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Surface plasmon resonance imaging for real-time, label-free analysis of protein interactions with carbohydrate microarrays

机译:表面等离振子共振成像可实时,无标记地分析与碳水化合物微阵列的蛋白质相互作用

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Plant lectin recognition of glycans was evaluated by SPR imaging using a model array of N-biotinylated aminoethyl glycosides of β-d-glucose (negative control), α-d-mannose (conA-responsive), β-d-galactose (RCA120-responsive) and N-acetyl-β-d-glucosamine (WGA-responsive) printed onto neutravidin-coated gold chips. Selective recognition of the cognate ligand was observed when RCA120 was passed over the array surface. Limited or no binding was observed for the non-cognate ligands. SPR imaging of an array of 40 sialylated and unsialylated glycans established the binding preference of hSiglec7 for α2-8-linked disialic acid structures over α2-6-sialyl-LacNAcs, which in turn were recognized and bound with greater affinity than α2-3-sialyl-LacNAcs. Affinity binding data could be obtained with as little as 10–20 μg of lectin per experiment. The SPR imaging technique was also able to establish selective binding to the preferred glycan ligand when analyzing crude culture supernatant containing 10–20 μg of recombinant hSiglec7-Fc. Our results show that SPR imaging provides results that are in agreement with those obtained from fluorescence based carbohydrate arrays but with the added advantage of label-free analysis.
机译:通过SPR成像使用β-d-葡萄糖(阴性对照),α-d-甘露糖(conA响应),β-d-半乳糖(RCA < sub> 120 响应)和N-乙酰基-β-d-葡萄糖胺(WGA响应)印刷在涂有中性生物素的金芯片上。当RCA 120 通过阵列表面时,观察到同源配体的选择性识别。对于非同源配体观察到有限或没有结合。 SPR成像的40个唾液酸化和未唾液酸化聚糖阵列建立了hSiglec7对α2-8连接的二唾液酸结构比α2-6-唾液酸-LacNAcs的结合偏好,后者被识别并以比α2-3-唾液酸-LacNAcs。每个实验中仅需10-20μg的凝集素就可以获得亲和力结合数据。当分析含有10–20μg重组hSiglec7-Fc的粗培养上清液时,SPR成像技术还能够与优选的聚糖配体建立选择性结合。我们的结果表明,SPR成像所提供的结果与基于荧光的碳水化合物阵列所获得的结果一致,但具有无标记分析的额外优势。

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