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荧光适体传感器用于可卡因的链替代扩增检测。

Fluorescence aptameric sensor for strand displacement amplification detection of cocaine.

机构信息

State Key Laboratory for Chemo/Biosensing and Chemometrics, College of Chemistry and Chemical Engineering, Hunan University, Changsha 410082, P. R. China.

出版信息

Anal Chem. 2010 Feb 15;82(4):1358-64. doi: 10.1021/ac902416u.

Abstract

A new fluorescence method based on aptamer-target interactions has been developed for cocaine detection with target-induced strand displacement. Here we describe new probes, the hairpin-probe and the single strand-probe (ss-probe), that possess two recognition sequences of cocaine aptamer. In the presence of cocaine, both probes would associate with the target to form a tripartite complex. The conformational change in the hairpin-probe causes the opening of a hairpin structure and the hybridization to primer. With polymerase and the dNTPs, the replication of the single-stranded domain of hairpin-probe triggers the process of primer extension. When the hairpin-probe is converted into a fully double-stranded form, the ss-probe and cocaine are displaced to bind another hairpin-probe and initiate new amplification cycles. Fluorescence signal generation would be observed upon SYBR Green I intercalating into the new DNA double helix. The new protocol design permits detection of as low as 2 nM cocaine in a closed tube, offering a convenient approach for a homogeneous assay. Compared with previously reported cocaine aptameric sensors, our new method is highly sensitive, selective, and economical.

摘要

一种基于适体-靶相互作用的新荧光法已被开发用于可卡因检测,其基于靶诱导的链位移。在这里,我们描述了两种新的探针,发夹探针和单链探针(ss-probe),它们都具有可卡因适体的两个识别序列。在可卡因存在的情况下,这两种探针都会与靶标结合形成三部分复合物。发夹探针的构象变化导致发夹结构的打开和与引物的杂交。在聚合酶和 dNTPs 的作用下,发夹探针的单链区域的复制引发引物延伸过程。当发夹探针转化为完全双链形式时,ss-probe 和可卡因被置换以结合另一个发夹探针并引发新的扩增循环。当 SYBR Green I 插入新的 DNA 双链时,会观察到荧光信号的产生。新的方案设计允许在封闭管中检测低至 2 nM 的可卡因,提供了一种用于均相测定的简便方法。与以前报道的可卡因适体传感器相比,我们的新方法具有高灵敏度、选择性和经济性。

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