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Protective and therapeutic effect of apocynin on bleomycin induced lung fibrosis in rats

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dc.contributor.author Kılıç, Talat
dc.contributor.author Parlakpınar, Hakan
dc.contributor.author Taşlıdere, Elif
dc.contributor.author Yıldız, Sedat
dc.contributor.author Polat, Alaadin
dc.contributor.author Vardı, Nigar
dc.contributor.author Çolak, Cemil
dc.contributor.author Ermiş, Hilal
dc.date.accessioned 2017-08-18T06:44:10Z
dc.date.available 2017-08-18T06:44:10Z
dc.date.issued 2015
dc.identifier.citation Kılıç, T. Parlakpınar, H. Taşlıdere, E. Yıldız, S. Polat, A. Vardı, N. Çolak, C. Ermiş, H. (2015). Protective and therapeutic effect of apocynin on bleomycin induced lung fibrosis in rats. Inflammation. 38, (3); 1166-1180. tr_TR
dc.identifier.uri http://hdl.handle.net/11616/7615
dc.description.abstract We aimed to investigate the preventive and therapeutic effect of apocynin (APO) on bleomycin (BLC)-induced lung injury in rats. Rats were assigned into groups as follows: control group; APO group, 20 mg/kg APO was given intraperitoneal for 29 days; BLC-1 and BLC-2 groups, a single intratracheal injection of BLC (2.5 mg/kg); APO+BLC-preventive group, 20 mg/kg APO was administered 12 h before the intratracheal BLC injection and continued for 14 days; BLC+APO-treatment group, 20 mg/kg APO was given on the 14th day after the intratracheal BLC injection and continued to sacrifice. The BLC-1 group was sacrificed on the 14th day of BLC administration to validate BLCinduced lung inflammation and fibrosis on the 14th of study initiation. All other groups were sacrificed on the 29th day after BLC administration. The semiquantitative histopathological assessment, tissue levels of malondialdehyde (MDA), superoxide dismutase, catalase (CAT), glutathione peroxidase (GPx), reduced glutathione (GSH), total antioxidant capacity, total oxidant status (TOS), and oxidative stress index (OSI) were measured. An addition to the serum myeloperoxidase (MPO), the cell count and cytokines (IL-1β, IL-6, and IL-8) of bronchoalveolar lavage (BAL) fluid were assayed. BLC-provoked histological changes were significantly detected compared to the control group. APO restored these histological damages in different quantity in the treatment and prevention groups. BLC caused a significant decrease in GSH, CAT, and GPX, which were accompanied with significantly the increased MDA, TOS levels, and OSI in the lung tissue concomitant with increased levels of the cellular account and proinflammatory cytokines in the BAL fluid. Otherwise, APO administration, both before and after BLC, reversed all biochemical markers and cytokine as well as histopathological changes induced by BLC. Interestingly, APO treatment reversed MPO activity in serum increased by BLC. In this study, both protective and therapeutic effects of APO against BLC-induced lung fibrosis were demonstrated for the first time. tr_TR
dc.language.iso eng tr_TR
dc.publisher Inflammation tr_TR
dc.relation.isversionof 10.1007/s10753-014-0081-1 tr_TR
dc.rights info:eu-repo/semantics/openAccess tr_TR
dc.subject Apocynin tr_TR
dc.subject Antioxidant tr_TR
dc.subject Bleomycin tr_TR
dc.subject Cytokine tr_TR
dc.subject Pulmonary fibrosis tr_TR
dc.title Protective and therapeutic effect of apocynin on bleomycin induced lung fibrosis in rats tr_TR
dc.type article tr_TR
dc.relation.journal Inflammation tr_TR
dc.contributor.department İnönü Üniversitesi tr_TR
dc.contributor.authorID 9217 tr_TR
dc.identifier.volume 38 tr_TR
dc.identifier.issue 3 tr_TR
dc.identifier.startpage 1166 tr_TR
dc.identifier.endpage 1180 tr_TR


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