Fluorescent labeling agents change binding profiles of glycan-binding proteins

聚糖 荧光 化学 生物化学 离解常数 凝集素 蛋白质阵列分析 糖蛋白 DNA微阵列 受体 量子力学 基因 物理 基因表达
作者
Yiyan Fei,Yung-Shin Sun,Yanhong Li,Kam Lau,Hai Yu,Harshal A. Chokhawala,Shengshu Huang,J. P. Landry,Xi Chen,X. D. Zhu
出处
期刊:Molecular BioSystems [The Royal Society of Chemistry]
卷期号:7 (12): 3343-3343 被引量:57
标识
DOI:10.1039/c1mb05332a
摘要

Interactions of glycan-binding proteins (GBPs) with glycans are essential in cell adhesion, bacterial/viral infection, and cellular signaling pathways. Experimental characterization of these interactions based on glycan microarrays typically involves (1) labeling GBPs directly with fluorescent reagents before incubation with the microarrays, or (2) labeling GBPs with biotin before the incubation and detecting the captured GBPs after the incubation using fluorescently labeled streptavidin, or (3) detecting the captured GBPs after the incubation using fluorescently labeled antibodies raised against the GBPs. The fluorescent signal is mostly measured ex situ after excess fluorescent materials are washed off. In this study, by using a label-free optical scanner for glycan microarray detection, we measured binding curves of 7 plant lectins to 24 glycans: four β1-4-linked galactosides, three β1-3-linked galactosides, one β-linked galactoside, one α-linked N-acetylgalactosaminide, eight α2-3-linked sialosides, and seven α2-6-linked sialosides. From association and dissociation constants deduced by global-fitting the binding curves, we found that (1) labeling lectins directly with fluorescent agents change binding profiles of lectins, in some cases by orders of magnitude; (2) those lectin–glycan binding reactions characterized with large dissociation rates, though biologically relevant, are easily missed or deemed insignificant in ex situ fluorescence-based assays as most captured lectins are washed off before detection. This study highlights the importance of label-free real-time detection of protein–ligand interactions and the potential pitfall in interpreting fluorescence-based assays for characterization of protein–glycan interactions.
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