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2. Nationwide quality assurance of high-throughput diagnostic molecular testing during the SARS-CoV-2 pandemic: role of the Belgian National Reference Centre

Author

Janssen, Reile, Cuypers, Lize, Laenen, Lies, Keyaerts, Els, Beuselinck, Kurt, Janssenswillen, Sunita, Slechten, Bram, Bode, Jannes, Wollants, Elke, Van Laethem, Kristel, Rector, Annabel, Bloemen, Mandy, Sijmons, Anke, de Schaetzen, Nathalie, Capron, Arnaud, Van Baelen, Kurt, Pascal, Thierry, Vermeiren, Céline, Bureau, Fabrice, Vandesompele, Jo, De Smet, Pieter, Uten, Wouter, Malonne, Hugues, Kerkhofs, Pierre, De Cock, Jo, Matheeussen, Veerle, Verhasselt, Bruno, Gillet, Laurent, Detry, Gautier, Bearzatto, Bertrand, Degosserie, Jonathan, Henin, Coralie, Pairoux, Gregor, Maes, Piet, Van Ranst, Marc, Lagrou, Katrien, Dequeker, Elisabeth, and André, Emmanuel

Published
2024
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3. Respiratory Viruses in Wastewater Compared with Clinical Samples, Leuven, Belgium

Author

Rector, Annabel, Bloemen, Mandy, Thijssen, Marijn, Pussig, Bram, Beuselinck, Kurt, Van Ranst, Marc, and Wollants, Elke

Subjects
Lung diseases -- Comparative analysis -- Health aspects, Wastewater -- Comparative analysis -- Health aspects, Influenza -- Health aspects -- Comparative analysis, Water treatment plants -- Health aspects -- Comparative analysis, Sewage -- Purification, Health
Abstract

Since the COVID-19 pandemic began, wastewater-based surveillance has been used to track circulation levels of SARS-CoV-2 (1,2). For that purpose, we began collecting samples from a regional wastewater treatment plant [...]

Published
2024
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6. An observational cohort study of histological screening for BK polyomavirus nephropathy following viral replication in plasma

Author

Cleenders, Evert, Koshy, Priyanka, Van Loon, Elisabet, Lagrou, Katrien, Beuselinck, Kurt, Andrei, Graciela, Crespo, Marta, De Vusser, Katrien, Kuypers, Dirk, Lerut, Evelyne, Mertens, Kris, Mineeva-Sangwo, Olga, Randhawa, Parmjeet, Senev, Aleksandar, Snoeck, Robert, Sprangers, Ben, Tinel, Claire, Van Craenenbroeck, Amaryllis, van den Brand, Jan, Van Ranst, Marc, Verbeke, Geert, Coemans, Maarten, and Naesens, Maarten

Published
2023
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7. Full-genome next-generation sequencing of hepatitis C virus to assess the accuracy of genotyping by the commercial assay LiPA and the prevalence of resistance-associated substitutions in a Belgian cohort

Author

Christensen, Kasper T., Pierard, Florian, Beuselinck, Kurt, Bonsall, David, Bowden, Rory, Lagrou, Katrien, Nevens, Frederik, Schrooten, Yoeri, Simmonds, Peter, Vandamme, Anne-Mieke, Van Wijngaerden, Eric, Dierckx, Tim, Cuypers, Lize, and Van Laethem, Kristel

Published
2022
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8. Centralised Air Sampling From a Ventilation System for the Surveillance of Respiratory Pathogens.

Author

Happaerts, Michiel, Geenen, Caspar, Michiels, Jade, Gorissen, Sarah, Swinnen, Jens, Beuselinck, Kurt, Laenen, Lies, Raymenants, Joren, Lorent, Natalie, Ombelet, Sien, Keyaerts, Els, André, Emmanuel, and Yun, Geun Young

Subjects
AIR sampling, AIR conditioning, COMMUNICABLE diseases, RESPIRATORY organs, SCALABILITY, VENTILATION
Abstract

Background: The COVID‐19 pandemic has triggered a renewed interest in indoor air sampling for infectious disease surveillance. However, scalability is currently limited, as samples are usually collected in a single indoor space. An alternative is to place the device within a heating, ventilation, and air conditioning system (HVAC), but this approach has not been tested against room air sampling. Methods: In this observational study, we sampled the air in an indoor fitness centre for 2 or 6 h, simultaneously in three locations of the main exercise hall and in the return plenum of the HVAC system. Samples were collected twice weekly for 11 weeks. All samples were tested for 29 respiratory pathogens using PCR. We compared the ventilation system and exercise hall air with regard to the presence and quantity of pathogens. Findings: Samples collected in two locations in the exercise hall had a similar overall sensitivity to the HVAC sampler for detecting pathogens, while a third sampling location was associated with significantly lower sensitivity. Overall, the pathogen concentration was similar in the ventilation system and the exercise hall air (ratio: 1.0; 95% CI: 0.8–1.3). Interpretation: Our results show that air sampling within a ventilation system can have equal sensitivity for detecting respiratory pathogens, compared to room‐based sampling. Thus, placing samplers within central ventilation systems could increase the scalability of air sampling for infectious disease surveillance. [ABSTRACT FROM AUTHOR]

Published
2024
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12. Diagnostic accuracy of digital RNA quantification versus real-time PCR for the detection of respiratory syncytial virus in nasopharyngeal aspirates from children with acute respiratory infection

Author

Bouzas, Maiara L., Oliveira, Juliana R., Queiroz, Artur, Fukutani, Kiyoshi F., Barral, Aldina, Rector, Annabel, Wollants, Elke, Keyaerts, Els, Van der Gucht, Winke, Van Ranst, Marc, Beuselinck, Kurt, de Oliveira, Camila I., Van Weyenbergh, Johan, and Nascimento-Carvalho, Cristiana M.

