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将微珠 DNA 处理与滚环扩增检测中的光磁检测相结合。

Integration of microbead DNA handling with optomagnetic detection in rolling circle amplification assays.

机构信息

Department of Health Technology, Technical University of Denmark, DTU Health Tech, Building 345C, DK-2800, Kongens Lyngby, Denmark.

Blusense Diagnostics ApS, Fruebjergvej 3, DK-2100, Copenhagen, Denmark.

出版信息

Mikrochim Acta. 2019 Jul 11;186(8):528. doi: 10.1007/s00604-019-3636-x.

DOI:10.1007/s00604-019-3636-x
PMID:31297615
Abstract

Rolling circle amplification (RCA) is a linear isothermal amplification technique that is widely applied in biomolecular assays due to its high specificity. Handling of a target sample using magnetic microbeads (MMBs) in a multi-step assay is appealing as the MMBs enable separation and transportation using an external magnet. Detection of amplicons using optomagnetic measurements of the rotational diffusion properties of magnetic nanoparticles (MNPs) is also appealing as it can be performed on any transparent sample container. Two strategies are described for integration of MMB sample handling in an RCA assay with on-chip optomagnetic detection of the amplification products. The first strategy relies on selective and irreversible release of the amplicons from the MMBs so that the binding of functionalized MNPs to the amplicons can be detected optomagnetically. The second strategy relies on the incorporation of MNPs into RCA products during RCA, followed by their separation on MMBs and subsequent optomagnetic detection upon release from the RCA products. Using MMB handling of RCA steps, the limits of detection (LODs) for a synthetic DNA target representative of Victoria Influenza type B were found to be between 4 and 20 pM with total assay times between 2 and 2.5 h. Without magnetic microbead sample handling, the LOD was 200 fM. The findings provide deeper insight into the use of magnetic microbeads as solid substrates to handle a DNA target for integration of RCA as well as other DNA-based assays. Graphical Abstract Schematic illustration of magnetic microbeads transporting a DNA target through the steps in a rolling circle amplification assay. Optomagnetic measurements detect the binding of magnetic nanoparticles to amplicons released from microbeads (top) or the pH-induced release of magnetic nanoparticles trapped in amplicons (bottom).

摘要

滚环扩增(RCA)是一种线性等温扩增技术,由于其高特异性,广泛应用于生物分子分析。在多步分析中使用磁性微球(MMB)处理靶样品很有吸引力,因为 MMB 可以使用外部磁铁进行分离和输送。使用磁纳米粒子(MNP)的旋转扩散特性的光磁测量来检测扩增子也很有吸引力,因为它可以在任何透明样品容器上进行。描述了两种将 MMB 样品处理集成到 RCA 测定中的策略,并对扩增产物进行片上光磁检测。第一种策略依赖于从 MMB 上选择性和不可逆地释放扩增子,以便可以光磁检测功能化 MNP 与扩增子的结合。第二种策略依赖于在 RCA 过程中将 MNP 掺入 RCA 产物中,然后在 MMB 上进行分离,随后从 RCA 产物中释放出来进行光磁检测。使用 MMB 处理 RCA 步骤,检测到维多利亚乙型流感的合成 DNA 靶标的检测限(LOD)在 4 到 20 pM 之间,总分析时间在 2 到 2.5 小时之间。没有磁性微球样品处理,LOD 为 200 fM。这些发现为使用磁性微球作为固体基底处理 DNA 靶标以整合 RCA 以及其他基于 DNA 的测定提供了更深入的了解。 摘要图 磁性微球通过滚环扩增测定中的步骤运输 DNA 靶标的示意图。光磁测量检测从微球中释放的磁纳米粒子与扩增子的结合(顶部)或捕获在扩增子中的磁纳米粒子的 pH 诱导释放(底部)。

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