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Dumbbell probe-mediated cascade isothermal amplification: A novel strategy for label-free detection of microRNAs and its application to real sample assay

机译:哑铃探针介导的级联等温扩增:一种无标记的微小RNA检测新策略及其在真实样品分析中的应用

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摘要

Considering the great significance of microRNAs (miRNAs) in cancer detection and typing, the development of sensitive, specific, quantitative, and low-cost methods for the assay of expression levels of miRNAs is desirable. We describe a highly efficient amplification platform for ultrasensitive analysis of miRNA (taking let-7a miRNA as a model analyte) based on a dumbbell probe-mediated cascade isothermal amplification (DP-CIA) strategy. The method relies on the circularization of dumbbell probe by binding target miRNA, followed by rolling circle amplification (RCA) reaction and an autonomous DNA machine performed by nicking/polymerization/displacement cycles that continuously produces single-stranded G-quadruplex to assemble with hemin to generate a color signal. In terms of the high sensitivity (as low as 1 zmol), wide dynamic range (covering 9 orders of magnitude), good specificity (even single-base difference) and easy operation (one probe and three enzymes), the proposed label-free assay is successfully applied to direct detection of let-7a miRNA in real sample (total RNA extracted from human lung tissue), demonstrating an attractive alternative for miRNA analysis for gene expression profiling and molecular diagnostics, particularly for early cancer diagnosis.
机译:考虑到微小RNA(miRNA)在癌症检测和分型中的巨大意义,需要开发灵敏,特异,定量和低成本的方法来测定miRNA的表达水平。我们描述了一个高效的扩增平台,用于基于哑铃探针介导的级联等温扩增(DP-CIA)策略的miRNA(以let-7a miRNA作为模型分析物)的超灵敏分析。该方法依靠结合靶标miRNA的哑铃探针环化,然后进行滚环扩增(RCA)反应和通过切刻/聚合/置换循环进行的自主DNA机器,该循环连续产生单链G-四链体以与血红素组装成产生颜色信号。就高灵敏度(低至1 zmol),宽动态范围(覆盖9个数量级),良好的特异性(甚至单碱基差异)和易于操作(一种探针和三种酶)而言,建议的无标记该检测方法成功地用于直接检测实际样品中的let-7a miRNA(从人肺组织中提取的总RNA),为miRNA分析,基因表达谱分析和分子诊断(尤其是早期癌症诊断)展示了一种有吸引力的替代方法。

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