Published
2018
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14. Blood Mucorales PCR to track down Aspergillus and Mucorales co-infections in at-risk hematology patients: A case-control study.

Author

Aerts, Robina, Bevers, Sien, Beuselinck, Kurt, Schauwvlieghe, Alexander, Lagrou, Katrien, and Maertens, Johan

Subjects
MIXED infections, CASE-control method, HEMATOLOGY, ASPERGILLUS, MEDICAL screening, ANTIFUNGAL agents
Abstract

Introduction: Serum Mucorales PCR can precede the final diagnosis of invasive mucormycosis by several days or weeks and could therefore be useful as a non-invasive screening tool. Methods: We assessed the performance of a commercial Mucorales PCR assay (MucorGenius®, PathoNostics, Maastricht, The Netherlands) on prospectively collected banked sera from hematology patients at risk for invasive mould infections. We evaluated if there is an underestimated incidence of missed Mucorales co-infections in patients with invasive aspergillosis (IA). We tested Mucorales PCR on the sera of all patients with a diagnosis of at least possible IA (EORTC-MSGERC consensus criteria) before the start of any antifungal therapy, and in a control group of similar high-risk hematology patients without IA (in a 1:4 ratio). When a positive Mucorales PCR was observed, at least 5 serum samples taken before and after the positive one were selected. Results: Mucorales PCR was performed in 46 diagnostic serum samples of cases and in 184 controls. Serum Mucorales PCR was positive in 4 cases of IA (8.7%; 12.9% of probable cases) and in 1 control case (0.5%) (p=0.0061, OR=17.43 (1.90-159.96). Post-mortem cultures of the positive control became positive for Rhizopus arrhizus. Mortality of IA cases with and without a positive Mucorales PCR was not significantly different. Only in the PCR positive control case, serial serum samples before and after the diagnostic sample were also positive. Discussion: It is not entirely clear what a positive Mucorales PCR in these cases implies since the 4 Mucorales PCR positive cases were treated with antifungals with activity against Mucorales. In addition, PCR was positive only once. This study does not provide enough evidence to implement Mucorales PCR screening. However, our findings emphasize once more the importance of considering the possibility of dual mould infections, even in patients with a positive galactomannan detection. [ABSTRACT FROM AUTHOR]

Published
2022
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15. Nationwide Harmonization Effort for Semi-Quantitative Reporting of SARS-CoV-2 PCR Test Results in Belgium.

Author

Cuypers, Lize, Bode, Jannes, Beuselinck, Kurt, Laenen, Lies, Dewaele, Klaas, Janssen, Reile, Capron, Arnaud, Lafort, Yves, Paridaens, Henry, Bearzatto, Bertrand, Cauchie, Mathieu, Huwart, Aline, Degosserie, Jonathan, Fagnart, Olivier, Overmeire, Yarah, Rouffiange, Arlette, Vandecandelaere, Ilse, Deffontaine, Marine, Pilate, Thomas, and Yin, Nicolas

Subjects
DIAGNOSTIC use of polymerase chain reaction, VIRAL shedding, CONTACT tracing, SUPPLY & demand, STANDARD deviations, MEDICAL personnel, OPTIMISM
Abstract

From early 2020, a high demand for SARS-CoV-2 tests was driven by several testing indications, including asymptomatic cases, resulting in the massive roll-out of PCR assays to combat the pandemic. Considering the dynamic of viral shedding during the course of infection, the demand to report cycle threshold (Ct) values rapidly emerged. As Ct values can be affected by a number of factors, we considered that harmonization of semi-quantitative PCR results across laboratories would avoid potential divergent interpretations, particularly in the absence of clinical or serological information. A proposal to harmonize reporting of test results was drafted by the National Reference Centre (NRC) UZ/KU Leuven, distinguishing four categories of positivity based on RNA copies/mL. Pre-quantified control material was shipped to 124 laboratories with instructions to setup a standard curve to define thresholds per assay. For each assay, the mean Ct value and corresponding standard deviation was calculated per target gene, for the three concentrations (107, 105 and 103 copies/mL) that determine the classification. The results of 17 assays are summarized. This harmonization effort allowed to ensure that all Belgian laboratories would report positive PCR results in the same semi-quantitative manner to clinicians and to the national database which feeds contact tracing interventions. [ABSTRACT FROM AUTHOR]

Published
2022
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17. No SARS‐CoV‐2 carriage observed in children attending daycare centers during the intial weeks of the epidemic in Belgium.

