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RNA干扰微阵列:哺乳动物细胞中的高通量功能丧失遗传学

RNA interference microarrays: high-throughput loss-of-function genetics in mammalian cells.

作者信息

Silva Jose M, Mizuno Hana, Brady Amy, Lucito Robert, Hannon Gregory J

机构信息

Watson School of Biological Sciences, Cold Spring Harbor Laboratory, 1 Bungtown Road, Cold Spring Harbor, NY 11724, USA.

出版信息

Proc Natl Acad Sci U S A. 2004 Apr 27;101(17):6548-52. doi: 10.1073/pnas.0400165101. Epub 2004 Apr 14.

Abstract

RNA interference (RNAi) is a biological process in which a double-stranded RNA directs the silencing of target genes in a sequence-specific manner. Exogenously delivered or endogenously encoded double-stranded RNAs can enter the RNAi pathway and guide the suppression of transgenes and cellular genes. This technique has emerged as a powerful tool for reverse genetic studies aimed toward the elucidation of gene function in numerous biological models. Two approaches, the use of small interfering RNAs and short hairpin RNAs (shRNAs), have been developed to permit the application of RNAi technology in mammalian cells. Here we describe the use of a shRNA-based live-cell microarray that allows simple, low-cost, high-throughput screening of phenotypes caused by the silencing of specific endogenous genes. This approach is a variation of "reverse transfection" in which mammalian cells are cultured on a microarray slide spotted with different shRNAs in a transfection carrier. Individual cell clusters become transfected with a defined shRNA that directs the inhibition of a particular gene of interest, potentially producing a specific phenotype. We have validated this approach by targeting genes involved in cytokinesis and proteasome-mediated proteolysis.

摘要

RNA干扰(RNAi)是一种生物学过程,其中双链RNA以序列特异性方式指导靶基因的沉默。外源性递送或内源性编码的双链RNA可进入RNAi途径并指导转基因和细胞基因的抑制。这项技术已成为反向遗传学研究的有力工具,旨在阐明众多生物学模型中的基因功能。已经开发出两种方法,即使用小干扰RNA和短发夹RNA(shRNA),以允许在哺乳动物细胞中应用RNAi技术。在这里,我们描述了一种基于shRNA的活细胞微阵列的使用,该微阵列允许对由特定内源性基因沉默引起的表型进行简单、低成本、高通量的筛选。这种方法是“反向转染”的一种变体,其中哺乳动物细胞在涂有不同shRNA的转染载体的微阵列载玻片上培养。单个细胞簇被特定的shRNA转染,该shRNA指导对特定感兴趣基因的抑制,可能产生特定的表型。我们通过靶向参与胞质分裂和蛋白酶体介导的蛋白水解的基因验证了这种方法。

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