Interlaboratory assays from the fungal PCR Initiative and the Modimucor Study Group to improve qPCR detection of Mucorales DNA in serum: one more step toward standardization

Steffi Rocchi; Emeline Scherer; P Lewis White; Audrey Guitton; Alexandre Alanio; Françoise Botterel; Marie Elisabeth Bougnoux; Maria José Buitrago; Massimo Cogliati; Marjorie Cornu; Celine Damiani; Julie Denis; Damien Dupont; Stefan Fuchs; Rebecca Gorton; Pieter-Jan Haas; Ferry Hagen; Rasmus Hare; Xavier Iriart; Corné H W Klaassen; Michaela Lackner; Martina Lengerova; Willem J G Melchers; Florent Morio; Philippe Poirier; Jan Springer; Stephane Valot; Birgit Willinger; Cristina Mazzi; Mario Cruciani; Rosemary Barnes; J Peter Donnelly; Jürgen Loeffler; Laurence Millon

doi:10.1128/jcm.01525-24

Interlaboratory assays from the fungal PCR Initiative and the Modimucor Study Group to improve qPCR detection of Mucorales DNA in serum: one more step toward standardization

J Clin Microbiol. 2024 Dec 31:e0152524. doi: 10.1128/jcm.01525-24. Online ahead of print.

Authors

Steffi Rocchi¹, Emeline Scherer^{1

2}, P Lewis White^{3

4}, Audrey Guitton¹, Alexandre Alanio^{5

6}, Françoise Botterel⁷, Marie Elisabeth Bougnoux⁸, Maria José Buitrago^{9

10}, Massimo Cogliati¹¹, Marjorie Cornu¹², Celine Damiani¹³, Julie Denis¹⁴, Damien Dupont¹⁵, Stefan Fuchs¹⁶, Rebecca Gorton¹⁷, Pieter-Jan Haas¹⁸, Ferry Hagen¹⁹, Rasmus Hare²⁰, Xavier Iriart^{21

22}, Corné H W Klaassen²³, Michaela Lackner²⁴, Martina Lengerova²⁵, Willem J G Melchers²⁶, Florent Morio²⁷, Philippe Poirier²⁸, Jan Springer²⁹, Stephane Valot³⁰, Birgit Willinger³¹, Cristina Mazzi³², Mario Cruciani³³, Rosemary Barnes³⁴, J Peter Donnelly³⁵, Jürgen Loeffler²⁹, Laurence Millon^{1