Author

Desmet, Stefanie, Ekinci, Esra, Wouters, Ine, Decru, Bram, Beuselinck, Kurt, Malhotra‐Kumar, Surbhi, and Theeten, Heidi

Subjects
DAY care centers, SARS-CoV-2, EPIDEMICS, COMMON cold, POLYMERASE chain reaction
Abstract

To gain knowledge about the role of young children attending daycare in the severe acute respiratory syndrome coronavirus 2 (SARS‐CoV‐2) epidemic, a random sample of children (n = 84) aged between 6 and 30 months attending daycare in Belgium was studied shortly after the start of the epidemic (February 29th) and before the lockdown (March 18th) by performing in‐house SARS‐CoV‐2 real‐time polymerase chain reaction. No asymptomatic carriage of SARS‐CoV‐2 was detected, whereas common cold symptoms were common (51.2%). Our study shows that in Belgium, there was no sign of early introduction into daycare centers at the moment children being not yet isolated at home, although the virus was clearly circulating. It is clear that more evidence is needed to understand the actual role of young children in the transmission of SARS‐CoV‐2 and their infection risk when attending daycare. [ABSTRACT FROM AUTHOR]

Published
2021
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18. Laboratory information system requirements to manage the COVID-19 pandemic: A report from the Belgian national reference testing center.

Author

Weemaes, Matthias, Martens, Steven, Cuypers, Lize, Elslande, Jan Van, Hoet, Katrien, Welkenhuysen, Joris, Goossens, Ria, Wouters, Stijn, Houben, Els, Jeuris, Kirsten, Laenen, Lies, Bruyninckx, Katrien, Beuselinck, Kurt, André, Emmanuel, Depypere, Melissa, Desmet, Stefanie, Lagrou, Katrien, Ranst, Marc Van, Verdonck, Ann K L C, and Goveia, Jermaine

Abstract

Objective: The study sought to describe the development, implementation, and requirements of laboratory information system (LIS) functionality to manage test ordering, registration, sample flow, and result reporting during the coronavirus disease 2019 (COVID-19) pandemic.Materials and Methods: Our large (>12 000 000 tests/y) academic hospital laboratory is the Belgian National Reference Center for severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) testing. We have performed a moving total of >25 000 SARS-CoV-2 polymerase chain reaction tests in parallel to standard routine testing since the start of the outbreak. A LIS implementation team dedicated to develop tools to remove the bottlenecks, primarily situated in the pre- and postanalytical phases, was established early in the crisis.Results: We outline the design, implementation, and requirements of LIS functionality related to managing increased test demand during the COVID-19 crisis, including tools for test ordering, standardized order sets integrated into a computerized provider order entry module, notifications on shipping requirements, automated triaging based on digital metadata forms, and the establishment of databases with contact details of other laboratories and primary care physicians to enable automated reporting. We also describe our approach to data mining and reporting of actionable daily summary statistics to governing bodies and other policymakers.Conclusions: Rapidly developed, agile extendable LIS functionality and its meaningful use alleviates the administrative burden on laboratory personnel and improves turnaround time of SARS-CoV-2 testing. It will be important to maintain an environment that is conducive for the rapid adoption of meaningful LIS tools after the COVID-19 crisis. [ABSTRACT FROM AUTHOR]

Published
2020
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19. Serial Detection of Circulating Mucorales DNA in Invasive Mucormycosis: A Retrospective Multicenter Evaluation.

Author

Mercier, Toine, Reynders, Marijke, Beuselinck, Kurt, Guldentops, Ellen, Maertens, Johan, and Lagrou, Katrien

Subjects
MUCORALES, FUNGAL DNA, MUCORMYCOSIS, BLOOD testing, MYCOSES, POLYMERASE chain reaction
Abstract

Invasive mucormycosis is a fungal infection with high mortality. Early diagnosis and initiation of appropriate treatment is essential to improve survival. However, current diagnostic tools suffer from low sensitivity, leading to delayed or missed diagnoses. Recently, several PCR assays for the detection of Mucorales DNA have been developed. We retrospectively assessed the diagnostic and kinetic properties of a commercial Mucorales PCR assay (MucorGenius®, PathoNostics) on serial blood samples from patients with culture-positive invasive mucormycosis and found an overall sensitivity of 75%. Importantly, a positive test preceded a positive culture result by up to 81 days (median eight days, inter-quartile range 1.75-16.25). After initiation of appropriate therapy, the average levels of circulating DNA decreased after one week and stabilized after two weeks. In conclusion, detection of circulating Mucorales DNA appears to be a good, fast diagnostic test that often precedes the final diagnosis by several days to weeks. This test could be especially useful in cases in which sampling for culture or histopathology is not feasible. [ABSTRACT FROM AUTHOR]

Published
2019
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22. Epidemiology of respiratory viruses in bronchoalveolar lavage samples in a tertiary hospital.

