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2. How to: Surveillance of Clostridium difficile infections

Author

Allerberger, F., Delmée, M., Van Broeck, J., Vatcheva-Dobrevska, R., Dobreva, E., Matica, B., Pieridou, D., Krůtová, M., Nyč, O., Olesen, B., Märtin, P., Mentula, S., Barbut, F., Arvand, M., von Müller, L., Papaparaskevas, J., Pászti, J., Hajdu, Á., Gudnason, T., Burns, K., Spigaglia, P., Vulāne, K., Debacker, M., Scicluna, E., Melillo, T., Kuijper, E.J., Crobach, M.T., Kacelnik, O., Astrup, E., Pituch, H., Oleastro, M., Wiuff, C., Coia, J., Nováková, E., Kolman, J., Grilc, E., Rupnik, M., Bouza, E., Reigadas, E., Åkerlund, T., Tschudin-Sutter, S., Wilcox, M.H., Fairley, D., Morris, T., Krutova, M., Kinross, P., and Hajdu, A.

Published
2018
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5. Designation of the European Working Group on Legionella Infection (EWGLI) Amplified Fragment Length Polymorphism Types of Legionella pneumophila Serogroup 1 and Results of Intercentre Proficiency Testing Using a Standard Protocol

Author

Fry, N., Bangsborg, J., Bergmans, A., Bernander, S., Etienne, J., Franzin, L., Gaia, V., Hasenberger, P., Baladrón Jiménez, B., Jonas, D., Lindsay, D., Mentula, S., Papoutsi, A., Struelens, M., Uldum, S., Visca, P., Wannet, W., and Harrison, T.

Published
2002
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10. How to: Surveillance of Clostridium difficile infections

Author

Krutova, M., primary, Kinross, P., additional, Barbut, F., additional, Hajdu, A., additional, Wilcox, M.H., additional, Kuijper, E.J., additional, Allerberger, F., additional, Delmée, M., additional, Van Broeck, J., additional, Vatcheva-Dobrevska, R., additional, Dobreva, E., additional, Matica, B., additional, Pieridou, D., additional, Krůtová, M., additional, Nyč, O., additional, Olesen, B., additional, Märtin, P., additional, Mentula, S., additional, Arvand, M., additional, von Müller, L., additional, Papaparaskevas, J., additional, Pászti, J., additional, Hajdu, Á., additional, Gudnason, T., additional, Burns, K., additional, Spigaglia, P., additional, Vulāne, K., additional, Debacker, M., additional, Scicluna, E., additional, Melillo, T., additional, Crobach, M.T., additional, Kacelnik, O., additional, Astrup, E., additional, Pituch, H., additional, Oleastro, M., additional, Wiuff, C., additional, Coia, J., additional, Nováková, E., additional, Kolman, J., additional, Grilc, E., additional, Rupnik, M., additional, Bouza, E., additional, Reigadas, E., additional, Åkerlund, T., additional, Tschudin-Sutter, S., additional, Fairley, D., additional, and Morris, T., additional

Published
2018
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11. Survey of diagnostic and typing capacity for Clostridium difficile infection in Europe, 2011 and 2014

Author

Dorp, S.M. van, Notermans, D.W., Alblas, J., Gastmeier, P., Mentula, S., Nagy, E., Spigaglia, P., Ivanova, K., Fitzpatrick, F., Barbut, F., Morris, T., Wilcox, M.H., Kinross, P., Suetens, C., Kuijper, E.J., and European Clostridium Difficile Inf

Subjects
0301 basic medicine, Diarrhea, medicine.medical_specialty, Epidemiology, 030106 microbiology, Convenience sample, Polymerase Chain Reaction, Ribotyping, Microbiology, 03 medical and health sciences, 0302 clinical medicine, Virology, Environmental health, Surveys and Questionnaires, Medicine, Humans, 030212 general & internal medicine, Typing, Infection surveillance, business.industry, Clinical Laboratory Techniques, Clostridioides difficile, Public Health, Environmental and Occupational Health, Pcr ribotyping, Clostridium difficile, Europe, Population Surveillance, Clostridium Infections, business, Clinical Laboratory Information Systems, Laboratories
Abstract

