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Two-Dimensional Trap for Ultrasensitive Quantification of Transient Protein Interactions

机译:二维陷阱用于瞬时蛋白相互作用的超灵敏定量

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摘要

We present an ultrasensitive technique for quantitative protein protein interaction analysis in a two-dimensional format based on phase-separated, micropatterned membranes. Interactions between proteins captured to lipid probes via an affinity tag trigger partitioning into the liquid-ordered phase, which is readily quantified by fluorescence imaging. Based on a calibration with well-defined low-affinity protein protein interactions, equilibrium dissociation constants >1 mM were quantified. Direct capturing of proteins from mammalian cell lysates enabled us to detect homo- and heterodimerization of signal transducer and activator of transcription proteins. Using the epidermal growth factor receptor (EGFR) as a model system, quantification of low-affinity interactions between different receptor domains contributing to EGFR dimerization was achieved. By exploitation of specific features of the membrane-based assay, the regulation of EGFR dimerization by lipids was demonstrated.
机译:我们提出了一种超敏感技术,用于基于相分离的微图案膜的二维格式的定量蛋白质相互作用分析。通过亲和标签捕获到脂质探针的蛋白质之间的相互作用触发了分配进入液相序列的过程,可以通过荧光成像轻松地对其进行定量。基于具有明确定义的低亲和力蛋白质相互作用的标定,对> 1 mM的平衡解离常数进行了定量。从哺乳动物细胞裂解物中直接捕获蛋白质使我们能够检测信号转导子和转录蛋白激活子的同二聚和异二聚化。使用表皮生长因子受体(EGFR)作为模型系统,可量化有助于EGFR二聚化的不同受体域之间的低亲和力相互作用。通过利用基于膜的测定的特定特征,证明了脂质对EGFR二聚化的调节。

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