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DNA mimics of red fluorescent proteins (RFP) based on G-quadruplex-confined synthetic RFP chromophores

机译:基于G-四链体限制的合成RFP发色团的红色荧光蛋白(RFP)的DNA模拟

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摘要

Red fluorescent proteins (RFPs) have emerged as valuable biological markers for biomolecule imaging in living systems. Developing artificial fluorogenic systems that mimic RFPs remains an unmet challenge. Here, we describe the design and synthesis of six new chromophores analogous to the chromophores in RFPs. We demonstrate, for the first time, that encapsulating RFP chromophore analogues in canonical DNA G-quadruplexes (G4) can activate bright fluorescence spanning red and far-red spectral regions (Em = 583−668 nm) that nearly match the entire RFP palette. Theoretical calculations and molecular dynamics simulations reveal that DNA G4 greatly restricts radiationless deactivation of chromophores induced by a twisted intramolecular charge transfer (TICT). These DNA mimics of RFP exhibit attractive photophysical properties comparable or superior to natural RFPs, including high quantum yield, large Stokes shifts, excellent anti-photobleaching properties, and two-photon fluorescence. Moreover, these RFP chromophore analogues are a novel and distinctive type of topology-selective G4 probe specific to parallel G4 conformation. The DNA mimics of RFP have been further exploited for imaging of target proteins. Using cancer-specific cell membrane biomarkers as targets, long-term real-time monitoring in single live cell and two-photon fluorescence imaging in tissue sections have been achieved without the need for genetic coding.
机译:红色荧光蛋白(RFPs)已成为生命系统中生物分子成像的有价值的生物标记。开发模拟RFP的人工荧光系统仍然是一项尚未解决的挑战。在这里,我们描述了六个类似于RFP中发色团的新发色团的设计和合成。我们首次证明了将RFP生色团类似物封装在规范的DNA G四联体(G4)中可以激活几乎与整个RFP调色板匹配的跨越红色和远红色光谱区域(Em = 583-668 nm)的明亮荧光。理论计算和分子动力学模拟表明,DNA G4极大地限制了分子内电荷转移(TICT)引起的生色团的无辐射失活。 RFP的这些DNA模拟物表现出与天然RFP相当或更好的诱人的光物理特性,包括高量子产率,大的斯托克斯位移,出色的抗光漂白特性和双光子荧光。此外,这些RFP生色团类似物是一种新颖且独特的拓扑选择性G4探针,专门针对平行G4构象。 RFP的DNA模仿物已被进一步用于靶蛋白成像。使用癌症特异性细胞膜生物标志物作为靶标,无需基因编码即可实现单活细胞的长期实时监测和组织切片中的双光子荧光成像。

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