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基于点击化学连接辅助杂交结合杂交链式反应信号放大的无酶等温检测微小RNA

Enzyme-free and isothermal detection of microRNA based on click-chemical ligation-assisted hybridization coupled with hybridization chain reaction signal amplification.

作者信息

Oishi Motoi

机构信息

Division of Materials Science, Faculty of Pure and Applied Sciences, University of Tsukuba, 1-1-1 Tennoudai, Tsukuba, Ibaraki, 305-8573, Japan,

出版信息

Anal Bioanal Chem. 2015 May;407(14):4165-72. doi: 10.1007/s00216-015-8629-y. Epub 2015 Mar 31.

DOI:10.1007/s00216-015-8629-y
PMID:25822161
Abstract

An enzyme-free and isothermal microRNA (miRNA) detection method has been developed based on click-chemical ligation-assisted hybridization coupled with hybridization chain reaction (HCR) on magnetic beads (MBs). The click-chemical ligation between an azide-modified probe DNA and a dibenzocyclooctyne-modified probe DNA occurred through the hybridization of target miRNA (miR-141). HCR on MBs was performed by the addition of DNA hairpin monomers (H1 and H2). After magnetic separation and denaturation/rehybridization of HCR products ([H1/H2] n ), the resulting HCR products were analyzed by the fluorescence emitted from an intercalative dye, allowing amplification of the fluorescent signal. The proposed assay had a limit of detection of 0.55 fmol, which was 230-fold more sensitive than that of the HCR on the MBs coupled with a conventional sandwich hybridization assay (without click-chemical ligation) (limit of detection 127 fmol). Additionally, the proposed assay could discriminate between miR-141 and other miR-200 family members. In contrast to quantitative reverse transcription polymerase chain reaction techniques using enzymes and thermal cycling, this is an enzyme-free assay that can be conducted under isothermal conditions and can specifically detect miR-141 in fetal bovine serum.

摘要

基于点击化学连接辅助杂交与磁珠(MBs)上的杂交链式反应(HCR),开发了一种无酶等温微小RNA(miRNA)检测方法。叠氮化物修饰的探针DNA与二苯并环辛炔修饰的探针DNA之间的点击化学连接通过靶标miRNA(miR-141)的杂交发生。通过添加DNA发夹单体(H1和H2)在MBs上进行HCR。在对HCR产物([H1/H2]n)进行磁分离和变性/再杂交后,通过嵌入染料发出的荧光对所得的HCR产物进行分析,从而实现荧光信号的放大。所提出的检测方法的检测限为0.55 fmol,比与传统夹心杂交检测法(无点击化学连接)结合的MBs上的HCR(检测限为127 fmol)灵敏度高230倍。此外,所提出的检测方法可以区分miR-141和其他miR-200家族成员。与使用酶和热循环的定量逆转录聚合酶链反应技术不同,这是一种无酶检测方法,可以在等温条件下进行,并且可以特异性地检测胎牛血清中的miR-141。

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