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Design of a protein tag and fluorogenic probe with modular structure for live-cell imaging of intracellular proteins

机译:用于细胞内蛋白质活细胞成像的具有模块化结构的蛋白质标签和荧光探针的设计

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Conditional fluorescence imaging is a powerful technique for precise spatiotemporal analysis of proteins in live cells upon administration of a synthetic probe. To be applicable to various biological phenomena, probes must be membrane-permeable, have a high signal-to-noise ratio, and work quickly. To date, few probes meet all of these requirements. Here, we designed a fluorogenic probe (AcFCANB) that could label intracellular proteins fused to the photoactive yellow protein (PYP) tag in live cells within 30 min and used it to image heterochromatin protein 1 localization in nuclei. AcFCANB is based on a modular platform consisting of fluorophore, ligand and quencher. We accelerated the labeling reaction by strategic mutations of charged residues on the surface of PYP. A simple model based on molecular dynamics simulations quantitatively reproduced the cooperative effect of multiple mutations on labeling rate.
机译:使用合成探针后,条件荧光成像是一种用于精确分析活细胞中蛋白质的时空分析的强大技术。为了适用于各种生物现象,探头必须是可透过膜的,具有高信噪比且工作迅速。迄今为止,很少有探头能够满足所有这些要求。在这里,我们设计了一种荧光探针(AcFCANB),可以在30分钟内在活细胞中标记与光敏黄色蛋白(PYP)标签融合的细胞内蛋白,并用它来成像异染色质蛋白1在细胞核中的定位。 AcFCANB基于包含荧光团,配体和淬灭剂的模块化平台。我们通过PYP表面带电残基的战略突变来加速标记反应。基于分子动力学模拟的简单模型定量再现了多个突变对标记率的协同作用。

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