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Establishment of an accurate and fast detection method using molecular beacons in loop-mediated isothermal amplification assay

机译:在环介导等温扩增测定中的分子信标的建立准确和快速的检测方法

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This study established a constant-temperature fluorescence quantitative detection method, combining loop-mediated isothermal amplification (LAMP) with molecular beacons. The advantages of LAMP are its convenience and efficiency, as it does not require a thermocycler and results are easily visualized by the naked eye. However, a major disadvantage of current LAMP techniques is the use of indirect evaluation methods (e.g., electrophoresis, SYBR Green I dye, precipitation, hydroxynaphthol blue dye, the turbidimetric method, calcein/Mn2+ dye, and the composite probe method), which cannot distinguish between the desired products and products of nonspecific amplification, thereby leading to false positives. Use of molecular beacons avoids this problem because molecular beacons produce fluorescence signals only when binding to target DNA, thus acting as a direct indicator of amplification products. Our analyses determined the optimal conditions for molecular beacons as an evaluation tool in LAMP: beacon length of 25–45?bp, beacon concentration of 0.6–1?pmol/μL, and reaction temperature of 60–65?°C. In conclusion, we validated a novel molecular beacon loop-mediated isothermal amplification method (MB-LAMP), realizing the direct detection of LAMP product.
机译:该研究建立了恒温荧光定量检测方法,将环形介导的等温扩增(灯)与分子信标结合。灯的优点是其便利性和效率,因为它不需要热循环仪,结果很容易被肉眼可视化。然而,目前灯技术的主要缺点是使用间接评估方法(例如,电泳,SYBR Green I染料,沉淀,羟基萘酚蓝染料,浊度法,Calcein / Mn2 +染料和复合探针方法)不能区分所需的产品和非特异性扩增的产品,从而导致误报。使用分子信标避免这种问题,因为仅当与靶DNA结合时仅产生荧光信号,从而作用为扩增产物的直接指示剂。我们的分析确定了作为灯的评估工具的分子信标的最佳条件:信标长度为25-45〜45磅,信标浓度为0.6-1≤PMOL/μL,反应温度为60-65Ω·℃。总之,我们验证了一种新型分子信标环介导的等温扩增方法(MB-LAMP),实现了灯产品的直接检测。

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