链置换扩增触发的3D DNA滚环辅助CRISPR/Cas12a电化学发光级联信号放大用于灵敏检测Ec-16S rDNA
Strand displacement amplification triggered 3D DNA roller assisted CRISPR/Cas12a electrochemiluminescence cascaded signal amplification for sensitive detection of Ec-16S rDNA.
作者信息
Wang Shujing, Liu Yaqi, Liu Ruifang, Xie Li, Yang Hongmei, Ge Shenguang, Yu Jinghua
机构信息
Institute for Advanced Interdisciplinary Research(iAIR), University of Jinan, Jinan, 250022, PR China.
Shandong Provincial Key Laboratory of Radiation Oncology, Cancer Research Center, Shandong Cancer Hospital and Institute, Shandong First Medical University and Shandong Academy of Medical Sciences, Jinan, Shandong, 250117, PR China.
出版信息
Anal Chim Acta. 2024 Feb 22;1291:342213. doi: 10.1016/j.aca.2024.342213. Epub 2024 Jan 3.
BACKGROUND
Escherichia coli can cause gastrointestinal infection, urinary tract infection and other infectious diseases. Accurate detection of Escherichia coli 16S rDNA (Ec-16S rDNA) in clinical practice is of great significance for the identification and treatment of related diseases. At present, there are various types of sensors that can achieve accurate detection of Ec-16S rDNA. Electrochemiluminescence (ECL) has attracted considerable attention from researchers, which causes excellent performance in bioanalysis. Based on the previous research, it is significance to develop a novel, sensitive and efficient ECL biosensor.
RESULTS
In this work, an ECL biosensor for the detection of Ec-16S rDNA was constructed by integrating CRISPR/Cas12a technology with the cascade signal amplification strategy consisting of strand displacement amplification (SDA) and dual-particle three-dimensional (3D) DNA rollers. The amplification products of SDA triggered the operation of the DNA rollers, and the products generated by the DNA rollers activated CRISPR/Cas12a to cleave the signal probe, thereby realizing the change of the ECL signal. The cascade amplification strategy realized the exponential amplification of the target signal and greatly improved the sensitivity. Manganese dioxide nanoflowers (MnO NFs) as a co-reaction promoter effectively enhanced the ECL intensity of tin disulfide quantum dots (SnS QDs). A new ternary ECL system (SnS QDs/SO/MnO NFs) was prepared, which made the change of ECL intensity of biosensor more significant. The proposed biosensor had a response range of 100 aM-10 nM and a detection limit of 27.29 aM (S/N = 3).
SIGNIFICANCE AND NOVELTY
Herein, the cascade signal amplification strategy formed by SDA and dual-particle 3D DNA rollers enabled the ECL biosensor to have high sensitivity and low detection limit. At the same time, the cascade signal amplification strategy was integrated with CRISPR/Cas12a to enable the biosensor to efficiently detect the target. It can provide a new idea for the detection of Ec-16S rDNA in disease diagnosis and clinical analysis.
背景
大肠杆菌可引起胃肠道感染、尿路感染等传染病。在临床实践中准确检测大肠杆菌16S核糖体DNA(Ec-16S rDNA)对相关疾病的诊断和治疗具有重要意义。目前,有多种类型的传感器可实现对Ec-16S rDNA的准确检测。电化学发光(ECL)引起了研究人员的广泛关注,其在生物分析中表现出优异的性能。基于先前的研究,开发一种新型、灵敏且高效的ECL生物传感器具有重要意义。
结果
在本研究中,通过将CRISPR/Cas12a技术与由链置换扩增(SDA)和双粒子三维(3D)DNA滚环组成的级联信号放大策略相结合,构建了一种用于检测Ec-16S rDNA的ECL生物传感器。SDA的扩增产物触发DNA滚环的运行,DNA滚环产生的产物激活CRISPR/Cas12a以切割信号探针,从而实现ECL信号的变化。级联放大策略实现了目标信号的指数级放大并大大提高了灵敏度。二氧化锰纳米花(MnO NFs)作为共反应促进剂有效增强了二硫化锡量子点(SnS QDs)的ECL强度。制备了一种新的三元ECL体系(SnS QDs/SO/MnO NFs),这使得生物传感器的ECL强度变化更加显著。所提出的生物传感器的响应范围为100 aM-10 nM,检测限为27.29 aM(S/N = 3)。
意义与创新
在此,由SDA和双粒子3D DNA滚环形成的级联信号放大策略使ECL生物传感器具有高灵敏度和低检测限。同时,级联信号放大策略与CRISPR/Cas12a相结合,使生物传感器能够高效检测目标物。它可为疾病诊断和临床分析中Ec-16S rDNA的检测提供新思路。
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