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A strategy for absolute proteome quantification with mass spectrometry by hierarchical use of peptide-concatenated standards

机译:通过分层使用肽级联的标准品对质谱进行绝对蛋白质组定量的策略

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摘要

The accurate and precise absolute abundance of proteins can be determined using mass spectrometry by spiking the sample with stable isotope-labeled standards. In this study, we developed a strategy of hierarchical use of peptide-concatenated standards (PCSs) to quantify more proteins over a wider dynamic range. Multiple primary PCSs were used for quantification of many target proteins. Unique "ID-tag peptides" were introduced into individual primary PCSs, allowing us to monitor the exact amounts of individual PCSs using a "secondary PCS" in which all "ID-tag peptides" were concatenated. Furthermore, we varied the copy number of the "ID-tag peptide" in each PCS according to a range of expression levels of target proteins. This strategy accomplished absolute quantification over a wider range than that of the measured ratios. The quantified abundance of budding yeast proteins showed a high reproducibility for replicate analyses and similar copy numbers per cell for ribosomal proteins, demonstrating the accuracy and precision of this strategy. A comparison with the absolute abundance of transcripts clearly indicated different post-transcriptional regulation of expression for specific functional groups. Thus, the approach presented here is a faithful method for the absolute quantification of proteomes and provides insights into biological mechanisms, including the regulation of expressed protein abundance.
机译:可以通过使用稳定同位素标记的标准品加标样,使用质谱法确定蛋白质的准确和精确的绝对丰度。在这项研究中,我们开发了一种分级使用肽连接标准品(PCS)的策略,以在更宽的动态范围内定量更多的蛋白质。多个主要PCS用于定量许多靶蛋白。独特的“ ID标签肽”被引入单个初级PCS中,从而使我们能够使用“次级PCS”(其中所有“ ID标签肽”串联在一起)来监视单个PCS的确切数量。此外,我们根据靶蛋白的表达水平范围改变了每个PCS中“ ID标签肽”的拷贝数。该策略在比测量比率更大的范围内实现了绝对定量。定量出芽的酵母蛋白显示出重复分析的高再现性,核糖体蛋白每个细胞的拷贝数相似,证明了该策略的准确性和精确性。与转录本的绝对丰度的比较清楚地表明,特定功能基团的转录后表达调控不同。因此,本文介绍的方法是对蛋白质组进行绝对定量的忠实方法,并提供了生物学机制的见解,包括对表达的蛋白质丰度的调节。

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