Design of Large Stokes Shift Fluorescent Proteins Based on Excited State Proton Transfer of an Engineered Photobase

荧光团 化学 荧光 斯托克斯位移 激发态 光化学 生物物理学 量子产额 光激发 质子 光学 原子物理学 物理 量子力学 生物
作者
Elizabeth Moreira dos Santos,Wei Sheng,Rahele Esmatpour Salmani,Setare Tahmasebi Nick,Alireza Ghanbarpour,Hadi Gholami,Chrysoula Vasileiou,James H. Geiger,Babak Borhan
出处
期刊:Journal of the American Chemical Society [American Chemical Society]
卷期号:143 (37): 15091-15102 被引量:70
标识
DOI:10.1021/jacs.1c05039
摘要

The incredible potential for fluorescent proteins to revolutionize biology has inspired the development of a variety of design strategies to address an equally broad range of photophysical characteristics, depending on potential applications. Of these, fluorescent proteins that simultaneously exhibit high quantum yield, red-shifted emission, and wide separation between excitation and emission wavelengths (Large Stokes Shift, LSS) are rare. The pursuit of LSS systems has led to the formation of a complex, obtained from the marriage of a rationally engineered protein (human cellular retinol binding protein II, hCRBPII) and different fluorogenic molecules, capable of supporting photobase activity. The large increase in basicity upon photoexcitation leads to protonation of the fluorophore in the excited state, dramatically red-shifting its emission, leading to an LSS protein/fluorophore complex. Essential for selective photobase activity is the intimate involvement of the target protein structure and sequence that enables Excited State Proton Transfer (ESPT). The potential power and usefulness of the strategy was demonstrated in live cell imaging of human cell lines.
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