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Bottom-up mass spectrometric sequencing of microRNA

机译:MicroRNA的自下而上的质谱测序

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The increasing interest in microRNA (miRNA) as diagnostic biomarkers or potential drug targets has raised the demand for more accurate miRNA detection. One way to improve the accuracy is by using mass spectrometry (MS) to measure miRNA directly. Matrix-assisted laser desorption/ionization (MALDI) MS stands apart from other MS techniques due to the fact that a MALDI matrix is required for sample preparation. In this study, by exploiting the acidity of MALDI matrix and its mixing with miRNA prior to MS measurements, a simple method to generate RNA sequencing ladders is developed. The method utilizes the MALDI matrix to hydrolyze RNA at high temperature. The resulting sequencing ladders are ready to be measured without any desalting. By using MALDI SpiralTOF MS, the monoisotopic mass of each RNA fragment was measured. The RNA sequence was determined by sequentially comparing nucleotide compositions that were calculated from measured monoisotopic masses. The use of nucleotide compositions to assist the spectral interpretation has the advantages on distinguishing the complementary sequencing ladders, and allows the nucleotide identity at each position to be crosschecked multiple times. Together with the analysis of both complementary sequencing ladders, 100% sequence coverage and sequence accuracy were achieved in a blinded study.
机译:对MicroRNA(miRNA)的兴趣日益增加,作为诊断生物标志物或潜在的药物靶标的提高了对更准确的miRNA检测的需求。提高精度的一种方法是通过使用质谱(MS)直接测量miRNA。基质辅助激光解吸/电离(MALDI)MS由于样品制备所需的MALDI基质是由于MALDI基质所需的其他MS技术。在本研究中,通过在MS测量之前利用MARDI基质的酸度及其与miRNA的混合,开发了产生RNA测序梯子的简单方法。该方法利用MALDI基质在高温下水解RNA。所得到的测序梯子可以在没有任何脱盐的情况下测量。通过使用MALDI SPIRALTOF MS,测量每个RNA片段的单同位素质量。通过顺序地比较由测量的单同步体质量计算的核苷酸组合物来确定RNA序列。使用核苷酸组合物来帮助光谱解释具有区分互补测序梯子的优点,并允许多次交叉检查每个位置的核苷酸同一性。与互补测序梯子的分析一起,在盲化的研究中实现了100%序列覆盖和序列精度。

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