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Heat Inactivation of Different Types of SARS-CoV-2 Samples: What Protocols for Biosafety, Molecular Detection and Serological Diagnostics?

Boris Pastorino, Franck Touret, Magali Gilles, Xavier de Lamballerie, Rémi N. Charrel

2020Viruses149 citationsDOIOpen Access PDF

Abstract

Standard precautions to minimize the risk of SARS-CoV-2 transmission implies that infected cell cultures and clinical specimens may undergo some sort of inactivation to reduce or abolish infectivity. We evaluated three heat inactivation protocols (56 °C-30 min, 60 °C-60 min and 92 °C-15 min) on SARS-CoV-2 using (i) infected cell culture supernatant, (ii) virus-spiked human sera (iii) and nasopharyngeal samples according to the recommendations of the European norm NF EN 14476-A2. Regardless of the protocol and the type of samples, a 4 Log10 TCID50 reduction was observed. However, samples containing viral loads > 6 Log10 TCID50 were still infectious after 56 °C-30 min and 60 °C-60 min, although infectivity was < 10 TCID50. The protocols 56 °C-30 min and 60 °C-60 min had little influence on the RNA copies detection, whereas 92 °C-15 min drastically reduced the limit of detection, which suggests that this protocol should be avoided for inactivation ahead of molecular diagnostics. Lastly, 56 °C-30 min treatment of serum specimens had a negligible influence on the results of IgG detection using a commercial ELISA test, whereas a drastic decrease in neutralizing titers was observed.

Topics & Concepts

InfectivitySerologyTiterVirologyBiosafetySevere acute respiratory syndrome coronavirus 2 (SARS-CoV-2)Detection limitVirusBiologyViral loadNeutralizing antibodyCoronavirus disease 2019 (COVID-19)Molecular biologyChemistryAntibodyMedicineImmunologyChromatographyInfectious disease (medical specialty)BiotechnologyPathologyDiseaseSARS-CoV-2 detection and testingSARS-CoV-2 and COVID-19 ResearchInfection Control and Ventilation
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