Sample-to-answer centrifugal microfluidic droplet PCR platform for quantitation of viral load

IF 6.1 2区工程技术 Q1 BIOCHEMICAL RESEARCH METHODS

Lab on a Chip Pub Date : 2024-09-11 DOI:10.1039/d4lc00533c

Lidija Malic, Liviu Clime, Byeong-Ui Moon, Christina Nassif, Dillon Da Fonte, Daniel Brassard, Ljuboje Lukic, Matthias Geissler, Keith J Morton, Denis Charlebois, Teodor Veres

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引用次数: 0

Abstract

Droplet digital polymerase chain reaction (ddPCR) stands out as a highly sensitive diagnostic technique that is gaining traction in infectious disease diagnostics due to its ability to quantitate very low numbers of viral gene copies. By partitioning the sample into thousands of droplets, ddPCR enables precise and absolute quantification without relying on a standard curve. Despite these advantages, current ddPCR systems often exhibit relatively low levels of integration, and the analytical process remains dependent on elaborate workflows for up-front sample preparation. Here, we introduce a fully-integrated system seamlessly combining viral lysis, nucleic acid extraction, emulsification, reverse transcription (RT) ddPCR, and fluorescence readout within a sample-to-answer format. The system comprises a disposable microfluidic cartridge housing buffers and reagents required for the assay, and a centrifugal platform that allows for pneumatic actuation of liquids during rotation, enabling automation of the workflow. Highly monodisperse droplets (~50 µm in diameter) are produced using centrifugal step emulsification and automatically transferred to an integrated heating module for amplification, thus limiting shear-induced merging of droplets during thermal cycling. The platform is equipped with a miniature fluorescence microscope enabling on-chip automated read-out of droplets after RT-ddPCR. As a use case, we demonstrate sample-to-answer detection of SARS-CoV-2 N and E genes, along with RNase P endogenous reference, using hydrolysis probes and multiplexed amplification within single droplets, achieving a low limit of detection of 0.1 copy/µL. We also tested 14 nasopharyngeal swab specimens from patients and were able to accurately distinguish positive and negative SARS-CoV-2 samples with 100% accuracy, surpassing results obtained by conventional real-time amplification. Being fully integrated, the assay facilitates potential deployment outside of specialized laboratories, opening new possibilities for quantitative, high-sensitivity detection of pathogens.

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用于病毒载量定量的样本到答案离心微流控液滴 PCR 平台

液滴数字聚合酶链反应（ddPCR）是一种高灵敏度的诊断技术，由于它能够定量检测极少量的病毒基因拷贝，因此在传染病诊断领域越来越受到重视。通过将样本分成数千个液滴，ddPCR 无需依赖标准曲线即可实现精确和绝对的定量。尽管具有这些优势，但目前的 ddPCR 系统通常集成度较低，分析过程仍然依赖于前期样品制备的复杂工作流程。在此，我们介绍一种完全集成的系统，它将病毒裂解、核酸提取、乳化、反转录 (RT) ddPCR 和荧光读数无缝地结合在一起，并采用从样品到答案的格式。该系统由一个一次性微流控芯片盒和一个离心平台组成，前者装有检测所需的缓冲液和试剂，后者可在旋转过程中对液体进行气动驱动，从而实现工作流程的自动化。利用离心阶跃乳化产生高单分散液滴（直径约 50 微米），并自动转移到集成加热模块进行扩增，从而限制了热循环过程中剪切引起的液滴合并。该平台配备了微型荧光显微镜，可在 RT-ddPCR 后在芯片上自动读出液滴。作为一个使用案例，我们展示了使用水解探针和单液滴内的多重扩增对 SARS-CoV-2 N 和 E 基因以及 RNase P 内源性参考进行的样本到答案检测，实现了 0.1 拷贝/微升的低检测限。我们还检测了 14 份患者鼻咽拭子标本，能够准确区分 SARS-CoV-2 阳性和阴性样本，准确率达到 100%，超过了传统实时扩增的结果。由于该检测方法是完全集成的，因此可以在专业实验室以外的地方使用，为定量、高灵敏度地检测病原体提供了新的可能性。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

Lab on a Chip 工程技术-化学综合

CiteScore

11.10

自引率

8.20%

发文量

434

审稿时长

2.6 months

期刊介绍： Lab on a Chip is the premiere journal that publishes cutting-edge research in the field of miniaturization. By their very nature, microfluidic/nanofluidic/miniaturized systems are at the intersection of disciplines, spanning fundamental research to high-end application, which is reflected by the broad readership of the journal. Lab on a Chip publishes two types of papers on original research: full-length research papers and communications. Papers should demonstrate innovations, which can come from technical advancements or applications addressing pressing needs in globally important areas. The journal also publishes Comments, Reviews, and Perspectives.