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Application of capillary isotachophoresis-based multidimensional separations coupled with electrospray ionization-tandem mass spectrometry for characterization of mouse brain mitochondrial proteome

机译:基于毛细管等速电泳的多维分离结合电喷雾电离串联质谱在表征小鼠脑线粒体蛋白质组学中的应用

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摘要

By employing a capillary ITP (CITP)/CZE-based proteomic technology, a total of 1795 distinct mouse Swiss-Prot protein entries (or 1705 nonredundant proteins) are identified from synaptic mitochondria isolated from mouse brain. The ultrahigh resolving power of CITP/CZE is evidenced by the large number of distinct peptide identifications measured from each CITP fraction together with the low peptide fraction overlapping among identified peptides. The degree of peptide overlapping among CITP fractions is even lower than that achieved using combined CIEFano-RP LC separations for the analysis of the same mitochondrial sample. When evaluating the protein sequence coverage by the number of distinct peptides mapping to each mitochondrial protein identification, CITP/CZE similarly achieves superior performance with 1041 proteins (58%) having 3 or more distinct peptides, 233 (13%) having 2 distinct peptides, and 521 (29%) having a single distinct peptide. The reproducibility of protein identifications is found to be around 86% by comparing proteins identified from repeated runs of the same mitochondrial sample. The analysis of the mouse mitochondrial proteome by two CITP/CZE runs results in the detection of 2095 distinct mouse Swiss-Prot protein entries (or 1992 nonredundant proteins), corresponding to 59% coverage of the updated Maestro mitochondrial reference set. The collective analysis from combined CITP/CZE and CIEF-based proteomic studies yields the identification of 2191 distinct mitochondrial protein entries (or 2082 nonredundant proteins), corresponding to 76% coverage of the MitoP2-database reference set.
机译:通过使用基于毛细管ITP(CITP)/ CZE的蛋白质组学技术,从小鼠脑中分离出的突触线粒体共鉴定出1795种不同的小鼠Swiss-Prot蛋白条目(或1705种非冗余蛋白)。 CITP / CZE具有超高的分辨能力,这是由从每个CITP馏分测得的大量独特肽鉴定以及鉴定出的肽之间重叠的低肽馏分所证明的。 CITP馏分之间的肽重叠程度甚至比使用CIEF / nano-RP LC组合分离分析同一线粒体样品所获得的重叠程度还要低。当通过映射到每个线粒体蛋白质鉴定的独特肽的数量评估蛋白质序列的覆盖率时,CITP / CZE同样具有104种具有3种或3种以上独特肽的蛋白质(58%),233种具有2种独特肽的蛋白质(13%), 521(29%)具有单个不同的肽。通过比较从同一线粒体样品的重复运行中鉴定出的蛋白质,发现蛋白质鉴定的可重复性约为86%。通过两次CITP / CZE运行对小鼠线粒体蛋白质组进行分析,结果是检测到2095个不同的小鼠Swiss-Prot蛋白条目(或1992年非冗余蛋白),相当于更新的Maestro线粒体参考集的59%覆盖率。来自结合CITP / CZE和基于CIEF的蛋白质组学研究的集体分析得出了2191个不同的线粒体蛋白质条目(或2082个非冗余蛋白质)的标识,对应于MitoP2数据库参考集的76%覆盖率。

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