Author

Drieghe, Stefanie, Ryckaert, Inge, Beuselinck, Kurt, Lagrou, Katrien, and Padalko, Elizaveta

Subjects
*EPIDEMIOLOGY, *RESPIRATORY infections, *BRONCHOALVEOLAR lavage, *DISEASE prevalence, *IMMUNOCOMPROMISED patients, *VIRUS diseases, *POLYMERASE chain reaction, *PATIENTS
Abstract

Abstract: Background: The prevalence of respiratory viruses in adults is largely underexplored, as most studies focus on children. Additionally, in severely ill or immunocompromised adults, where respiratory infections are mostly attributed to bacteria and fungi; respiratory viruses can lead to severe complications. Objectives: To evaluate the epidemiology of respiratory viruses in bronchoalveolar lavage fluid (BAL) specimens from patients with lower respiratory tract disease. The study population consisted of different groups including immunocompetent patients (control patients), solid organ transplant recipients, patients with haematological malignancies and other immunocompromised adults. Study design: A total of 134 BAL fluid specimens collected during 2009–2011 were retrospectively assessed with the new commercial multiplex real-time PCR FTD Respiratory 21 Plus®, targeting 18 different viruses and 2 atypical bacterial pathogens. Results: Viral or atypical bacterial pathogens were detected in 29.1% of BAL fluid specimens. Coronaviruses were most prevalent (13.4%), followed by rhinoviruses (5.2%), RSV (4.5%) and bocaviruses (3.7%). Comparing the total number of viruses detected, a statistically significant difference was observed between the control group and patients with haematological malignancies (27.5% vs. 57.1%, p <0.05). Conclusion: In conclusion, our study highlights the high prevalence of respiratory viruses in BAL fluid specimens from adult patients with lower respiratory tract disease. The methods to be used should be sensitive and cover a wide range of potential pathogens. The specific patient population can also influence the detection rates of respiratory viruses. [Copyright &y& Elsevier]

Published
2014
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23. Nationwide Harmonization Effort for Semi-Quantitative Reporting of SARS-CoV-2 PCR Test Results in Belgium

Author

Lize Cuypers, Jannes Bode, Kurt Beuselinck, Lies Laenen, Klaas Dewaele, Reile Janssen, Arnaud Capron, Yves Lafort, Henry Paridaens, Bertrand Bearzatto, Mathieu Cauchie, Aline Huwart, Jonathan Degosserie, Olivier Fagnart, Yarah Overmeire, Arlette Rouffiange, Ilse Vandecandelaere, Marine Deffontaine, Thomas Pilate, Nicolas Yin, Isabel Micalessi, Sandrine Roisin, Veronique Moons, Marijke Reynders, Sophia Steyaert, Coralie Henin, Elena Lazarova, Dagmar Obbels, François E. Dufrasne, Hendri Pirenne, Raf Schepers, Anaëlle Collin, Bruno Verhasselt, Laurent Gillet, Stijn Jonckheere, Philippe Van Lint, Bea Van den Poel, Yolien Van der Beken, Violeta Stojkovic, Maria-Grazia Garrino, Hannah Segers, Kevin Vos, Maaike Godefroid, Valerie Pede, Friedel Nollet, Vincent Claes, Inge Verschraegen, Pierre Bogaerts, Marjan Van Gysel, Judith Leurs, Veroniek Saegeman, Oriane Soetens, Merijn Vanhee, Gilberte Schiettekatte, Evelyne Huyghe, Steven Martens, Ann Lemmens, Heleen Nailis, Kim Laffineur, Deborah Steensels, Elke Vanlaere, Jérémie Gras, Gatien Roussel, Koenraad Gijbels, Michael Boudewijns, Catherine Sion, Wim Achtergael, Wim Maurissen, Luc Iliano, Marianne Chantrenne, Geert Vanheule, Reinoud Flies, Nicolas Hougardy, Mario Berth, Vanessa Verbeke, Robin Morent, Anne Vankeerberghen, Sébastien Bontems, Kaat Kehoe, Anneleen Schallier, Giang Ho, Kristof Bafort, Marijke Raymaekers, Yolande Pypen, Amelie Heinrichs, Wim Schuermans, Dominique Cuigniez, Salah Eddine Lali, Stefanie Drieghe, Dieter Ory, Marie Le Mercier, Kristel Van Laethem, Inge Thoelen, Sarah Vandamme, Iqbal Mansoor, Carl Vael, Maxime De Sloovere, Katrien Declerck, Elisabeth Dequeker, Stefanie Desmet, Piet Maes, Katrien Lagrou, Emmanuel André, Dufrasne, Francois/0000-0001-6288-7936, Yin, Nicolas/0000-0003-1706-6869, Van Laethem, Kristel/0000-0001-6036-2271, Micalessi, Isabel, Ory , Dieter, Dequeker, Elisabeth, CLAES , Vincent, Verhasselt, Bruno, Moons, Veronique, Soetens, Oriane, Godefroid, Maaike, Verschraegen, Inge, Pirenne, Hendri, Gillet, Laurent, Heinrichs, Amelie, Huwart, Aline, Vanhee, Merijn, Vandamme, Sarah, Maurissen, Wim, Laenen , Lies, Reynders , Marijke, Thoelen, Inge, Gras, Jeremie, Berth, Mario, Obbels, Dagmar, Vanheule, Geert, Maes, Piet, Bafort, Kristof, Flies, Reinoud, Janssen, Reile, van den Poel, Bea, Bontems, Sebastien, Schepers , Raf, Overmeire, Yarah, Boudewijns, Michael, van der Beken, Yolien, Cuypers , Lize, Bode, Jannes, Vos, Kevin, Paridaens, Henry, Achtergael, Wim, Saegeman, Veroniek, Rouffiange, Arlette, Dewaele, Klaas, Pypen, Yolande, Yin, Nicolas, Drieghe, Stefanie, Nailis, Heleen, Kehoe, Kaat, DE SMET, Stefanie, Verbeke, Vanessa, Vanlaere, Elke, Vael, Carl, Van Laethem, Kristel, Segers, Hannah, Pede, Valerie, Deffontaine, Marine, Martens , Steven, Lemmens, Ann, Vankeerberghen, Anne, Lagrou, Katrien, Iliano, Luc, Chantrenne, Marianne, Laffineur, Kim, Bearzatto, Bertrand, Vandecandelaere, Ilse, Sion, Catherine, Andre, Emmanuel, Cuigniez, Dominique, Pilate, Thomas, Capron, Arnaud, Nollet, Friedel, Roisin, Sandrine, Gijbels, Koenraad, Van Lint, Philippe, Bogaerts, Pierre, Lafort, Yves, Henin, Coralie, Van Gysel, Marjan, Huyghe, Evelyne, Lali, Salah Eddine, Roussel, Gatien, Garrino, Maria-Grazia, Schuermans, Wim, Steyaert, Sophia, Le Mercier, Marie, De Sloovere, Maxime, Leurs, Judith, STEENSELS, Deborah, Declerck, Katrien, Dufrasne, Francois E., Fagnart, Olivier, Ho, Giang, Lazarova, Elena, Schallier, Anneleen, Beuselinck, Kurt, Morent, Robin, Hougardy, Nicolas, Raymaekers, Marijke, Jonckheere, Stijn, Stojkovic, Violeta, Degosserie, Jonathan, Cauchie, Mathieu, Schiettekatte, Gilberte, Collin, Anaelle, Mansoor, Iqbal, Faculty of Economic and Social Sciences and Solvay Business School, Faculty of Medicine and Pharmacy, Supporting clinical sciences, Microbiology and Infection Control, Clinical Biology, Experimental Pharmacology, Department of Clinical Microbiology, Faculty of Psychology and Educational Sciences, UCL - (MGD) Laboratoire de biologie clinique, and UCL - SSS/IREC/MONT - Pôle Mont Godinne

