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Profiling of core fucosylated N-glycans using a novel bacterial lectin that specifically recognizes α16 fucosylated chitobiose

机译:使用特异性识别α16岩藻糖基化壳二糖的新型细菌凝集素对核心岩藻糖基化N-聚糖进行分析

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摘要

A novel fucose-binding lectin (SL2-1) from the bacterium Streptomyces rapamycinicus was identified by analysis of metagenomic DNA sequences. SL2-1 belongs to a new group of bacterial fucose-specific lectins that have no similarity to known bacterial fucose-binding proteins, but are related to certain eukaryotic fucose-binding lectins. The 17 kDa protein was expressed recombinantly in E. coli and purified by affinity chromatography. Glycan microarray analysis with fluorescently labeled recombinant SL2-1 demonstrated its ability to bind to core α1-6 fucosylated N-glycans, but not to core α1-3 fucosylated N-glycans, or other α1-2, α1-3 and α1-4 fucosylated oligosaccharides. The minimal high affinity binding epitope of SL2-1 was α1-6 fucosylated di-n-acetylchitobiose. The recombinant lectin was efficient in detection of N-glycan core fucosylation using lectin blotting and lectin ELISA assays. Finally, a workflow using SL2-1 for selective and quantitative profiling of core fucosylated N-glycans using UPLC-HILIC-FLR analysis was established. The approach was validated for selective capture and analysis of core fucosylated N-glycans present in complex glycan mixtures derived from mammalian serum IgG.
机译:通过对宏基因组DNA序列的分析,鉴定了一种来自细菌链霉菌的新型岩藻糖结合凝集素(SL2-1)。 SL2-1属于一类新的细菌岩藻糖特异性凝集素,与已知的细菌岩藻糖结合蛋白没有相似性,但与某些真核岩藻糖结合凝集素有关。 17 kDa蛋白在大肠杆菌中重组表达并通过亲和层析纯化。用荧光标记的重组SL2-1进行的糖微阵列分析显示其结合核心α1-6岩藻糖基化N-聚糖的能力,但不结合核心α1-3岩藻糖基化N-聚糖或其他α1-2,α1-3和α1-4的能力。岩藻糖基化低聚糖。 SL2-1的最小的高亲和力结合表位是α1-6岩藻糖基化的二-正乙酰基壳二糖。使用凝集素印迹和凝集素ELISA分析,重组凝集素可有效检测N-聚糖核心岩藻糖基化。最后,建立了使用SL2-1使用UPLC-HILIC-FLR分析对岩藻糖基化N-聚糖进行选择性和定量分析的工作流程。该方法经验证可用于选择性捕获和分析源自哺乳动物血清IgG的复杂聚糖混合物中存在的核心岩藻糖基化N-聚糖。

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