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Yanıkta doku kültürünün avantajları

dc.contributor.advisorSelmanpakoğlu, Naki
dc.contributor.authorAçıkel, Cengiz
dc.date.accessioned2023-09-26T11:54:59Z
dc.date.available2023-09-26T11:54:59Z
dc.date.submitted2018-08-06
dc.date.issued1997
dc.identifier.urihttps://acikbilim.yok.gov.tr/handle/20.500.12812/755984
dc.description.abstractÖZET 2 - 4 cm 2' lik deri biyopsisinin epidermisi tripsin + EDTA solüsyonu içerisinde +4 derecede 18 saat inkübe edilerek dermişten ayrıldı. Elde edilen epidermal hücreler proliferasyon yeteneği mitomisin - C ile durdurulan 3T3 fare fibroblastlan ile birlikte, 75 cm 2' lik polistren flasklarda kültüre edildi. Bazal vasat olarak HAM F12 + DMEM ( 1:1 ) kullanıldı. Bazal vasata fetal sığır serumu, L - glutamin, adenin, insülin, hidrokortizon, transferrin, 3,37,5 - triiyodo - L - tironin eklendi. Kültürler 37 ° C ve % 5 CO 2' li etüvde inkübe edildi ve haftada üç kez vasat değiştirildi. Kültürün ikinci gününden itibarin vasata kolera toksini ve epidermal büyüme faktörü de eklendi. 8-10 gün sonra kültür % 80 konfluent oldu ve subkültürler yapıldı. Sekonder kültürler 10 günde konfluent hale gelip stratifiye oldular. Flasklar kızgın tel yardımı ile açıldı. Kültüre epitel flask zemininden dispaz ile muamele edilerek bir tabaka halinde ayrıldı. Epitel üzerine parafin emdirilmiş gazlı bez metal küplerle monte edildi ve bazal taraf üstte olacak şekilde transport kabma aktarıldı. Sonuçta birkaç santimetre karelik bir deri örneğinden elde edilen keratinositlerin invitro ve seri kültürü ile büyük miktarlarda, greftlenebilir kalitede epitel elde edildi. 46
dc.description.abstractSUMMARY The epidermis of the cutaneous biopsy ( 2 - 4 cm 2 ) was separated from dermis after incubation with trypsin + EDTA solution at +4 ° C for 18 hours. Epidermal cells were cocultured with 3T3 murine fibroblasts whose proliferation was arrested by mitomycin - C in 75 cm polystrain flasks. HAM F12 + DMEM ( 1:1 ) was used as a basal medium. Supplements were fetal bovine serum, L - glutamine, adenin, insulin, hydrocortisone, transferrin, 3,37,5 - triiodo - L thyronine. The cultures were incubated at 37 ° C in humidifed athmosphere containing 5 % CO 2 and medium was changed three times weekly. After two days in culture cholera toxin and epidermal growth factor were added to the medium. The cultures were nearly confluent after 8-10 days and subcultured. The secondary cultures became confluent and stratified within 10 days. Flasks were opened by means of a hot wire. Cultured epithelia were enzymatically detached as a coherent sheet from the culture using dispase treatment. Paraffin impregnated tulle gras was mounted on epithelium with metal clips and transferred to transport vessel together basal side up. As a conclusion, large amounts of graftable epithelia were generated using in vitro and serially culture of keratinocytes obtained from a piece of skin sample. 47en_US
dc.languageTurkish
dc.language.isotr
dc.rightsinfo:eu-repo/semantics/embargoedAccess
dc.rightsAttribution 4.0 United Statestr_TR
dc.rights.urihttps://creativecommons.org/licenses/by/4.0/
dc.subjectPlastik ve Rekonstrüktif Cerrahitr_TR
dc.subjectPlastic and Reconstructive Surgeryen_US
dc.titleYanıkta doku kültürünün avantajları
dc.typedoctoralThesis
dc.date.updated2018-08-06
dc.contributor.departmentPlastik ve Rekonstrüktif Cerrahi Ana Bilim Dalı
dc.subject.ytmTissue culture
dc.subject.ytmBurns
dc.identifier.yokid58927
dc.publisher.instituteTıp Fakültesi
dc.publisher.universityGÜLHANE ASKERİ TIP AKADEMİSİ
dc.type.submedicineThesis
dc.identifier.thesisid58927
dc.description.pages60
dc.publisher.disciplineDiğer


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