Aptamer-based Cas14a1 biosensor for amplification-free live pathogenic detection

CRISPR-Cas systems have been employed to detect a large variety of pathogenic microorganisms by simply changing the guide RNA sequence. However, these platforms usually rely on nucleic acid extraction and amplification to achieve good sensitivity. Herein, we developed a new platform for the highly s...

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Veröffentlicht in:Biosensors & bioelectronics 2022-09, Vol.211, p.114282-114282, Article 114282
Hauptverfasser: Wei, Yangdao, Tao, Zhenzhen, Wan, Lu, Zong, Chengli, Wu, Jiajia, Tan, Xiao, Wang, Buhua, Guo, Zixuan, Zhang, Ling, Yuan, Haoyu, Wang, Peng, Yang, Zhiqing, Wan, Yi
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Sprache:eng
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Zusammenfassung:CRISPR-Cas systems have been employed to detect a large variety of pathogenic microorganisms by simply changing the guide RNA sequence. However, these platforms usually rely on nucleic acid extraction and amplification to achieve good sensitivity. Herein, we developed a new platform for the highly specific and sensitive detection of live staphylococcus aureus (S. aureus) based on an Aptamer-based Cas14a1 Biosensor (ACasB), without the need for nucleic acid extraction or amplification. First, the S. aureus specific aptamer was hybrid with a blocker DNA. After the live S. aureus was added, the blocker can be released upon bacteria-aptamer binding. Finally, the released blocker can activate Cas14a1 protein by binding with the sgRNA to generate a change of fluorescent intensity. The ACasB indicates high specificity and sensitivity: it can directly distinguish 400 CFU/ml live S. aureus cells. Comparable to qPCR, the Cas14a1-aptamer biosensor can detect S. aureus with 100% accuracy in complex samples. Therefore, this ACasB for the on-site detection of live S. aureus can broaden its applications in food safety and environmental monitoring. [Display omitted]
ISSN:0956-5663
1873-4235
DOI:10.1016/j.bios.2022.114282