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一种使用改良型微小RNA操纵子在鸡中进行RNA干扰的强大系统。

A robust system for RNA interference in the chicken using a modified microRNA operon.

作者信息

Das Raman M, Van Hateren Nick J, Howell Gareth R, Farrell Elizabeth R, Bangs Fiona K, Porteous Victoria C, Manning Elizabeth M, McGrew Michael J, Ohyama Kyoji, Sacco Melanie A, Halley Pam A, Sang Helen M, Storey Kate G, Placzek Marysia, Tickle Cheryll, Nair Venugopal K, Wilson Stuart A

机构信息

Department of Molecular Biology and Biotechnology, The University of Sheffield, Firth Court, Western Bank, Sheffield S10 2TN, UK.

出版信息

Dev Biol. 2006 Jun 15;294(2):554-63. doi: 10.1016/j.ydbio.2006.02.020. Epub 2006 Mar 30.

Abstract

RNA interference (RNAi) provides an effective method to silence gene expression and investigate gene function. However, RNAi tools for the chicken embryo have largely been adapted from vectors designed for mammalian cells. Here we present plasmid and retroviral RNAi vectors specifically designed for optimal gene silencing in chicken cells. The vectors use a chicken U6 promoter to express RNAs modelled on microRNA30, which are embedded within chicken microRNA operon sequences to ensure optimal Drosha and Dicer processing of transcripts. The chicken U6 promoter works significantly better than promoters of mammalian origin and in combination with a microRNA operon expression cassette (MOEC), achieves up to 90% silencing of target genes. By using a MOEC, we show that it is also possible to simultaneously silence two genes with a single vector. The vectors express either RFP or GFP markers, allowing simple in vivo tracking of vector delivery. Using these plasmids, we demonstrate effective silencing of Pax3, Pax6, Nkx2.1, Nkx2.2, Notch1 and Shh in discrete regions of the chicken embryonic nervous system. The efficiency and ease of use of this RNAi system paves the way for large-scale genetic screens in the chicken embryo.

摘要

RNA干扰(RNAi)为沉默基因表达和研究基因功能提供了一种有效方法。然而,用于鸡胚的RNAi工具大多是从为哺乳动物细胞设计的载体改造而来。在此,我们展示了专门为在鸡细胞中实现最佳基因沉默而设计的质粒和逆转录病毒RNAi载体。这些载体使用鸡U6启动子来表达基于微小RNA30构建的RNA,这些RNA嵌入鸡微小RNA操纵子序列中,以确保转录本得到最佳的Drosha和Dicer加工。鸡U6启动子的效果明显优于哺乳动物来源的启动子,并且与微小RNA操纵子表达盒(MOEC)结合使用时,可实现高达90%的靶基因沉默。通过使用MOEC,我们证明了用单个载体同时沉默两个基因也是可行的。这些载体表达红色荧光蛋白(RFP)或绿色荧光蛋白(GFP)标记,便于在体内简单追踪载体递送情况。利用这些质粒,我们在鸡胚神经系统的离散区域证明了对Pax3、Pax6、Nkx2.1、Nkx2.2、Notch1和Shh的有效沉默。该RNAi系统的高效性和易用性为在鸡胚中进行大规模遗传筛选铺平了道路。

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