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本文引用的文献

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Ion trapping for ion mobility spectrometry measurements in a cyclical drift tube.在循环漂移管中进行离子淌度谱测量的离子捕集。
Anal Chem. 2013 Aug 6;85(15):7003-8. doi: 10.1021/ac4015066. Epub 2013 Jul 15.
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A database of alkaline-earth-coordinated peptide cross sections: insight into general aspects of structure.碱土金属配位肽截面数据库:对结构的一般方面的洞察。
J Am Soc Mass Spectrom. 2013 May;24(5):768-79. doi: 10.1007/s13361-013-0579-z. Epub 2013 Mar 20.
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Improving qualitative and quantitative performance for MS(E)-based label-free proteomics.提高基于 MS(E)的无标记蛋白质组学的定性和定量性能。
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High-definition differential ion mobility spectrometry with resolving power up to 500.高分辨差分离子淌度谱技术,分辨率高达 500。
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Ion mobility mass spectrometry of peptide ions: effects of drift gas and calibration strategies.肽离子的离子淌度质谱分析:漂移气体和校准策略的影响。
Anal Chem. 2012 Aug 21;84(16):7124-30. doi: 10.1021/ac3014498. Epub 2012 Aug 10.
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Ion mobility-mass spectrometry for structural proteomics.离子淌度-质谱用于结构蛋白质组学。
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How hot are your ions in TWAVE ion mobility spectrometry?TWAVE 离子淌度谱仪中离子有多热?
J Am Soc Mass Spectrom. 2012 Mar;23(3):553-62. doi: 10.1007/s13361-011-0313-7. Epub 2011 Dec 28.
8
Structural stability from solution to the gas phase: native solution structure of ubiquitin survives analysis in a solvent-free ion mobility-mass spectrometry environment.从溶液到气相的结构稳定性:在无溶剂离子淌度-质谱环境中分析天然溶液状态下的泛素结构仍能保持稳定。
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Mass spectrometry: come of age for structural and dynamical biology.质谱法:结构和动态生物学的时代已经到来。
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10
Number of solution states of bradykinin from ion mobility and mass spectrometry measurements.缓激肽的溶液态数目来自离子淌度和质谱测量。
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行波离子迁移谱质谱仪上的大规模碰撞截面分析

Large-scale collision cross-section profiling on a traveling wave ion mobility mass spectrometer.

作者信息

Lietz Christopher B, Yu Qing, Li Lingjun

机构信息

Department of Chemistry, University of Wisconsin, Madison, WI, 53705, USA.

出版信息

J Am Soc Mass Spectrom. 2014 Dec;25(12):2009-19. doi: 10.1007/s13361-014-0920-1. Epub 2014 May 21.

DOI:10.1007/s13361-014-0920-1
PMID:24845359
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC4224635/
Abstract

Ion mobility (IM) is a gas-phase electrophoretic method that separates ions according to charge and ion-neutral collision cross-section (CCS). Herein, we attempt to apply a traveling wave (TW) IM polyalanine calibration method to shotgun proteomics and create a large peptide CCS database. Mass spectrometry methods that utilize IM, such as HDMS(E), often use high transmission voltages for sensitive analysis. However, polyalanine calibration has only been demonstrated with low voltage transmission used to prevent gas-phase activation. If polyalanine ions change conformation under higher transmission voltages used for HDMS(E), the calibration may no longer be valid. Thus, we aimed to characterize the accuracy of calibration and CCS measurement under high transmission voltages on a TW IM instrument using the polyalanine calibration method and found that the additional error was not significant. We also evaluated the potential error introduced by liquid chromatography (LC)-HDMS(E) analysis, and found it to be insignificant as well, validating the calibration method. Finally, we demonstrated the utility of building a large-population peptide CCS database by investigating the effects of terminal lysine position, via LysC or LysN digestion, on the formation of two structural sub-families formed by triply charged ions.

摘要

离子淌度(IM)是一种气相电泳方法,可根据电荷和离子-中性碰撞截面(CCS)分离离子。在此,我们尝试将行波(TW)IM聚丙氨酸校准方法应用于鸟枪法蛋白质组学,并创建一个大型肽CCS数据库。利用IM的质谱方法,如HDMS(E),通常使用高传输电压进行灵敏分析。然而,聚丙氨酸校准仅在用于防止气相活化的低电压传输情况下得到证明。如果聚丙氨酸离子在用于HDMS(E)的较高传输电压下改变构象,校准可能不再有效。因此,我们旨在使用聚丙氨酸校准方法在TW IM仪器上表征高传输电压下校准和CCS测量的准确性,发现额外误差不显著。我们还评估了液相色谱(LC)-HDMS(E)分析引入的潜在误差,发现其也不显著,从而验证了校准方法。最后,我们通过研究经LysC或LysN消化后末端赖氨酸位置对由三价离子形成的两个结构亚家族形成的影响,证明了构建大型肽CCS数据库的实用性。