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Imaging and determining friction forces of specific interactions between human IgG and rat anti-human IgG

机译:成像并确定人IgG和大鼠抗人IgG之间特异性相互作用的摩擦力

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摘要

Covalently immobilized rat anti-human immunoglobulin (IgG) monolayers on thiol-modified gold substrates and human IgG linked with the tips were fabricated using the self-assembled monolayer method, and interactions between these systems were studied by friction force microscopy (FFM). In addition to observation of distinct nanostructures of protein monolayers due to recognition events, FFM also quantified the friction force due to protein–protein-specific interactions. The average friction force due to interactions between the antigen functionalized tip and the antibody monolayer was determined as 200–250 pN, significantly greater than that between either the bare tip and the antibody monolayer (0–50 pN), or the blocked antigen tip and the antibody monolayer (50–100 pN), indicative of antigen/antibody-specific interactions. These results, taken together, suggest that FFM is not only capable of tracking recognition events, but also quantifying the friction force due to specific interactions between biological molecules, such as antigen and antibody.
机译:使用自组装单层方法制备了在硫醇修饰的金底物上共价固定的大鼠抗人免疫球蛋白(IgG)单层和与尖端连接的人IgG,并通过摩擦力显微镜(FFM)研究了这些系统之间的相互作用。除了观察到由于识别事件引起的蛋白质单分子层的独特纳米结构外,FFM还量化了由于蛋白质-蛋白质特异性相互作用而产生的摩擦力。抗原官能化末端与抗体单层之间相互作用产生的平均摩擦力被确定为200–250 pN,显着大于裸末端与抗体单层(0–50 pN)或封闭的抗原末端之间的平均摩擦力。单层抗体(50-100 pN),表示抗原/抗体特异性相互作用。这些结果加在一起表明,FFM不仅能够跟踪识别事件,而且能够量化由于生物分子(例如抗原和抗体)之间的特定相互作用而产生的摩擦力。

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