Activatable Raman Probes Utilizing Enzyme-Induced Aggregate Formation for Selective Ex Vivo Imaging

被引:15
|
作者
Fujioka, Hiroyoshi [1 ,2 ]
Kawatani, Minoru [2 ,3 ]
Spratt, Spencer John [4 ]
Komazawa, Ayumi [1 ]
Misawa, Yoshihiro [2 ,3 ]
Shou, Jingwen [4 ]
Mizuguchi, Takaha [4 ]
Kosakamoto, Hina [5 ]
Kojima, Ryosuke [3 ]
Urano, Yasuteru [1 ,3 ]
Obata, Fumiaki [5 ,6 ]
Ozeki, Yasuyuki [4 ]
Kamiya, Mako [2 ,3 ,7 ]
机构
[1] Univ Tokyo, Grad Sch Pharmaceut Sci, Tokyo 1130033, Japan
[2] Tokyo Inst Technol, Dept Life Sci & Technol, Yokohama, Kanagawa 2268501, Japan
[3] Univ Tokyo, Grad Sch Med, Tokyo 1130033, Japan
[4] Univ Tokyo, Grad Sch Engn, Dept Elect Engn & Informat Syst, Tokyo 1138656, Japan
[5] RIKEN Ctr Biosyst Dynam Res, Kobe, Hyogo 6500047, Japan
[6] Kyoto Univ, Grad Sch Biostudies, Kyoto 6068501, Japan
[7] Tokyo Inst Technol, Living Syst Mat LiSM Res Grp, Int Res Frontiers Initiat IRFI, Yokohama, Kanagawa 2268501, Japan
关键词
FLUORESCENT-PROBE; PYRONIN-Y; VISUALIZATION; SENSITIVITY; TISSUE; CELLS;
D O I
10.1021/jacs.2c12381
中图分类号
O6 [化学];
学科分类号
0703 ;
摘要
Detecting multiple enzyme activities simultaneously with high spatial specificity is a promising strategy to investigate complex biological phenomena, and Raman imaging would be an excellent tool for this purpose due to its high multiplexing capabilities. We previously developed activatable Raman probes based on 9CN-pyronins, but specific visualization of cells with target enzyme activities proved difficult due to leakage of the hydrolysis products from the target cells after activation. Here, focusing on rhodol bearing a nitrile group at the position of 9 (9CN-rhodol), we established a novel mechanism for Raman signal activation based on a combination of aggregate formation (to increase local dye concentration) and the resonant Raman effect along with the bathochromic shift of the absorption, and utilized it to develop Raman probes. We selected the 9CN-rhodol derivative 9CN-JCR as offering a suitable combination of increased stimulated Raman scattering (SRS) signal intensity and high aggregate-forming ability, resulting in good retention in target cells after probe activation. By using isotope-edited 9CN-JCR-based probes, we could simultaneously detect beta-galactosidase, gamma-glutamyl transpeptidase, and dipeptidyl peptidase-4 activities in live cultured cells and distinguish cell regions expressing target enzyme activity in Drosophila wing disc and fat body ex vivo.
引用
收藏
页码:8871 / 8881
页数:11
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