Ultrasensitive and Specific Clustered Regularly Interspaced Short Palindromic Repeats Empowered a Plasmonic Fiber Tip System for Amplification-Free Monkeypox Virus Detection and Genotyping

The urgent necessity for highly sensitive diagnostic tools has been accentuated by the ongoing mpox (monkeypox) virus pandemic due to the complexity in identifying asymptomatic and presymptomatic carriers. Traditional polymerase chain reaction-based tests, despite their effectiveness, are hampered b...

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Published inACS Nano Vol. 17; no. 13; pp. 12903 - 12914
Main Authors Chen, Yuzhi, Chen, Zhi, Li, Tianzhong, Qiu, Meng, Zhang, Jinghan, Wang, Yan, Yuan, Wu, Ho, Aaron Ho-Pui, Al-Hartomy, Omar, Wageh, Swelm, Al-Sehemi, Abdullah G., Shi, Xin, Li, Jingfeng, Xie, Zhongjian, Xuejin, Li, Zhang, Han
Format Journal Article
LanguageEnglish
Published United States American Chemical Society 11.07.2023
American Chemical Society (ACS)
Subjects
Biosensing Techniques
Genotype
Humans
Monkeypox virus
Mpox (monkeypox)
Mutation
Pandemics
Monkeypox virus
Surface plasmon resonance-based fiber tip
Clustered regularly interspaced short palindromic repeats (CRISPR)
Amplification-free
Biosensor
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Summary:The urgent necessity for highly sensitive diagnostic tools has been accentuated by the ongoing mpox (monkeypox) virus pandemic due to the complexity in identifying asymptomatic and presymptomatic carriers. Traditional polymerase chain reaction-based tests, despite their effectiveness, are hampered by limited specificity, expensive and bulky equipment, labor-intensive operations, and time-consuming procedures. In this study, we present a clustered regularly interspaced short palindromic repeats (CRISPR)/Cas12a-based diagnostic platform with a surface plasmon resonance-based fiber tip (CRISPR-SPR-FT) biosensor. The compact CRISPR-SPR-FT biosensor, with a 125 μm diameter, offers high stability and portability, enabling exceptional specificity for mpox diagnosis and precise identification of samples with a fatal mutation site (L108F) in the F8L gene. The CRISPR-SPR-FT system can analyze viral double-stranded DNA from mpox virus without amplification in under 1.5 h with a limit of detection below 5 aM in plasmids and about 59.5 copies/μL when in pseudovirus-spiked blood samples. Our CRISPR-SPR-FT biosensor thus offers fast, sensitive, portable, and accurate target nucleic acid sequence detection.
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ISSN:1936-0851
1936-086X
1936-086X
DOI:10.1021/acsnano.3c05007