USMF logo

Institutional Repository in Medical Sciences
of Nicolae Testemitanu State University of Medicine and Pharmacy
of the Republic of Moldova
(IRMS – Nicolae Testemitanu SUMPh)

Biblioteca Stiintifica Medicala
DSpace

University homepage  |  Library homepage

 
 
Please use this identifier to cite or link to this item: http://hdl.handle.net/20.500.12710/14091
Full metadata record
DC FieldValueLanguage
dc.contributor.authorCobzac, Vitalie
dc.contributor.authorJian, Mariana
dc.contributor.authorMadan, Vadim
dc.contributor.authorCroitor, Gheorghe
dc.contributor.authorNacu, Viorel
dc.date.accessioned2020-12-15T12:12:58Z
dc.date.available2020-12-15T12:12:58Z
dc.date.issued2016
dc.identifier.citationCOBZAC, Vitalie, JIAN, Mariana, MADAN, Vadim et al. Method of chondrocytes isolation from hyaline cartilage. In: Arta Medica. 2016, nr. 4(61), pp. 47-48. ISSN 1810-1852.en_US
dc.identifier.issn1810-1852
dc.identifier.urihttps://artamedica.md/old_issues/ArtaMedica_61.pdf
dc.identifier.urihttp://repository.usmf.md/handle/20.500.12710/14091
dc.descriptionLaboratory of Tissue Engineering and Cells Cultures, State University of Medicine and Pharmacy “Nicolae Testemițanu”, Republic of Moldova, Al VIII-lea Congres Naţional de Ortopedie și Traumatologie cu participare internaţională 12-14 octombrie 2016en_US
dc.description.abstractThe aim of this study is isolation of chondrocytes from articular hyaline cartilage and their expansion in cell cultures for further transplantation in a cartilage defect. Materials and methods: The study was performed on 9 New Zealand White rabbit 6 months old. Under sterile conditions, slices of hyaline cartilage were harvested from unbearing area of knee joint, followed by 0,25% tripsină-EDTA treatment for 30 min and 0,6% collagenase for 6 hours. The cells were cultivated in cell culture flasks by 10000 ±500 cell/cm2 and incubated at 37 ° C with 5% CO2 in DMEM with 10% FBS. The cells were expanded in culture up to 21 days to a confluence of 80%. The cells was counted by a hemocytometer. The chondrocytes were stained with Safranin O and toluidine blue/fast green. Results: From approximately 50±10 mg of cartilage were isolated 4x105 ±5x104 cells. At staining chondrocytes with Safranin O, the nuclei were black, the cytoplasm gray-green and and cartilage, mucin were orange to red. At staining chondrocytes with toluidine blue/fast green, the nuclei appeared dark blue, the cartilage blue, deep purple and background green. Conclusion The method of chondrocytes isolation from hyaline cartilage is efficient and it was confirmed by in vitro cell staining with Safranin O and toluidine blue/fast green. Our further purpose is implantation in vitro of expanded chondrocytes on tridimensional scaffold and their transplantation in an osteochondral defect.en_US
dc.language.isoenen_US
dc.publisherAsociaţia chirurgilor “Nicolae Anestiadi” din Republica Moldovaen_US
dc.subjectchondrocyteen_US
dc.subjectisolationen_US
dc.subjecthyalineen_US
dc.subjectcartilageen_US
dc.titleMethod of chondrocytes isolation from hyaline cartilageen_US
dc.typeOtheren_US
Appears in Collections:Arta Medica Vol. 61, No 4, 2016 ediție specială

Files in This Item:
File Description SizeFormat 
Method_of_chondrocytes_isolation_from_hyaline_cartilage.pdf259.02 kBAdobe PDFView/Open


Items in DSpace are protected by copyright, with all rights reserved, unless otherwise indicated.

 

Valid XHTML 1.0! DSpace Software Copyright © 2002-2013  Duraspace - Feedback