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Spatiotemporal-Controlled Reporter for Cell-Surface Proteolytic Enzyme Activity Visualization

机译:用于细胞表面蛋白水解酶活性的时尚记者可视化

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摘要

Live-cell imaging of cell-surface-associated proteolytic enzymes is crucial to understand their biological roles and functions in both physiological and pathological processes. However, the complexity of the cell membrane environment increases difficulties in specifically investigating targeted proteolytic activities within the microenvironment. Towards this end, a unique, photoremovable, furin-responsive peptide probe that can undergo spatiotemporal control through UV-light illumination has been designed and synthesized to aid in visualizing the activity of a cell-surface-associated protease enzyme, furin, in live cells. Prior to light irradiation, the photolabile moiety, 4,5-dimethoxy-2-nitrobenzyl, in the peptide sequence of the reporter will block furin-like enzymatic hydrolysis, and thus, no fluorescence will be observed. Upon simple light illumination, photolysis will occur, thereby revealing the uncaged peptide probe, which can undergo enzyme hydrolysis and lead to an increase in fluorescence signal; this allows the real-time imaging of endogenous cell-surface-associated furin-like enzyme function in living cells through precise spatial and temporal resolution.
机译:细胞表面相关蛋白水解酶的活细胞成像至关重要,以了解其生理和病理过程中的生物作用和功能。然而,细胞膜环境的复杂性增加了在微环境中具体研究靶向蛋白水解活性的困难。朝向此目的,设计和合成了可以通过UV光照射进行时尚控制的独特,光放大的Furin-encorperive肽探针,以帮助可视化细胞表面相关蛋白酶酶,Furin,活细胞中的活性。在光照射之前,在报告者的肽序列中,光映射部分,4,5-二甲氧基-2-硝基苄基将阻断Furin样酶水解,因此,不会观察到荧光。在简单的光照照射后,将发生光解,从而显示出未透过的肽探针,其可以经历酶水解并导致荧光信号的增加;这允许通过精确的空间和时间分辨率在活细胞中实时成像。

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