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'RNA 漫步' 是一种研究小 RNA 与其靶标之间 RNA-RNA 相互作用的新方法。

'RNA walk' a novel approach to study RNA-RNA interactions between a small RNA and its target.

机构信息

The Mina and Everard Goodman Faculty of Life Sciences, Bar Ilan University, Ramat-Gan, Israel.

出版信息

Nucleic Acids Res. 2010 Jan;38(1):e5. doi: 10.1093/nar/gkp872. Epub 2009 Oct 23.

Abstract

In this study we describe a novel method to investigate the RNA-RNA interactions between a small RNA and its target that we termed 'RNA walk'. The method is based on UV-induced AMT cross-linking in vivo followed by affinity selection of the hybrid molecules and mapping the intermolecular adducts by RT-PCR or real-time PCR. Domains carrying the cross-linked adducts fail to efficiently amplify by PCR compared with non-cross-linked domains. This method was calibrated and used to study the interaction between a special tRNA-like molecule (sRNA-85) that is part of the trypanosome signal recognition particle (SRP) complex and the ribosome. Four contact sites between sRNA-85 and rRNA were identified by 'RNA walk' and were further fine-mapped by primer extension. Two of the contact sites are expected; one contact site mimics the interaction of the mammalian Alu domain of SRP with the ribosome and the other contact sites include a canonical tRNA interaction. The two other cross-linked sites could not be predicted. We propose that 'RNA walk, is a generic method to map target RNA small RNAs interactions in vivo.

摘要

在这项研究中,我们描述了一种研究小 RNA与其靶标之间 RNA-RNA 相互作用的新方法,我们称之为“RNA 漫步”。该方法基于 UV 诱导的体内 AMT 交联,然后通过亲和选择杂交分子,并通过 RT-PCR 或实时 PCR 对分子间加合物进行作图。与非交联结构域相比,携带交联加合物的结构域不能有效地进行 PCR 扩增。该方法经过校准并用于研究特殊 tRNA 样分子 (sRNA-85) 与核糖体之间的相互作用,sRNA-85 是原生动物信号识别颗粒 (SRP) 复合物的一部分。通过“RNA 漫步”鉴定了 sRNA-85 和 rRNA 之间的四个接触位点,并通过引物延伸进一步精确定位。其中两个接触位点是预期的;一个接触位点模拟了哺乳动物 SRP Alu 结构域与核糖体的相互作用,而其他接触位点包括一个典型的 tRNA 相互作用。另外两个交联位点无法预测。我们提出“RNA 漫步”是一种在体内绘制靶 RNA 与小 RNA 相互作用的通用方法。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/b588/2800229/85cbd0347a72/gkp872f1.jpg

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