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dc.contributor.authorZorbozan, O. and Harman, M. and Evren, V. and Erdoǧan, M.A. and Kilavuz, A. and Tunali, V. and Çavuş, I. and Yilmaz, O. and Özbilgin, A. and Turgay, N.
dc.date.accessioned2020-07-02T06:08:39Z
dc.date.available2020-07-02T06:08:39Z
dc.date.issued2018
dc.identifier.citationcited By 0
dc.identifier.urihttps://www.scopus.com/inward/record.uri?eid=2-s2.0-85044835497&doi=10.5578%2fmb.66350&partnerID=40&md5=dd6363c5dcfb37e47a6ea842350c90fc
dc.identifier.urihttp://hdl.handle.net/20.500.12481/11740
dc.description.abstractLeishmaniasis is a vector-borne zoonotic disease that shows different clinical features like cutaneous, mucocutaneous, visceral and viscerotropic forms. The protocols used in the treatment of leishmaniasis are toxic and have many limitations during administration. One of the limitations of treatment is the resistance against the protocols in practice. There is also a need to define new treatment options especially for resistant patients. Ex-vivo models using primary cell cultures may be a good source for evaluating new drug options in patients with antimony resistance, in addition to in-vitro and in-vivo studies. In this study, it was aimed to define a new ex-vivo culture model to evaluate treatment options in patients with cutaneous leishmaniasis who did not respond to treatment. In our experimental model of ex-vivo infection, Leishmania tropica promastigotes isolated from a case previously diagnosed with cutaneous leishmaniasis were used. The primary astroglial cell culture used for the ex-vivo model was prepared from 2-3 days old neonatal Sprague Dawley rat brains under sterile conditions by the modification McCarthy's method. The astroglia cells, which reached sufficient density, were infected with antimony resistant Ltropica promastigotes. After 24 hours of incubation, the supernatant on the cells were collected, the cell culture plate was dried at room temperature, then fixed with methyl alcohol and stained with Giemsa to search for Ltropica amastigotes. Amastigotes were intensely observed in glia cells in primary cell cultures infected with Ltropica promastigotes. No promastigotes were seen on Giemsa stained preparations of the precipitates prepared from the bottom sediment after the centrifugation of the liquid medium removed from the infected plates. In this study, promastigotes from a cutaneous leishmaniasis patient unable to respond to pentavalent antimony therapy were shown to infect rat glia cells and converted to amastigote form. This amastigote glial cell model, as far as we know, is the first model in the literature produced by Ltropica. The occurrence of Ltropica amastigote forms in glia cells may be indicative of the ability of Leishmania species to infect the central nervous system. The central nervous system may be an area for the Leishmania amastigotes to escape from the immune system in cases of leishmaniasis without a treatment response. Our study is important because it is the first study to show the infection of glia cells with L.tropica amastigotes. © 2018 Ankara Microbiology Society. All rights reserved.
dc.language.isoTurkish
dc.publisherAnkara Microbiology Society
dc.titleInfecting glial cells with antimony resistant Leishmania tropica: A new ex-vivo model [Glia Hücrelerinin Antimona Dirençli Leishmania tropica ile Enfekte Edilmesi: Yeni Bir ex-vivo Modeli]
dc.typeArticle
dc.contributor.departmentEge University, Faculty of Medicine, Department of Parasitology, Bornova, Izmir, Turkey; Dicle University, Faculty of Medicine, Department of Dermatology, Diyarbakir, Turkey; Ege University, Faculty of Medicine, Department of Physiology, Izmir, Turkey; Ege University, Faculty of Medicine, Department of Geriatric, Izmir, Turkey; Celal Bayar University, Faculty of Medicine, Department of Parasitology, Manisa, Turkey
dc.identifier.DOI-ID10.5578/mb.66350
dc.identifier.volume52
dc.identifier.pages49-55


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