Author: Perchetti, Garrett A.; Zhu, Haiying; Mills, Margaret G.; Shrestha, Lasata; Wagner, Cassia; Bakhash, Shah Mohamed; Lin, Michelle J.; Xie, Hong; Huang, Meeiâ€Li; Mathias, Patrick; Bedford, Trevor; Jerome, Keith R.; Greninger, Alexander L.; Roychoudhury, Pavitra
Title: Specific allelic discrimination of N501Y and other SARSâ€CoVâ€2 mutations by ddPCR detects B.1.1.7 lineage in Washington State Cord-id: rsbh30zf Document date: 2021_7_3
ID: rsbh30zf
Snippet: Realâ€time epidemiological tracking of variants of concern (VOCs) can help limit the spread of more contagious forms of severe acute respiratory syndrome coronavirus 2 (SARSâ€CoVâ€2), such as those containing the N501Y mutation. Typically, genetic sequencing is required to be able to track VOCs in realâ€time. However, sequencing can take time and may not be accessible in all laboratories. Genotyping by RTâ€ddPCR offers an alternative to rapidly detect VOCs through discrimination of specific
Document: Realâ€time epidemiological tracking of variants of concern (VOCs) can help limit the spread of more contagious forms of severe acute respiratory syndrome coronavirus 2 (SARSâ€CoVâ€2), such as those containing the N501Y mutation. Typically, genetic sequencing is required to be able to track VOCs in realâ€time. However, sequencing can take time and may not be accessible in all laboratories. Genotyping by RTâ€ddPCR offers an alternative to rapidly detect VOCs through discrimination of specific alleles such as N501Y, which is associated with increased transmissibility and virulence. Here we describe the first cases of the B.1.1.7 lineage of SARSâ€CoVâ€2 detected in Washington State by using a combination of reverseâ€transcription polymerase chain reaction (RTâ€PCR), RTâ€ddPCR, and nextâ€generation sequencing. We initially screened 1035 samples positive for SARSâ€CoVâ€2 by our CDCâ€based laboratoryâ€developed assay using ThermoFisher's multiplex RTâ€PCR COVIDâ€19 assay over four weeks from late December 2020 to early January 2021. S gene target failures (SGTF) were subsequently assayed by RTâ€ddPCR to confirm four mutations within the S gene associated with the B.1.1.7 lineage: a deletion at amino acid (AA) 69â€70 (ACATGT), deletion at AA 145, (TTA), N501Y mutation (TAT), and S982A mutation (GCA). All four targets were detected in two specimens; followâ€up sequencing revealed a total of 9 mutations in the S gene and phylogenetic clustering within the B.1.1.7 lineage. Next, we continued screening samples for SGTF detecting 23 additional B.1.1.7 variants by RTâ€ddPCR and confirmed by sequencing. As VOCs become increasingly prevalent, molecular diagnostic tools like RTâ€ddPCR can be utilized to quickly, accurately, and sensitively distinguish more contagious lineages of SARSâ€CoVâ€2.
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