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首页> 外文期刊>Sensors >Label-Free Fluorescence Assay of S1 Nuclease and Hydroxyl Radicals Based on Water-Soluble Conjugated Polymers and WS 2 Nanosheets
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Label-Free Fluorescence Assay of S1 Nuclease and Hydroxyl Radicals Based on Water-Soluble Conjugated Polymers and WS 2 Nanosheets

机译:基于水溶性共轭聚合物和WS 2纳米片的S1核酸酶和羟自由基的无标记荧光测定

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摘要

We developed a new method for detecting S1 nuclease and hydroxyl radicals based on the use of water-soluble conjugated poly[9,9-bis(6,6-( N,N,N -trimethylammonium)-fluorene)-2,7-ylenevinylene-co-alt-2,5-dicyano-1,4-phenylene)] (PFVCN) and tungsten disulfide (WS 2 ) nanosheets . Cationic PFVCN is used as a signal reporter, and single-layer WS 2 is used as a quencher with a negatively charged surface. The ssDNA forms complexes with PFVCN due to much stronger electrostatic interactions between cationic PFVCN and anionic ssDNA, whereas PFVCN emits yellow fluorescence. When ssDNA is hydrolyzed by S1 nuclease or hydroxyl radicals into small fragments, the interactions between the fragmented DNA and PFVCN become weaker, resulting in PFVCN being adsorbed on the surface of WS 2 and the fluorescence being quenched through fluorescence resonance energy transfer. The new method based on PFVCN and WS 2 can sense S1 nuclease with a low detection limit of 5 × 10 ?6 U/mL. Additionally, this method is cost-effective by using affordable WS 2 as an energy acceptor without the need for dye-labeled ssDNA. Furthermore, the method provides a new platform for the nuclease assay and reactive oxygen species, and provides promising applications for drug screening.
机译:我们开发了一种基于水溶性共轭聚[9,9-双(6,6-(N,N,N-三甲基铵)-芴)-2,7-的S1核酸酶和羟基自由基检测新方法亚乙烯基-co-alt-2,5-二氰基-1,4-亚苯基]](PFVCN)和二硫化钨(WS 2)纳米片。阳离子PFVCN用作信号报告器,单层WS 2用作表面带负电的淬灭剂。由于阳离子PFVCN与阴离子ssDNA之间更强的静电相互作用,因此ssDNA与PFVCN形成复合物,而PFVCN发出黄色荧光。当ssDNA被S1核酸酶或羟基自由基水解成小片段时,片段化的DNA与PFVCN之间的相互作用变弱,导致PFVCN吸附在WS 2的表面上,并通过荧光共振能量转移使荧光猝灭。基于PFVCN和WS 2的新方法可以检测S1核酸酶,检测限低至5×10?6 U / mL。此外,该方法通过使用负担得起的WS 2作为能量受体而具有成本效益,而无需染料标记的ssDNA。此外,该方法为核酸酶测定和活性氧种类提供了新的平台,并为药物筛选提供了有希望的应用。

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