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A lentiviral microRNA-based system for single-copy polymerase II-regulated RNA interference in mammalian cells

机译:基于慢病毒microRNA的系统,用于哺乳动物细胞中单拷贝聚合酶II调控的RNA干扰

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摘要

The advent of RNA interference has led to the ability to interfere with gene expression and greatly expanded our ability to perform genetic screens in mammalian cells. The expression of short hairpin RNA (shRNA) from polymerase III promoters can be encoded in transgenes and used to produce small interfering RNAs that down-regulate specific genes. In this study, we show that polymerase II-transcribed shRNAs display very efficient knockdown of gene expression when the shRNA is embedded in a microRNA context. Importantly, our shRNA expression system [called PRIME (potent RNA interference using microRNA expression) vectors] allows for the multicistronic cotranscription of a reporter gene, thereby facilitating the tracking of shRNA production in individual cells. Based on this system, we developed a series of lentiviral vectors that display tetracycline-responsive knockdown of gene expression at single copy. The high penetrance of these vectors will facilitate genomewide loss-of-function screens and is an important step toward using bar-coding strategies to follow loss of specific sequences in complex populations.
机译:RNA干扰的出现导致了干扰基因表达的能力,并大大扩展了我们在哺乳动物细胞中进行基因筛选的能力。来自聚合酶III启动子的短发夹RNA(shRNA)的表达可以在转基因中编码,并用于产生下调特定基因的小干扰RNA。在这项研究中,我们表明,当shRNA嵌入microRNA时,聚合酶II转录的shRNA表现出非常有效的基因表达抑制。重要的是,我们的shRNA表达系统(称为PRIME(使用microRNA表达的潜在RNA干扰)载体)可实现报告基因的多顺反子共转录,从而有助于追踪单个细胞中shRNA的产生。基于此系统,我们开发了一系列慢病毒载体,这些载体在单拷贝时显示出四环素反应性基因表达的敲低。这些载体的高渗透性将促进全基因组功能丧失筛选,并且是朝着使用条形码策略追踪复杂人群中特定序列丧失的重要一步。

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