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首页> 外文期刊>Journal of chromatography, A: Including electrophoresis and other separation methods >Application of a strong anion exchange material in electrostatic repulsion-hydrophilic interaction chromatography for selective enrichment of glycopeptides
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Application of a strong anion exchange material in electrostatic repulsion-hydrophilic interaction chromatography for selective enrichment of glycopeptides

机译:强阴离子交换材料在静电排斥-亲水相互作用色谱中选择性富集糖肽的应用

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摘要

Glycoproteins are involved in various cellular activities, including inter- and extracellular signaling. However, glycopeptide signals are significantly suppressed by coeluting non-glycosylated peptides in mass spectrometry-based analysis. For detailed elucidation of the biological functions of glycoproteins, selective enrichment of glycopeptides from non-glycosylated peptides is crucial. In the present study, a SAX material, XCharge SAX, was used in a column in the ERLIC mode with the aim of specifically enriching glycopeptides. Enrichment conditions were initially optimized, and selectivity, glycosylation heterogeneity coverage and detection sensitivity of XCharge SAX were subsequently assessed. In the selectivity assessment, glycopeptides were effectively isolated from a peptide mixture (human serum immunoglobulin G (IgG) and human serum albumin digests) and a tryptic digest of human serum using XCharge SAX. In the evaluation of glycosylation heterogeneity coverage, five glycosites and eleven glycopeptides from horseradish peroxidase were identified after enrichment with XCharge SAX. In detection sensitivity assessment, glycopeptides within four orders of magnitude were identified after enrichment with XCharge SAX. In addition, volatile solvents were used in the loading and eluting buffers so that desalting was not necessary for ERLIC fractions. Our results collectively support the utility of XCharge SAX as a suitable chromatographic material for global glycosylation site analysis.
机译:糖蛋白参与各种细胞活动,包括细胞间和细胞外信号传导。但是,在基于质谱的分析中,共洗脱非糖基化的肽会显着抑制糖肽信号。为了详细阐明糖蛋白的生物学功能,从非糖基化肽中选择性富集糖肽至关重要。在本研究中,以ERLIC模式在色谱柱中使用了SAX材料XCharge SAX,目的是专门富集糖肽。最初优化了富集条件,随后评估了XCharge SAX的选择性,糖基化异质性覆盖范围和检测灵敏度。在选择性评估中,使用XCharge SAX从肽混合物(人血清免疫球蛋白G(IgG)和人血清白蛋白消化物)和人血清的胰蛋白酶消化物中有效分离了糖肽。在评估糖基化异质性覆盖率时,在用XCharge SAX富集后,从辣根过氧化物酶中鉴定出5个糖位和11个糖肽。在检测灵敏度评估中,用XCharge SAX富集后,鉴定出四个数量级内的糖肽。此外,在上样和洗脱缓冲液中使用了挥发性溶剂,因此对于ERLIC馏分而言,脱盐不是必需的。我们的研究结果共同支持XCharge SAX作为适用于全局糖基化位点分析的色谱材料的效用。

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