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Separation of β-Amyloid Tryptic Peptide Species with Isomerized and Racemized L-Aspartic Residues with Ion Mobility in Structures for Lossless Ion Manipulations

机译:无损离子处理结构中具有离子迁移性的异构化和消旋化L-天冬氨酸残基的β-淀粉样蛋白胰蛋白酶肽种类的分离

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摘要

Accumulation of β-amyloid (Aβ) is one of the hallmarks of Alzheimer’s disease. The deposition of β-amyloid plaques is likely to start years in advance of manifestation of clinical symptoms, although the exact timing is unknown. Over the years, Aβ peptides undergo both post-translational modification and stereoisomerization. Analysis of the resulting stereoisomers is particularly challenging because of their identical elemental composition and similar physicochemical properties. Herein, we have utilized our recently developed structures for lossless ion manipulations ion mobility-mass spectrometry platform (SLIM IM-MS), in conjunction with serpentine ultralong path with extended routing (SUPER), to baseline resolve four distinct sets of Aβ17–28 tryptic peptide epimers on a rapid (~1 s) time scale. We discovered that sodium adduct ions, [M + H + Na]2+, allowed baseline SLIM SUPER IM resolution for all Aβ epimer sets assessed, while such baseline separations were unachievable for their [M + 2H]2+ doubly protonated ions.
机译:β-淀粉样蛋白(Aβ)的积累是阿尔茨海默氏病的标志之一。尽管尚不清楚确切的时机,但β-淀粉样蛋白斑块的沉积可能在临床症状出现之前的数年开始。多年来,Aβ肽同时经历翻译后修饰和立体异构化。由于其立体组成相同,理化性质相似,因此对所得立体异构体的分析尤其具有挑战性。在这里,我们将我们最新开发的结构用于无损离子处理离子迁移质谱仪(SLIM IM-MS),结合蛇形超长路径和扩展路径(SUPER),以基线解析四组不同的Aβ17-28胰蛋白酶(〜1 s)时间尺度上的肽差向异构体。我们发现,[M + H + Na] 2 + 钠加合物离子可对所有评估的Aβ差向异构体进行基线SLIM SUPER IM拆分,而对于它们的[M + 2H]无法实现基线分离 2 + 双质子化离子。

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