2}

Affiliations

¹ Chrono-environnement UMR6249, CNRS, University of Franche-Comté, Besançon, Bourgogne-Franche-Comté, France.
² Parasitology-Mycology Department, Besançon University Hospital, Besançon, Bourgogne-Franche-Comté, France.
³ Public Health Wales Mycology Reference Laboratory, University Hospital of Wales, Cardiff, Wales, United Kingdom.
⁴ Division of Infection and Immunity, Centre for Trials Research, Cardiff, Wales, United Kingdom.
⁵ Laboratoire de parasitologie-mycologie, AP-HP, Hôpital Saint-Louis, Paris, Île-de-France, France.
⁶ Mycology Department, Institut Pasteur, Université Paris Cité, National Reference Center for Invasive Mycoses and Antifungals, Translational Mycology research group, Paris, Île-de-France, France.
⁷ Unité de Parasitologie-Mycologie, Département de Prévention, Diagnostic et Traitement des Infections, CHU Henri Mondor, Assistance Publique des Hôpitaux de Paris (APHP), Créteil, France.
⁸ Parasitology-Mycology Unit, Necker Enfants Malades Hospital, APHP, Paris, Île-de-France, France.
⁹ Mycology Reference Laboratory, Centro Nacional de Microbiologia, Instituto de Salud Carlos III, Madrid, Community of Madrid, Spain.
¹⁰ CIBERINFEC, ISCIII-CIBER de Enfermedades Infecciosas, Instituto de Salud Carlos III, Madrid, Community of Madrid, Spain.
¹¹ Department of Biomedical Sciences for Health, Università degli Studi di Milano, Milan, Italy.
¹² Université de Lille, Inserm U1285, CHU Lille, Laboratoire de Parasitologie-Mycologie, CNRS, UMR 8576, UGSF-Unité de Glycobiologie Structurale et Fonctionnelle, Lille, Hauts-de-France, France.
¹³ Laboratoire de Parasitologie et Mycologie Médicales, Centre de Biologie Humaine, CHU Amiens Picardie, Agents Infectieux, Résistance et Chimiothérapie (AGIR), UR 4294, Université de Picardie Jules Verne, Amiens, Hauts-de-France, France.
¹⁴ Laboratoire de Parasitologie et de Mycologie Médicale, Hôpitaux Universitaires de Strasbourg, Strasbourg, Grand Est, France.
¹⁵ Institut des Agents Infectieux, Service de Parasitologie et Mycologie Médicale, Hospices Civils de Lyon, Hôpital Croix-Rousse, Lyon, Auvergne-Rhône-Alpes, France.
¹⁶ Molecular Diagnostics, Institute of Hygiene and Medical Microbiology, Medical University of Innsbruck, Innsbruck, Tyrol, Austria.
¹⁷ Health Services Laboratories, London, United Kingdom.
¹⁸ Department of Medical Microbiology, University Medical Center Utrecht, Utrecht, the Netherlands.
¹⁹ Westerdijk Fungal Biodiversity Institute, Utrecht, the Netherlands.
²⁰ Mycology Unit, Department for Bacteria, Parasites and Fungi, Statens Serum Institut, Copenhagen, Capital Region of Denmark, Denmark.
²¹ Service de Parasitologie-Mycologie, CHU Toulouse, Toulouse, France.
²² Institut Toulousain des Maladies Infectieuses et Inflammatoires (Infinity), Université de Toulouse, CNRS UMR5051, INSERM UMR1291, Universite Paul Sabatier, Toulouse, Occitanie, France.
²³ Department of Medical Microbiology and Infectious Diseases, Erasmus MC University Medical Center Rotterdam, Rotterdam, South Holland, The Netherlands.
²⁴ Mycology Research Group, Institute for Hygiene and Medical Microbiology, Medical University of Innsbruck (MUI), Innsbruck, Tyrol, Austria.
²⁵ Department of Internal Medicine-Hematology and Oncology, University Hospital Brno, Brno, South Moravian Region, Czechia.
²⁶ Department of Medical Microbiology, Radboud University Medical Center, Nijmegen, Gelderland, the Netherlands.
²⁷ Nantes Université, CHU Nantes, Cibles et Médicaments des Infections et de l'Immunité, Nantes, France.
²⁸ Laboratoire de Parasitologie-Mycologie, CHU Clermont-Ferrand, 3IHP, Paris, France.
²⁹ Department of Internal Medicine II, WÜ4i, University Hospital Wuerzburg, Wuerzburg, Germany.
³⁰ Laboratoire de Parasitologie-Mycologie, Plateforme de Biologie Hospitalo-Universitaire Gérard Mack, Dijon, France.
³¹ Division of Clinical Microbiology, Department of Laboratory Medicine, Medical University of Vienna, Vienna, Austria.
³² IRCCS Sacro Cuore Don Calabria Hospital, Negrar di Valpolicella, Verona, Italy.
³³ Fungal PCR Initiative (FPCRI), Verona, Italy.
³⁴ Medical Microbiology and Infectious Diseases, Cardiff University School of Medicine, Cardiff, United Kingdom.
³⁵ Fungal PCR Initiative (FPCRI), Nijmegen, the Netherlands.

PMID: 39745482
DOI: 10.1128/jcm.01525-24

Abstract

The aim of this study was to identify parameters influencing DNA extraction and PCR amplification efficiencies in an attempt to standardize Mucorales qPCR. The Fungal PCR Initiative Mucorales Laboratory Working Group distributed two panels of simulated samples to 26 laboratories: Panel A (six sera spiked with Mucorales DNA and one negative control serum) and Panel B (six Mucorales DNA extracts). Panel A underwent DNA extraction in each laboratory according to the local procedure and were sent to a central laboratory for testing using three different qPCR techniques: one in-house qPCR assay and two commercial assays (MucorGenius and Fungiplex). Panel B DNA extracts were PCR amplified in each laboratory using local procedures: nine in-house qPCR assays and two commercial kits (MucorGenius and MycoGENIE). All data were compiled and anonymously analyzed at the central laboratory. For Panel A, a total of six different automated platforms and five manual extraction methods were used. Positive rates were 64%, 70%, and 89%, for the MucorGenius, Fungiplex, and the in-house qPCR assay, respectively. Using a large volume of serum for DNA extraction provided the highest analytical sensitivity (82.5% for 1 mL compared with 62.7% for smaller volumes, P < 0.01). For Panel B, five in-house qPCR assays and two commercial kits had >78% positivity. Using larger PCR input volumes (≥7 µL) was associated with the highest sensitivity at 95.5% compared to 58.3% when lower input volumes were used (P < 0.01). Using larger sample volumes for nucleic acid extraction and DNA template volumes for PCR amplification significantly improves the performance of Mucorales qPCR when testing serum.

Importance: Mucormycosis is a life-threatening mold infection affecting immunosuppressed patients but also other patients with diabetes or trauma. Better survival is linked to shorter delays in diagnosis and treatment initiation. Detection of Mucorales-free DNA in serum or plasma using quantitative PCR allows a prompt diagnosis and earlier treatment. Several techniques and protocols of quantitative Mucorales PCR are used in Europe, and improving performance remains a common objective of laboratories participating in the fungal PCR Initiative Working Group. This study, which combined results from 26 laboratories in Europe, showed that the main parameters underpinning sensitivity are the preanalytical variables (volume of serum used for DNA extraction and DNA template volume), irrespective of the extraction platforms and qPCR assay/platform.

Keywords: Mucorales PCR; interlaboratory assay; mucormycosis; standardization.