Subjects
SARS-CoV-2, PCR, semi-quantitative reporting, RNA copies/mL, infectivity, COVID-19/diagnosis, COVID-19, Real-Time Polymerase Chain Reaction, mL, Infectious Diseases, Belgium, SARS-CoV-2/genetics, Virology, Humans, RNA copies, Human medicine, Belgium/epidemiology, Pandemics
Abstract

From early 2020, a high demand for SARS-CoV-2 tests was driven by several testing indications, including asymptomatic cases, resulting in the massive roll-out of PCR assays to combat the pandemic. Considering the dynamic of viral shedding during the course of infection, the demand to report cycle threshold (Ct) values rapidly emerged. As Ct values can be affected by a number of factors, we considered that harmonization of semi-quantitative PCR results across laboratories would avoid potential divergent interpretations, particularly in the absence of clinical or serological information. A proposal to harmonize reporting of test results was drafted by the National Reference Centre (NRC) UZ/KU Leuven, distinguishing four categories of positivity based on RNA copies/mL. Pre-quantified control material was shipped to 124 laboratories with instructions to setup a standard curve to define thresholds per assay. For each assay, the mean Ct value and corresponding standard deviation was calculated per target gene, for the three concentrations (10(7), 10(5) and 10(3) copies/mL) that determine the classification. The results of 17 assays are summarized. This harmonization effort allowed to ensure that all Belgian laboratories would report positive PCR results in the same semi-quantitative manner to clinicians and to the national database which feeds contact tracing interventions. UZ/KU Leuven: as National Reference Center for Respiratory Pathogens, is supported by Sciensano, which is gratefully acknowledged. We would like to acknowledge additional staff members of the participating laboratories that contributed to this study: Jean-Luc Gala, Benoit Kabamba, Elsa Wiam, Valentin Coste, Paul Blanpain, Jean Ruelle, Ari Serbetciyan, Nicolas Pinte, Ophélie Simon and the entire UCLouvain federal testing platform COVID-19 team (all affiliation 4), Aurore Demars (affiliation 7), Laura Vanden Daele (affiliation 9), Hanne Valgaeren (affiliation 22), Guillaume Bayon-Vicente (affiliation 23), Fabrice Bureau, Claire Gourzonès and Joey Schyns (affiliation 28), Stéphanie Evrard (affiliation 42), Clara Ceyssens (affiliation 58), Jorn Hellemans (affiliation 77), Bram Slechten (affiliation 86) and the entire team of the laboratory of microbiology of UZA (affiliation 89) and of the UZA Federal testing platform COVID-19 (affiliation 85) for their boundless dedication.

Published
2022

24. Multicenter study of the performance of NTM Elite agar for the detection of nontuberculous mycobacteria from patients with cystic fibrosis.

