%0 Journal Article %A Thompson, Jamie L. %A Downie Ruiz Velasco, Angela %A Cardall, Alice %A Tarbox, Rebecca %A Richardson, Jaineeta %A Clarke, Gemma %A Lister, Michelle %A Howson-Wells, Hannah C. %A Fleming, Vicki M. %A Khakh, Manjinder %A Sloan, Tim %A Duckworth, Nichola %A Walsh, Sarah %A Denning, Chris %A McClure, C. Patrick %A Benest, Andrew V. %A Seedhouse, Claire H. %T Comparative effects of viral-transport-medium heat inactivation upon downstream SARS-CoV-2 detection in patient samples %D 2021 %J Journal of Medical Microbiology, %V 70 %N 3 %@ 1473-5644 %C 001301 %R https://doi.org/10.1099/jmm.0.001301 %K COVID-19 %K RT-qPCR testing %K SARS-CoV-2 %K viral transport media %I Microbiology Society, %X Introduction. The COVID-19 pandemic, which began in 2020 is testing economic resilience and surge capacity of healthcare providers worldwide. At the time of writing, positive detection of the SARS-CoV-2 virus remains the only method for diagnosing COVID-19 infection. Rapid upscaling of national SARS-CoV-2 genome testing presented challenges: (1) Unpredictable supply chains of reagents and kits for virus inactivation, RNA extraction and PCR-detection of viral genomes. (2) Rapid time to result of <24 h is required in order to facilitate timely infection control measures. Hypothesis. Extraction-free sample processing would impact commercially available SARS-CoV-2 genome detection methods. Aim. We evaluated whether alternative commercially available kits provided sensitivity and accuracy of SARS-CoV-2 genome detection comparable to those used by regional National Healthcare Services (NHS). Methodology. We tested several detection methods and tested whether detection was altered by heat inactivation, an approach for rapid one-step viral inactivation and RNA extraction without chemicals or kits. Results. Using purified RNA, we found the CerTest VIASURE kit to be comparable to the Altona RealStar system currently in use, and further showed that both diagnostic kits performed similarly in the BioRad CFX96 and Roche LightCycler 480 II machines. Additionally, both kits were comparable to a third alternative using a combination of Quantabio qScript one-step Quantitative Reverse Transcription Polymerase Chain Reaction (qRT-PCR) mix and Centre for Disease Control and Prevention (CDC)-accredited N1 and N2 primer/probes when looking specifically at borderline samples. Importantly, when using the kits in an extraction-free protocol, following heat inactivation, we saw differing results, with the combined Quantabio-CDC assay showing superior accuracy and sensitivity. In particular, detection using the CDC N2 probe following the extraction-free protocol was highly correlated to results generated with the same probe following RNA extraction and reported clinically (n=127; R2=0.9259). Conclusion. Our results demonstrate that sample treatment can greatly affect the downstream performance of SARS-CoV-2 diagnostic kits, with varying impact depending on the kit. We also showed that one-step heat-inactivation methods could reduce time from swab receipt to outcome of test result. Combined, these findings present alternatives to the protocols in use and can serve to alleviate any arising supply-chain issues at different points in the workflow, whilst accelerating testing, and reducing cost and environmental impact. %U https://www.microbiologyresearch.org/content/journal/jmm/10.1099/jmm.0.001301