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使用均匀场漂移管离子淌度质谱分析天然蛋白质结构的条件及 TWIM-MS 的稳定校准标准品的特性。

Conditions for Analysis of Native Protein Structures Using Uniform Field Drift Tube Ion Mobility Mass Spectrometry and Characterization of Stable Calibrants for TWIM-MS.

机构信息

School of Chemistry, University of Wollongong, Wollongong, NSW, 2522, Australia.

Molecular Horizons, University of Wollongong, Wollongong, NSW, 2522, Australia.

出版信息

J Am Soc Mass Spectrom. 2019 Feb;30(2):256-267. doi: 10.1007/s13361-018-2074-z. Epub 2018 Oct 15.

DOI:10.1007/s13361-018-2074-z
PMID:30324262
Abstract

Determination of collisional cross sections (CCS) by travelling wave ion mobility mass spectrometry (TWIM-MS) requires calibration against standards for which the CCS has been measured previously by drift tube ion mobility mass spectrometry (DTIM-MS). The different extents of collisional activation in TWIM-MS and DTIM-MS can give rise to discrepancies in the CCS of calibrants across the two platforms. Furthermore, the conditions required to ionize and transmit large, folded proteins and assemblies may variably affect the structure of the calibrants and analytes. Stable hetero-oligomeric phospholipase A (PDx) and its subunits were characterized as calibrants for TWIM-MS. Conditions for acquisition of native-like TWIM (Synapt G1 HDMS) and DTIM (Agilent 6560 IM-Q-TOF) mass spectra were optimized to ensure the spectra exhibited similar charge state distributions. CCS measurements (DTIM-MS) for ubiquitin, cytochrome c, holo-myoglobin, serum albumin and glutamate dehydrogenase were in good agreement with other recent results determined using this and other DTIM-MS instruments. PDx and its β and γ subunits were stable across a wide range of cone and trap voltages in TWIM-MS and were stable in the presence of organic solvents. The CCS of PDx and its subunits were determined by DTIM-MS and were used as calibrants in determination of CCS of native-like cytochrome c, holo-myoglobin, carbonic anhydrase, serum albumin and haemoglobin in TWIM-MS. The CCS values were in good agreement with those measured by DTIM-MS where available. These experiments demonstrate conditions for analysis of native-like proteins using a commercially available DTIM-MS instrument, characterize robust calibrants for TWIM-MS, and present CCS values determined by DTIM-MS and TWIM-MS for native proteins to add to the current literature database. Graphical Abstract ᅟ.

摘要

用行波离子迁移质谱(TWIM-MS)测定碰撞截面(CCS)需要用先前已用漂移管离子迁移质谱(DTIM-MS)测定 CCS 的标准品进行校准。TWIM-MS 和 DTIM-MS 中碰撞激活的程度不同,可能会导致两种平台上校准品的 CCS 存在差异。此外,使大的折叠蛋白质和组装体电离和传输所需的条件可能会不同程度地影响校准品和分析物的结构。稳定的异源寡聚磷脂酶 A(PDx)及其亚基被表征为 TWIM-MS 的校准品。优化了获得类似天然 TWIM(Synapt G1 HDMS)和 DTIM(Agilent 6560 IM-Q-TOF)质谱的条件,以确保谱图显示出相似的电荷状态分布。用 DTIM-MS 测定的泛素、细胞色素 c、血红蛋白全酶、血清白蛋白和谷氨酸脱氢酶的 CCS 值与使用该 DTIM-MS 和其他 DTIM-MS 仪器测定的其他近期结果非常吻合。PDx 及其β和γ亚基在 TWIM-MS 中在广泛的锥和阱电压范围内稳定,并且在存在有机溶剂时稳定。用 DTIM-MS 测定 PDx 及其亚基的 CCS,并将其用作在 TWIM-MS 中测定类似天然的细胞色素 c、血红蛋白全酶、碳酸酐酶、血清白蛋白和血红蛋白的 CCS 的校准品。CCS 值与 DTIM-MS 测定的那些值吻合良好。这些实验证明了使用市售 DTIM-MS 仪器分析类似天然蛋白质的条件,表征了 TWIM-MS 的稳健校准品,并提供了 DTIM-MS 和 TWIM-MS 测定的类似天然蛋白质的 CCS 值,以补充当前的文献数据库。

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