化学
核酸外切酶
清脆的
Cas9
核酸
多重位移放大
核糖核酸
T7 RNA聚合酶
抄写(语言学)
分子生物学
计算生物学
DNA
聚合酶链反应
聚合酶
生物化学
噬菌体
基因
生物
DNA提取
哲学
大肠杆菌
语言学
作者
Decai Zhang,Benshun Tian,Yong Ling,Ye Long,Xiao Meng,Kaixuan Yuan,Xinqiang Zhang,Guansheng Zheng,Xinying Li,Judun Zheng,Yuhui Liao,Bowen Shu,Bing Gu
出处
期刊:Analytical Chemistry
[American Chemical Society]
日期:2024-06-11
卷期号:96 (25): 10451-10458
被引量:13
标识
DOI:10.1021/acs.analchem.4c01800
摘要
-cleavage of the linker strands inhibiting split G-Quadruplex (G4) assembly, thereby inducing fluorescence attenuation proportion to the input RNA target. We first performed step-by-step validation of the entire assay process and optimized the reaction parameters. Using the optimal conditions, T7/G4-CRISPR was capable of detecting as low as 3.6 pM target RNA, obtaining ∼100-fold improvement in sensitivity compared with the most direct Cas12a assays. Meanwhile, its excellent specificity could discriminate single nucleotide variants adjacent to the toehold region and allow species-specific pathogen identification. Furthermore, we applied it for analyzing bacterial 16S rRNA in 40 clinical urine samples, exhibiting a sensitivity of 90% and a specificity of 100% when validated by RT-quantitative PCR. Therefore, we envision that T7/G4-CRISPR will serve as a promising RNA sensing approach to expand the toolbox of CRISPR-based diagnostics.
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