Sensitive fluorescence detection of SARS-CoV-2 RNA in clinical samples via one-pot isothermal ligation and transcription
- PMID: 32948855
- PMCID: PMC7499000
- DOI: 10.1038/s41551-020-00617-5
Sensitive fluorescence detection of SARS-CoV-2 RNA in clinical samples via one-pot isothermal ligation and transcription
Abstract
The control of viral outbreaks requires nucleic acid diagnostic tests that are sensitive, simple and fast. Here, we report a highly sensitive and specific one-pot assay for the fluorescence-based detection of RNA from pathogens. The assay, which can be performed within 30-50 min of incubation time and can reach a limit of detection of 0.1-attomolar RNA concentration, relies on a sustained isothermal reaction cascade producing an RNA aptamer that binds to a fluorogenic dye. The RNA aptamer is transcribed by the T7 RNA polymerase from the ligation product of a promoter DNA probe and a reporter DNA probe that hybridize with the target single-stranded RNA sequence via the SplintR ligase (a Chlorella virus DNA ligase). In 40 nasopharyngeal SARS-CoV-2 samples, the assay reached positive and negative predictive values of 95 and 100%, respectively. We also show that the assay can rapidly detect a range of viral and bacterial RNAs.
Conflict of interest statement
Patent applications have been submitted by J.W.L., G.Y.J., C.H.W., S.J. and G.S. based on the results of this study (PCT/KR2020/005331 (Patent Cooperation Treaty) and 10-2020-0048912 (Republic of Korea)).
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Comment in
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Rapid and frequent testing.Nat Biomed Eng. 2020 Dec;4(12):1121-1122. doi: 10.1038/s41551-020-00670-0. Nat Biomed Eng. 2020. PMID: 33293723 No abstract available.
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