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Diazo Coupling Method for Covalent Attachment of Proteins to Solid Substrates

机译:重氮偶联法将蛋白质共价结合到固体基质上

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We describe a process for covalently linking proteins to glass microscope slides and microbeads in a manner that optimizes the reactivity of the immobilized proteins and that is suitable for high-throughput microarray and flow cytometry analysis.The method involves the diazo coupling of proteins onto activated self-assembled monolayers formed from p-aminophenyl trimethoxysilane.Proteins immobilized by this method maintained bioactivity and produced enhanced levels of protein-protein interaction,low background fluorescence,and high selectivity.The binding of immobilized proteins to their specific binding partner was analyzed quantitatively and successfully correlated with solution concentrations.Diazotized surfaces bound more efficiently to proteins containing a hexahistidine tag than those without a his-tag.Moreover,significantly higher reactivity of the immobilized bis-tagged proteins was observed on diazotized surfaces than on amine-terminated surfaces.Results suggest that his-tagged proteins are immobilized by reaction of the his-tag with the diazotized surface,thus offering the possibility for preferential orientation of covalently bound proteins.
机译:我们描述了一种将蛋白质与玻璃显微镜载玻片和微珠共价连接的方法,该方法可以优化固定化蛋白质的反应性,适用于高通量微阵列和流式细胞仪分析。该方法涉及将蛋白质重氮偶合到活化的自我上对氨基苯基三甲氧基硅烷形成的单分子组装膜。通过该方法固定化的蛋白质保持了生物活性,并增强了蛋白质-蛋白质相互作用的水平,降低了背景荧光,选择性高。定量分析了固定化蛋白质与其特异性结合伴侣的结合情况与没有组氨酸标签的蛋白质相比,重氮化的表面与含六组氨酸标签的蛋白质的结合效率更高。此外,在重氮化的表面上观察到的固定化双标签蛋白质的反应性比在胺端基的表面上要高得多。被他标记的蛋白质通过组氨酸标签与重氮化表面的反应而被固定,从而为共价结合的蛋白质的优先取向提供了可能性。

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