Development of a multiplex tandem pcr (Mt‐pcr) assay for the detection of emerging sars‐cov‐2 variants

Abstract

The emergence of variants of SARS‐CoV‐2 has created challenges for the testing infra-structure. Although large‐scale genome sequencing of SARS‐CoV‐2 has facilitated hospital and public health responses, access to sequencing facilities globally is variable and turnaround times can be significant, so there is a requirement for rapid and cost‐effective alternatives. Applying a polymer-ase chain reaction (PCR)‐based single nucleotide polymorphism (SNP) approach enables rapid (<4 h) identification of SARS‐CoV‐2 lineages from nucleic acid extracts, through the presence or absence of a panel of defined of genomic polymorphisms. For example, the B.1.1.7 lineage (“UK”, “Alpha”, or “Kent” variant) is characterised by 23 mutations compared to the reference strain, and the most biologically significant of these are found in the S gene. We have developed a SARS‐CoV‐2 typing assay focused on five positions in the S gene (HV69/70, N501, K417, E484 and P681). This configu-ration can identify a range of variants, including all the “Variants of Concern” currently designated by national and international public health bodies. The panel has been evaluated using a range of clinical isolates and standardised control materials at four UK hospitals and shows excellent con-cordance with the known lineage information derived from full sequence analysis. The assay has a turnaround time of about three hours for a set of up to 24 samples and has been utilised to identify emerging variants in a clinical setting.