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Engineered Janus probes modulate nucleic acid amplification to expand the dynamic range for direct detection of viral genomes in one microliter crude serum samples

机译:工程Janus探针可调节核酸扩增,扩大动态范围,可直接检测一微升粗血清样品中的病毒基因组

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The viral genome load in diverse clinical samples varies over several orders of magnitude (e.g. 1–104 copies per μL), thus a dynamic range-extended and sensitive analysis method is highly desired. However, existing well-developed nucleic acid amplification systems always suffer from either a limited dynamic range or modest sensitivity for analysis of these samples. Herein, we propose a general engineered Janus probe to modulate the thermodynamics and kinetic properties of the amplification reaction. Through rational regulation, the Janus system improves the performance by both reducing the background and enhancing the signal, expanding the operative dynamic range by 2 orders of magnitude. This proposed approach achieves a detection limit for hepatitis B virus (HBV) DNA of down to 3 copies and can be successfully applied for direct quantification of the HBV genome in one microliter crude serum samples without any pretreatment. The results are consistent with clinical diagnosis and hold considerable potential to discriminate healthy volunteers and patients at different disease stages. Whereas, following the same operation, the representative well-developed system provided serious false-negative results using such trace amounts of samples from clinically confirmed positive patients.
机译:不同临床样品中病毒基因组的负载量变化了几个数量级(每μL例如 1–10 4 个拷贝),因此动态范围非常需要扩展和灵敏的分析方法。然而,现有的发达的核酸扩增系统对于这些样品的分析总是受到有限的动态范围或中等灵敏度的困扰。在本文中,我们提出了一种通用的Janus探针来调节扩增反应的热力学和动力学性质。通过合理的调节,Janus系统通过降低背景和增强信号,将操作动态范围扩大2个数量级来提高性能。该方法可将乙型肝炎病毒(HBV)DNA的检出限降低至3份,并且无需任何预处理即可成功用于一微升粗血清样品中HBV基因组的直接定量。结果与临床诊断相符,并且具有区分健康志愿者和处于不同疾病阶段的患者的巨大潜力。而经过相同的操作,具有代表性的发达系统使用来自临床确诊阳性患者的痕量样品提供了严重的假阴性结果。

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