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Method for Comparative Analysis of Ribonucleic Acids Using Isotope Labeling and Mass Spectrometry

机译:同位素标记和质谱法比较核糖核酸的方法

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Here, we describe a method for the comparative analysis of ribonucleic acids (RNAs). This method allows sequence or modification information from a previously uncharacterized RNA to be obtained by direct comparison with a reference RNA, whose sequence or modification information is known. This simple and rapid method is enabled by the differential labeling of two RNA samples. One sample, the reference RNA, is labeled with ~(16)O during enzymatic digestion. The second sample, the candidate or unknown RNA, is labeled with ~(18)O. By combining the two digests, digestion products that share the same sequence or post-transcriptional modification(s) between the reference and candidate will appear as doublets separated by 2 Da. Sequence or modification differences between the two will generate singlets that can be further characterized to identify how the candidate sequence differs from the reference. We illustrate the application of this approach for sequencing individual RNAs and demonstrate how this method can be used to identify sequence-specific differences in RNA modification. This comparative analysis of RNA digests (CARD) approach is scalable to multiple candidate RNAs using one or multiple reference RNAs and is compatible with existing methods for quantitative analysis of RNAs.
机译:在这里,我们描述了一种比较分析核糖核酸(RNA)的方法。该方法允许通过与参考RNA(其序列或修饰信息是已知的)直接比较来获得先前未表征的RNA的序列或修饰信息。通过两个RNA样品的差异标记,可以实现这种简单而快速的方法。在酶促消化过程中,一个样品(参考RNA)被〜(16)O标记。第二个样品是候选RNA或未知RNA,标有〜(18)O。通过将两种消化物合并,在参考物和候选物之间共享相同序列或转录后修饰的消化产物将显示为双峰,相距2 Da。两者之间的序列或修饰差异将产生单峰,可进一步表征这些峰以鉴定候选序列与参考序列的差异。我们说明了这种方法对单个RNA测序的应用,并演示了如何使用此方法来鉴定RNA修饰中的序列特异性差异。这种RNA消化的比较分析(CARD)方法可使用一个或多个参考RNA扩展到多个候选RNA,并且与现有的RNA定量分析方法兼容。

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