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用于动力学实验的tRNA荧光标记

Fluorescent labeling of tRNAs for dynamics experiments.

作者信息

Betteridge Thu, Liu Hanqing, Gamper Howard, Kirillov Stanislav, Cooperman Barry S, Hou Ya-Ming

机构信息

Department of Biochemistry and Molecular Biology, Thomas Jefferson University, Philadelphia, PA 19107, USA.

出版信息

RNA. 2007 Sep;13(9):1594-601. doi: 10.1261/rna.475407. Epub 2007 Jul 24.

DOI:10.1261/rna.475407
PMID:17652134
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1950756/
Abstract

Transfer RNAs (tRNAs) are substrates for complex enzymes, such as aminoacyl-tRNA synthetases and ribosomes, and play an essential role in translation of genetic information into protein sequences. Here we describe a general method for labeling tRNAs with fluorescent dyes, so that the activities and dynamics of the labeled tRNAs can be directly monitored by fluorescence during the ribosomal decoding process. This method makes use of the previously reported fluorescent labeling of natural tRNAs at dihydrouridine (D) positions, but extends the previous method to synthetic tRNAs by preparing tRNA transcripts and introducing D residues into transcripts with the yeast enzyme Dus1p dihydrouridine synthase. Using the unmodified transcript of Escherichia coli tRNAPro as an example, which has U17 and U17a in the D loop, we show that Dus1p catalyzes conversion of one of these Us (mostly U17a) to D, and that the modified tRNA can be labeled with the fluorophores proflavin and rhodamine 110, with overall labeling yields comparable to those obtained with the native yeast tRNAPhe. Further, the transcript of yeast tRNAPhe, modified by Dus1p and labeled with proflavin, translocates on the ribosome at a rate similar to that of the proflavin-labeled native yeast tRNAPhe. These results demonstrate that synthetic tRNA transcripts, which may be designed to contain mutations not found in nature, can be labeled and studied. Such labeled tRNAs should have broad utility in research that involves studies of tRNA maturation, aminoacylation, and tRNA-ribosome interactions.

摘要

转运RNA(tRNA)是诸如氨酰-tRNA合成酶和核糖体等复杂酶的作用底物,在将遗传信息转化为蛋白质序列的翻译过程中发挥着至关重要的作用。在此,我们描述了一种用荧光染料标记tRNA的通用方法,这样在核糖体解码过程中,标记后的tRNA的活性和动态变化就可以通过荧光直接监测。该方法利用了先前报道的在二氢尿嘧啶(D)位置对天然tRNA进行荧光标记的方法,但通过制备tRNA转录本并利用酵母酶Dus1p二氢尿嘧啶合成酶将D残基引入转录本,将先前的方法扩展到了合成tRNA。以大肠杆菌tRNAPro的未修饰转录本为例,其D环中有U17和U17a,我们发现Dus1p催化这些U中的一个(大多是U17a)转化为D,并且修饰后的tRNA可以用荧光染料原黄素和罗丹明110进行标记,总体标记产率与天然酵母tRNAPhe的标记产率相当。此外,经Dus1p修饰并用原黄素标记的酵母tRNAPhe转录本在核糖体上的转运速率与原黄素标记的天然酵母tRNAPhe相似。这些结果表明,可以对可能设计为包含自然界中未发现的突变的合成tRNA转录本进行标记和研究。这种标记的tRNA在涉及tRNA成熟、氨酰化和tRNA-核糖体相互作用研究的科研中应具有广泛的用途。

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