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一步法多重荧光检测 microRNAs 基于双链特异性核酸酶信号放大。

One-step, multiplexed fluorescence detection of microRNAs based on duplex-specific nuclease signal amplification.

机构信息

State Key Laboratory of Bioreactor Engineering, East China University of Science and Technology , Meilong Road 130, Shanghai, 200237, China.

出版信息

J Am Chem Soc. 2012 Mar 21;134(11):5064-7. doi: 10.1021/ja300721s. Epub 2012 Mar 8.

DOI:10.1021/ja300721s
PMID:22394262
Abstract

Traditional molecular beacons, widely applied for detection of nucleic acids, have an intrinsic limitation on sensitivity, as one target molecule converts only one beacon molecule to its fluorescent form. Herein, we take advantage of the duplex-specific nuclease (DSN) to create a new signal-amplifying mechanism, duplex-specific nuclease signal amplification (DSNSA), to increase the detection sensitivity of molecular beacons (Taqman probes). DSN nuclease is employed to recycle the process of target-assisted digestion of Taqman probes, thus, resulting in a significant fluorescence signal amplification through which one target molecule cleaves thousands of probe molecules. We further demonstrate the efficiency of this DSNSA strategy for rapid direct quantification of multiple miRNAs in biological samples. Our experimental results showed a quantitative measurement of sequence-specific miRNAs with the detection limit in the femtomolar range, nearly 5 orders of magnitude lower than that of conventional molecular beacons. This amplification strategy also demonstrated a high selectivity for discriminating differences between miRNA family members. Considering the superior sensitivity and specificity, as well as the multiplex and simple-to-implement features, this method promises a great potential of becoming a routine tool for simultaneously quantitative analysis of multiple miRNAs in tissues or cells, and supplies valuable information for biomedical research and clinical early diagnosis.

摘要

传统的分子信标广泛应用于核酸检测,但由于一个靶标分子只能将一个信标分子转化为荧光形式,因此存在固有灵敏度限制。在此,我们利用双链特异性核酸酶(DSN)创建了一种新的信号放大机制,即双链特异性核酸酶信号放大(DSNSA),以提高分子信标(Taqman 探针)的检测灵敏度。DSN 核酸酶用于回收靶标辅助 Taqman 探针消化的过程,从而通过一个靶标分子切割数千个探针分子实现显著的荧光信号放大。我们进一步证明了这种 DSNSA 策略在生物样品中快速直接定量检测多种 miRNA 的效率。我们的实验结果表明,该方法能够以皮摩尔级的检测限进行序列特异性 miRNA 的定量测量,比传统的分子信标低 5 个数量级。这种扩增策略还表现出区分 miRNA 家族成员差异的高选择性。鉴于其出色的灵敏度和特异性,以及多重性和易于实现的特点,该方法有望成为组织或细胞中同时定量分析多种 miRNA 的常规工具,并为生物医学研究和临床早期诊断提供有价值的信息。

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