İZOİMPERATORİN ARACILIKLI ANTİKANSER AKTİVİTE: MİTOKONDRİYAL DİSFONKSİYONUN HEPG2 HÜCRELERİNDEKİ ROLÜ

Q4 Pharmacology, Toxicology and Pharmaceutics Ankara Universitesi Eczacilik Fakultesi Dergisi Pub Date : 2023-07-24 DOI:10.33483/jfpau.1312637
Ali Ergüç, Ege Arzuk, Gökay Albayrak, Fuat Karakuş, Hayati Okur, Şüra Baykan
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Abstract

Objective: The first goal of the present study is to investigate the role of mitochondria due to the Crabtree effect in HepG2 cells exposed to ISO in either glucose- or galactose-conditioned media. The second aim is to predict the interactions between electron transport chain (ETC) complexes and ISO, which might be the possible reason for mitochondrial dysfunction. Material and Method: Cell viability and membrane damage for HepG2 cells exposed to ISO (12.5, 25, 50, 100, and 250 µM) were assessed by MTT and LDH leakage assays in either glucose- or galactose-conditioned media. The affinity of ISO to ETC complexes was also determined by a molecular docking study. Result and Discussion: MTT assay showed that 250 µM ISO leads to cytotoxic activity in glucose-conditioned media, while 25 µM and higher concentrations of ISO decrease cell viability in galactose-conditioned media. A membrane damage assay conducted in a glucose-conditioned media assay revealed that 250 µM ISO disrupts the cell membrane. 100 and 250 µM ISO increased membrane damage in galactose-conditioned media. According to docking simulations, binding affinities of ISO to ETC complexes are in descending order: Complex IV > Complex I > Complex III > Complex II. Inhibition of complex IV by ISO inhibits the transfer of electrons from cytochrome c to oxygen, and the proton gradient collapses. The present study proposed that ISO leads to mitochondrial dysfunction via inhibition of the ETC.
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目的:本研究的第一个目标是研究在葡萄糖或半乳糖条件培养基中暴露于ISO的HepG2细胞中由于Crabtree效应引起的线粒体的作用。第二个目的是预测电子传输链(ETC)复合物与ISO之间的相互作用,这可能是线粒体功能障碍的原因。材料和方法:在葡萄糖或半乳糖条件培养基中,通过MTT和LDH渗漏测定评估暴露于ISO(12.5、25、50、100和250µM)的HepG2细胞的细胞活力和膜损伤。ISO与ETC复合物的亲和力也通过分子对接研究确定。结果和讨论:MTT分析显示,250µM ISO在葡萄糖条件培养基中具有细胞毒性活性,而25µM和更高浓度的ISO降低了半乳糖条件培养基的细胞活力。在葡萄糖条件培养基测定中进行的膜损伤测定显示,250µM ISO会破坏细胞膜。在半乳糖条件培养基中,100和250µM ISO增加了膜损伤。根据对接模拟,ISO与ETC复合物的结合亲和力按降序排列:复合物IV>复合物I>复合物III>复合物II。ISO对复合物IV的抑制抑制了电子从细胞色素c向氧的转移,质子梯度崩溃。本研究提出ISO通过抑制ET导致线粒体功能障碍。
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来源期刊
Ankara Universitesi Eczacilik Fakultesi Dergisi
Ankara Universitesi Eczacilik Fakultesi Dergisi Pharmacology, Toxicology and Pharmaceutics-Pharmaceutical Science
CiteScore
0.80
自引率
0.00%
发文量
70
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