One-Pot CRISPR-Cas12a-Based Viral DNA Detection via HRP-Enriched Extended ssDNA-Modified Au@Fe 3 O 4 Nanoparticles.
Dong Hyeok ParkIzzati HaizanMin Ju AhnMin Yu ChoiMin Jung KimJin-Ha ChoiPublished in: Biosensors (2024)
In the context of virus outbreaks, the need for early and accurate diagnosis has become increasingly urgent. In addition to being crucial for effective disease control, timely and precise detection of viral infections is also necessary for the implementation of essential public health measures, especially during pandemics. Among these measures, point-of-care testing (POCT) stands out as a powerful approach with the potential to revolutionize the landscape of viral diagnosis. In this study, we developed a one-pot clustered regularly interspaced short palindromic repeats (CRISPR)-Cas12a-based viral DNA detection system tailored for POCT; this method utilizes multi-enzyme-modified Au@Fe 3 O 4 nanoparticles. As an alternative to nucleic acid amplification, our method uses single-stranded DNA elongation to facilitate multi-enzyme modification; this guarantees heightened sensitivity and expedites the diagnostic process. We achieved a satisfactory limit of detection of 0.25 nM, demonstrating the remarkable sensitivity of the method without the need for sophisticated equipment. The incorporation of Au@Fe 3 O 4 magnetic nanoparticles facilitates sample separation, further streamlining the workflow and reinforcing the simplicity of our method. This integrated approach offers a practical solution for sensitive viral DNA detection in POCT scenarios, advancing the field of rapid and accurate diagnostics.
Keyphrases
- nucleic acid
- loop mediated isothermal amplification
- crispr cas
- sars cov
- public health
- label free
- sensitive detection
- circulating tumor
- real time pcr
- cell free
- genome editing
- healthcare
- magnetic nanoparticles
- risk assessment
- photodynamic therapy
- gold nanoparticles
- smoking cessation
- quantum dots
- circulating tumor cells