Suboptimal laboratory diagnostics for Clostridium difficile infection (CDI) impedes its surveillance and control across Europe. We evaluated changes in local laboratory CDI diagnostics and changes in national diagnostic and typing capacity for CDI during the European C. difficile Infection Surveillance Network (ECDIS-Net) project, through cross-sectional surveys in 33 European countries in 2011 and 2014. In 2011, 126 (61%) of a convenience sample of 206 laboratories in 31 countries completed a survey on local diagnostics. In 2014, 84 (67%) of these 126 laboratories in 26 countries completed a follow-up survey. Among laboratories that participated in both surveys, use of CDI diagnostics deemed ‘optimal’ or ‘acceptable’ increased from 19% to 46% and from 10% to 15%, respectively (p C. difficile typing method increased from 22/31 countries in 2011 to 26/32 countries in 2014; for PCR ribotyping from 20/31 countries to 23/32 countries, and specifically for capillary PCR ribotyping from 7/31 countries to 16/32 countries. While our study indicates improved diagnostic capability and national capacity for capillary PCR ribotyping across European laboratories between 2011 and 2014, increased use of ‘optimal’ diagnostics should be promoted.

Published
2016

13. Lactobacillus reuteri DSM 17938 for managing infant colic: protocol for an individual participant data meta-analysis

Author

Sung, V, Cabana, MD, D'Amico, F, Deshpande, G, Dupont, C, Indrio, F, Mentula, S, Partty, A, Savino, F, Szajewska, H, Tancredi, D, Sung, V, Cabana, MD, D'Amico, F, Deshpande, G, Dupont, C, Indrio, F, Mentula, S, Partty, A, Savino, F, Szajewska, H, and Tancredi, D

Abstract

INTRODUCTION: Infant colic, or excessive crying of unknown cause in infants less than 3 months old, is common and burdensome. Its aetiology is undetermined, and consensus on its management is still lacking. Recent studies suggest a possible link between infant colic and gut microbiota, indicating probiotics to be a promising treatment. However, only a few strains have been tested, and results from randomised controlled trials are conflicting. It is important to clarify whether probiotics are effective for treating infant colic in general, and to identify whether certain subgroups of infants with colic would benefit from particular strains of probiotics. METHODS AND ANALYSIS: Through an individual participant data meta-analysis (IPDMA), we aim to identify whether the probiotic Lactobacillus reuteri DSM 17938 is effective in the management of infant colic, and to clarify whether its effects differ according to feeding method (breast vs formula vs combined), proton pump inhibitor exposure, and antibiotic exposure. The primary outcomes are infant crying duration and treatment success (at least 50% reduction in crying time from baseline) at 21 days postintervention. Individual participant data from all studies will be modelled simultaneously in multilevel generalised linear mixed-effects regression models to account for the nesting of participants within studies. Subgroup analyses of participant-level and intervention-level characteristics will be undertaken on the primary outcomes to assess if the intervention effect differs between certain groups of infants. ETHICS AND DISSEMINATION: Approved by the Royal Children's Hospital Human Research Ethics Committee (HREC 34081). Results will be reported in a peer-reviewed journal in 2015. TRIAL REGISTRATION NUMBER: PROSPERO CRD42014013210.

Published
2014

18. Designation of the European Working Group on Legionella Infection (EWGLI) amplified fragment length polymorphism types of Legionella pneumophila serogroup 1 and results of intercentre proficiency testing Using a standard protocol

Author

Fry, N K, Bangsborg, Jette Marie, Bergmans, A, Bernander, S, Etienne, J, Franzin, L, Gaia, V, Hasenberger, P, Baladrón Jiménez, B, Jonas, D, Lindsay, D, Mentula, S, Papoutsi, A, Struelens, M, Uldum, S A, Visca, P, Wannet, W, Harrison, T G, Fry, N K, Bangsborg, Jette Marie, Bergmans, A, Bernander, S, Etienne, J, Franzin, L, Gaia, V, Hasenberger, P, Baladrón Jiménez, B, Jonas, D, Lindsay, D, Mentula, S, Papoutsi, A, Struelens, M, Uldum, S A, Visca, P, Wannet, W, and Harrison, T G

