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High levels of apoptosis are induced in human glioma cell lines by co-administration of peptide nucleic acids targeting miR-221 and miR-222

机译:通过共同施用靶向miR-221和miR-222的肽核酸在人神经胶质瘤细胞系中诱导高水平的凋亡

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The biological activity of a combined treatment of U251, U373 and T98G glioma cell lines with two anti-miR PNAs, directed against miR?221 and miR?222 and conjugated with an ocataarginine tail (R8-PNA-a221 and R8-PNA-a222) for efficient cellular delivery, was determined. Apoptosis was analyzed, and the effect of the combined treatment of glioma cells with either or both PNAs on the reversion of drug-resistance phenotype was assessed in the temozolomide-resistant T98G glioma cell line. Selectivity of PNA/miRNA interactions was studied by surface plasmon resonance (SPR)-based Biacore analysis. Specificity of the PNA effects at the cellular level was analyzed by RT-qPCR. These experiments support the concept that the effects of R8-PNA-a221 and R8-PNA-a222 are specific. The studies on apoptosis confirmed that the R8-PNA-a221 induces apoptosis and demonstrated the pro-apoptotic effects of R8-PNA-a222. Remarkably, increased pro-apoptotic effects were obtained with the co-administration of both anti-miR?221 and anti-miR?222 PNAs. In addition, co-administration of R8-PNA-a221 and R8-PNA-a222 induced apoptosis of TMZ-treated T98G cells at a level higher than that obtained following singular administration of R8-PNA-a221 or R8-PNA-a222.
机译:用两种针对miR?221和miR?222并与ocataarginine尾巴缀合的抗miR PNA联合治疗U251,U373和T98G胶质瘤细胞系的生物学活性(R8-PNA-a221和R8-PNA-a222确定有效的细胞递送。分析了细胞凋亡,并在耐替莫唑胺的T98G神经胶质瘤细胞系中评估了用一种或两种PNA联合治疗胶质瘤细胞对耐药表型逆转的影响。通过基于表面等离振子共振(SPR)的Biacore分析研究了PNA / miRNA相互作用的选择性。通过RT-qPCR分析PNA作用在细胞水平上的特异性。这些实验支持以下概念:R8-PNA-a221和R8-PNA-a222的作用是特定的。凋亡研究证实,R8-PNA-a221诱导细胞凋亡,并证明了R8-PNA-a222的促凋亡作用。值得注意的是,同时施用抗miR?221和抗miR?222 PNA可获得增强的促凋亡作用。另外,R8-PNA-a221和R8-PNA-a222的共同施用诱导了TMZ处理的T98G细胞的凋亡,其水平高于单独施用R8-PNA-a221或R8-PNA-a222后获得的水平。

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