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天然大分子组装体的被困离子淌度谱技术。

Trapped Ion Mobility Spectrometry of Native Macromolecular Assemblies.

机构信息

Department of Chemistry and Biochemistry, Florida International University, Miami, Florida 33199, United States.

Biomolecular Sciences Institute, Florida International University, Miami, Florida 33199, United States.

出版信息

Anal Chem. 2021 Feb 9;93(5):2933-2941. doi: 10.1021/acs.analchem.0c04556. Epub 2021 Jan 25.

Abstract

The structural elucidation of native macromolecular assemblies has been a subject of considerable interest in native mass spectrometry (MS), and more recently in tandem with ion mobility spectrometry (IMS-MS), for a better understanding of their biochemical and biophysical functions. In the present work, we describe a new generation trapped ion mobility spectrometer (TIMS), with extended mobility range ( = 0.185-1.84 cm·V·s), capable of trapping high-molecular-weight (MW) macromolecular assemblies. This compact 4 cm long TIMS analyzer utilizes a convex electrode, quadrupolar geometry with increased pseudopotential penetration in the radial dimension, extending the mobility trapping to high-MW species under native state (i.e., lower charge states). The TIMS capabilities to perform variable scan rate () mobility measurements over short time (100-500 ms), high-mobility resolution, and ion-neutral collision cross-section (CCS) measurements are presented. The trapping capabilities of the convex electrode TIMS geometry and ease of operation over a wide gas flow, rf range, and electric field trapping range are illustrated for the first time using a comprehensive list of standards varying from CsI clusters ( = 6-73), Tuning Mix oligomers ( = 1-5), common proteins (e.g., ubiquitin, cytochrome C, lysozyme, concanavalin ( = 1-4), carbonic anhydrase, β clamp ( = 1-4), topoisomerase IB, bovine serum albumin ( = 1-3), topoisomerase IA, alcohol dehydrogenase), IgG antibody (e.g., avastin), protein-DNA complexes, and macromolecular assemblies (e.g., GroEL and RNA polymerase ( = 1-2)) covering a wide mass (up to / 19 000) and CCS range (up to 22 000 Å with <0.6% relative standard deviation (RSD)).

摘要

天然大分子组装体的结构阐明一直是天然质谱(MS)领域的研究热点,最近结合离子淌度谱(IMS-MS)技术,以更好地了解其生化和生物物理功能。在本工作中,我们描述了一种新型的离子阱淌度谱仪(TIMS),具有扩展的淌度范围( = 0.185-1.84 cm·V·s),能够捕获高分子量(MW)的大分子组装体。这个紧凑的 4 cm 长 TIMS 分析器采用凸面电极,四极几何形状,在径向维度上增加了伪势穿透,在天然状态下(即低电荷态)扩展了对高分子量物种的淌度捕获。TIMS 具有在短时间(100-500 ms)内进行可变扫描速率()淌度测量、高淌度分辨率和离子-中性碰撞截面(CCS)测量的能力。首次展示了凸面电极 TIMS 几何形状的捕获能力和在宽气流、射频范围和电场捕获范围下的操作简便性,使用了一系列标准品,范围从 CsI 团簇( = 6-73)、调谐混合物低聚物( = 1-5)、常见蛋白质(如泛素、细胞色素 C、溶菌酶、伴刀豆球蛋白( = 1-4)、碳酸酐酶、β 夹( = 1-4)、拓扑异构酶 IB、牛血清白蛋白( = 1-3)、拓扑异构酶 IA、醇脱氢酶)、IgG 抗体(如阿瓦斯汀)、蛋白-DNA 复合物和大分子组装体(如 GroEL 和 RNA 聚合酶( = 1-2)),涵盖了广泛的质量(高达 / 19 000)和 CCS 范围(高达 22 000 Å,相对标准偏差(RSD)<0.6%)。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/cb0e/8327357/804373a9c59f/nihms-1725917-f0002.jpg

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