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An analytical method to control the surface density and stability of DNA-gold nanoparticles for an optimized biosensor

机译:一种控制DNA-金纳米粒子对优化生物传感器的表面密度和稳定性的分析方法

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摘要

DNA functionalized gold nanoparticles (DNA-AuNPs) have shown great potential for biosensing as they combine the excellent optical properties of gold nanoparticles and the molecular recognition function of DNA. Since the DNA density determines the assay performance and the stability of the conjugate, a precise control of the surface density of DNA-AuNP is crucial for an optimized biosensor. Here we report a simple assay for quantifying multiple unlabeled DNAs on AuNPs. The assay relies on potassium cyanide (KCN) to first dissolve the AuNPs, which then releases surface bound DNA for quantification through a double-stranded DNA dye. Using this analytical quantification method, we investigated several strategies to control the surface density of DNA-AuNPs. Besides the precise control of DNA density, the stability of DNA-AuNPs after conjugation is also important in developing a biosensor with optimal performance. Without proper storing conditions, DNA-AuNPs are unstable and aggregate over time. To overcome this problem, we developed a long-term storage solution to ensure the stability and quality of DNA-AuNPs after conjugation which would benefit any DNA-AuNP-based biosensor.
机译:DNA官能化金纳米颗粒(DNA-AUNP)显示了生物传感的巨大潜力,因为它们结合了金纳米颗粒的优异光学性质和DNA的分子识别功能。由于DNA密度决定了测定性能和缀合物的稳定性,因此对DNA-AUNP的表面密度的精确控制对于优化的生物传感器至关重要。在这里,我们报告了一种简单的测定,用于量化在AUNP上的多个未标记的DNA。测定依赖于氰化钾(KCN)首先溶解αUNP,然后通过双链DNA染料释放表面结合的DNA以定量。使用这种分析量化方法,我们研究了一种控制DNA-AUNP的表面密度的几种策略。除了对DNA密度的精确控制之外,缀合后DNA-AUNP的稳定性在开发具有最佳性能的生物传感器方面也很重要。没有适当的储存条件,DNA-AUNPS随着时间的推移不稳定并且聚集。为了克服这个问题,我们开发了一个长期的存储解决方案,以确保缀合后DNA-AUNP的稳定性和质量,这些缀合后会受益于任何基于DNA-AUNP的生物传感器。

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