Biomolecular Mass Spectrometry and Proteomics, Bijvoet Center for Biomolecular Research and Utrecht Institute for Pharmaceutical Sciences, Utrecht University, Padualaan 8, 3584 CH, Utrecht, The Netherlands.
Netherlands Proteomics Centre, Padualaan 8, 3584 CH, Utrecht, The Netherlands.
Nat Commun. 2020 Jun 26;11(1):3244. doi: 10.1038/s41467-020-17010-0.
Bioorthogonal chemistry introduces affinity-labels into biomolecules with minimal disruption to the original system and is widely applicable in a range of contexts. In proteomics, immobilized metal affinity chromatography (IMAC) enables enrichment of phosphopeptides with extreme sensitivity and selectivity. Here, we adapt and combine these superb assets in a new enrichment strategy using phosphonate-handles, which we term PhosID. In this approach, click-able phosphonate-handles are introduced into proteins via 1,3-dipolar Huisgen-cycloaddition to azido-homo-alanine (AHA) and IMAC is then used to enrich exclusively for phosphonate-labeled peptides. In interferon-gamma (IFNγ) stimulated cells, PhosID enabled the identification of a large number of IFN responsive newly synthesized proteins (NSPs) whereby we monitored the differential synthesis of these proteins over time. Collectively, these data validate the excellent performance of PhosID with efficient analysis and quantification of hundreds of NSPs by single LC-MS/MS runs. We envision PhosID as an attractive and alternative tool for studying stimuli-sensitive proteome subsets.
生物正交化学通过最小化对原始系统的干扰,将亲和标签引入生物分子中,并且在多种情况下广泛适用。在蛋白质组学中,固定化金属亲和层析(IMAC)能够以极高的灵敏度和选择性富集磷酸肽。在这里,我们通过点击化学,将可点击的膦酸酯手柄通过 1,3-偶极环加成反应引入到带有叠氮基同型丙氨酸(AHA)的蛋白质中,然后使用 IMAC 仅富集膦酸酯标记的肽。在干扰素-γ(IFNγ)刺激的细胞中,PhosID 能够鉴定出大量的 IFN 响应新合成的蛋白质(NSPs),我们可以通过监测这些蛋白质随时间的差异合成来监测它们。总的来说,这些数据验证了 PhosID 的出色性能,通过单次 LC-MS/MS 运行即可有效地分析和定量数百个 NSPs。我们设想 PhosID 是一种有吸引力的替代工具,可用于研究刺激敏感的蛋白质组亚群。
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