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Microchip capillary gel electrophoresis combined with lectin affinity enrichment employing magnetic beads for glycoprotein analysis

机译:微芯片毛细管电泳结合凝集素亲和力富集使用磁珠进行糖蛋白分析

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摘要

Due to the constant search for reliable methods to investigate glycoproteins in complex biological samples, an alternative approach combining affinity enrichment with rapid and sensitive analysis on-a-chip is presented. Glycoproteins were specifically captured by lectin-coated magnetic beads, eluted by competitive sugars, and investigated with microchip capillary gel electrophoresis (MCGE), i.e., CGE-on-a-chip. We compared our results to sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) data, which turned out to be in very good agreement. While SDS-PAGE offers the possibility of subsequent mass spectrometric analysis of captured and separated analytes, MCGE scores with time savings, higher throughput, and lower sample consumption as well as quality control (QC) and process analytical technology (PAT) applicability. Due to these advantages, a lectin-based glycoprotein capture protocol can easily be optimized. In our case, two different types of magnetic beads were tested and compared regarding lectin binding. The selectivity of our strategy was demonstrated with a set of model glycoproteins, as well as with human serum and serum depleted from high-abundance proteins. The specificity of the capturing method was investigated revealing to a certain degree an unspecific binding between each sample and the beads themselves, which has to be considered for any specific enrichment and data interpretation. In addition, two glycoproteins from Trichoderma atroviride, a fungus with mycoparasitic activity and only barely studied glycoproteome, were enriched by means of a lectin and so identified for the first time. >Graphical abstractGlycoproteins from biological samples were detected by microchip capillary gel electrophoresis after lectin affinity enrichment using magnetic beads and elution with respective competitive monosaccharides
机译:由于不断寻求可靠的方法来研究复杂生物样品中的糖蛋白,因此提出了一种将亲和力富集与芯片上快速灵敏分析相结合的替代方法。糖蛋白被凝集素包被的磁珠特异性捕获,被竞争性糖洗脱,并通过微芯片毛细管凝胶电泳(MCGE),即CGE-on-a-chip研究。我们将结果与十二烷基硫酸钠-聚丙烯酰胺凝胶电泳(SDS-PAGE)数据进行了比较,结果非常吻合。尽管SDS-PAGE提供了随后对捕获和分离的分析物进行质谱分析的可能性,但MCGE评分可节省时间,提高通量并降低样品消耗,并具有质量控制(QC)和过程分析技术(PAT)的适用性。由于这些优点,可以轻松优化基于凝集素的糖蛋白捕获方案。在我们的案例中,测试了两种不同类型的磁珠并比较了凝集素的结合。我们的策略的选择性通过一组模型糖蛋白以及人血清和从高丰度蛋白质中耗尽的血清得到证明。研究了捕获方法的特异性,在一定程度上揭示了每个样品与珠子本身之间的非特异性结合,对于任何特异性的富集和数据解释都必须考虑到这种结合。此外,通过凝集素富集了来自木霉阿特罗韦德的两种糖蛋白,这是一种具有霉菌寄生活性的真菌,只有很少研究的糖蛋白组学,因此首次被鉴定出来。 <!-fig ft0-> <!-fig @ position =“ anchor” mode =文章f4-> <!-fig mode =“ anchred” f5-> >图形摘要<!-无花果/图形|无花果/替代品/图形模式=“锚定” m1-> <!-标题a7->使用磁珠富集凝集素并通过各自的竞争性洗脱后,通过微芯片毛细管凝胶电泳检测生物样品中的糖蛋白单糖

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