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基于硅胶珠的微流控芯片与集成光电二极管的快速捕获和检测技术,可在飞摩尔范围内对滚环扩增产物进行检测。

Silica bead-based microfluidic device with integrated photodiodes for the rapid capture and detection of rolling circle amplification products in the femtomolar range.

机构信息

Instituto de Engenharia de Sistemas e Computadores - Microsistemas e Nanotecnologias (INESC MN) and IN - Institute of Nanoscience and Nanotechnology, Lisbon, Portugal; IBB - Institute for Bioengineering and Biosciences, Instituto Superior Técnico, Universidade de Lisboa, Lisbon, Portugal.

Science for Life Laboratory, Department of Biochemistry and Biophysics, Stockholm University, SE-171 65 Solna, Sweden.

出版信息

Biosens Bioelectron. 2019 Mar 1;128:68-75. doi: 10.1016/j.bios.2018.12.004. Epub 2018 Dec 18.

DOI:10.1016/j.bios.2018.12.004
PMID:30634076
Abstract

The rapid and sensitive detection of specific nucleic acid sequences at the point-of-care (PoC) is becoming increasingly in demand for a variety of emergent biomedical applications ranging from infectious disease diagnostics to the screening of antimicrobial resistance. To meet such demand, considerable efforts have been invested towards the development of portable and integrated analytical devices combining microfluidics with miniaturized signal transducers. Here, we demonstrate the combination of rolling circle amplification (RCA)-based nucleic acid amplification with an on-chip size-selective trapping of amplicons on silica beads (~8 nL capture chamber) coupled with a thin-film photodiode (200 × 200 µm area) fluorescence readout. Parameters such as the flow rate of the amplicon solution and trapping time were optimized as well as the photodiode measurement settings, providing minimum detection limits below 0.5 fM of targeted nucleic acids and requiring only 5 μL of pre-amplified sample. Finally, we evaluated the analytical performance of our approach by benchmarking it against a commercial instrument for RCA product (RCP) quantification and further investigated the effect of the number of RCA cycles and elongation times (ranging from 10 to 120 min). Moreover, we provide a demonstration of the application for diagnostic purposes by detecting RNA from influenza and Ebola viruses, thus highlighting its suitability for integrated PoC systems.

摘要

在即时检测(Point-of-care,PoC)中,对特定核酸序列进行快速、灵敏的检测,对于各种新兴的生物医学应用(从传染病诊断到抗生素耐药性筛查)的需求日益增长。为了满足这一需求,研究人员投入了相当大的努力,开发了将微流控技术与微型信号传感器相结合的便携式集成分析设备。在这里,我们展示了基于滚环扩增(Rolling circle amplification,RCA)的核酸扩增与在芯片上对扩增子进行基于大小的选择性捕获(~8 nL 捕获室)相结合的方法,该方法与薄膜光电二极管(200×200 µm 面积)荧光读出相耦合。我们优化了扩增物溶液的流速和捕获时间等参数,以及光电二极管的测量设置,从而实现了针对目标核酸的最低检测限低于 0.5 fM,并且仅需 5 µL 预扩增样品。最后,我们通过将其与商用 RCA 产物(RCA product,RCP)定量的仪器进行基准测试,评估了我们方法的分析性能,并进一步研究了 RCA 循环数和延伸时间(范围从 10 到 120 分钟)的影响。此外,我们通过检测流感病毒和埃博拉病毒的 RNA 来演示其在诊断中的应用,从而突出了其在集成 PoC 系统中的适用性。

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