Author

André E, Lorent N, Beuselinck K, Deiwick S, Dupont L, Gafsi J, Laenen L, Raymaekers L, Van Bleyenbergh P, Perry JD, and Kahl BC

Subjects
Humans, Bacteriological Techniques methods, Female, Male, Cystic Fibrosis microbiology, Cystic Fibrosis complications, Nontuberculous Mycobacteria isolation & purification, Nontuberculous Mycobacteria growth & development, Nontuberculous Mycobacteria genetics, Nontuberculous Mycobacteria classification, Mycobacterium Infections, Nontuberculous microbiology, Mycobacterium Infections, Nontuberculous diagnosis, Sputum microbiology, Agar, Culture Media chemistry
Abstract

The performance of a novel selective agar was evaluated against the performance of conventional mycobacterial cultures, i.e., a combination of the mycobacterial growth indicator tube (MGIT) with Löwenstein-Jensen (LJ), for the detection of nontuberculous mycobacteria (NTM) in sputum samples from people with cystic fibrosis (pwCF). Two hundred eighty-three sputum samples (231 fresh sputum and 52 spiked sputum) from 143 pwCF were collected. They were inoculated without prior decontamination on NTM Elite agar (30°C ± 2°C for 28 days) and inoculated on both MGIT and LJ (35°C-37°C for 6-8 weeks) after N-acetyl-L-cysteine-2% sodium hydroxide decontamination. NTM were identified by Matrix-Assisted Laser Desorption Ionization/Time of Flight Mass Spectrometry and/or PCR, and whole-genome sequencing. A total of 67 NTM were recovered overall by the combination of all culture media. NTM Elite agar allowed the recovery of 65 NTM (97%), compared to 22 for the conventional MGIT and LJ media combination (32.8%), including 22 NTM for MGIT (32.8%) and 3 NTM with the LJ medium (4.5%). For Mycobacterium abscessus complex, the sensitivity of NTM Elite agar was 95% compared with a sensitivity of 30% for the conventional MGIT and LJ media combination. Overall, 17.3% of cultures on NTM Elite agar were contaminated with other micro-organisms vs 46.3% on MGIT and 77% on LJ. This study shows that the novel selective agar (NTM Elite agar) significantly outperforms the conventional MGIT and LJ media combination in terms of sensitivity, selectivity, and ease of culture, without the requirement of an L3 laboratory.IMPORTANCENontuberculous mycobacteria (NTM) are significant pulmonary pathogens in patients with pre-existing structural lung conditions such as cystic fibrosis, bronchiectasis, or chronic obstructive pulmonary disease. Mycobacterium avium complex and Mycobacterium abscessus complex (MABSC) are the most frequently isolated organisms. Compared to the recommended culture method for NTM, which combines solid and liquid culture media, NTM Elite agar enables a faster/easier diagnosis and speeds up identification and susceptibility testing as the final reading is at 28 days instead of 6-8 weeks for the conventional mycobacterial cultures. In addition, for the NTM Elite agar, no decontamination stage before inoculation is necessary, unlike the conventional mycobacterial cultures. NTM Elite agar is derived from a formulation of medium adapted to rapidly growing mycobacteria (RGM). The medium enables the growth of RGM while suppressing other flora. It is supported with published clinical data showing the benefits of this medium., Competing Interests: J.G. is an employee of bioMérieux. The Newcastle upon Tyne Hospitals, UK, represented by John Perry, receive ongoing funding from bioMérieux, France, for the development and evaluation of culture media. UZ Leuven and Munster University Hospital received funding from bioMérieux, France, for the evaluation of NTM culture media.

Published
2024
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25. Beta-d-Glucan for Diagnosing Pneumocystis Pneumonia: a Direct Comparison between the Wako β-Glucan Assay and the Fungitell Assay.

Author

Mercier T, Guldentops E, Patteet S, Beuselinck K, Lagrou K, and Maertens J

Subjects
Biomarkers, Case-Control Studies, Humans, Pneumocystis carinii classification, Pneumocystis carinii genetics, Pneumonia, Pneumocystis microbiology, ROC Curve, Reproducibility of Results, Sensitivity and Specificity, Molecular Diagnostic Techniques methods, Molecular Diagnostic Techniques standards, Pneumonia, Pneumocystis blood, Pneumonia, Pneumocystis diagnosis, beta-Glucans blood
Abstract

Measuring serum beta-d-glucan (BDG) is a useful tool for supporting a quantitative PCR (qPCR)-based diagnosis of suspected Pneumocystis pneumonia (PCP) with bronchoalveolar lavage (BAL) fluid. Since the 2000s, the Fungitell assay was the only BDG assay which was FDA cleared and Conformité Européenne (CE) marked. However, the Wako β-glucan test was also recently CE marked and commercialized. We analyzed archived sera from 116 PCP cases (who were considered to have PCP based on compatible clinical and radiological findings plus a BAL fluid qPCR threshold cycle value of ≤28) and 114 controls (those with a BAL fluid qPCR threshold cycle value of >45 and no invasive fungal infection) using the Fungitell and Wako assays in parallel and assessed their diagnostic performance using the manufacturer's proposed cutoffs of 80 pg/ml and 11 pg/ml, respectively. We found the Wako assay to be more specific (0.98 versus 0.87, P  < 0.001) and the Fungitell assay to be more sensitive (0.78 versus 0.85, P  = 0.039) at the proposed cutoffs. Overall performance, as determined by the area under the receiver operating characteristic curve, was similar for both assays. We determined a new Wako assay cutoff (3.616 pg/ml) to match the sensitivity of the Fungitell assay (0.88 at a cutoff of ≥60 pg/ml). Using this newly proposed cutoff, the specificity of the Wako assay was significantly better than that of the Fungitell assay (0.89 versus 0.82, P  = 0.011). In conclusion, the Wako assay performed excellently compared to the Fungitell assay for the diagnosis of presumed PCP based on qPCR. In addition, contrary to the Fungitell assay, the Wako assay allows for single-sample testing with lower inter- and intrarun variability. Finally, we propose an optimized cutoff for the Wako assay to reliably exclude PCP., (Copyright © 2019 American Society for Microbiology.)

