenses/by-nc/4.0/
dc.subjectAutologous chondrocyte implantationes_ES
dc.subjectCartilagees_ES
dc.subjectCell therapyes_ES
dc.subjectOsteoarthritises_ES
dc.titleCryopreservation effect on proliferative and chondrogenic potential of human chondrocytes isolated from superficial and deep cartilagees_ES
dc.typejournal articlees_ES
dspace.entity.typePublication
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relation.isAuthorOfPublicationdba2fb6d-5f3d-4532-8375-9ddef1781493
relation.isAuthorOfPublicationf357279a-035a-4279-a553-99cfd79bd2bb
relation.isAuthorOfPublication.latestForDiscoveryb97cdc77-829e-45af-8641-cc62c8553d56

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