Sensitive detection and quantification of SARS-CoV-2 in saliva

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作者
Mustafa Fatih Abasiyanik
Blake Flood
Jing Lin
Sefika Ozcan
Sherin J. Rouhani
Athalia Pyzer
Jonathan Trujillo
Chaojie Zhen
Ping Wu
Stephen Jumic
Andrew Wang
Thomas F. Gajewski
Peng Wang
Madeline Hartley
Bekim Ameti
Rachael Niemiec
Marian Fernando
Vasudha Mishra
Peter Savage
Bulent Aydogan
Cindy Bethel
Scott Matushek
Kathleen G. Beavis
Nishant Agrawal
Jeremy Segal
Savaş Tay
Evgeny Izumchenko
机构
[1] University of Chicago,Pritzker School of Molecular Engineering
[2] University of Chicago,Department of Pathology
[3] University of Chicago,Section of Hematology and Oncology, Pritzker School of Medicine
[4] University of Chicago,Section of Hospital Medicine, Department of Medicine
[5] University of Chicago,Radiation and Cellular Oncology
[6] University of Chicago Medicine,Microbiology Laboratory
[7] University of Chicago,Section of Otolaryngology
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Saliva has significant advantages as a test medium for detection of SARS-CoV-2 infection in patients, such as ease of collection, minimal requirement of supplies and trained personnel, and safety. Comprehensive validation in a large cohort of prospectively collected specimens with unknown SARS-CoV-2 status should be performed to evaluate the potential and limitations of saliva-based testing. We developed a saliva-based testing pipeline for detection of SARS-CoV-2 nucleic acids using real-time reverse transcription PCR (RT-PCR) and droplet digital PCR (ddPCR) readouts, and measured samples from 137 outpatients tested at a curbside testing facility and 29 inpatients hospitalized for COVID-19. These measurements were compared to the nasal swab results for each patient performed by a certified microbiology laboratory. We found that our saliva testing positively detects 100% (RT-PCR) and 93.75% (ddPCR) of curbside patients that were identified as SARS-CoV-2 positive by the Emergency Use Authorization (EUA) certified nasal swab testing assay. Quantification of viral loads by ddPCR revealed an extremely wide range, with 1 million-fold difference between individual patients. Our results demonstrate for both community screening and hospital settings that saliva testing reliability is on par with that of the nasal swabs in detecting infected cases, and has potential for higher sensitivity when combined with ddPCR in detecting low-abundance viral loads that evade traditional testing methods.
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