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Identification of leucocyte surface protein interactions by high-throughput screening with multivalent reagents

机译:通过多价试剂高通量筛选鉴定白细胞表面蛋白相互作用

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摘要

We describe a high-throughput screening system to detect interactions between leucocyte surface proteins, taking into account that these interactions are usually of very low affinity. The method involves producing the extracellular regions of leucocyte proteins with tags so that they can be bound to nanoparticles to provide an avid reagent to screen over an array of 36 similar proteins immobilized using the Proteon™ XPR36 with detection by surface plasmon resonance. The system was tested using established interactions that could be detected without spurious binding. The ability to detect new interactions was shown by identifying a new interaction between carcinoembryonic antigen-related cell adhesion molecule 1 and carcinoembryonic antigen-related cell adhesion molecule 8.
机译:考虑到这些相互作用通常亲和力很低,我们描述了一种高通量筛选系统来检测白细胞表面蛋白之间的相互作用。该方法涉及产生带有标签的白细胞蛋白质的胞外区域,以便它们可以与纳米颗粒结合,从而提供一种狂热试剂,以筛选通过Proteon™XPR36固定化的36种相似蛋白质的阵列,并通过表面等离振子共振进行检测。使用已建立的交互作用对系统进行了测试,可以在没有虚假绑定的情况下进行检测。通过鉴定癌胚抗原相关的细胞粘附分子1和癌胚抗原相关的细胞粘附分子8之间的新相互作用,显示了检测新相互作用的能力。

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