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An activity-dependent proximity ligation platform for spatially resolved quantification of active enzymes in single cells

机译:一个活动依赖的邻近连接平台用于空间分辨单个细胞中活性酶的定量

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摘要

Integration of chemical probes into proteomic workflows enables the interrogation of protein activity, rather than abundance. Current methods limit the biological contexts that can be addressed due to sample homogenization, signal-averaging, and bias toward abundant proteins. Here we report a platform that integrates family-wide chemical probes with proximity-dependent oligonucleotide amplification and imaging to quantify enzyme activity in native contexts with high spatial resolution. Application of this method, activity-dependent proximity ligation (ADPL), to serine hydrolase and cysteine protease enzymes enables quantification of differential enzyme activity resulting from endogenous changes in localization and expression. In a competitive format, small-molecule target engagement with endogenous proteins in live cells can be quantified. Finally, retention of sample architecture enables interrogation of complex environments such as cellular co-culture and patient samples. ADPL should be amenable to diverse probe and protein families to detect active enzymes at scale and resolution out of reach with current methods.
机译:将化学探针整合到蛋白质组学工作流程中可以查询蛋白质活性而不是蛋白质含量。当前的方法限制了由于样品均质化,信号平均和偏向丰富蛋白质而可能解决的生物学问题。在这里,我们报告了一个平台,该平台将全家族的化学探针与邻近依赖性寡核苷酸扩增和成像相集成,以量化具有高空间分辨率的天然环境中的酶活性。该方法的活性依赖的邻近连接(ADPL)在丝氨酸水解酶和半胱氨酸蛋白酶上的应用可以量化由内源性定位和表达变化引起的酶活性差异。以竞争性形式,可以定量与活细胞中内源蛋白质的小分子靶标结合。最后,保留样品结构可以询问复杂的环境,例如细胞共培养和患者样品。 ADPL应该适合各种探针和蛋白质家族,以现有方法无法大规模地检测活性酶和分离度。

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