化学
离子阱
色谱法
蛋白质组学
质谱法
分馏
肽
串联质谱法
蛋白质组
自下而上蛋白质组学
自上而下的蛋白质组学
鸟枪蛋白质组学
分析化学(期刊)
蛋白质质谱法
生物化学
基因
作者
Xinyan Fu,Jie Hong,Yanbing Zhai,Kefu Liu,Wei Xu
标识
DOI:10.1021/acs.analchem.3c00532
摘要
In bottom-up proteomics, the complexity of the proteome requires advanced peptide separation and/or fractionation methods to acquire an in-depth understanding of protein profiles. Proposed earlier as a solution-phase ion manipulation device, liquid phase ion traps (LPITs) were used in front of mass spectrometers to accumulate target ions for improved detection sensitivity. In this work, an LPIT-reversed phase liquid chromatography-tandem mass spectrometry (LPIT-RPLC-MS/MS) platform was established for deep bottom-up proteomics. LPIT was used here as a robust and effective method for peptide fractionation, which also shows good reproducibility and sensitivity on both qualitative and quantitative levels. LPIT separates peptides based on their effective charges and hydrodynamic radii, which is orthogonal to that of RPLC. With excellent orthogonality, the integration of LPIT with RPLC-MS/MS could effectively increase the number of peptides and proteins being detected. When HeLa cells were analyzed, peptide and protein coverages were increased by ∼89.2% and 50.3%, respectively. With high efficiency and low cost, this LPIT-based peptide fraction method could potentially be used in routine deep bottom-up proteomics.
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