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通过液相色谱-质谱联用(LC-MS)对转移 RNA 进行全局鉴定。

Global identification of transfer RNAs by liquid chromatography-mass spectrometry (LC-MS).

机构信息

Rieveschl Laboratories for Mass Spectrometry, Department of Chemistry, PO Box 210172, University of Cincinnati, Cincinnati, OH 45221-0172, United States.

出版信息

J Proteomics. 2012 Jun 27;75(12):3450-64. doi: 10.1016/j.jprot.2011.09.015. Epub 2011 Sep 29.

DOI:10.1016/j.jprot.2011.09.015
PMID:21982830
Abstract

Transfer ribonucleic acid (tRNA) is the non-coding RNA that links the processes of gene transcription with protein translation. While tRNAs have, individually, been studied for many years, few approaches exist for the global identification of tRNAs at the RNA and posttranscriptional RNA levels. Previously our lab introduced the concept of signature enzymatic digestion products (SDPs) for tRNA identification using matrix-assisted laser desorption/ionization mass spectrometry (MALDI-MS). SDPs enable the direct determination of tRNA identity based on mass spectrometry detection of unique m/z values from enzymatic digestion products. Here we have examined the applicability of liquid chromatography-mass spectrometry (LC-MS) and liquid chromatography tandem mass spectrometry (LC-MS/MS) for global identification of bacterial tRNAs via their SDPs using Escherichia coli as the model system. Optimal ultra high performance and high performance liquid chromatography (UPLC vs. HPLC) conditions were identified to address the hundreds of enzymatic digestion products present in the sample. The use of LC-MS/MS improves the accuracy of SDP assignments through confirming sequence information. The combination of mass unique SDP detection along with MS/MS sequencing yielded the identification of all tRNA families from E. coli and nearly doubles the number of specific SDPs detected over that previously obtained using MALDI-MS. This article is part of a Special Section entitled: Understanding genome regulation and genetic diversity by mass spectrometry.

摘要

转移核糖核酸 (tRNA) 是将基因转录过程与蛋白质翻译过程联系起来的非编码 RNA。虽然 tRNA 已经被研究了很多年,但在 RNA 和转录后 RNA 水平上对 tRNA 进行全局鉴定的方法很少。以前,我们实验室提出了使用基质辅助激光解吸/电离质谱 (MALDI-MS) 鉴定 tRNA 的特征酶切产物 (SDP) 的概念。SDP 能够基于从酶切产物中检测到的独特 m/z 值的质谱检测,直接确定 tRNA 的身份。在这里,我们研究了通过其 SDP 使用大肠杆菌作为模型系统通过液相色谱-质谱 (LC-MS) 和液相色谱串联质谱 (LC-MS/MS) 对细菌 tRNA 进行全局鉴定的适用性。确定了最佳的超高效和高效液相色谱 (UPLC 与 HPLC) 条件,以解决样品中存在的数百种酶切产物。LC-MS/MS 的使用通过确认序列信息提高了 SDP 分配的准确性。质量独特的 SDP 检测与 MS/MS 测序的结合产生了从大肠杆菌中鉴定所有 tRNA 家族的结果,并比以前使用 MALDI-MS 检测到的特定 SDP 数量增加了近一倍。本文是一个特刊的一部分,标题为:通过质谱理解基因组调控和遗传多样性。

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