A strategy for electrochemical biosensing based on dendritic HCR amplification for detection of RNA m5C and m6A methylation

IF 6 2区 化学 Q1 CHEMISTRY, ANALYTICAL Analytica Chimica Acta Pub Date : 2025-02-13 DOI:10.1016/j.aca.2025.343796
Mimi Li , Lina Wang , Yue Hu , Yi Liu , Shuang Xu , Kexing Peng , Chenghong Li , Hui Huang , Lichao Fang , Lulu Li , Huamin Liu , Xiaolong Wang , Junsong Zheng
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Abstract

Sensitive and efficient detection of RNA methylation sites is considered an integral part of epigenetic assessment. Contrary to previous studies on the detection of RNA m5C or m6A methylation alone, this study innovatively designed a biosensor capable of detecting RNA m5C or m6A methylation at the same time. Substances with specific electrochemical reactions such as ferrocene (FC) or methylene blue (MB) were modified onto the hairpin probe. When the hairpin probe was activated under specific conditions, it triggered a dendritic nonlinear hybridization chain reaction (HCR), which resulted in signal amplification. Gold (Au) and iron tetraoxide (Fe3O4) composite nanomaterials were employed as the linking materials: the carboxylated ends of Fe3O4 were connected to an antibody that specifically recognizes the m5C and m6A methylation sites, while Au nanoparticle ends adhering to the carboxylated Fe3O4 surface are connected to the HCR enhanced signal amplifier. The m5C antibody was linked to Fc-containing HCR amplification products by this material, and similarly, the m6A antibody was linked to MB-containing amplifiers. Thus, the dandelion complex, a multifunctional body with methyl recognition and signal amplification, was formed. The capture probe immobilized on the surface of the gold electrode by Au–S recognized the target RNA sequence by base complementary pairing. Upon addition of the dandelion complex, due to its multi-functionality, the amplified signals were carried to the electrode by the antigen-antibody recognition mechanism, generating a current signal. The positions and heights of the current signal peaks enabled rapid determination of target RNA methyl modification sites and their abundance. The detection limits of this biosensor for RNA m5C and m6A were 4.68 × 10−16 M and 1.10 × 10−15 M, respectively, and the linear range was from 10−15 mol/L to 10−8 mol/L. The sensor developed in this study has the advantages of cost-effectiveness, ease of fabrication, and fast response time, and has the potential to be promoted for RNA methylation detection.

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基于树突状HCR扩增检测RNA m5C和m6A甲基化的电化学生物传感策略
敏感和有效的检测RNA甲基化位点被认为是表观遗传评估的一个组成部分。与以往仅检测RNA m5C或m6A甲基化的研究不同,本研究创新性地设计了一种能够同时检测RNA m5C或m6A甲基化的生物传感器。二茂铁(FC)或亚甲基蓝(MB)等具有特定电化学反应的物质被修饰到发夹探针上。当发夹探针在特定条件下被激活时,它会引发树枝状非线性杂交链反应(HCR),导致信号放大。采用金(Au)和四氧化二铁(Fe3O4)复合纳米材料作为连接材料:将Fe3O4的羧基化端连接到特异性识别m5C和m6A甲基化位点的抗体上,而粘附在羧基化Fe3O4表面的金纳米颗粒端连接到HCR增强信号放大器上。m5C抗体通过该材料连接到含fc的HCR扩增产物,同样,m6A抗体连接到含mb的扩增产物。这样,蒲公英复合物,一个具有甲基识别和信号放大的多功能体,就形成了。用Au-S固定在金电极表面的捕获探针通过碱基互补配对识别靶RNA序列。添加蒲公英复合物后,由于蒲公英复合物的多功能性,放大后的信号被抗原-抗体识别机制携带到电极上,产生电流信号。当前信号峰的位置和高度可以快速确定目标RNA甲基修饰位点及其丰度。该生物传感器对RNA m5C和m6A的检出限分别为4.68×10-16 M和1.10×10-15 M,线性范围为10-15 mol/L ~ 10-8 mol/L。本研究开发的传感器具有成本效益高、制作方便、响应时间快等优点,在RNA甲基化检测中具有推广应用的潜力。
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ferrous chloride tetrahydrate
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iron chloride hexahydrate
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N-Hydroxy succinimide (NHS)
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1-(3-Dimethylaminopropyl)-3-ethylcarbodiimide hydrochloride (EDC)
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sodium citrate
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chloroauric acid
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anhydrous ethanol
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potassium permanganate
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oleic acid
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sodium hydroxide
来源期刊
Analytica Chimica Acta
Analytica Chimica Acta 化学-分析化学
CiteScore
10.40
自引率
6.50%
发文量
1081
审稿时长
38 days
期刊介绍: Analytica Chimica Acta has an open access mirror journal Analytica Chimica Acta: X, sharing the same aims and scope, editorial team, submission system and rigorous peer review. Analytica Chimica Acta provides a forum for the rapid publication of original research, and critical, comprehensive reviews dealing with all aspects of fundamental and applied modern analytical chemistry. The journal welcomes the submission of research papers which report studies concerning the development of new and significant analytical methodologies. In determining the suitability of submitted articles for publication, particular scrutiny will be placed on the degree of novelty and impact of the research and the extent to which it adds to the existing body of knowledge in analytical chemistry.
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