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使用基于香豆素的探针进行快速谷胱甘肽检测和通用肽/蛋白质标记以追踪细胞穿透

Rapid GSH detection and versatile peptide/protein labelling to track cell penetration using coumarin-based probes.

作者信息

Xue Li, Yu Dehao, Sun Jing, Guan Liangyu, Xie Chengzhi, Wang Luo, Jia Yuanyuan, Tian Junyu, Fan Heli, Sun Huabing

机构信息

The Province and Ministry Co-sponsored Collaborative Innovation Center for Medical Epigenetics, Tianjin Medical University; Tianjin Key Laboratory on Technologies Enabling Development of Clinical Therapeutics and Diagnostics, School of Pharmacy, Tianjin Medical University, Tianjin 300070, P. R. China.

School of Pharmacy, Jinzhou Medical University, Jinzhou, Liaoning 121001, P. R. China.

出版信息

Analyst. 2023 Jan 31;148(3):532-538. doi: 10.1039/d2an01510b.

DOI:10.1039/d2an01510b
PMID:36349786
Abstract

Biothiols play essential roles in balancing the redox state and modulating cellular functions. Fluorescent probes for monitoring/labelling biothiols often suffer from slow reaction rates, strong background fluorescence and cytotoxic byproduct release. Thus, developing facile and versatile probes to overcome the challenges is still in high demand. Here, we report four coumarin-maleimides as fast responding and fluorogenic probes to detect GSH or label peptides/proteins. The probes quantitatively and selectively react with GSH Michael addition within 1-2 min, achieving an 11-196-fold increase in fluorescence quantum yield blockage of the photoinduced electron transfer (PET) process. Optimized probe 4 is applied for the detection of GSH (A549 cells) and (zebrafish embryos). Taking advantage of the fast Michael addition between the maleimide moiety and the sulfhydryl group, we expand the application of our method for fluorescent labelling of peptides/proteins and for tracking their cellular uptake process. The labelling strategy works for both Cys-bearing and Cys-free proteins after the introduction of a sulfhydryl group using Traut's reagent. Fluorescence assay reveals that the TAT-peptide can efficiently enter cells, but H3 protein, part of nucleosomes, prefers to bind on the cell membrane by electrostatic interactions, shedding light on the cellular uptake activity of nucleosomes and affording a potential membrane staining strategy. Overall, our study illustrates the broad potential of coumarin-maleimide based dual-functional probes for GSH detection and versatile protein labelling in biochemical research.

摘要

生物硫醇在平衡氧化还原状态和调节细胞功能方面发挥着重要作用。用于监测/标记生物硫醇的荧光探针常常存在反应速率慢、背景荧光强以及细胞毒性副产物释放等问题。因此,开发简便且通用的探针来克服这些挑战仍然具有很高的需求。在此,我们报道了四种香豆素-马来酰亚胺作为快速响应且具有荧光性的探针,用于检测谷胱甘肽(GSH)或标记肽/蛋白质。这些探针在1 - 2分钟内通过迈克尔加成与GSH进行定量且选择性的反应,实现了荧光量子产率11 - 196倍的增加,这是由于光诱导电子转移(PET)过程受阻。优化后的探针4用于检测A549细胞和斑马鱼胚胎中的GSH。利用马来酰亚胺部分与巯基之间快速的迈克尔加成反应,我们拓展了该方法在肽/蛋白质荧光标记及其细胞摄取过程追踪方面的应用。在使用特劳特试剂引入巯基后,该标记策略对含半胱氨酸(Cys)和不含Cys的蛋白质均有效。荧光分析表明,TAT肽能够有效地进入细胞,但核小体的一部分H3蛋白更倾向于通过静电相互作用结合在细胞膜上,这揭示了核小体的细胞摄取活性,并提供了一种潜在的膜染色策略。总体而言,我们的研究说明了基于香豆素-马来酰亚胺的双功能探针在生化研究中用于GSH检测和通用蛋白质标记的广阔潜力。

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