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Universal Low-Background Fluorophore Platform via Structural Reprogramming of Oxazine 1 with Julolidine for Activatable Probe Design

化学 荧光团 重编程 光化学 聚集诱导发射 荧光 纳米技术 生物化学 光学 物理 材料科学 细胞
作者
Dianfeng Dai,Zhimin Zhang,Mo Ma,Chen Zhao,Jingkang Li,Siqi Zhang,Pinyi Ma,Bo Zhang,Daqian Song
出处
期刊:Analytical Chemistry [American Chemical Society]
卷期号:97 (38): 21071-21078 被引量:1
标识
DOI:10.1021/acs.analchem.5c04331
摘要

Fluorescent probes play a vital role in biological detection and imaging; however, their application is often hampered by high background fluorescence, which compromises detection sensitivity and reduces the signal-to-noise ratio. Oxazine 1 is a modifiable near-infrared fluorophore that can be used to develop low-background probes. Nonetheless, it suffers from limitations such as insufficient red-shifted emission, low fluorescence quantum yield, and poor cellular uptake. To address these limitations, we designed and synthesized two new oxazine derivatives, JSO and JDO, by replacing the diethylamino donor group of oxazine 1 with a rigid julolidine moiety. This structural modification effectively enhanced electron-donating ability, suppressed nonradiative decay, and improved membrane permeability. Compared to oxazine 1, the emission wavelength of JDO was red-shifted (703 nm), and its fluorescence quantum yield increased 2-fold. JDO also had superior intracellular accumulation and excellent pH stability and photostability. By leveraging these advantages, we developed a novel peroxynitrite (ONOO-)-responsive probe, JDO-ONOO, as a proof-of-concept demonstration to validate the design platform. Through strategic disruption of the fluorophore's conjugated structure, JDO-ONOO emitted ultralow background fluorescence, and in the presence of ONOO-, the fluorescence switched to a "turn-on" mode, resulting in a 130-fold increase in intensity. The probe had high sensitivity (LOD = 3.7 nM), rapid response, and excellent selectivity under physiological conditions. It was successfully employed in the fluorescence imaging of ONOO- in living cells and in multiple mouse models of inflammation. Overall, this study presents a universal strategy for developing next-generation low-background fluorescent probes, demonstrated through ONOO- detection.
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