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A bi-functional siRNA construct induces RNA interference and also primes PCR amplification for its own quantification

机译:双功能siRNA构建体可诱导RNA干扰,还可引发PCR扩增以进行自身定量

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摘要

RNA interference (RNAi) is a process of post-transcriptional gene silencing initiated by double-stranded RNAs, including short interfering RNA (siRNA). Silencing is sequence-specific and RNAi has rapidly become central to the study of gene function. RNAi also carries promise for selective silencing of viral and endogenous genes causal for disease. To detect the very low levels of siRNA effective for RNAi we modified the 3' end of the sense strand of siRNA with a nuclease-resistant DNA hairpin. We show that the modified siRNA-DNA construct (termed 'crook' siRNA) functions as a primer for the PCR and describe a novel, yet simple PCR protocol for its quantification (amolar levels/cell). When transfected into mammalian cells, crook siRNA induces selective mRNA knock-down equivalent to its unmodified siRNA counterpart. This new bifunctional siRNA construct will enable future in vivo studies on the uptake, distribution and pharmacokinetics of siRNA, and is particularly important for the development of siRNA-based therapeutics. More generally, PCR-based detection of siRNA carries wide-ranging applications for RNAi reverse genetics.
机译:RNA干扰(RNAi)是转录后基因沉默的过程,该过程由双链RNA(包括短干扰RNA(siRNA))引发。沉默是序列特异性的,RNAi已迅速成为基因功能研究的中心。 RNAi还有望选择性沉默导致疾病的病毒和内源基因。为了检测对RNAi有效的极低水平的siRNA,我们用耐核酸酶的DNA发夹修饰了siRNA有义链的3'末端。我们显示,修改后的siRNA-DNA构建体(称为“ crook” siRNA)起PCR引物的作用,并描述了一种新颖但简单的PCR协议以对其进行定量(无定型水平/细胞)。当被转染到哺乳动物细胞中时,弯曲的siRNA诱导选择性的mRNA敲低,等同于其未修饰的siRNA对应物。这种新的双功能siRNA构建体将使未来对siRNA的吸收,分布和药代动力学的体内研究成为可能,并且对于基于siRNA的治疗剂的开发特别重要。更普遍地,基于PCR的siRNA检测在RNAi反向遗传学中具有广泛的应用。

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