A highly sensitive fluorescent light-up probe for real-time detection of the endogenous protein target and its antagonism in live cells

被引:18
|
作者
Geng, Junlong [1 ]
Goh, Walter L. [2 ]
Zhang, Chongjing [3 ]
Lane, David P. [2 ]
Liu, Bin [1 ,3 ]
Ghadessy, Farid [2 ]
Tan, Yen Nee [1 ]
机构
[1] ASTAR, Inst Mat Res Engn, Singapore 117602, Singapore
[2] ASTAR, Lab P53, Singapore 138648, Singapore
[3] Natl Univ Singapore, Dept Chem & Biomol Engn, Singapore 117576, Singapore
基金
新加坡国家研究基金会;
关键词
AGGREGATION-INDUCED EMISSION; TUMOR-SUPPRESSOR PATHWAY; P53; PATHWAY; CANCER-CELLS; LIVING CELLS; IN-SITU; MDM2; BIOPROBE; INHIBITION; APOPTOSIS;
D O I
10.1039/c5tb00819k
中图分类号
TB3 [工程材料学]; R318.08 [生物材料学];
学科分类号
0805 ; 080501 ; 080502 ;
摘要
Real-time detection and monitoring of cancer-related biomolecular interactions in live cells are of paramount importance for disease diagnostics and drug screening. Herein, we developed a target-specific fluorescent light-up probe for cellular detection of Mdm2, the key negative regulator of the p53 tumour suppressor protein. Conjugation of a uniquely designed fluorogen (TPECM) with aggregation induced-emission properties, to a specific p53-derived peptide (12.1Pep) targeting Mdm2, yielded a cell-permeable probe (TPECM-12.1Pep) with turn-on fluorescence properties for real-time live cell imaging of Mdm2. This specific light-up probe is almost non-fluorescent in its isolated state but is highly emissive upon binding to Mdm2, enabling quantitative detection of both Mdm2 and its antagonism. Using a model compound (Nutlin-3a), we demonstrate that the as-developed probes can be used to screen p53-Mdm2 inhibiting drug candidates, both in vitro and in cells. Furthermore, the probe activity can be accurately monitored in cells using a fluorescently activated cell sorting machine. These features will expedite research in the areas of drug discovery, clinical diagnostics and fundamental cell biology.
引用
收藏
页码:5933 / 5937
页数:5
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