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毛细管电泳-非接触电导检测法分析糖蛋白中的单糖组成。

Monosaccharide profiling of glycoproteins by capillary electrophoresis with contactless conductivity detection.

机构信息

Faculty of Science, Department of Analytical Chemistry, Charles University, Prague, Czech Republic.

出版信息

Electrophoresis. 2022 Oct;43(20):1963-1970. doi: 10.1002/elps.202200033. Epub 2022 Aug 27.

DOI:10.1002/elps.202200033
PMID:35961667
Abstract

Saccharides form one of the major constituents of biological macromolecules in living organisms. Many biological processes including protein folding, stability, immune response and receptor activation are regulated by glycosylation. In this work, we optimized a capillary electrophoresis method with capacitively coupled contactless conductivity detection for the separation of eight monosaccharides commonly found in glycoproteins, namely D-glucose, D-galactose, D-mannose, N-acetyl-D-glucosamine, N-acetyl-D-galactosamine, D-fucose, N-acetylneuraminic acid, and D-xylose. A highly alkaline solution of 50 mM sodium hydroxide, 22.5 mM disodium phosphate, and 0.2 mM CTAB (pH 12.4) was used as a background electrolyte in a 10 µm id capillary. To achieve baseline separation of all analytes, a counter-directional pressure of -270 kPa was applied during the separation. The limits of detection of our method were below 7 µg/ml (i.e., 1.5 pg or 1 mg/g protein) and the limits of quantification were below 22 µg/ml (i.e., 5 pg or 3 mg/g protein). As a proof of concept of our methodology, we performed an analysis of monosaccharides released from fetuin glycoprotein by acid hydrolysis. The results show that, when combined with an appropriate pre-concentration technique, the developed method can be used as a monosaccharide profiling tool in glycoproteomics and complement the routinely used LC-MS/MS analysis.

摘要

糖是生物体内生物大分子的主要组成部分之一。许多生物过程,包括蛋白质折叠、稳定性、免疫反应和受体激活,都受到糖基化的调节。在这项工作中,我们优化了一种带有电容耦合非接触电导检测的毛细管电泳方法,用于分离八种常见于糖蛋白中的单糖,即 D-葡萄糖、D-半乳糖、D-甘露糖、N-乙酰-D-葡萄糖胺、N-乙酰-D-半乳糖胺、D-岩藻糖、N-乙酰神经氨酸和 D-木糖。在 10 µm id 毛细管中,使用 50 mM 氢氧化钠、22.5 mM 磷酸二氢钠和 0.2 mM CTAB(pH 12.4)的高碱性溶液作为背景电解质。为了实现所有分析物的基线分离,在分离过程中施加了-270 kPa 的反向压力。我们方法的检测限低于 7 µg/ml(即 1.5 pg 或 1 mg/g 蛋白质),定量限低于 22 µg/ml(即 5 pg 或 3 mg/g 蛋白质)。作为我们方法学的概念验证,我们对酸水解胎球蛋白释放的单糖进行了分析。结果表明,当与适当的预浓缩技术结合使用时,该方法可用于糖蛋白质组学中的单糖分析,并补充常规使用的 LC-MS/MS 分析。

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