A Rationally Designed CRISPR/Cas12a Assay Using a Multimodal Reporter for Various Readouts

清脆的 计算生物学 化学 环介导等温扩增 报告基因 核酸 DNA 基因 生物 生物化学 基因表达
作者
Jean de Dieu Habimana,Omar Mukama,Obed Boadi Amissah,Yirong Sun,Eric Karangwa,Yujie Liu,Samson Mugisha,Na Cheng,Ling Wang,Jianlin Chen,Sihao Deng,Rongqi Huang,Zhiyuan Li
出处
期刊:Analytical Chemistry [American Chemical Society]
卷期号:95 (31): 11741-11750 被引量:8
标识
DOI:10.1021/acs.analchem.3c01876
摘要

The CRISPR/Cas systems offer a programmable platform for nucleic acid detection, and CRISPR/Cas-based diagnostics (CRISPR-Dx) have demonstrated the ability to target nucleic acids with greater accuracy and flexibility. However, due to the configuration of the reporter and the underlying labeling mechanism, almost all reported CRISPR-Dx rely on a single-option readout, resulting in limitations in end-point result readouts. This is also associated with high reagent consumption and delays in diagnostic reports due to protocol differences. Herein, we report for the first time a rationally designed Cas12a-based multimodal universal reporter (CAMURE) with improved sensitivity that harnesses a dual-mode reporting system, facilitating options in end-point readouts. Through systematic configurations and optimizations, our novel universal reporter achieved a 10-fold sensitivity enhancement compared to the DETECTR reporter. Our unique and versatile reporter could be paired with various readouts, conveying the same diagnostic results. We applied our novel reporter for the detection of staphylococcal enterotoxin A due to its high implication in staphylococcal food poisoning. Integrated with loop-mediated isothermal amplification, our multimodal reporter achieved 10 CFU/mL sensitivity and excellent specificity using a real-time fluorimeter, in-tube fluorescence, and lateral flow strip readouts. We also propose, using artificially contaminated milk samples, a fast (2–5 min) Triton X-100 DNA extraction approach with a comparable yield to the commercial extraction kit. Our CAMURE could be leveraged to detect all gene-encoding SEs by simply reprogramming the guide RNA and could also be applied to the detection of other infections and disease biomarkers.
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