首页> 外文期刊>Langmuir: The ACS Journal of Surfaces and Colloids >Tuning Toehold Length and Temperature to Achieve Rapid, Colorimetric Detection of DNA from the Disassembly of DNA-Gold Nanoparticle Aggregates
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Tuning Toehold Length and Temperature to Achieve Rapid, Colorimetric Detection of DNA from the Disassembly of DNA-Gold Nanoparticle Aggregates

机译:调整脚趾的长度和温度,以实现从金纳米颗粒DNA的分解中快速进行比色检测。

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摘要

Gold nanoparticles have been widely utilized to achieve colorimetric detection for various diagnostic applications. One of the most frequently used methods for DNA detection involves the aggregation of DNA-modified gold nanoparticles driven by target DNA hybridization. This process, however, is intrinsically slow, limiting its use in rapid diagnostics. Here we take advantage of the reverse process: the disassembly of preformed aggregates triggered by the addition of target DNA via a strand displacement mechanism. A systematic study of the dependence of the disassembly rate on temperature, with and without toeholds, has delivered a system that produces an extremely rapid colorimetric response. Furthermore, using an optimal toehold length of 5 nucleotides, target triggered disassembly is rapid over a wide range of ambient temperatures. Using this overhang system, simple visualization of low picomole amounts of target DNA is possible within 10 min at room temperature.
机译:金纳米颗粒已被广泛用于各种诊断应用中的比色检测。 DNA检测最常用的方法之一涉及由靶DNA杂交驱动的DNA修饰金纳米颗粒的聚集。但是,此过程本质上很慢,限制了其在快速诊断中的使用。在这里,我们利用了反向过程的优势:通过链置换机制添加目标DNA触发的预制聚集体的分解。对有或没有脚尖的分解速度对温度的依赖性的系统研究提供了一种产生极快色度响应的系统。此外,使用5个核苷酸的最佳鞋头长度,在广泛的环境温度范围内,目标触发的拆卸迅速。使用此突出系统,可以在室温下10分钟之内简单可视化低picomole量的目标DNA。

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