环介导等温扩增
DNA
Cas9
计算生物学
核酸
底漆延伸
PCR的应用
底漆(化妆品)
多重位移放大
聚合酶链反应
生物
分子生物学
清脆的
化学
遗传学
基序列
基因
DNA提取
多重聚合酶链反应
有机化学
作者
Ting Wang,Yong Liu,Huanhuan Sun,Bin‐Cheng Yin,Bang‐Ce Ye
标识
DOI:10.1002/anie.201901292
摘要
We have developed an ingenious method, termed Cas9 nickase-based amplification reaction (Cas9nAR), to amplify a target fragment from genomic DNA at a constant temperature of 37 °C. Cas9nAR employs a sgRNA:Cas9n complex with a single-strand nicking property, a strand-displacing DNA polymerase, and two primers bearing the cleavage sequence of Cas9n, to promote cycles of DNA replication through priming, extension, nicking, and displacement reaction steps. Cas9nAR exhibits a zeptomolar limit of detection (2 copies in 20 μL of reaction system) within 60 min and a single-base discrimination capability. More importantly, the underlying principle of Cas9nAR offers simplicity in primer design and universality in application. Considering the superior sensitivity and specificity, as well as the simple-to-implement, rapid, and isothermal features, Cas9nAR holds great potential to become a routine assay for the quantitative detection of nucleic acids in basic and applied studies.
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