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基于 CRISPR/Cas12a 和金纳米棒的诊断生物传感器的设计,实现了 miRNA 的直接、快速和灵敏检测。

Designing a CRISPR/Cas12a- and Au-Nanobeacon-Based Diagnostic Biosensor Enabling Direct, Rapid, and Sensitive miRNA Detection.

机构信息

College of Chemistry and Chemical Engineering, Central South University, Changsha 410083, P. R. China.

出版信息

Anal Chem. 2022 May 3;94(17):6566-6573. doi: 10.1021/acs.analchem.2c00401. Epub 2022 Apr 22.

Abstract

Direct, rapid, sensitive, and selective detection of nucleic acids in complex biological fluids is crucial for medical early diagnosis. We herein combine the trans-cleavage ability of clustered regularly interspaced short palindromic repeats (CRISPR)/Cas12a with Au-nanobeacon to establish a CRISPR-based biosensor, providing rapid miRNA detection with high speed and attomolar sensitivity. In this strategy, we first report that the trans-cleavage activity of CRISPR/cas12a, which was previously reported to be triggered only by target ssDNA or dsDNA, can be activated by the target miRNA directly. Therefore, this method is direct, i.e., does not need the conversion of miRNA into its complementary DNA (cDNA). Meanwhile, as compared to the traditional ssDNA reporters and molecular beacon (MB) reporters, the Au-nanobeacon reporters exhibit improved reaction kinetics and sensitivity. In this assay, the miRNA-21 could be detected with very high sensitivity in only 5 min. Finally, the proposed strategy enables rapid, sensitive, and selective miRNA determination in complex biological samples, providing a potential tool for medical early diagnosis.

摘要

直接、快速、敏感和选择性地检测复杂生物流体中的核酸对于医学早期诊断至关重要。我们在此将成簇规律间隔短回文重复(CRISPR)/Cas12a 的转切割能力与 Au-纳米信标结合,建立了基于 CRISPR 的生物传感器,可实现快速 miRNA 检测,具有高速度和皮摩尔灵敏度。在该策略中,我们首次报道了 CRISPR/cas12a 的转切割活性,先前报道该活性仅被靶 ssDNA 或 dsDNA 触发,可被靶 miRNA 直接激活。因此,该方法是直接的,即不需要将 miRNA 转化为其互补 DNA(cDNA)。同时,与传统的 ssDNA 报告子和分子信标(MB)报告子相比,Au-纳米信标报告子表现出改进的反应动力学和灵敏度。在该测定中,miRNA-21 仅在 5 分钟内即可被非常高灵敏度地检测到。最后,该策略能够在复杂的生物样品中快速、灵敏和选择性地测定 miRNA,为医学早期诊断提供了一种潜在的工具。

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