All-photonic kinase inhibitors: light-controlled release-and-report inhibition

被引:3
作者
Fleming, Cassandra L. [1 ,2 ]
Benitez-Martin, Carlos [1 ]
Bernson, Elin [3 ]
Xu, Yongjin [2 ]
Kristenson, Linnea [4 ]
Inghardt, Tord [5 ]
Lundback, Thomas [6 ]
Thoren, Fredrik B. [7 ]
Grotli, Morten [2 ]
Andreasson, Joakim [1 ]
机构
[1] Chalmers Univ Technol, Dept Chem & Chem Engn, Phys Chem, SE-41296 Gothenburg, Sweden
[2] Univ Gothenburg, Dept Chem & Mol Biol, Box 462, SE-40530 Gothenburg, Sweden
[3] Univ Gothenburg, Inst Clin Sci, Sahlgrenska Acad, TIMM Lab,Sahlgrenska Ctr Canc Res,Dept Obstet & Gy, SE-41296 Gothenburg, Sweden
[4] Univ Gothenburg, Inst Biomed, Sahlgrenska Acad, TIMM Lab,Sahlgrenska Ctr Canc Res,Dept Infect Dis, SE-41296 Gothenburg, Sweden
[5] Cardiovasc Renal & Metab, Innovat Med & Early Dev, AstraZeneca, SE-43183 Molndal, Sweden
[6] Mechanist & Struct Biol, Discovery Sci R&D, AstraZeneca, SE-43183 Molndal, Sweden
[7] Univ Gothenburg, Inst Biomed, Sahlgrenska Acad, TIMM Lab,Sahlgrenska Ctr Canc Res,Dept Med Biochem, SE-41296 Gothenburg, Sweden
基金
瑞典研究理事会;
关键词
PHOTOREMOVABLE PROTECTING GROUPS; LCK; DISCOVERY; TYROSINE; DESIGN; POTENT; SAR;
D O I
10.1039/d4sc00390j
中图分类号
O6 [化学];
学科分类号
0703 ;
摘要
Light-responsive molecular tools targeting kinases affords one the opportunity to study the underlying cellular function of selected kinases. In efforts to externally control lymphocyte-specific protein tyrosine kinase (LCK) activity, the development of release-and-report LCK inhibitors is described, in which (i) the release of the active kinase inhibitor can be controlled externally with light; and (ii) fluorescence is employed to report both the release and binding of the active kinase inhibitor. This introduces an unprecedented all-photonic method for users to both control and monitor real-time inhibitory activity. A functional cellular assay demonstrated light-mediated LCK inhibition in natural killer cells. The use of coumarin-derived caging groups resulted in rapid cellular uptake and non-specific intracellular localisation, while a BODIPY-derived caging group predominately localised in the cellular membrane. This concept of release-and-report inhibitors has the potential to be extended to other biorelevant targets where both spatiotemporal control in a cellular setting and a reporting mechanism would be beneficial. An all-photonic method is described, in which (i) the release of an active kinase inhibitor is controlled externally with light; and (ii) fluorescence is employed to report both the release and binding of the inhibitor to its corresponding target.
引用
收藏
页码:6897 / 6905
页数:9
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