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Ultrasensitive detection of lead ions based on a DNA-labelled DNAzyme sensor

机译:基于DNA标记的DNAzyme传感器的铅离子超灵敏检测

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摘要

Here, we report a facile approach for highly sensitive and selective detection of aqueous lead ions that uses a real-time quantitative polymerase chain reaction technology and a lead-dependent DNAzyme, termed GR-5. In this method, the substrate DNA is cleaved at the site of the adenosine ribonucleotide by GR-5 DNAzyme in the presence of lead ions, resulting in a decrease in template DNA available for PCR and a consequent change in signal detection (cycle threshold (Ct) value). This novel approach takes advantage of the exponential amplification of PCR and the specific recognition of the GR-5 lead-dependent DNAzyme to provide Pb2+-specific detection with an excellent linear relationship between Ct value and Pb2+ concentration within a range of 1-500 nM. The correlation coefficient of the standard curve was 0.9898, and the limit of detection was 0.7 nM. Moreover, this sensor showed good selectivity for Pb2+ ions over other metal ions.
机译:在这里,我们报告了一种使用实时定量聚合酶链反应技术和铅依赖型DNA酶(称为GR-5)进行水铅离子的高灵敏度和选择性检测的简便方法。在这种方法中,存在铅离子的情况下,GR-5 DNAzyme会在腺苷核糖核苷酸的位点切割底物DNA,导致可用于PCR的模板DNA减少,从而导致信号检测发生变化(循环阈值(Ct )值)。这种新方法利用了PCR的指数扩增和GR-5铅依赖性DNAzyme的特异性识别,可提供Pb2 +特异性检测,并且Ct值与Pb2 +浓度在1-500 nM之间具有极好的线性关系。标准曲线的相关系数为0.9898,检出限为0.7 nM。而且,该传感器对Pb2 +离子的选择性优于其他金属离子。

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