Abstract

The utility of amplified fragment length polymorphism (AFLP) analysis as a genotyping method for the epidemiological typing of Legionella pneumophila serogroup 1 has been previously demonstrated. This study (i). reports recommendations for the designation of the European Working Group on Legionella Infections (EWGLI) AFLP types, (ii). describes the EWGLI AFLP types identified for the 130 strains in the EWGLI culture collection, and (iii). reports the results of a newly introduced international programme of proficiency testing. Following preliminary analysis of 20 epidemiologically unrelated isolates, 16 major AFLP types were identified. A coded proficiency panel, comprising 12 additional isolates representing 9 of these 16 AFLP types, was sent to 17 centres in 14 European countries where it was analysed following a previously determined standard protocol. The identity of each coded strain (recorded as AFLP type 001-016 or untypeable) was determined by participants with reference to these 16 AFLP types, either visually or using gel analysis software where available, and reported to the coordinating centre. Nine of the 12 strains, including an epidemiologically related pair and two pairs of unrelated isolates of the same type, were correctly identified to the correct AFLP type by all or all but one of the participants. Seven laboratories correctly identified all 12 isolates, and a further seven laboratories correctly identified 11. Type identification scores ranged from 75% (1 centre), 83% (2 centres), and 92% (7 centres) to 100% (7 centres). The AFLP method as described is robust and rapid and allows the genotypic comparison of isolates of Legionella pneumophila between different testing centres without the need for exchange of the strains studied.

Published
2002

21. Pan-European Study on Culture-Proven Legionnaires' Disease: Distribution of Legionella pneumophila Serogroups and Monoclonal Subgroups.

Author

Helbig, J. H., Bernander, S., Pastoris, M. Castellani, Etienne, J., Gaia, V., Lauwers, S., Lindsay, D., Lück, P. C., Marques, T., Mentula, S., Peeters, M. F., Pelaz, C., Struelens, M., Uldum, S. A., Wewalka, G., and Harrison, T. G.

Subjects
LEGIONNAIRES' disease, LEGIONELLA pneumophila, MONOCLONAL antibodies, MICROBIAL virulence, NOSOCOMIAL infections
Abstract

This pan-European study included unrelated strains of Legionella pneumophila obtained from 1,335 cases of Legionnaires' disease. The isolates were serotyped into the serogroups 1 to 15 by monoclonal antibodies (MAb) and/or rabbit antisera. Additionally, MAb subgrouping was undertaken for isolates belonging to serogroups 1, 4, and 5. Monoclonal types of serogroup 1 were subdivided as having, or not having, the virulence-associated epitope recognized by the MAb 3/1 (Dresden Panel). This epitope is not present on strains belonging to any other serogroups. Taking all Legionella incidents together, MAb 3/1-positive cases were most frequent (66.8%); 11.7% of the isolates belonged to MAb 3/1-negative serogroup 1 subgroups and 21.5% to other serogroups, with serogroups 3 and 6 predominating. Among all serotypes discriminated in this study, monoclonal subtype Philadelphia was the most frequent. If categories of infection were considered, the proportion of MAb 3/1-negative strains differed significantly (P<0.0005) between community-acquired cases (139/510; 27.3%) and travel-associated (42/295; 14.2%) or hospital-acquired infections (176/329; 53.5%). Moreover, taking distribution in different European areas into account, the proportion of MAb 3/1-negative strains was significantly higher in the Scandinavian region than in the Mediterranean countries or the UK for both community-acquired (48.7% vs. 18.6% or 12.0%; P<0.0005) and nosocomial cases (87.7% vs. 32.6% or 52.6%; P≤0.0007). [ABSTRACT FROM AUTHOR]

Published
2002
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23. Designation of the European Working Group on Legionella Infection (EWGLI) amplified fragment length polymorphism types of Legionella pneumophila serogroup 1 and results of intercentre proficiency testing Using a standard protocol

Author

L. Franzin, Marc Struelens, A.M.C. Bergmans, B. Baladrón Jiménez, Timothy G. Harrison, Norman K. Fry, Petra Hasenberger, Diane S. J. Lindsay, Sverker Bernander, Jette M Bangsborg, Jerome Etienne, Daniel Jonas, S. Mentula, Paolo Visca, Wim J. B. Wannet, Valeria Gaia, Androniki Papoutsi, Søren A. Uldum, Fry, Nk, Bangsborg, Jm, Bergmans, A, Bernander, S, Etienne, J, Franzin, L, Gaia, V, Hasenberger, P, BALADRON JIMENEZ, B, Jonas, D, Lindsay, D, Mentula, S, Papoutsi, A, Struelens, M, Uldum, Sa, Visca, Paolo, Wannet, W, and Harrison, Tg

