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Attomole quantification and global profile of RNA modifications: Epitranscriptome of human neural stem cells

机译:Attomole定量和RNA修饰的整体概况:人类神经干细胞的转录组。

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Exploration of the epitranscriptome requires the development of highly sensitive and accurate technologies in order to elucidate the contributions of the more than 100 RNA modifications to cell processes. A highly sensitive and accurate ultra-high performance liquid chromatography-tandem mass spectrometry method was developed to simultaneously detect and quantify 28 modified and four major nucleosides in less than 20 min. Absolute concentrations were calculated using extinction coefficients of each of the RNA modifications studied. A comprehensive RNA modifications database of UV profiles and extinction coefficient is reported within a 2.3-5.2 % relative standard deviation. Excellent linearity was observed 0.99227-0.99999 and limit of detection values ranged from63.75 attomoles to 1.21 femtomoles. The analytical performance was evaluated by analyzing RNA modifications from 100 ng of RNA from human pluripotent stem cell-derived neural cells. Modifications were detected at concentrations four orders of magnitude lower than the corresponding parental nucleosides, and as low as 23.01 femtograms, 64.09 attomoles. Direct and global quantitative analysis of RNA modifications are among the advantages of this new approach.
机译:探索转录组需要开发高度敏感和准确的技术,以阐明100多种RNA修饰对细胞过程的贡献。开发了一种高度灵敏,准确的超高效液相色谱-串联质谱方法,可以在不到20分钟的时间内同时检测和定量分析28种修饰核苷和4种主要核苷。使用研究的每种RNA修饰的消光系数计算绝对浓度。报告了一个完整的UV谱和消光系数的RNA修饰数据库,相对标准偏差在2.3-5.2%之内。观察到0.99227-0.99999的极佳线性度,检测值的范围从63.75 tom到1.21飞摩尔。通过分析来自人多能干细胞的神经细胞的100 ng RNA的RNA修饰来评估分析性能。在比相应亲代核苷低四个数量级的浓度下检测到修饰,其低至23.01飞克,64.09原子。 RNA修饰的直接和全局定量分析是这种新方法的优点。

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