Published
2019
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26. Comparison of PCR-Electrospray Ionization Mass Spectrometry with 16S rRNA PCR and Amplicon Sequencing for Detection of Bacteria in Excised Heart Valves.

Author

Peeters B, Herijgers P, Beuselinck K, Peetermans WE, Herregods MC, Desmet S, and Lagrou K

Subjects
Bacteria chemistry, Bacteria classification, Bacteria genetics, False Negative Reactions, Humans, RNA, Ribosomal, 16S genetics, Retrospective Studies, Sensitivity and Specificity, Bacteria isolation & purification, Endocarditis diagnosis, Heart Valves microbiology, Polymerase Chain Reaction methods, Sequence Analysis, DNA methods, Spectrometry, Mass, Electrospray Ionization methods
Abstract

Identification of the causative pathogen of infective endocarditis (IE) is crucial for adequate management and therapy. A broad-range PCR-electrospray ionization mass spectrometry (PCR-ESI-MS) technique was compared with broad-spectrum 16S rRNA PCR and amplicon sequencing (16S rRNA PCR) for the detection of bacterial pathogens in 40 heart valves obtained from 34 definite infective endocarditis patients according to the modified Duke criteria and six nonendocarditis patients. Concordance between the two molecular techniques was 98% for being positive or negative, 97% for concordant identification up to the genus level, and 77% for concordant identification up to the species level. Sensitivity for detecting the causative pathogen (up to the genus level) in excised heart valves was 88% for 16S rRNA PCR and 85% for PCR-ESI-MS; the specificity was 83% for both methods. The two molecular techniques were significantly more sensitive than valve culture (18%) and accurately identified bacteria in excised heart valves. In eight patients with culture-negative IE, the following results were obtained: concordant detection of Coxiella burnetii (n = 2), Streptococcus gallolyticus (n = 1), Propionibacterium acnes (n = 1), and viridans group streptococci (n = 1) by both molecular tests, detection of P. acnes by PCR-ESI-MS whereas the 16S rRNA PCR was negative (n = 1), and a false-negative result by both molecular techniques (n = 2). In one case of IE caused by viridans streptococci, PCR-ESI-MS was positive for Enterococcus spp. The advantages of PCR-ESI-MS compared to 16S rRNA PCR are its automated workflow and shorter turnaround times., (Copyright © 2016, American Society for Microbiology. All Rights Reserved.)

Published
2016
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27. Detection of perinatal cytomegalovirus infection and sensorineural hearing loss in belgian infants by measurement of automated auditory brainstem response.

Author

Verbeeck J, Van Kerschaver E, Wollants E, Beuselinck K, Stappaerts L, and Van Ranst M

Subjects
Belgium, Case-Control Studies, Evoked Potentials, Auditory, Brain Stem, Follow-Up Studies, Humans, Infant, Infant, Newborn, Sensitivity and Specificity, Urine virology, Cytomegalovirus isolation & purification, Cytomegalovirus Infections complications, Hearing Loss, Sensorineural diagnosis, Polymerase Chain Reaction methods
Abstract

Since auditory disability causes serious problems in the development of speech and in the total development of a child, it is crucial to diagnose possible hearing impairment as soon as possible after birth. This study evaluates the neonatal hearing screening program in Flanders, Belgium. The auditory ability of 118,438 babies was tested using the automated auditory brainstem response. We selected 194 babies with indicative hearing impairment and 332 matched controls to investigate the association between the presence of human cytomegalovirus (HCMV) in urine samples and sensorineural hearing loss and to analyze the sensibility and specificity of a cell culture assay and a quantitative PCR detection method. Our results indicate that significantly more babies with confirmed hearing impairment were HCMV positive after birth. Further, based on the results of our study, babies with HCMV viral loads above 4.5 log copies/ml urine seem to be 1.4 times more likely to have confirmed hearing impairment. Our follow-up study suggests that the hearing impairment of children infected with HCMV after birth is less likely to improve than that of HCMV-negative infants. Our results confirm that the presence of HCMV before or shortly after birth influences the outcome of hearing impairment.

Published
2008
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28. Automated extraction of viral-pathogen RNA and DNA for high-throughput quantitative real-time PCR.

