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采用离子阱-飞行时间质谱仪的碰撞池中 193nm 紫外光光解对肽和蛋白质进行构象特征分析。

Conformational Characterization of Peptides and Proteins by 193 nm Ultraviolet Photodissociation in the Collision Cell of a Trapped Ion Mobility Spectrometry-Time-of-Flight Mass Spectrometer.

机构信息

Department of Chemistry, The University of Texas at Austin, Austin, Texas 78712, United States.

Bruker Daltonics GmbH & Co. KG, Bremen 28359, Germany.

出版信息

Anal Chem. 2024 Oct 15;96(41):16154-16161. doi: 10.1021/acs.analchem.4c02686. Epub 2024 Oct 4.

Abstract

Ultraviolet photodissociation (UVPD) has been shown to be a versatile ion activation strategy for the characterization of peptides and intact proteins among other classes of biological molecules. Combining the high-performance mass spectrometry (MS/MS) capabilities of UVPD with the high-resolution separation of trapped ion mobility spectrometry (TIMS) presents an opportunity for enhanced structural elucidation of biological molecules. In the present work, we integrate a 193 nm excimer laser in a TIMS-time-of-flight (TIMS-TOF) mass spectrometer for UVPD in the collision cell and use it for the analysis of several mass-mobility-selected species of ubiquitin and myoglobin. The resultant data displayed differences in fragmentation that could be correlated with changes in protein conformation. Additionally, this mobility-resolved UVPD strategy was applied to collision-induced unfolded ions of ubiquitin to follow changes in fragmentation patterns relating to the extent of protein unfolding. This platform and methodology offer new opportunities for exploring how conformational variations are manifested in the fragmentation patterns of gas-phase ions.

摘要

紫外光解(UVPD)已被证明是一种通用的离子活化策略,可用于鉴定肽和完整蛋白质等其他类生物分子。将紫外光解的高性能质谱(MS/MS)能力与被困离子淌度谱(TIMS)的高分辨率分离相结合,为生物分子的结构阐明提供了机会。在本工作中,我们在 TIMS-飞行时间(TIMS-TOF)质谱仪中集成了 193nm 准分子激光器,用于在碰撞池中进行紫外光解,并将其用于分析几种质量-淌度选择的泛素和肌红蛋白物种。所得数据显示出碎片的差异,这些差异可以与蛋白质构象的变化相关联。此外,这种具有流动性分辨能力的紫外光解策略还应用于泛素的碰撞诱导展开离子,以跟踪与蛋白质展开程度相关的碎片模式变化。该平台和方法为探索构象变化如何在气相离子的碎片模式中表现出来提供了新的机会。

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