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制备热带爪蟾卵提取物以鉴定微管相关RNA。

Production of Xenopus tropicalis egg extracts to identify microtubule-associated RNAs.

作者信息

Sharp Judith A, Blower Mike D

机构信息

Department of Molecular Biology, Massachusetts General Hospital, MA, USA.

出版信息

J Vis Exp. 2013 Jun 27(76):50434. doi: 10.3791/50434.

Abstract

Many organisms localize mRNAs to specific subcellular destinations to spatially and temporally control gene expression. Recent studies have demonstrated that the majority of the transcriptome is localized to a nonrandom position in cells and embryos. One approach to identify localized mRNAs is to biochemically purify a cellular structure of interest and to identify all associated transcripts. Using recently developed high-throughput sequencing technologies it is now straightforward to identify all RNAs associated with a subcellular structure. To facilitate transcript identification it is necessary to work with an organism with a fully sequenced genome. One attractive system for the biochemical purification of subcellular structures are egg extracts produced from the frog Xenopus laevis. However, X. laevis currently does not have a fully sequenced genome, which hampers transcript identification. In this article we describe a method to produce egg extracts from a related frog, X. tropicalis, that has a fully sequenced genome. We provide details for microtubule polymerization, purification and transcript isolation. While this article describes a specific method for identification of microtubule-associated transcripts, we believe that it will be easily applied to other subcellular structures and will provide a powerful method for identification of localized RNAs.

摘要

许多生物体将信使核糖核酸(mRNA)定位到特定的亚细胞位置,以在空间和时间上控制基因表达。最近的研究表明,转录组的大部分都定位在细胞和胚胎中的非随机位置。一种识别定位mRNA的方法是通过生物化学方法纯化感兴趣的细胞结构,并识别所有相关的转录本。利用最近开发的高通量测序技术,现在可以直接识别与亚细胞结构相关的所有RNA。为了便于转录本识别,有必要使用具有全基因组序列的生物体。用于亚细胞结构生物化学纯化的一个有吸引力的系统是由非洲爪蟾(Xenopus laevis)产生的卵提取物。然而,非洲爪蟾目前没有全基因组序列,这阻碍了转录本的识别。在本文中,我们描述了一种从相关的热带爪蟾(X. tropicalis)制备卵提取物的方法,热带爪蟾具有全基因组序列。我们提供了微管聚合、纯化和转录本分离的详细信息。虽然本文描述了一种识别微管相关转录本的特定方法,但我们相信它将很容易应用于其他亚细胞结构,并将为识别定位RNA提供一种强大的方法。

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