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采用双特异性核酸酶和 MoS 纳米片检测血浆外泌体 microRNA 进行肺癌诊断。

In situ detection of plasma exosomal microRNA for lung cancer diagnosis using duplex-specific nuclease and MoS nanosheets.

机构信息

College of Public Health, Zhengzhou University, Zhengzhou 450001, China.

出版信息

Analyst. 2021 Mar 21;146(6):1924-1931. doi: 10.1039/d0an02193h. Epub 2021 Jan 25.

DOI:10.1039/d0an02193h
PMID:33491014
Abstract

MicroRNAs (miRNAs) encapsulated in tumor-derived exosomes are becoming ideal biomarkers for the early diagnosis and prognosis of lung cancer. However, the accuracy and sensitivity are often hampered by the extraction process of exosomal miRNA using traditional methods. Herein, this study developed a fluorogenic quantitative detection method for exosomal miRNA using the fluorescence quenching properties of molybdenum disulfide (MoS) nanosheets and the enzyme-assisted signal amplification properties of duplex-specific nuclease (DSN). First, a fluorescently-labeled nucleic acid probe was used to hybridize the target miRNA to form a DNA/RNA hybrid structure. Under the action of the DSN, the DNA single strand in the DNA/RNA hybrid strand was selectively digested into smaller oligonucleotide fragments. At the same time, the released miRNA target triggers the next reaction cycle, so as to achieve signal amplification. Then, MoS was used to selectively quench the fluorescence of the undigested probe leaving the fluorescent signal of the fluorescently-labeled probe fragments. The fluorometric signals for miRNA-21 had a maximum excitation/emission wavelength of 488/518 nm. Most importantly, the biosensor was then applied for the accurate quantitative detection of miRNA-21 in exosome lysates extracted from human plasma and this method was able to successfully distinguish lung cancer patients from healthy people. This biosensor provides a simple, rapid, and a highly specific quantitative method for exosomal miRNA and has promising potential to be used in the early diagnosis of lung cancer.

摘要

微小 RNA(miRNAs)包裹在肿瘤衍生的外泌体中,成为肺癌早期诊断和预后的理想生物标志物。然而,外泌体 miRNA 的传统提取方法往往会影响其准确性和灵敏度。在此,本研究利用二硫化钼(MoS)纳米片的荧光猝灭特性和双链特异性核酸酶(DSN)的酶辅助信号放大特性,开发了一种用于外泌体 miRNA 的荧光定量检测方法。首先,用荧光标记的核酸探针与靶 miRNA 杂交形成 DNA/RNA 杂合结构。在 DSN 的作用下,DNA/RNA 杂合链中的 DNA 单链被选择性地消化成较小的寡核苷酸片段。同时,释放的 miRNA 靶触发下一个反应循环,从而实现信号放大。然后,MoS 选择性猝灭未被消化的探针的荧光,从而留下荧光标记探针片段的荧光信号。miRNA-21 的荧光信号具有最大激发/发射波长为 488/518nm。最重要的是,该生物传感器随后被应用于从人血浆中提取的外泌体裂解物中 miRNA-21 的准确定量检测,该方法能够成功地区分肺癌患者和健康人。该生物传感器为外泌体 miRNA 的简单、快速和高特异性定量方法提供了新的思路,有望用于肺癌的早期诊断。

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