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A Chemical Approach for Profiling Intracellular AKT Signaling Dynamics from Single Cells

机译:一种从单细胞分析细胞内AKT信号动力学的化学方法

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We present here a novel chemical method to continuously analyze intracellular AKT signaling activities at single-cell resolution, without genetic manipulations. A pair of cyclic peptide-based fluorescent probes were developed to recognize the phosphorylated Ser474 site and a distal epitope on AKT. A Forster resonance energy transfer signal is generated upon concurrent binding of the two probes onto the same AKT protein, which is contingent upon the Ser474 phosphorylation. Intracellular delivery of the probes enabled dynamic measurements of the AKT signaling activities. We further implemented this detection strategy on a microwell single-cell platform, and interrogated the AKT signaling dynamics in a human glioblastoma cell line. We resolved unique features of the single-cell signaling dynamics following different perturbations. Our study provided the first example of monitoring the temporal evolution of cellular signaling heterogeneities and unveiled biological information that was inaccessible to other methods.
机译:我们在这里提出了一种新颖的化学方法,可以连续分析细胞内AKT信号以单细胞分辨率的活动,而无需进行基因操作。开发了一对基于环状肽的荧光探针,以识别磷酸化的Ser474位点和AKT的远端表位。当两个探针同时结合到相同的AKT蛋白上时,就会产生Forster共振能量转移信号,这取决于Ser474的磷酸化作用。探针的细胞内递送使得能够动态测量AKT信号传导活性。我们进一步在微孔单细胞平台上实现了这种检测策略,并询问了人类胶质母细胞瘤细胞系中的AKT信号动力学。我们解决了不同扰动后单细胞信号动力学的独特特征。我们的研究提供了监测细胞信号异质性随时间变化的第一个例子,并揭示了其他方法无法获得的生物学信息。

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