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Functional studies of the PI(3)-kinase signalling pathway employing synthetic and expressed siRNA

机译:使用合成和表达的siRNA的PI(3)激酶信号通路的功能研究

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摘要

RNA interference (RNAi) is a RNA-mediated sequence-specific gene silencing mechanism. Recently, this mechanism has been used to down-regulate protein expression in mammalian cells by applying synthetic- or vector-generated small interfering RNAs (siRNAs). However, for the evaluation of this new knockdown technology, it is crucial to demonstrate biological consequences beyond protein level reduction. Here, we demonstrate that this new siRNA-based technology is suitable to analyse protein functions using the phosphatidylinositol (PI) 3-kinase signal transduction pathway as a model system. We demonstrate stable and transient siRNA-mediated knockdown of one of the PI 3-kinase catalytic subunits, p110β, which leads to inhibition of invasive cell growth in vitro as well as in a tumour model system. Importantly, this result is consistent with loss-of-function phenotypes induced by conventional RNase H-dependent antisense molecules or treatment with the PI 3-kinase inhibitor . RNAi knockdown of the downstream kinases Akt1 and Akt2 does not reduce cell growth on extracellular matrix. Our data show that synthetic siRNAs, as well as vector-based expression of siRNAs, are a powerful new tool to interfere with signal transduction processes for the elucidation of gene function in mammalian cells.
机译:RNA干扰(RNAi)是RNA介导的序列特异性基因沉默机制。最近,已通过应用合成或载体产生的小干扰RNA(siRNA),将该机制用于下调哺乳动物细胞中的蛋白质表达。但是,对于评估这种新的基因敲除技术,至关重要的是证明降低蛋白质水平之外的生物学后果。在这里,我们证明了这种基于siRNA的新技术适合使用磷脂酰肌醇(PI)3-激酶信号转导途径作为模型系统来分析蛋白质功能。我们证明PI 3激酶催化亚基之一,p110β的稳定和短暂的siRNA介导的敲低,导致体外和肿瘤模型系统中侵袭性细胞生长的抑制。重要的是,该结果与常规RNA酶H依赖性反义分子或用PI 3激酶抑制剂治疗引起的功能丧失表型一致。下游激酶Akt1和Akt2的RNAi敲低不会减少细胞外基质上的细胞生长。我们的数据表明,合成的siRNA以及基于载体的siRNA表达是一种强大的新工具,可干扰信号转导过程来阐明哺乳动物细胞中的基因功能。

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