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使用亲水相互作用液相色谱-质谱联用技术分析生物样品中普鲁卡因酰胺衍生化的硫酸乙酰肝素二糖。

Analysis of procainamide-derivatised heparan sulphate disaccharides in biological samples using hydrophilic interaction liquid chromatography mass spectrometry.

作者信息

Antia Imeobong U, Mathew Kurian, Yagnik Darshna R, Hills Frank A, Shah Ajit J

机构信息

Glycan Research Group, Department of Natural Sciences, Faculty of Science and Technology, Middlesex University, London, UK.

出版信息

Anal Bioanal Chem. 2018 Jan;410(1):131-143. doi: 10.1007/s00216-017-0703-1. Epub 2017 Nov 2.

DOI:10.1007/s00216-017-0703-1
PMID:29098336
Abstract

Glycosaminoglycans (GAGs) are a family of linear heteropolysaccharides made up of repeating disaccharide units that are found on the surface and extracellular matrix of animal cells. They are known to play a critical role in a wide range of cellular processes including proliferation, differentiation and invasion. To elucidate the mechanism of action of these molecules, it is essential to quantify their disaccharide composition. Analytical methods that have been reported involve either chemical or enzymatic depolymerisation of GAGs followed by separation of non-derivatised (native) or derivatised disaccharide subunits and detection by either UV/fluorescence or MS. However, the measurement of these disaccharides is challenging due to their hydrophilic and labile nature. Here we report a pre-column LC-MS method for the quantification of GAG disaccharide subunits. Heparan sulphate (HS) was extracted from cell lines using a combination of molecular weight cutoff and anion exchange spin filters and digested using a mixture of heparinases I, II and III. The resulting subunits were derivatised with procainamide, separated using hydrophilic interaction liquid chromatography and detected using electrospray ionisation operated in positive ion mode. Eight HS disaccharides were separated and detected together with an internal standard. The limit of detection was found to be in the range 0.6-4.9 ng/mL. Analysis of HS extracted from all cell lines tested in this study revealed a significant variation in their composition with the most abundant disaccharide being the non-sulphated ∆UA-GlcNAc. Some structural functional relationships are discussed demonstrating the viability of the pre-column method for studying GAG biology. Graphical abstract Extraction and HILIC UPLC-MS analysis of procainamide-labelled heparan sulphate disaccharides.

摘要

糖胺聚糖(GAGs)是一类线性杂多糖,由重复的二糖单元组成,存在于动物细胞表面和细胞外基质中。已知它们在包括增殖、分化和侵袭在内的广泛细胞过程中发挥关键作用。为了阐明这些分子的作用机制,对其二糖组成进行定量至关重要。已报道的分析方法包括对GAGs进行化学或酶解聚,然后分离未衍生化(天然)或衍生化的二糖亚基,并通过紫外/荧光或质谱进行检测。然而,由于这些二糖具有亲水性和易降解性,对其进行测量具有挑战性。在此,我们报告一种用于定量GAG二糖亚基的柱前液相色谱-质谱方法。使用截留分子量和阴离子交换旋转过滤器从细胞系中提取硫酸乙酰肝素(HS),并用肝素酶I、II和III的混合物进行消化。所得亚基用普鲁卡因酰胺衍生化,通过亲水相互作用液相色谱分离,并使用正离子模式下的电喷雾电离进行检测。八种HS二糖与内标一起被分离和检测。检测限在0.6 - 4.9 ng/mL范围内。对本研究中测试的所有细胞系提取的HS进行分析,结果显示其组成存在显著差异,最丰富的二糖是未硫酸化的ΔUA-GlcNAc。讨论了一些结构功能关系,证明了柱前方法在研究GAG生物学方面的可行性。图形摘要 普鲁卡因酰胺标记的硫酸乙酰肝素二糖的提取和亲水相互作用超高效液相色谱-质谱分析

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