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Addition of gold nanoparticles to real-time PCR: effect on PCR profile and SYBR Green I fluorescence

机译:金纳米颗粒添加到实时PCR中:对PCR谱图和SYBR Green I荧光的影响

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摘要

Real-time quantitative polymerase chain reaction (qPCR) is the industry standard technique for the quantitative analysis of nucleic acids due to its unmatched sensitivity and specificity. Optimisation and improvements of this fundamental technique over the past decade have largely consisted of attempts to allow faster and more accurate ramping between critical temperatures by improving assay reagents and the thermal geometry of the PCR chamber. Small gold nanoparticles (Au-NPs) have been reported to improve PCR yield under fast cycling conditions. In this study, we investigated the effect of Au-NPs on optimised real-time qPCR assays by amplifying DNA sequences from genetically modified canola in the presence and absence of 0.9 nM Au-NPs of diameter 12 ± 2nm. Contrary to expectations, we found that Au-NPs altered the PCR amplification profile when using a SYBR Green I detection system due to fluorescence quenching; furthermore, high-resolution melt (HRM) analysis demonstrated that Au-NPs destabilised the double-stranded PCR product. The results indicate that effects on the assay detection system must be carefully evaluated before Au-NPs are included in any qPCR assay.
机译:实时定量聚合酶链反应(qPCR)由于其无与伦比的灵敏度和特异性,是核酸定量分析的行业标准技术。在过去的十年中,对该基本技术的优化和改进主要包括通过改进测定试剂和PCR室的热几何形状,在临界温度之间实现更快,更准确的升温的尝试。据报道,小金纳米粒子(Au-NPs)在快速循环条件下可提高PCR产量。在这项研究中,我们通过在存在和不存在直径为12±2nm的0.9 nM Au-NP的情况下,从转基因油菜中扩增DNA序列,研究了Au-NP在优化的实时qPCR分析中的作用。与预期相反,我们发现当使用SYBR Green I检测系统时,由于荧光猝灭,Au-NP改变了PCR扩增曲线。此外,高分辨率熔解(HRM)分析表明Au-NPs使双链PCR产物不稳定。结果表明,在任何qPCR分析中都包含Au-NP之前,必须仔细评估对分析检测系统的影响。

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