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在高灵敏度飞行时间质谱仪中,强低能电子束使生物分子离解。

Dissociation of Biomolecules by an Intense Low-Energy Electron Beam in a High Sensitivity Time-of-Flight Mass Spectrometer.

机构信息

Sciex, 71 Four Valley Drive Concord, Ontario L4K 4V8, Canada.

出版信息

J Am Soc Mass Spectrom. 2021 Aug 4;32(8):1964-1975. doi: 10.1021/jasms.0c00425. Epub 2021 Jun 3.

Abstract

We report the progress on an electron-activated dissociation (EAD) device coupled to a quadrupole TOF mass spectrometer (QqTOF MS) developed in our group. This device features a new electron beam optics design allowing up to 100 times stronger electron currents in the reaction cell. The electron beam current reached the space-charge limit of 0.5 μA at near-zero electron kinetic energies. These advances enable fast and efficient dissociation of various analytes ranging from singly charged small molecules to multiply protonated proteins. Tunable electron energy provides access to different fragmentation regimes: ECD, hot ECD, and electron-impact excitation of ions from organics (EIEIO). The efficiency of the device was tested on a wide range of precursor charge states. The EAD device was installed in a QqTOF MS employing a novel trap-and-release strategy facilitating spatial mass focusing of ions at the center of the TOF accelerator. This technique increased the sensitivity 6-10 times and allows for the first time comprehensive structural lipidomics on an LC time scale. The system was evaluated for other compound classes such as intact proteins and glycopeptides. Application of hot ECD for the analysis of glycopeptides resulted in rich fragmentation with predominantly peptide backbone fragments; however, glycan fragments attributed to the ECD process were also observed. A standard small protein ubiquitin (8.6 kDa) was sequenced with 90% cleavage coverage at spectrum accumulation times of 100 ms and 98% at 800 ms. Comparable cleavage coverage for a medium-size protein (carbonic anhydrase: 29 kDa) could be achieved, albeit with longer accumulation times.

摘要

我们报告了我们小组开发的一种与四极杆飞行时间质谱仪(QqTOF MS)耦合的电子激活解离(EAD)装置的进展。该装置具有新的电子束光学设计,可在反应室中实现高达 100 倍的电子电流强度。电子束电流在接近零电子动能时达到 0.5 μA 的空间电荷限制。这些进展使得对各种分析物进行快速高效的解离成为可能,范围从单电荷小分子到多质子化蛋白质。可调谐电子能量可实现不同的碎裂模式:ECD、热 ECD 和电子冲击激发有机物中的离子(EIEIO)。该装置的效率在广泛的前体电荷状态下进行了测试。EAD 装置安装在 QqTOF MS 中,采用了一种新颖的捕获和释放策略,便于在 TOF 加速器的中心对离子进行空间质量聚焦。该技术将灵敏度提高了 6-10 倍,并首次允许在 LC 时间尺度上进行全面的结构脂质组学研究。该系统还针对其他化合物类别进行了评估,例如完整蛋白质和糖肽。热 ECD 用于糖肽分析可产生丰富的碎裂,主要为肽骨架片段;然而,也观察到归因于 ECD 过程的聚糖片段。在谱图累积时间为 100 ms 时,标准小蛋白泛素(8.6 kDa)的测序覆盖率达到 90%,在 800 ms 时达到 98%。虽然累积时间较长,但可以实现中大小蛋白质(碳酸酐酶:29 kDa)的可比切割覆盖率。

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