Subjects
DNA, Bacterial, Male, Microbiology (medical), Genotype, Legionella, Sensitivity and Specificity, Legionella pneumophila, Microbiology, Cohort Studies, Humans, Typing, Serotyping, Legionella pneumophila Serogroup 1, Genotyping, Genetics, biology, Molecular epidemiology, General Medicine, bacterial infections and mycoses, biology.organism_classification, Bacterial Typing Techniques, Electrophoresis, Gel, Pulsed-Field, Europe, Infectious Diseases, Genes, Bacterial, Female, Amplified fragment length polymorphism, Legionnaires' Disease, Polymorphism, Restriction Fragment Length
Abstract

The utility of amplified fragment length polymorphism (AFLP) analysis as a genotyping method for the epidemiological typing of Legionella pneumophila serogroup 1 has been previously demonstrated. This study (i). reports recommendations for the designation of the European Working Group on Legionella Infections (EWGLI) AFLP types, (ii). describes the EWGLI AFLP types identified for the 130 strains in the EWGLI culture collection, and (iii). reports the results of a newly introduced international programme of proficiency testing. Following preliminary analysis of 20 epidemiologically unrelated isolates, 16 major AFLP types were identified. A coded proficiency panel, comprising 12 additional isolates representing 9 of these 16 AFLP types, was sent to 17 centres in 14 European countries where it was analysed following a previously determined standard protocol. The identity of each coded strain (recorded as AFLP type 001-016 or untypeable) was determined by participants with reference to these 16 AFLP types, either visually or using gel analysis software where available, and reported to the coordinating centre. Nine of the 12 strains, including an epidemiologically related pair and two pairs of unrelated isolates of the same type, were correctly identified to the correct AFLP type by all or all but one of the participants. Seven laboratories correctly identified all 12 isolates, and a further seven laboratories correctly identified 11. Type identification scores ranged from 75% (1 centre), 83% (2 centres), and 92% (7 centres) to 100% (7 centres). The AFLP method as described is robust and rapid and allows the genotypic comparison of isolates of Legionella pneumophila between different testing centres without the need for exchange of the strains studied.

Published
2002

24. Evaluation of the STANDARD M10 MDR-TB and MTB/NTM assays for the detection of Mycobacterium tuberculosis , rifampicin and isoniazid resistance, and nontuberculous mycobacteria in a low-incidence setting.

Author

Luukinen B, Aittoniemi J, Miikkulainen-Lahti T, Mentula S, and Pätäri-Sampo A

Subjects
Humans, Mycobacterium Infections, Nontuberculous microbiology, Mycobacterium Infections, Nontuberculous diagnosis, Antitubercular Agents pharmacology, Microbial Sensitivity Tests, Molecular Diagnostic Techniques methods, Incidence, Rifampin pharmacology, Isoniazid pharmacology, Nontuberculous Mycobacteria drug effects, Nontuberculous Mycobacteria genetics, Nontuberculous Mycobacteria isolation & purification, Sensitivity and Specificity, Mycobacterium tuberculosis drug effects, Mycobacterium tuberculosis genetics, Tuberculosis, Multidrug-Resistant microbiology, Tuberculosis, Multidrug-Resistant diagnosis
Abstract

