Inhibition of c-FLIP by RNAi Enhances Sensitivity of the Human Osteogenic Sarcoma Cell Line U2OS to TRAILInduced Apoptosis

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Inhibition of c-FLIP by RNAi Enhances Sensitivity of the Human Osteogenic Sarcoma Cell Line U2OS to TRAILInduced Apoptosis

机译：RNAi对c-FLIP的抑制作用增强了人类成骨肉瘤细胞系U2OS对TRAIL诱导的细胞凋亡的敏感性

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To study effects of cellular FLICE (FADD-like IL-1β-converting enzyme)-inhibitory protein (c-FLIP)inhibition by RNA interference (RNAi) on sensitivity of U2OS cells to tumor necrosis factor (TNF)-relatedapoptosis-inducing ligand (TRAIL)-induced apoptosis, plasmid pSUPER-c-FLIP-siRNA was constructed andthen transfected into U2OS cells. A stable transfection cell clone U2OS/pSUPER-c-FLIP-siRNA was screenedfrom the c-FLIP-siRNA transfected cells. RT-PCR and Western blotting were applied to measure the expressionof c-FLIP at the levels of mRNA and protein. The results indicated that the expression of c-FLIP was significantlysuppressed by the c-FLIP-siRNA in the cloned U2OS/pSUPER-c-FLIP-siRNA as compared with the controlcells of U2OS/pSUPER. The cloned cell line of U2OS/pSUPER-c-FLIP-siRNA was further examined for TRAILinducedcell death and apoptosis in the presence of a pan-antagonist of inhibitor of apoptosis proteins (IAPs)AT406, with or without 4 hrs pretreatment with rocaglamide, an inhibitor of c-FLIP biosynthesis, for 24 hrs.Cell death effects and apoptosis were measured by the methods of MTT assay with 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide and flow cytometry, respectively. The results indicated that TRAIL-inducedcell death in U2OS/pSUPER-c-FLIP-siRNA was increased compared with control cells U2OS/pSUPER in thepresence or absence of AT406. Flow cytometry indicated that TRAIL-induced cell death effects proceeded throughcell apoptosis pathway. However, in the presence of rocaglamide, cell death or apoptotic effects of TRAIL weresimilar and profound in both cell lines, suggesting that the mechanism of action for both c-FLIP-siRNA androcaglamide was identical. We conclude that the inhibition of c-FLIP by either c-FLIP-siRNA or rocaglamidecan enhance the sensitivity of U2OS to TRAIL-induced apopotosis, suggesting that inhibition of c-FLIP is a goodtarget for anti-cancer therapy.

机译：研究RNA干扰（RNAi）抑制细胞FLICE（FADD样IL-1β转换酶）抑制蛋白（c-FLIP）对U2OS细胞对肿瘤坏死因子（TNF）相关凋亡诱导配体（（TRAIL）诱导的细胞凋亡，构建了质粒pSUPER-c-FLIP-siRNA，然后将其转染到U2OS细胞中。从c-FLIP-siRNA转染的细胞中筛选出稳定的转染细胞克隆U2OS / pSUPER-c-FLIP-siRNA。应用RT-PCR和Western blotting检测mRNA和蛋白水平上c-FLIP的表达。结果表明，与U2OS / pSUPER的对照细胞相比，克隆的U2OS / pSUPER-c-FLIP-siRNA中的c-FLIP-siRNA显着抑制了c-FLIP的表达。在凋亡蛋白抑制剂（IAPs）AT406泛拮抗剂存在下或不使用rocaglamide预处理4小时的情况下，进一步检查了克隆的U2OS / pSUPER-c-FLIP-siRNA细胞系TRAIL诱导的细胞死亡和凋亡。 c-FLIP生物合成抑制剂24小时。分别通过使用3-（4,5-二甲基噻唑-2-基）-2,5-二苯基四唑溴化物的MTT分析方法和流式细胞仪测量细胞死亡效应和凋亡。结果表明，在存在或不存在AT406的情况下，与对照细胞U2OS / pSUPER相比，TRAIL诱导的U2OS / pSUPER-c-FLIP-siRNA细胞死亡增加。流式细胞术表明TRAIL诱导的细胞死亡作用通过细胞凋亡途径进行。但是，在存在rocaglamide的情况下，TRAIL在两种细胞系中的细胞死亡或凋亡效应均相似且影响深远，这表明c-FLIP-siRNA和rocaglamide的作用机理相同。我们得出的结论是，通过c-FLIP-siRNA或rocaglamide抑制c-FLIP可以增强U2OS对TRAIL诱导的凋亡的敏感性，这表明对c-FLIP的抑制是抗癌治疗的良好靶标。

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《Asian Pacific Journal of Cancer Prevention》 |2015年第6期|共6页
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Inhibition of c-FLIP by RNAi Enhances Sensitivity of the Human Osteogenic Sarcoma Cell Line U2OS to TRAILInduced Apoptosis

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