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Real-time monitoring of caspase cascade activation in living cells

机译:生物细胞中Caspase级联激活的实时监测

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摘要

We introduce a simple, versatile and robust one-step technique that enables real-time imaging of multiple intracellular caspase activities in living cells without the need for complicated synthetic protocols. Conventional fluorogenic probes or recently reported activatable probes have been designed to target various proteases but are limited to extracellular molecules. Only a few have been applied to image intracellular proteases in living cells because most of these probes have limited cell-permeability. Our platform does not need complicated synthetic processes; instead it involves a straightforward peptide synthesis and a simple mixing step with a commercial transfection agent. The transfection agent efficiently delivered the highly quenched fluorogenic probes, comprised of distinctive pairs of dyes and quenchers, to the initiator caspase-8 and the effector caspase-3 in MDA-MB-435 cells, allowing dual-imaging of the activities of both caspases during the apoptotic process induced by TNF-related apoptosis induced ligand (TRAIL). With the combination of multiple fluorogenic probes, this simple platform can be applied to multiplexed imaging of selected intracellular proteases to study apoptotic processes in pathologies or for cell-based high throughput screening systems for drug discovery.
机译:我们介绍了一种简单,多功能和坚固的一步技术,可以在没有复杂合成方案的情况下实现活细胞中多个细胞内胱天蛋白酶活性的实时成像。常规的荧光探针或最近报道的可活化探针已经设计用于靶向各种蛋白酶,但仅限于细胞外分子。只有少数人应用于活细胞的图像细胞内蛋白酶,因为大多数这些探针具有有限的细胞渗透性。我们的平台不需要复杂的合成过程;相反,它涉及直接的肽合成和具有商业转染剂的简单混合步骤。转染剂有效地递送了由诸如MDA-MB-435细胞中的引发剂Caspase-8和效应Caspase-3的独特染料和猝灭剂的高淬火荧光探针。在MDA-MB-435细胞中,允许两种胱天蛋白酶的活动进行双重成像在TNF相关凋亡诱导配体(TRAIL)诱导的凋亡过程中。随着多种荧光探针的组合,该简单平台可以应用于所选细胞内蛋白酶的复用成像,以研究病理学中的凋亡过程或用于药物发现的细胞的高通量筛选系统。

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