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Development and validation of an RNAi screen for ABT-737 sensitizers

机译:用于ABT-737敏化剂的RNAi筛选的开发和验证

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Abstract: The chemical compound ABT-737 is a nanomolar inhibitor of several antiapoptotic Bcl-2 family members with potential therapeutic efficacy for a variety of cancers. Herein, we describe the development of a complementation-based RNAi assay that can be used to identify mechanisms of ABT-737-resistance. HeLa cells, which were resistant to ABT-737, were optimized for reverse-transfection efficiency and tested for siRNA-mediated silencing. The developed assay utilized HeLa cell reverse-transfection with 10 nM siRNA, followed by 48 h incubation, ABT-737 or DMSO treatment for 24 h, and cell viability measurement using ATPlite (which measures ATP levels as an indicator of cell viability). As a validation, the kinase subset of the Ambion Silencer Human Druggable Genome siRNA Library V2, which consisted of 865 genes (three siRNA sequences per gene), was screened. Several assay-positive siRNAs were tested and confirmed to sensitize cells to ABT-737. Transfection of cells with siRNAs targeting Bcl-2 family member Mcl-1 also potently sensitized HeLa cells to ABT-737. The current assay thus represents a screen that can be utilized to identify ABT-737-sensitizing siRNAs and correspondingly, potential new targets for drug discovery.
机译:摘要:化合物ABT-737是几种抗凋亡Bcl-2家族成员的纳摩尔抑制剂,对多种癌症都有潜在的治疗作用。在本文中,我们描述了可用于识别ABT-737抗性机制的基于互补的RNAi分析的发展。对ABT-737具有抗性的HeLa细胞经过优化,可提高逆转效率,并测试了siRNA介导的沉默。这项开发的检测方法是将HeLa细胞用10 nM siRNA进行转染,然后进行48小时孵育,ABT-737或DMSO处理24小时,并使用ATPlite(可测量ATP水平作为细胞生存能力的指标)进行细胞生存能力的测量。作为验证,筛选了Ambion Silencer人类药物基因组siRNA文库V2的激酶子集,该子集由865个基因组成(每个基因三个siRNA序列)。测试了几种测定阳性的siRNA,并确认它们使细胞对ABT-737敏感。用靶向Bcl-2家族成员Mcl-1的siRNA转染细胞也可以有效地使HeLa细胞对ABT-737敏感。因此,当前的检测方法代表了一种可用于识别ABT-737致敏siRNA以及相应地潜在的药物发现新靶标的筛选方法。

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