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DNA 瓦片和入侵堆积引物辅助 CRISPR-Cas12a 多重扩增系统,用于基于熵的电化学检测具有可调灵敏度的 microRNA。

DNA Tile and Invading Stacking Primer-Assisted CRISPR-Cas12a Multiple Amplification System for Entropy-Driven Electrochemical Detection of MicroRNA with Tunable Sensitivity.

机构信息

Key Laboratory of Interfacial Reaction & Sensing Analysis in Universities of Shandong, School of Chemistry and Chemical Engineering, University of Jinan, Nanxinzhuang West Road, Jinan 250022, P. R. China.

Key Laboratory of Analytical Science and Technology of Hebei Province, College of Chemistry and Materials Science, Hebei University, Baoding 071002, P. R. China.

出版信息

Anal Chem. 2023 Sep 12;95(36):13659-13667. doi: 10.1021/acs.analchem.3c02603. Epub 2023 Aug 25.

DOI:10.1021/acs.analchem.3c02603
PMID:37623910
Abstract

Conventional electrochemical detection of microRNA (miRNA) encounters issues of poor sensitivity and fixed dynamic range. Here, we report a DNA tile and invading stacking primer-assisted CRISPR-Cas12a multiple amplification strategy to construct an entropy-controlled electrochemical biosensor for the detection of miRNA with tunable sensitivity and dynamic range. To amplify the signal, a cascade amplification of the CRISPR-Cas12a system along with invading stacking primer signal amplification (ISPSA) was designed to detect trace amounts of miRNA-31 (miR-31). The target miR-31 could activate ISPSA and produce numerous DNAs, triggering the cleavage of the single-stranded linker probe (LP) that connects a methylene blue-labeled DNA tile with a DNA tetrahedron to form a Y-shaped DNA scaffold on the electrode. Based on the decrease of current, miR-31 can be accurately and efficiently detected. Impressively, by changing the loop length of the LP, it is possible to finely tune the entropic contribution while keeping the enthalpic contribution constant. This strategy has shown a tunable limit of detection for miRNA from 0.31 fM to 0.56 pM, as well as a dynamic range from ∼2200-fold to ∼270,000-fold. Moreover, it demonstrated satisfactory results in identifying cancer cells with a high expression of miR-31. Our strategy broadens the application of conventional electrochemical biosensing and provides a tunable strategy for detecting miRNAs at varying concentrations.

摘要

传统的电化学检测 miRNA(microRNA)会遇到灵敏度差和动态范围固定的问题。在这里,我们报告了一种 DNA 瓦片和入侵堆叠引物辅助的 CRISPR-Cas12a 多重扩增策略,用于构建具有可调灵敏度和动态范围的熵控电化学生物传感器来检测 miRNA。为了放大信号,设计了 CRISPR-Cas12a 系统的级联扩增以及入侵堆叠引物信号扩增(ISPSA)来检测痕量的 miRNA-31(miR-31)。目标 miR-31 可以激活 ISPSA 并产生大量 DNA,触发将亚甲基蓝标记的 DNA 瓦片与 DNA 四面体连接的单链连接探针(LP)的切割,在电极上形成 Y 形 DNA 支架。基于电流的减少,可以准确有效地检测 miR-31。令人印象深刻的是,通过改变 LP 的环长,可以在保持焓贡献不变的情况下精细调整熵贡献。该策略显示出对 miRNA 的可调检测限从 0.31 fM 到 0.56 pM,动态范围从约 2200 倍到约 270,000 倍。此外,它在识别高表达 miR-31 的癌细胞方面取得了令人满意的结果。我们的策略拓宽了传统电化学生物传感的应用,并为检测不同浓度的 miRNA 提供了一种可调策略。

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