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High-Field Asymmetric Waveform Ion Mobility Spectrometry and Native Mass Spectrometry: Analysis of Intact Protein Assemblies and Protein Complexes

机译:高场非对称波形离子迁移谱和天然质谱:完整蛋白质组装和蛋白质复合物的分析

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High-field asymmetric waveform ion mobility spectrometry (FAIMS) enables the separation of ions on the basis of their differential mobility in an asymmetric oscillating electric field. We, and others, have previously demonstrated the benefits of FAIMS for the analysis of peptides and denatured proteins. To date, FAIMS has not been integrated with native mass spectrometry of folded proteins and protein complexes, largely due to concerns over the heating effects associated with the high electric fields employed. Here, we demonstrate the newly introduced cylindrical FAIMS Pro device coupled with an Orbitrap Eclipse enables analysis of intact protein assemblies up to 147 kDa. No evidence for dissociation was detected suggesting that any field heating is insufficient to disrupt the noncovalent interactions governing these assemblies. Moreover, the FAIMS device was integrated into native liquid extraction surface analysis (LESA) MS of protein assemblies directly from thin tissue sections. Intact tetrameric hemoglobin (64 kDa) and trimeric reactive intermediate deiminase A (RidA, 43 kDa) were detected. Improvements in signal-to-noise of between 1.5x and 12X were observed for these protein assemblies on integration of FAIMS.
机译:高场非对称波形离子迁移光谱法(Faims)能够基于其在不对称振荡电场中的差动迁移率来分离离子。我们和其他人以前展示了Faims用于分析肽和变性蛋白质的好处。迄今为止,FAIMS尚未与折叠蛋白质和蛋白质复合物的天然质谱相结合,这主要是由于对采用的高电场相关的加热效果的担忧。在这里,我们展示了新推出的圆柱形Faims Pro设备,其与壁图Eclipse相结合,可以分析完整的蛋白质组件,最高可达147kDa。未检测到解离证据表明任何现场加热不足以破坏控制这些组件的非共价相互作用。此外,将指数装置直接从薄的组织部分纳入本地液体提取表面分析(LESA)蛋白质组件MS。检测完整的四聚体血红蛋白(64kDa)和三聚体反应性中间酶A(Rida,43kDa)。对于这些蛋白质组件,观察到噪声的噪音的改善对于这些蛋白质组件进行了融合。

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