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Analysis of a non-labeling protein array on biotin modified gold surfaces using atomic force microscopy and surface plasmon resonance

机译:使用原子力显微镜和表面等离子体共振分析生物素修饰的金表面上的非标记蛋白质阵列

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摘要

Streptavidin was used as a linker protein for binding a second biotinylated protein. To efficiently combine streptavidin without non-specific binding, a well-controlled array of biotin was prepared on a gold surface by a mixed self-assembly method. Two thiol derivatives containing hydroxyl and biotin functional groups, respectively, were used to fabricate the mixed self-assembled monolayer. The antibody was fragmented, modified with biotin, and added to the array on the streptavidin linker layer. Topographical changes to the array surface caused by protein immobilization were demonstrated by applying atomic force microscopy and ellipsometry. The resonance wavelengths of SPR spectra were red shifted according to the increase in thickness of the dielectric layer by protein immobilization. (C) 2007 Elsevier B.V. All rights reserved.
机译:链霉亲和素用作连接第二种生物素化蛋白的接头蛋白。为了有效地结合抗生蛋白链菌素而没有非特异性结合,通过混合自组装方法在金表面上制备了良好控制的生物素阵列。分别包含羟基和生物素官能团的两种硫醇衍生物被用于制造混合的自组装单层。将抗体片段化,用生物素修饰,然后添加到链霉亲和素接头层上的阵列中。通过应用原子力显微镜和椭偏仪证明了蛋白质固定化引起的阵列表面的形貌变化。 SPR光谱的共振波长根据蛋白质固定介电层厚度的增加而发生红移。 (C)2007 Elsevier B.V.保留所有权利。

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