Author

Beuselinck K, van Ranst M, and van Eldere J

Subjects
Automation, Cytomegalovirus genetics, Cytomegalovirus isolation & purification, DNA Virus Infections diagnosis, DNA Virus Infections virology, DNA, Viral blood, Edetic Acid, Hepacivirus genetics, Hepacivirus isolation & purification, Hepatitis B virus genetics, Hepatitis B virus isolation & purification, Herpesvirus 4, Human genetics, Herpesvirus 4, Human isolation & purification, Humans, Indicators and Reagents, RNA Virus Infections diagnosis, RNA Virus Infections virology, RNA, Viral blood, Sensitivity and Specificity, DNA, Viral isolation & purification, Polymerase Chain Reaction methods, RNA, Viral isolation & purification
Abstract

The performance of the m1000 system (Abbott Laboratories, Illinois) as a front-end extraction system for high-throughput "in-house" quantitative real-time PCR assays was analyzed and compared to that of manual extraction of plasma and serum samples (hepatitis C virus [HCV] and hepatitis B virus [HBV]) and EDTA-blood samples (cytomegalovirus [CMV] and Epstein-Barr virus [EBV]). Linearity of extraction was tested on dilution series of HCV and HBV reference materials. The correlation coefficient for standard curves based on repeated extraction runs was 0.97 +/- 0.06 for HCV and 0.97 +/- 0.03 for HBV, indicating a linear extraction from 100 to 1.0 x 10(5) HCV IU/ml and from 100 to 1.0 x 10(6) HBV IU/ml. Intra- and interrun variability was below 0.23 log(10) IU/ml for 2.98 to 5.28 log(10) HCV IU/ml and 2.70 to 5.20 log(10) HBV IU/ml. Correlation between automated and manual extraction was very good. For HCV, the correlation coefficient was 0.91 and the mean difference in viral load was 0.13 log(10) HCV IU/ml. For HBV, the correlation coefficient was 0.98 and the mean difference in viral load 0.61 log(10) HBV IU/ml. For CMV and EBV, the correlation coefficient was 0.98 and the mean difference in viral load 0.33 log(10) copies/ml. Accuracy was confirmed with a reference panel (QCMD, Glasgow, Scotland) for all four assays. No cross-contamination was observed when extracting strongly positive polyomavirus samples (8.10 log(10) copies/ml) interspersed with polyomavirus-negative samples. Automated extraction via the m1000 system offers a high reliability of extraction and resulted in a strong reduction of the required extraction hands-on time for high-throughput PCR compared to manual extraction protocols.

Published
2005
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29. Molecular typing and epidemiology of enteroviruses identified from an outbreak of aseptic meningitis in Belgium during the summer of 2000.

Author

Thoelen I, Lemey P, Van Der Donck I, Beuselinck K, Lindberg AM, and Van Ranst M

Subjects
Adolescent, Adult, Belgium epidemiology, Child, Child, Preschool, DNA-Binding Proteins cerebrospinal fluid, DNA-Binding Proteins genetics, Enterovirus classification, Enterovirus isolation & purification, Enterovirus B, Human genetics, Enterovirus B, Human isolation & purification, Enterovirus Infections cerebrospinal fluid, Enterovirus Infections virology, Genotype, Humans, Infant, Meningitis, Aseptic cerebrospinal fluid, Meningitis, Aseptic virology, Molecular Epidemiology, Molecular Sequence Data, Phylogeny, Plant Proteins, Polymerase Chain Reaction methods, RNA, Viral analysis, Trans-Activators, Transcription Factors cerebrospinal fluid, Transcription Factors genetics, Disease Outbreaks, Enterovirus genetics, Enterovirus Infections epidemiology, Meningitis, Aseptic epidemiology
Abstract

Non-polio enteroviruses are the most common cause of aseptic meningitis worldwide. From May to September 2000, a major outbreak of aseptic meningitis occurred in Belgium. Cerebrospinal fluid samples (CSF) of 122 patients were found to contain enterovirus RNA using diagnostic RT-PCR that targeted a 231-bp gene fragment in the 5' noncoding region. In addition, a molecular typing method was developed based on RT-nested PCR and sequencing directly from CSF(a) 358-bp fragment in the aminoterminal part of the VP1 capsid protein. To identify the enterovirus type, nucleotide sequences of the VP1 amplicons were compared to all the enterovirus VP1 sequences available in GenBank. Echovirus 30 (31.2%), echovirus 13 (23.8%), and echovirus 6 (20.5%) were identified most frequently during the epidemic. Coxsackievirus B5 was present in 15.6% of the samples, and could be subdivided in two distinct epidemic clusters, coxsackievirus B5a (10.7%) and B5b (4.9%). Other enteroviruses encountered were echovirus 16 (5.7%), echovirus 18 (1.6%), coxsackievirus B4 (0.8%) and echovirus 7 (0.8%). The high prevalence of echovirus 13, considered previously a rare serotype, indicates it is an emerging epidemic type. To verify the typing results and to explore further the intratypical genetic variation, phylogenetic analysis was carried out. Geographical clustering of most of the strains within each type and subtype could be observed. The RT-nested PCR strategy, carried out directly on clinical samples, is a simple and rapid method for adequate molecular typing of the Group B enteroviruses causing aseptic meningitis., (Copyright 2003 Wiley-Liss, Inc.)

Published
2003
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