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增强去簇化使基于离子淌度时间对齐的片段化的膜蛋白复合物的从头分析成为可能。

Enhanced Declustering Enables Native Top-Down Analysis of Membrane Protein Complexes using Ion-Mobility Time-Aligned Fragmentation.

机构信息

OMass Therapeutics, Chancellor Court, John Smith Drive, ARC Oxford OX4 2GX, United Kingdom.

Waters Corporation, Stamford Avenue, Altrincham Road, Wilmslow SK9 4AX, United Kingdom.

出版信息

J Am Soc Mass Spectrom. 2024 Aug 7;35(8):1891-1901. doi: 10.1021/jasms.4c00190. Epub 2024 Jul 15.

DOI:10.1021/jasms.4c00190
PMID:39007842
Abstract

Native mass spectrometry (MS) is proving to be a disruptive technique for studying the interactions of proteins, necessary for understanding the functional roles of these biomolecules. Recent research is expanding the application of native MS towards membrane proteins directly from isolated membrane preparations or from purified detergent micelles. The former results in complex spectra comprising several heterogeneous protein complexes; the latter enables therapeutic protein targets to be screened against multiplexed preparations of compound libraries. In both cases, the resulting spectra are increasingly complex to assign/interpret, and the key to these new directions of native MS research is the ability to perform native top-down analysis, which allows unambiguous peak assignment. To achieve this, detergent removal is necessary prior to MS analyzers, which allow selection of specific / values, representing the parent ion for downstream activation. Here, we describe a novel, enhanced declustering (ED) device installed into the first pumping region of a cyclic IMS-enabled mass spectrometry platform. The device enables declustering of ions prior to the quadrupole by imparting collisional activation through an oscillating electric field applied between two parallel plates. The positioning of the device enables liberation of membrane protein ions from detergent micelles. Quadrupole selection can now be utilized to isolate protein-ligand complexes, and downstream collision cells enable the dissociation and identification of binding partners. We demonstrate that ion mobility (IM) significantly aids in the assignment of top-down spectra, aligning fragments to their corresponding parent ions by means of IM drift time. Using this approach, we were able to confidently assign and identify a novel hit compound against MATE, obtained from multiplexed ligand libraries.

摘要

天然质谱(MS)被证明是一种用于研究蛋白质相互作用的颠覆性技术,这对于理解这些生物分子的功能作用至关重要。最近的研究将天然 MS 的应用扩展到了直接从分离的膜制剂或从纯化的去污剂胶束中分离的膜蛋白。前者导致包含几种异质蛋白质复合物的复杂光谱;后者使治疗性蛋白质靶标能够针对化合物库的多路复用制剂进行筛选。在这两种情况下,得到的光谱越来越难以分配/解释,而天然 MS 研究的这些新方向的关键是能够进行天然自上而下的分析,从而能够明确峰分配。为此,在 MS 分析仪之前需要去除去污剂,这允许选择代表下游激活的母离子的特定/ 值。在这里,我们描述了一种安装在循环 IMS 启用的质谱平台的第一抽气区中的新型增强解簇(ED)设备。该设备通过在两个平行板之间施加振荡电场来赋予离子碰撞活性,从而在进入四极之前对离子进行解簇。该设备的定位使膜蛋白离子能够从去污剂胶束中释放出来。现在可以利用四极选择来分离蛋白质-配体复合物,并且下游碰撞池可以使配体解离并鉴定结合伴侣。我们证明离子淌度(IM)通过 IM 漂移时间显著有助于自上而下的光谱分配,将片段与它们对应的母离子对齐。通过这种方法,我们能够自信地分配并鉴定从多路复用配体文库中获得的新型针对 MATE 的命中化合物。

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