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聚糖组学策略在二糖、寡糖和多糖唾液酸的有效连锁分析中的应用。

Glycomic strategy for efficient linkage analysis of di-, oligo- and polysialic acids.

机构信息

Institute of Biochemistry, Faculty of Medicine, University of Giessen, Friedrichstrasse 24, D-35392 Giessen, Germany.

出版信息

J Proteomics. 2012 Sep 18;75(17):5266-78. doi: 10.1016/j.jprot.2012.06.011. Epub 2012 Jun 20.

Abstract

Sialic acid polymers of glycoproteins and glycolipids are characterized by a high diversity in nature and are involved in distinct biological processes depending inter alia on the glycosidic linkages between the present sialic acid residues. Though suitable protocols are available for chain length and sialic acid determination, sensitive methods for linkage analysis of di-, oligo-, and polysialic acids (di/oligo/polySia) are still pending. In this study, we have established a highly sensitive glycomic strategy for this purpose which is based on permethylation of di/oligo/polySia after tagging their reducing ends with the fluorescent dye 1,2-diamino-4,5-methylenedioxybenzene (DMB). Using DMB-labeled sialic acid di/oligo/polymers glycosidic linkages could be efficiently determined and, optionally, the established working procedure can be combined with HPLC for in depth characterization of distinct di/oligo/polySia chains. Moreover, the outlined approach can be directly applied to mammalian tissue samples and linkage analysis of sialic acid polymers present in biopsy samples of neuroblastoma tissue demonstrating the usefulness of the outlined work flow to screen, for example, cancer tissue for the presence of distinct variants of di/oligo/polySia as potentially novel biomarkers. Hence, the described strategy offers a highly sensitive and efficient strategy for identification of glycosidic linkages in sialic acid di/oligo/polymers of glycoproteins and glycolipids.

摘要

糖蛋白和糖脂中的唾液酸聚合物具有高度多样化的性质,并且根据存在的唾液酸残基之间的糖苷键等,参与不同的生物学过程。尽管有适用于链长和唾液酸测定的合适方案,但双、寡、和多唾液酸(二/寡/多 Sia)的键合分析的敏感方法仍在等待中。在这项研究中,我们为此建立了一种高度敏感的糖组学策略,该策略基于用荧光染料 1,2-二氨基-4,5-亚甲基二氧基苯(DMB)标记其还原末端后对二/寡/多 Sia 进行甲基化。使用 DMB 标记的唾液酸二/寡/多聚合物可以有效地确定糖苷键合,并且可以根据需要将建立的工作程序与 HPLC 结合使用,以深入表征不同的二/寡/多 Sia 链。此外,所提出的方法可以直接应用于哺乳动物组织样品,并对神经母细胞瘤组织活检样品中存在的唾液酸聚合物进行键合分析,证明了所提出的工作流程在筛选例如癌症组织中存在不同变体的二/寡/多 Sia 作为潜在的新型生物标志物的有用性。因此,所描述的策略为鉴定糖蛋白和糖脂中的唾液酸二/寡/多聚合物中的糖苷键提供了一种高度敏感和有效的策略。

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