Evaluation of the Orbitrap Ascend Tribrid Mass Spectrometer for Shotgun Proteomics

轨道轨道 化学 质谱法 鸟枪蛋白质组学 蛋白质组学 自上而下的蛋白质组学 串联质谱法 定量蛋白质组学 背景(考古学) 色谱法 蛋白质质谱法 生物化学 古生物学 生物 基因
作者
Yuchen He,Evgenia Shishkova,Trenton M. Peters-Clarke,Dain R. Brademan,Michael S. Westphall,David Bergen,Jingjing Huang,Romain Huguet,Michael W. Senko,Vlad Zabrouskov,Graeme C. McAlister,Joshua J. Coon
出处
期刊:Analytical Chemistry [American Chemical Society]
卷期号:95 (28): 10655-10663 被引量:35
标识
DOI:10.1021/acs.analchem.3c01155
摘要

Mass spectrometry (MS)-based proteomics is a powerful technology to globally profile protein abundances, activities, interactions, and modifications. The extreme complexity of proteomics samples, which often contain hundreds of thousands of analytes, necessitates continuous development of MS techniques and instrumentation to improve speed, sensitivity, precision, and accuracy, among other analytical characteristics. Here, we systematically evaluated the Orbitrap Ascend Tribrid mass spectrometer in the context of shotgun proteomics, and we compared its performance to that of the previous generation of Tribrid instruments─the Orbitrap Eclipse. The updated architecture of the Orbitrap Ascend includes a second ion-routing multipole (IRM) in front of the redesigned C-trap/Orbitrap and a new ion funnel that allows gentler ion introduction, among other changes. These modifications in Ascend hardware configuration enabled an increase in parallelizable ion injection time during higher-energy collisional dissociation (HCD) Orbitrap tandem MS (FTMS2) analysis of ∼5 ms. This enhancement was particularly valuable in the analyses of limited sample amounts, where improvements in sensitivity resulted in up to 140% increase in the number of identified tryptic peptides. Further, analysis of phosphorylated peptides enriched from the K562 human cell line yielded up to ∼50% increase in the number of unique phosphopeptides and localized phosphosites. Strikingly, we also observed a ∼2-fold boost in the number of detected N-glycopeptides, likely owing to the improvements in ion transmission and sensitivity. In addition, we performed the multiplexed quantitative proteomics analyses of TMT11-plex labeled HEK293T tryptic peptides and observed 9-14% increase in the number of quantified peptides. In conclusion, the Orbitrap Ascend consistently outperformed its predecessor the Orbitrap Eclipse in various bottom-up proteomic analyses, and we anticipate that it will generate reproducible and in-depth datasets for numerous proteomic applications.
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