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基于二聚体分子信标的分子内链置换扩增可实现 miRNA 的稳健分析。

Dimeric-molecular beacon based intramolecular strand displacement amplification enables robust analysis of miRNA.

机构信息

Department of Clinical Laboratory, Jiujiang City Key Laboratory of Cell Therapy, Jiujiang NO.1 People's Hospital, Jiujiang, 332000, China.

College of Biological, Chemical Science and Engineering, Jiaxing University, Jiaxing, 314001, China.

出版信息

Talanta. 2024 Dec 1;280:126778. doi: 10.1016/j.talanta.2024.126778. Epub 2024 Aug 25.

DOI:10.1016/j.talanta.2024.126778
PMID:39191109
Abstract

Given the critical role of miRNAs in regulating gene expression and their potential as biomarkers for various diseases, accurate and sensitive miRNA detection is essential for early diagnosis and monitoring of conditions such as cancer. In this study, we introduce a dimeric molecular beacon (Di-MB) based isothermal strand displacement amplification (ISDA) system (Di-MB-ISDA) for enhanced miRNA detection. The Di-MB system is composed of two monomeric MBs (Mono-MBs) connected by a double-stranded DNA linker with single-stranded sequences in the middle, facilitating binding with the flexible arms of the Mono-MBs. This design forms a compact, high-density structure, significantly improving biostability against nuclease degradation. In the absence of target miRNA, the Di-MB maintains its stable structure. When target miRNA is present, it binds to the stem-loop regions, causing the hairpin structure to unfold and expose the stem sequences. These sequences serve as templates for the built-in primers, triggering DNA replication through an intramolecular recognition mechanism. This spatial confinement effect accelerates the strand displacement reaction, allowing the target miRNA to initiate additional reaction cycles and amplify the detection signal. The Di-MB-ISDA system addresses key challenges such as poor biostability and limited sensitivity seen in traditional methods. By enhancing biostability and optimizing reaction conditions, this system demonstrates robust performance for miRNA detection with a detection limit of 100 pM. The findings highlight the potential of Di-MB-ISDA for sensitive and accurate miRNA analysis, paving the way for its application in biomedical study and disease diagnosis in complex biological samples.

摘要

鉴于 miRNAs 在调控基因表达中的关键作用及其作为各种疾病生物标志物的潜力,准确、灵敏的 miRNA 检测对于癌症等疾病的早期诊断和监测至关重要。在本研究中,我们引入了一种基于二聚体分子信标(Di-MB)的等温链置换扩增(ISDA)系统(Di-MB-ISDA),用于增强 miRNA 的检测。Di-MB 系统由两个单体分子信标(Mono-MB)通过双链 DNA 连接子连接而成,连接子中间具有单链序列,有利于与 Monomer 的柔性臂结合。这种设计形成了一个紧凑、高密度的结构,显著提高了对核酸酶降解的生物稳定性。在没有靶标 miRNA 的情况下,Di-MB 保持其稳定的结构。当存在靶标 miRNA 时,它与茎环区域结合,导致发夹结构展开并暴露茎序列。这些序列充当内置引物的模板,通过分子内识别机制触发 DNA 复制。这种空间限制效应加速了链置换反应,使靶标 miRNA 能够启动额外的反应循环并放大检测信号。Di-MB-ISDA 系统解决了传统方法中存在的生物稳定性差和灵敏度有限等关键挑战。通过增强生物稳定性和优化反应条件,该系统在 miRNA 检测方面表现出了稳健的性能,检测限为 100 pM。研究结果表明,Di-MB-ISDA 具有用于灵敏和准确的 miRNA 分析的潜力,为其在复杂生物样本中的生物医学研究和疾病诊断中的应用铺平了道路。

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