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Sialic Acid-focused Quantitative Mouse Serum Glycoproteomics by Multiple Reaction Monitoring Assay

机译:唾液酸聚焦的小鼠血清糖皮质激素的多重反应监测分析

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摘要

Despite increasing importance of protein glycosylation, most of the large-scale glycoproteomics have been limited to profiling the sites of N-glycosylation. However, in-depth knowledge of protein glycosylation to uncover functions and their clinical applications requires quantitative glycoproteomics eliciting both peptide and glycan sequences concurrently. Here we describe a novel strategy for the multiplexed quantitative mouse serum glycoproteomics based on a specific chemical ligation, namely, reverse glycoblotting technique, focusing sialic acids and multiple reaction monitoring (MRM). LC-MS/MS analysis of de-glycosylated peptides identified 270 mouse serum peptides (95 glycoproteins) as sialylated glycopeptides, of which 67 glycopeptides were fully characterized by MS/MS analyses in a straightforward manner. We revealed the importance of a fragment ion containing innermost N-acetylglucosamine (GlcNAc) residue as MRM transitions regardless the sequence of the peptides. Versatility of the reverse glycoblotting-assisted MRM assays was demonstrated by quantitative comparison of 25 targeted glycopeptides from 16 proteins between mice with homo and hetero types of diabetes disease model.
机译:尽管蛋白质糖基化的重要性日益增加,但大多数大规模糖蛋白组学仅限于对N-糖基化位点进行分析。然而,深入了解蛋白质糖基化以揭示功能及其临床应用需要定量糖蛋白组学同时引发肽和聚糖序列。在这里,我们描述了一种基于特定化学连接的多重定量小鼠血清糖蛋白组学的新策略,即反向糖印迹技术,唾液酸聚焦和多反应监测(MRM)。糖基化肽段的LC-MS / MS分析确定了270种小鼠血清肽(95种糖蛋白)为唾液酸化糖肽,其中67种糖肽已通过MS / MS分析以直接方式完全表征。我们揭示了包含最里面的N-乙酰氨基葡萄糖(GlcNAc)残基的碎片离子作为MRM过渡的重要性,而与肽的序列无关。通过对具有同种和异种类型的糖尿病疾病模型的小鼠之间的来自16种蛋白质的25种靶向糖肽进行定量比较,证明了反向糖印迹辅助MRM分析的多功能性。

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