Confining Thiolysis of Dinitrophenyl Ether to a Luminescent Metal–Organic Framework with a Large Stokes Shift for Highly Efficient Detection of Hydrogen Sulfide in Rat Brain

化学 硫分解 二硝基苯基 硫化氢 发光 乙醚 硫化物 斯托克斯位移 组合化学 光化学 有机化学 硫黄 光电子学 多酚 原花青素 生物 物理 抗体 免疫学 抗氧化剂
作者
Mengxia Qin,Wenliang Ji,Pengcheng Huang,Fang‐Ying Wu,Lanqun Mao
出处
期刊:Analytical Chemistry [American Chemical Society]
卷期号:96 (36): 14697-14705 被引量:2
标识
DOI:10.1021/acs.analchem.4c03929
摘要

Hydrogen sulfide (H2S) is a gaseous signaling molecule that regulates various physiological and pathological processes in the central nervous system. It is vital to develop an effective method to detect H2S in vivo to elucidate its critical role. However, current fluorescent probes for accurate quantification of H2S still face big challenges due to complicated fabrication, small Stokes shift, unsatisfactory selectivity, and especially delayed response time. Herein, based on simple postsynthetic modification, we present an innovative strategy by confining H2S-triggered thiolysis of dinitrophenyl (DNP) ether within a luminescent metal–organic framework (MOF) to address those issues. Due to the cleavage of the DNP moiety by H2S, the nanoprobe gives rise to a remarkable fluorescence turn-on signal with a large Stokes shift of 190 nm and also provides high selectivity to H2S against various interferents including competing biothiols. In particular, by virtue of the unique structural property of the MOF, it exhibits an ultrafast sensing ability for H2S (only 5 s). Moreover, the fluorescence enhancement efficiency displays a good linear correlation with H2S concentration in the range of 0–160 μM with a detection limit of 0.29 μM. Importantly, these superior sensing performances enable the nanoprobe to measure the basal value and monitor the change of H2S level in the rat brain.
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