Litcius/Paper detail

DNA Extraction- and Amplification-Free Nucleic Acid Biosensor for the Detection of Foodborne Pathogens Based on CRISPR/Cas12a and Argonaute Protein-Mediated Cascade Signal Amplification

Rui Chen, Junpeng Zhao, Minjie Han, Yongzhen Dong, Feng Jiang, Yiping Chen

2023Journal of Agricultural and Food Chemistry40 citationsDOI

Abstract

A novel method for detecting low levels of viable foodborne pathogens, specifically Salmonella typhimurium ( S. typhimurium ), has been developed. Traditional nucleic acid assay, such as polymerase chain reaction (PCR), often requires complex DNA extraction and amplification, making it challenging to differentiate between viable and nonviable pathogens. This assay employed a phage as the recognition element to precisely identify and lyse viable S. typhimurium that can undergo DNA extraction. It combined the efficient trans-cleavage activities of CRISPR/Cas12a with the specific cleavage advantages of Argonaute proteins, enabling ultrasensitive detection. This double-enzyme-mediated nucleic acid test can accurately distinguish viable and nonviable S. typhimurium with a detection limit of 23 CFU/mL without DNA amplification. The method was successfully applied to common food samples, producing results consistent with quantitative PCR tests. This work provides a promising platform for easily detecting viable foodborne pathogens with high sensitivity without the need for DNA extraction and amplification.

Topics & Concepts

Nucleic acidCRISPRRecombinase Polymerase AmplificationBiologyMolecular beaconDNAPolymerase chain reactionMultiple displacement amplificationDNA extractionSalmonellaMolecular biologyComputational biologyOligonucleotideBiochemistryBacteriaGeneGeneticsCRISPR and Genetic EngineeringBiosensors and Analytical DetectionAdvanced biosensing and bioanalysis techniques