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High-Throughput Flow Cytometry Compatible Biosensor Based on Fluorogen Activating Protein Technology

机译:基于荧光激活蛋白质技术的高通量流式细胞术兼容生物传感器

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摘要

Monitoring the trafficking of multiple proteins simultaneously in live cells is of great interest because many receptor proteins are found to function together with others in the same cell. However, existing fluorescent labeling techniques have restricted the mechanistic study of functional receptor pairs. We have expanded a hybrid system combining fluorogen activating protein (FAP) technology and high-throughput flow cytometry to a new type of biosensor that is robust, sensitive, and versatile. This provides the opportunity to study multiple trafficking proteins in the same cell. Human beta2 adrenergic receptor (β2AR) fused with FAP AM2.2 and murine C-C chemokines receptor type 5 fused with FAP MG13 was chosen for our model system. The function of the receptor and the binding between MG13 and fluorogen MG-2p have been characterized by flow cytometry and confocal microscopy assays. The binding of fluorogen and the FAP pair is highly specific, while both FAP-tagged fusion proteins function similarly to their wild type counterparts. The system has successfully served as a counter screen assay to eliminate false positive compounds identified in a screen against NIH Molecular Libraries Small Molecule Repository targeting regulators of the human β2AR.
机译:在活细胞中同时监测多种蛋白质的运输非常重要,因为发现许多受体蛋白质在同一细胞中与其他蛋白质一起发挥作用。然而,现有的荧光标记技术限制了功能性受体对的机理研究。我们已经将结合了氟激活蛋白(FAP)技术和高通量流式细胞仪的混合系统扩展为一种新型的生物传感器,该传感器坚固,灵敏且用途广泛。这提供了研究同一细胞中多种运输蛋白的机会。选择与FAP AM2.2融合的人β2肾上腺素能受体(β2AR)和与FAP MG13融合的5型小鼠C-C趋化因子受体作为我们的模型系统。受体的功能以及MG13和氟MG-2p之间的结合已通过流式细胞术和共聚焦显微镜分析进行了表征。氟与FAP对的结合具有高度特异性,而两种带有FAP标签的融合蛋白的功能与其野生型对应物相似。该系统已成功用作反筛选试验,以消除针对人β2AR的NIH分子库小分子储存库的筛选中鉴定出的假阳性化合物。

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