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基于长探针和短探针的循环扩增的高效液相色谱法用于多种 microRNAs 的高灵敏度检测。

Highly Sensitive Detection of Multiple MicroRNAs by High-Performance Liquid Chromatography Coupled with Long and Short Probe-Based Recycling Amplification.

机构信息

School of Environmental and Chemical Engineering, Jiangsu University of Science and Technology, Zhenjiang 212003, Jiangsu Province, People's Republic of China.

School of Grain Science and Technology, Jiangsu University of Science and Technology, Zhenjiang 212003, Jiangsu Province, People's Republic of China.

出版信息

Anal Chem. 2020 Apr 7;92(7):5033-5040. doi: 10.1021/acs.analchem.9b05301. Epub 2020 Mar 20.

Abstract

This report demonstrated the utility of high-performance liquid chromatography (HPLC)-fluorescence detection for selective separation and sensitive quantification of multiple microRNAs (miRNAs). A duplex specific nuclease (DSN)-assisted target recycling amplification strategy was developed to enhance the signals of miRNAs, which alleviates the low sensitivity of conventional HPLC to nucleic acids. To separate the signals of different miRNAs, DNA probes with different lengths and base sequences were immobilized on magnetic beads. The application of an effective magnetic separation minimized the background signal and extended the dynamic range. This assay achieved a limit of detection of 0.39 fM for miRNA-122, 0.30 fM for miRNA-155, and 0.26 fM for miRNA-21, respectively. The proposed assay was successfully applied to detect simultaneously miRNA-122, miRNA-155, and miRNA-21 in serum samples from healthy persons and cervical cancer patients, and the results were then compared with those of quantitative real-time-polymerase chain reaction amplification.

摘要

本报告展示了高效液相色谱(HPLC)-荧光检测在选择性分离和灵敏定量多种 microRNAs(miRNAs)方面的应用。开发了一种双链特异性核酸酶(DSN)辅助的靶标循环扩增策略来增强 miRNAs 的信号,这缓解了常规 HPLC 对核酸灵敏度低的问题。为了分离不同 miRNAs 的信号,将具有不同长度和碱基序列的 DNA 探针固定在磁珠上。有效的磁分离应用最小化了背景信号并扩展了动态范围。该测定法分别对 miRNA-122 实现了 0.39 fM 的检测限、对 miRNA-155 实现了 0.30 fM 的检测限、对 miRNA-21 实现了 0.26 fM 的检测限。该方法成功应用于检测健康人和宫颈癌患者血清样本中的 miRNA-122、miRNA-155 和 miRNA-21,并将结果与定量实时聚合酶链反应扩增的结果进行了比较。

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