Results of the first German external quality assessment scheme for the detection of monkeypox virus DNA

Vierbaum, Laura; Wojtalewicz, Nathalie; Kaufmann, Anne; Goseberg, Sabine; Kaiser, Patricia; Grunert, Hans-Peter; Dühring, Ulf; Zimmermann, Anika; Scholz, Annemarie; Michel, Janine; Nitsche, Andreas; Rabenau, Holger F.; Obermeier, Martin; Schellenberg, Ingo; Zeichhardt, Heinz; Kammel, Martin

2023-04-28Zeitschriftenartikel

Vierbaum, Laura

Wojtalewicz, Nathalie

Kaufmann, Anne

Goseberg, Sabine

Kaiser, Patricia

Grunert, Hans-Peter

Dühring, Ulf

Zimmermann, Anika

Scholz, Annemarie

Michel, Janine

Nitsche, Andreas

Rabenau, Holger F.

Obermeier, Martin

Schellenberg, Ingo

Zeichhardt, Heinz

Kammel, Martin

Background: In May 2022, the monkeypox virus (MPXV) spread into non-endemic countries and the global community was quick to test the lessons learned from the SARS-CoV-2 pandemic. Due to its symptomatic resemblance to other diseases, like the non-pox virus varicella zoster (chickenpox), polymerase chain reaction methods play an important role in correctly diagnosing the rash-causing pathogen. INSTAND quickly established a new external quality assessment (EQA) scheme for MPXV and orthopoxvirus (OPXV) DNA detection to assess the current performance quality of the laboratory tests. Methods: We analyzed quantitative and qualitative data of the first German EQA for MPXV and OPXV DNA detection. The survey included one negative and three MPXV-positive samples with different MPX viral loads. The threshold cycle (Ct) or other measures defining the quantification cycle (Cq) were analyzed in an assay-specific manner. A Passing Bablok fit was used to investigate the performance at laboratory level. Results: 141 qualitative datasets were reported by 131 laboratories for MPXV detection and 68 qualitative datasets by 65 laboratories for OPXV detection. More than 96% of the results were correctly identified as negative and more than 97% correctly identified as positive. An analysis of the reported Ct/Cq values showed a large spread of these values of up to 12 Ct/Cq. Nevertheless, there is a good correlation of results for the different MPXV concentrations at laboratory level. Only a few quantitative results in copies/mL were reported (MPXV: N = 5; OPXV: N = 2), but the results correlated well with the concentration differences between the EQA samples, which were to a power of ten each. Conclusion: The EQA results show that laboratories performed well in detecting both MPXV and OPXV. However, Ct/Cq values should be interpreted with caution when conclusions are drawn about the viral load as long as metrological traceability is not granted.

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