Turn-on sensing for Ag+ based on AIE-active fluorescent probe and cytosine-rich DNA

被引:0
|
作者
Ke Ma
Hui Wang
Xing Li
Bin Xu
Wenjing Tian
机构
[1] Jilin University,State Key Laboratory of Supramolecular Structure and Materials
来源
Analytical and Bioanalytical Chemistry | 2015年 / 407卷
关键词
Chemical sensor; AIE fluorescent probe; Ag; detection; cytosine-rich DNA; Enzyme;
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学科分类号
摘要
An aggregation-induced-emission (AIE)-active molecule, 4,4ʹ-(1E,1ʹE)-2,2ʹ-(anthracene-9,10-diyl) bis (ethene-2,1-diyl) bis (N,N,N-trimethylbenzenaminium iodide) (DSAI), used as a label-free and turn-on fluorescent probe, was developed for Ag+ sensing. The cytosine-rich DNA (oligo-C) chosen as a base could be induced to form a hairpin structure in the presence of Ag+. To improve the sensitivity of Ag+ detection, we selected nuclease S1 to reduce the fluorescence intensity of DSAI via its strong ability to hydrolyze oligo-C. In the solution containing oligo-C, DSAI, and nuclease S1, in the absence of Ag+, oligo-C was broken into fragments by nuclease S1; this meant DSAI could not aggregate, leading to non-emission of the solution. In the presence of Ag+, oligo-C was induced to form a hairpin structure via the C–Ag+–C base pair and DSAI could aggregate on the surface of the hairpin structure to produce a strong emission. On increasing the amount of Ag+ in the solution containing oligo-C, DSAI, and nuclease S1, the fluorescence intensity of DSAI gradually increased, and the highest intensity was nearly 16-fold higher than the original intensity. The detection limit at a signal-to-noise ratio (S/N) of 3 was estimated to be 155 nmol L−1. The new sensing method provides simplicity, easy operation, and good sensitivity and selectivity for Ag+ detection.
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页码:2625 / 2630
页数:5
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