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Comparison of Different HILIC Stationary Phases in the Separation of Hemopexin and Immunoglobulin G Glycopeptides and Their Isomers

机译:不同HILIC固定阶段在血红蛋白和免疫球蛋白G糖肽及其异构体分离中的不同性静止阶段

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摘要

Protein glycosylation analysis is challenging due to the structural variety of complex conjugates. However, chromatographically separating glycans attached to tryptic peptides enables their site-specific characterization. For this purpose, we have shown the importance of selecting a suitable hydrophilic interaction liquid chromatography (HILIC) stationary phase in the separation of glycopeptides and their isomers. Three different HILIC stationary phases, i.e., HALO® penta-HILIC, Glycan ethylene bridged hybrid (BEH) Amide, and ZIC-HILIC, were compared in the separation of complex N-glycopeptides of hemopexin and Immunoglobulin G glycoproteins. The retention time increased with the polarity of the glycans attached to the same peptide backbone in all HILIC columns tested in this study, except for the ZIC-HILIC column when adding sialic acid to the glycan moiety, which caused electrostatic repulsion with the negatively charged sulfobetaine functional group, thereby decreasing retention. The HALO® penta-HILIC column provided the best separation results, and the ZIC-HILIC column the worst. Moreover, we showed the potential of these HILIC columns for the isomeric separation of fucosylated and sialylated glycoforms. Therefore, HILIC is a useful tool for the comprehensive characterization of glycoproteins and their isomers.
机译:由于结构多种复合缀合物,蛋白质糖基化分析是挑战性的。然而,附着于胰蛋白酶肽的色谱分离的聚糖使其能够特异性表征。为此目的,我们已经表明在分离糖肽及其异构体中选择合适的亲水性相互作用液相色谱(HILIC)固定相的重要性。在分离血红素和免疫球蛋白G糖蛋白G糖蛋白的复合N-糖苷肽的分离中,将三种不同的HILIC固定阶段,即Halo®Penta-hilic,甘油乙烯桥接杂交(BEN)酰胺和ZIC-HILIC进行比较。保留时间随着在本研究中测试的所有HILIC柱中连接到相同肽骨架的聚糖的极性而增加,除了将唾液酸添加到甘油部分时,除了ZIC-HILIC柱外,这导致带负电荷的磺基因的静电排斥功能组,从而降低保留。 Halo®Penta-HILIC柱提供了最佳的分离结果,ZIC-HILIC柱最坏。此外,我们展示了这些HILIC柱的潜力,用于岩藻糖基化和唾液酸糖化糖醇的异构分离。因此,HILIC是一种有用的工具,用于综合糖蛋白及其异构体的综合表征。

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