Determination of adenosine triphosphate based on the use of fluorescent terbium(III) organic frameworks and aptamer modified gold nanoparticles

被引:0
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作者
Chao Sun
Shiyu Zhao
Fei Qu
Wenli Han
Jinmao You
机构
[1] Qufu Normal University,The Key Laboratory of Life
[2] Qufu Normal University,Organic Analysis
[3] Beijing Institute of Technology,The Key Laboratory of Pharmaceutical Intermediates and Analysis of Natural Medicine
[4] Dalai Nur Sub-bureau of Hulunbuir Ecology and Enviroment Bureau,Beijing Key Laboratory of Photoelectronic/Electrophotonic Conversion Materials, Key Laboratory of Cluster Science, Ministry of Education, School of Chemistry and Chemical Engineering
[5] Chongqing Medical University,Laboratory Animal Center
[6] Chinese Academy of Science,Key Laboratory of Tibetan Medicine Research & Qinghai Provincial Key Laboratory of Tibetan Medicine Research, Northwest Institute of Plateau Biology
来源
Microchimica Acta | 2020年 / 187卷
关键词
Thiol-labeled aptamer; Steric repulsion; Electrostatic repulsion; Unlabeled aptamer; Inner filter effect; Dynamic quenching; Fluorescence resonance energy transfer; Biosensing; ATP-binding aptamer; Aggregation;
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学科分类号
摘要
A thiol-labeled adenosine triphosphate (ATP) binding aptamer is covalently linked on the surface of gold nanoparticles (AuNPs). This warrants protection of the red AuNPs from aggregation in high salt condition. The dispersed AuNPs can quench the fluorescence of the Tb(III)-MOFs at 547 nm with the excitation wavelength of 290 nm. This is ascribed to the combined action of inner filter effect, dynamic quenching and fluorescence resonance energy transfer. If the aptamer binds ATP to form folded structures, the AuNPs aggregate in high salt medium and the green fluorescence of the Tb(III)-MOFs is recovered. This method shows good sensitivity and selectivity for ATP, and the linear range is from 0.5 to 10 μM of ATP with the detection limitat of 0.32 μM. It was applied to the determination of ATP in (spiked) human plasma with satisfactory recoveries (from 93.2% to 106.3%). Oppositely, when the unlabeled aptamer is used instead of thiol-labeled aptamer in this process, the ATP-aptamer complexes rather than unlabeled aptamer provide greater protection for AuNPs against salt-induced aggregation. It is found that when the aptamer covalently binds to AuNPs, the steric hindrance is dominant for the stabilization of AuNPs; for unlabeled aptamer, the electrostatic repulsion is responsible for their stability, irrespective of whether ATP is present or not. These two different forces lead to the aggregation or dispersion of AuNPs with addition of target in salt solution.
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