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An optimized approach for enrichment of glycoproteins from cell culture lysates using native multi-lectin affinity chromatography

机译:使用天然多凝集素亲和色谱从细胞培养物裂解物中富集糖蛋白的优化方法

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摘要

Lectins are capable of recognizing specific glycan structures and serve as invaluable tools for the separation of glycosylated proteins from nonglycosylated proteins in biological samples. We report on the optimization of native multi-lectin affinity chromatography, combining three lectins, namely, concanavalin A, jacalin, and wheat germ agglutinin for fractionation of cellular glycoproteins from MCF-7 breast cancer lysate. We evaluated several conditions for optimum recovery of total proteins and glycoproteins such as low pH and saccharide elution buffers, and the inclusion of detergents in binding and elution buffers. Optimum recovery was observed with overnight incubation of cell lysate with lectins at 4°C, and inclusion of detergent in binding and saccharide elution buffers. Total protein and bound recoveries were 80 and 9%, respectively. Importantly, we found that high saccharide strength elution buffers were not necessary to release bound glycoproteins. This study demonstrates that multi-lectin affinity chromatography can be extended to total cell lysate to investigate the cellular glycoproteome.
机译:凝集素能够识别特定的聚糖结构,并且是从生物样品中的非糖基化蛋白中分离糖基化蛋白的宝贵工具。我们报告了对天然多凝集素亲和色谱的优化,结合了三种凝集素,即伴刀豆球蛋白A,jacalin和小麦胚芽凝集素,用于从MCF-7乳腺癌裂解物中分离细胞糖蛋白。我们评估了总蛋白和糖蛋白的最佳回收率的几种条件,例如低pH和糖洗脱缓冲液,以及结合和洗脱缓冲液中包含去污剂。通过在4℃下用凝集素孵育细胞裂解液过夜,并在结合和糖洗脱缓冲液中加入去污剂,观察到最佳回收率。总蛋白质和结合回收率分别为80%和9%。重要的是,我们发现高糖强度洗脱缓冲液对于释放结合的糖蛋白不是必需的。这项研究表明,多凝集素亲和层析可以扩展到总细胞裂解物中,以研究细胞糖蛋白组。

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