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在用于即时检测系统的集成微流控装置中高效富集游离靶序列。

Efficient enrichment of free target sequences in an integrated microfluidic device for point-of-care detection systems.

机构信息

CEIT-Basque Research and Technology Alliance (BRTA), Manuel Lardizabal 15, 20018 Donostia, San Sebastián, Spain; Universidad de Navarra, Tecnun, Manuel Lardizabal 13, 20018 Donostia, San Sebastián, Spain.

CEIT-Basque Research and Technology Alliance (BRTA), Manuel Lardizabal 15, 20018 Donostia, San Sebastián, Spain; Universidad de Navarra, Tecnun, Manuel Lardizabal 13, 20018 Donostia, San Sebastián, Spain; Group of Bioengineering in Regeneration and Cancer, Biogipuzkoa Health Research Institute, San Sebastian, Spain.

出版信息

Nanomedicine. 2024 Oct;61:102771. doi: 10.1016/j.nano.2024.102771. Epub 2024 Jul 2.

DOI:10.1016/j.nano.2024.102771
PMID:38960366
Abstract

Nucleic acid biomarker detection has great importance in the diagnosis of disease, the monitoring of disease progression and the classification of patients according to treatment decision making. Nucleic acid biomarkers found in the blood of patients have generated a lot of interest due to the possibility of being detected non-invasively which makes them ideal for monitoring and screening tests and particularly amenable to point-of-care (POC) or self-testing. A major challenge to POC molecular diagnostics is the need to enrich the target to optimise detection. In this work, we describe a microfabricated device for the enrichment of short dsDNA target sequences, which is especially valuable for potential detection methods, as it improves the probability of effectively detecting the target in downstream analyses. The device integrated a heating element and a temperature sensor with a microfluidic chamber to carry out the denaturation of the dsDNA combined with blocking-probes to enrich the target. This procedure was validated by fluorescence resonance energy transfer (FRET) technique, labelling DNA with a fluorophore and a quencher. As proof of concept, a 23-mer long dsDNA sequence corresponding to the L858R mutation of the EGFR gene was used. The qualitative results obtained determined that the most optimal blocking rate was obtained with the incorporation of 11/12-mer blocking-probes at a total concentration of 6 μM. This device is a powerful DNA preparation tool, which is an indispensable initial step for subsequent detection of sequences via nucleic acid hybridisation methods.

摘要

核酸生物标志物检测在疾病诊断、疾病进展监测以及根据治疗决策对患者进行分类方面具有重要意义。由于可以非侵入性地检测到患者血液中的核酸生物标志物,因此引起了人们的极大兴趣,这使得它们非常适合用于监测和筛查试验,尤其适合于即时检测 (POC) 或自我检测。POC 分子诊断的一个主要挑战是需要富集目标以优化检测。在这项工作中,我们描述了一种用于富集短 dsDNA 靶序列的微加工设备,这对于潜在的检测方法特别有价值,因为它提高了在下游分析中有效检测目标的概率。该设备集成了加热元件和温度传感器以及微流控室,以进行 dsDNA 的变性,并结合阻断探针来富集目标。该过程通过荧光共振能量转移 (FRET) 技术进行了验证,该技术通过荧光团和猝灭剂对 DNA 进行标记。作为概念验证,使用了对应于 EGFR 基因 L858R 突变的 23 个碱基对长的 dsDNA 序列。定性结果确定,在总浓度为 6 μM 时,掺入 11/12 个碱基对的阻断探针可获得最佳阻断率。该设备是一种强大的 DNA 制备工具,是随后通过核酸杂交方法检测序列不可或缺的初始步骤。

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