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拟南芥、玉米、豌豆和烟草叶绿体提取物中外源RNA编辑的检测。

Assay of editing of exogenous RNAs in chloroplast extracts of Arabidopsis, maize, pea, and tobacco.

作者信息

Hayes Michael L, Hanson Maureen R

机构信息

Department of Molecular Biology and Genetics, Cornell University, Ithaca, New York, USA.

出版信息

Methods Enzymol. 2007;424:459-82. doi: 10.1016/S0076-6879(07)24021-2.

Abstract

Nucleotides within transcripts of chloroplasts and mitochondria are modified through C-to-U RNA editing in vascular plants. The specific protein components and enzymatic machinery required for editing have not been defined. A consensus sequence is not present around all editing sites, complicating the discovery of cis-sequence elements critical for editing. Chloroplast extracts capable of carrying out editing in vitro along with precise quantification of editing extent of exogenous transcripts will facilitate identification of both cis and trans factors. We have optimized an in vitro assay originally developed to study editing in tobacco and pea chloroplasts and have expanded the assay to include the study of chloroplast editing in the model species Arabidopsis and the monocot maize. The superior genetic resources in these two species can now be utilized in conjunction with biochemical analysis to dissect the editing apparatus. We have improved the assay conditions for editing in vitro, achieving efficient editing (as much as 92%) with certain RNA substrates. Unlike the initial assay that relied on qualitative analysis, we are able to achieve precise quantification of editing activity within 1% through a simple poisoned primer extension (PPE) assay with radiolabeled oligonucleotides.

摘要

在维管植物中,叶绿体和线粒体转录本中的核苷酸通过C到U的RNA编辑进行修饰。编辑所需的特定蛋白质成分和酶机制尚未明确。并非所有编辑位点周围都存在共有序列,这使得对编辑至关重要的顺式序列元件的发现变得复杂。能够在体外进行编辑的叶绿体提取物以及对外源转录本编辑程度的精确量化,将有助于鉴定顺式和反式因子。我们优化了最初用于研究烟草和豌豆叶绿体编辑的体外测定方法,并将该测定方法扩展到包括对模式植物拟南芥和单子叶植物玉米叶绿体编辑的研究。现在可以结合这两个物种优越的遗传资源和生化分析来剖析编辑装置。我们改进了体外编辑的测定条件,使用某些RNA底物可实现高效编辑(高达92%)。与最初依赖定性分析的测定方法不同,我们通过使用放射性标记寡核苷酸的简单中毒引物延伸(PPE)测定法,能够在1%的范围内实现对编辑活性的精确量化。

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