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首页> 外文期刊>Mikrochimica Acta: An International Journal for Physical and Chemical Methods of Analysis >Electrochemical strategy for ultrasensitive detection of microRNA based on MNAzyme-mediated rolling circle amplification on a gold electrode
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Electrochemical strategy for ultrasensitive detection of microRNA based on MNAzyme-mediated rolling circle amplification on a gold electrode

机译:基于MNAzyme介导的金电极滚环扩增的microRNA超灵敏检测的电化学策略

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摘要

The authors describe an electrochemical strategy for ultrasensitive and specific detection of microRNA (miRNA). It is based on both multicomponent nucleic acid enzyme (MNAzyme) amplification and rolling circle amplification (RCA). In the presence of target miRNAs, partial enzyme A (partzyme A) and partial enzyme B (partzyme B) are assembled to form active MNAzymes. Once formed, the MNAzymes catalyze the cleavage of the hairpin substrates to liberate biotinylated fragments which hybridized with the capture probes immobilized on a gold electrode. The RCA is then initiated to form a product that binds many detection probes. Finally, the amperometric signal (best acquired at a working voltage of 0.22 V vs. Ag/AgCl) is obtained by employing the streptavidinylated alkaline phosphatase as the enzyme. This biosensor has a 1.66 fM detection limit, and a dynamic range that extends from 10 fM to 1 nM. It displays specificity down to single mismatch discrimination of target miRNAs and good reproducibility. It was successfully applied to the determination of miRNA in total RNA samples extracted from human breast adenocarcinoma MCF-7 cells.
机译:作者介绍了用于microRNA(miRNA)的超灵敏和特异性检测的电化学策略。它基于多组分核酸酶(MNAzyme)扩增和滚环扩增(RCA)。在存在靶miRNA的情况下,组装部分酶A(部分酶A)和部分酶B(部分酶B)以形成活性MNA酶。一旦形成,MNA酶就催化发夹底物的裂解以释放生物素化的片段,该片段与固定在金电极上的捕获探针杂交。然后启动RCA形成结合许多检测探针的产物。最后,通过使用链霉亲和素化碱性磷酸酶作为酶获得安培信号(最好在0.22 V对Ag / AgCl的工作电压下获得)。该生物传感器的检测极限为1.66 fM,动态范围从10 fM扩展到1 nM。它显示出特异性低至靶miRNA的单个错配判别和良好的再现性。它已成功地用于测定从人乳腺腺癌MCF-7细胞提取的总RNA样品中的miRNA。

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