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Deconvolution of mixture spectra and increased throughput of peptide identification by utilization of intensified complementary ions formed in tandem mass spectrometry

机译:利用串联质谱中形成的增强互补离子对混合物光谱进行反卷积并提高肽鉴定的通量

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摘要

A cornerstone of mass spectrometry based proteomics is to relate with high statistical significance experimentally obtained tandem mass spectrometry (MS/MS) data to peptide sequences from a protein database. Most sequence specific fragment ions in MS/MS spectra are represented by a subset of complementary ion pairs. Here, we investigated the reliabilities of complementary ion pairs formed in CAD and CAD/ETD MS/MS and developed a reliability-based approach of intensification of ion signals of complementary pairs prior to database searching. In a large-scale proteomics experiment using high-resolution orbitrap mass spectrometry, an increase in the number of peptide identifications was obtained relative to the original CAD MS/MS spectra when intensified golden complementary (+18.6%) and CAD complementary pairs (+17.2%) were submitted to the Mascot search engine. This also exceeded the results obtained by deisotoping/deconvolution of CAD MS/MS spectra. A novel approach for extracting sequence-specific fragment ions of co-isolated peptides was developed based on the complementarity rules. This technique demonstrated an impressive gain of 42.4% more peptide identifications as compared with the use of the initial data set.
机译:基于质谱的蛋白质组学的基石与具有高统计意义的实验相关联,该实验是通过实验获得的串联质谱(MS / MS)数据与蛋白质数据库中的肽序列相关联的。 MS / MS谱图中大多数序列特定的碎片离子由互补离子对的子集表示。在这里,我们研究了在CAD和CAD / ETD MS / MS中形成的互补离子对的可靠性,并在数据库搜索之前开发了一种基于可靠性的增强互补对离子信号的方法。在使用高分辨率orbitrap质谱仪进行的大规模蛋白质组学实验中,当金色互补(+ 18.6%)和CAD互补对(+17.2)增强时,相对于原始CAD MS / MS谱图,肽鉴定的数量增加了%)已提交给Mascot搜索引擎。这也超过了通过对CAD MS / MS光谱进行去同位素/去卷积获得的结果。基于互补规则,开发了一种提取共分离肽的序列特异性片段离子的新方法。与使用初始数据集相比,该技术显示出令人印象深刻的肽鉴定增加了42.4%。

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