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Rapid conditional knock-down-knock-in system for mammalian cells

机译:哺乳动物细胞的快速条件敲除敲入系统

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摘要

RNA interference (RNAi) is a powerful tool to analyze gene function in mammalian cells. However, the interpretation of RNAi knock-down phenotypes can be hampered by off-target effects or compound phenotypes, as many proteins combine multiple functions within one molecule and coordinate the assembly of multimolecular complexes. Replacing the endogenous protein with ectopic wild-type or mutant forms can exclude off-target effects, preserve complexes and unravel specific roles of domains or modifications. Therefore, we developed a rapid-knock-down-knock-in system for mammalian cells. Stable polyclonal cell lines were generated within 2 weeks by simultaneous selection of two episomal vectors. Together these vectors mediated reconstitution and knock-down in a doxycycline-dependent manner to allow the analysis of essential genes. Depletion was achieved by an artificial miRNA-embedded siRNA targeting the untranslated region of the endogenous, but not the ectopic mRNA. To prove effectiveness, we tested 17 mutants of WDR12, a factor essential for ribosome biogenesis and cell proliferation. Loss-off function phenotypes were rescued by the wild-type and six mutant forms, but not by the remaining mutants. Thus, our system is suitable to exclude off-target effects and to functionally analyze mutants in cells depleted for the endogenous protein.
机译:RNA干扰(RNAi)是分析哺乳动物细胞中基因功能的强大工具。但是,脱靶效应或复合表型可能会妨碍RNAi敲除表型的解释,因为许多蛋白质在一个分子内结合了多种功能并协调了多分子复合物的组装。用异位野生型或突变体形式替代内源蛋白可以排除脱靶作用,保留复合物并阐明结构域或修饰的特定作用。因此,我们为哺乳动物细胞开发了一种快速敲低敲入系统。通过同时选择两种附加型载体,在2周内生成了稳定的多克隆细胞系。这些载体一起以强力霉素依赖的方式介导了重组和敲除,从而可以分析必需基因。通过靶向内源非翻译区域而不是异位mRNA的人工miRNA嵌入的siRNA来实现耗竭。为了证明有效性,我们测试了WDR12的17个突变体,这是核糖体生物发生和细胞增殖所必需的因子。功能丧失的表型可以通过野生型和六种突变体形式来挽救,而不能通过其余的突变体来挽救。因此,我们的系统适用于排除脱靶效应,并在功能上分析了内源蛋白质耗尽的细胞中的突变体。

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