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RNA interference by expression of short-interfering RNAs and hairpin RNAs in mammalian cells

机译:通过在哺乳动物细胞中表达短干扰RNA和发夹RNA来干扰RNA

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摘要

Duplexes of 21-nt RNAs, known as short-interfering RNAs (siRNAs), efficiently inhibit gene expression by RNA interference (RNAi) when introduced into mammalian cells. We show that siRNAs can be synthesized by in vitro transcription with T7 RNA polymerase, providing an economical alternative to chemical synthesis of siRNAs. By using this method, we show that short hairpin siRNAs can function like siRNA duplexes to inhibit gene expression in a sequence-specific manner. Further, we find that hairpin siRNAs or siRNAs expressed from an RNA polymerase III vector based on the mouse U6 RNA promoter can effectively inhibit gene expression in mammalian cells. U6-driven hairpin siRNAs dramatically reduced the expression of a neuron-specific β-tubulin protein during the neuronal differentiation of mouse P19 cells, demonstrating that this approach should be useful for studies of differentiation and neurogenesis. We also observe that mismatches within hairpin siRNAs can increase the strand selectivity of a hairpin siRNA, which may reduce self-targeting of vectors expressing siRNAs. Use of hairpin siRNA expression vectors for RNAi should provide a rapid and versatile method for assessing gene function in mammalian cells, and may have applications in gene therapy.
机译:21 nt RNA的双链体(称为短干扰RNA(siRNA))在导入哺乳动物细胞后,可通过RNA干扰(RNAi)有效抑制基因表达。我们表明,可以通过体外转录与T7 RNA聚合酶合成siRNA,为siRNA的化学合成提供了一种经济的选择。通过使用此方法,我们表明,短发夹siRNA可以像siRNA双链体一样发挥功能,以序列特异性方式抑制基因表达。此外,我们发现发夹siRNA或从基于小鼠U6 RNA启动子的RNA聚合酶III载体表达的siRNA可以有效抑制哺乳动物细胞中的基因表达。在小鼠P19细胞的神经元分化过程中,U6驱动的发夹siRNA显着降低了神经元特异性β-微管蛋白的表达,表明该方法对分化和神经发生的研究应是有用的。我们还观察到发夹siRNA内的错配会增加发夹siRNA的链选择性,这可能会降低表达siRNA的载体的自我定位。将发夹siRNA表达载体用于RNAi应该为评估哺乳动物细胞中的基因功能提供一种快速而通用的方法,并且可能在基因治疗中得到应用。

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