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Short-range RNA-RNA crosslinking methods to determine rRNA structure and interactions.

机译:短程RNA-RNA交联方法可确定rRNA的结构和相互作用。

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We describe details of procedures to analyze RNA-RNA crosslinks made by far-UV irradiation (< 300 nm) or made by irradiation with near-UV light (320-365 nm) on RNA containing photosensitive nucleotides, in the present case containing 4-thiouridine. Zero-length crosslinks of these types must occur because of the close proximity of the participants through either specific interactions or transient contacts in the folded RNA structure, so they are valuable monitors of the conformation of the RNA. Procedures to produce crosslinks in the 16S ribosomal RNA and between the 16S rRNA and mRNA or tRNA are described. Gel electrophoresis conditions are described that separate the products according to their structure to allow the determination of the number and frequency of the crosslinking products. Gel electrophoresis together with an ultracentrifugation procedure for the efficient recovery of RNA from the polyacrylamide gels allows the purification of molecules containing different crosslinks. These separation techniques allow the analysis of the sites of crosslinking by primer extension and RNA sequencing techniques. The procedures are applicable to other types of RNA molecules with some differences to control levels of crosslinking and separation conditions. Copyright 2001 Elsevier Science (USA).
机译:我们描述了程序的细节,以分析由远紫外线(<300 nm)或由近紫外线(320-365 nm)照射在含光敏核苷酸的RNA上形成的RNA-RNA交联,在本例中,该光敏核苷酸为4-硫尿苷。由于参与者通过折叠RNA结构中的特定相互作用或短暂接触而非常接近,因此必须发生这些类型的零长度交联,因此它们是RNA构象的重要监测者。描述了在16S核糖体RNA中以及16S rRNA与mRNA或tRNA之间产生交联的程序。描述了根据产物的结构分离产物的凝胶电泳条件,从而可以确定交联产物的数量和频率。凝胶电泳和超速离心程序可从聚丙烯酰胺凝胶中有效回收RNA,从而可以纯化含有不同交联键的分子。这些分离技术允许通过引物延伸和RNA测序技术分析交联位点。该程序适用于其他类型的RNA分子,但存在一些差异以控制交联和分离条件的水平。版权所有2001 Elsevier Science(美国)。

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