Rapid detection is crucial for tuberculosis (TB) control. GeneXpert (Cepheid) is a widely used PCR system, known for its simplicity, random access, and point-of-care compatibility. SD BIOSENSOR recently introduced a similar system, STANDARD M10, including a Mycobacterium tuberculosis (MTB) and rifampicin (RIF) and isoniazid resistance (herein, MDR-TB) assay and an MTB/nontuberculous mycobacteria (NTM) assay. We evaluated these assays for the potential to replace the established Xpert MTB/RIF Ultra assay in a low-TB incidence setting. We analyzed 160 clinical respiratory samples (45 MTB-positive and 35 NTM-positive) and further 24 drug-resistant MTB, 30 mycobacterial species (2 MTB, 28 NTM), and 37 non-mycobacterial isolates. Compared with culture, clinical sensitivities and specificities for MTB detection were 88.9% (95% confidence interval [CI] = 76.1-95.6%) and 97.4% (CI = 92.3-99.4%) with Xpert Ultra, 88.9% (95% CI = 76.1-95.6%) and 98.3% (CI = 93.5-99.9%) with M10 MDR-TB, and 84.4% (CI = 70.9-94.4%) and 98.3% (CI = 93.5-99.9%) with M10 MTB/NTM, respectively. For NTM detection, M10 MTB/NTM showed sensitivity and specificity of 65.7% (CI = 49.1-79.2%) and 96.8% (CI = 91.8-99.0%). Compared with phenotypic drug susceptibility testing (DST), sensitivity and specificity for detecting RIF resistance were 100% (CI = 77.3-100%) and 95.6% (CI = 84.4-99.6%) with Xpert Ultra, and 100% (CI = 74.9-100%) and 95.5% (CI = 84.0-99.6%) with M10 MDR-TB. M10 MDR-TB showed 92.3% sensitivity (CI = 74.7-99.0%) and 100% specificity (CI = 87.3-100%) for detecting isoniazid resistance. All discrepancies in DST by PCR were concordant with whole-genome sequencing. While M10 MDR-TB demonstrated great potential as an alternative to Xpert Ultra, M10 MTB/NTM had limitations in NTM screening. Additionally, the M10 sputum pretreatment did not inactivate MTB efficiently, which should be considered in process risk assessment., Importance: The molecular diagnostic STANDARD M10 system is highly analogous to the widely established GeneXpert system, which significantly increases the relevance of this evaluation study in the field of rapid detection of M. tuberculosis . To our knowledge, this is the first clinical evaluation describing the performance of the STANDARD M10 MDR-TB and MTB/NTM assays, including an extensive analytical specificity panel (inclusivity and exclusivity) for the detection of M. tuberculosis , drug resistance, and nontuberculous mycobacteria., Competing Interests: The authors declare no conflict of interest.

Published
2024
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25. Transmission of drug-resistant Mycobacterium tuberculosis isolates between Finnish- and foreign-born cases, 2014-2021: A molecular epidemiological study.

Author

Zhu J, Haanpera M, Mentula S, Vapalahti O, Soini H, Sironen T, Kant R, and Zakham F

Subjects
Humans, Antitubercular Agents therapeutic use, Finland epidemiology, Molecular Epidemiology, Genotype, Mycobacterium tuberculosis genetics, Tuberculosis, Multidrug-Resistant diagnosis, Tuberculosis, Multidrug-Resistant drug therapy, Tuberculosis, Multidrug-Resistant epidemiology, Tuberculosis microbiology
Abstract

Background: Data on the molecular epidemiology and transmission of drug-resistant Mycobacterium tuberculosis (MTB) in low-incidence settings with immigration from high-incidence settings is limited., Method: We included 115 drug-resistant (DR) MTB isolates with whole-genome sequencing data isolated in Finland between 2014 and 2021. Potential transmission clusters were identified using a threshold of 12 single-nucleotide polymorphisms (SNPs). Highly related clusters were identified using a threshold of 5 SNPs., Result: Of the 115 DR MTB isolates, 31 (27.0%) isolates were from Finnish-born cases and 84 (73.0%) were from foreign-born cases. The proportion of multidrug-resistant (MDR) MTB isolates (30/84, 35.7%) from foreign-born cases was higher than that of MDR MTB isolates from Finnish-born cases (8/31, 25.8%). Lineage 2 (40/115, 34.8%) and lineage 4 (40/115, 34.8%) were the most prevalent lineages. A total of 25 (21.7%) isolates were classified into eight potential transmission clusters (≤12 SNPs). Furthermore, five highly related clusters (≤5 SNPs) were identified, including three DR MTB isolates from Finnish-born cases and 14 DR isolates from foreign-born cases., Conclusion: The risk of DR MTB transmission between Finnish- and foreign-born persons is not negligible. Further research on clustering analysis in drug-susceptible MTB is worth to inform tuberculosis management and control in low-incidence settings with increasing immigration., Competing Interests: Declaration of competing interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2024 The Authors. Published by Elsevier Ltd.. All rights reserved.)

Published
2024
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26. Tap water as the source of a Legionnaires' disease outbreak spread to several residential buildings and one hospital, Finland, 2020 to 2021.

Author

Mentula S, Kääriäinen S, Jaakola S, Niittynen M, Airaksinen P, Koivula I, Lehtola M, Mauranen E, Mononen I, Savolainen R, Haatainen S, and Lyytikäinen O

Subjects
Humans, Middle Aged, Aged, Aged, 80 and over, Finland epidemiology, Retrospective Studies, Hospitals, Water, Disease Outbreaks, Water Microbiology, Legionnaires' Disease diagnosis, Legionnaires' Disease epidemiology, Legionnaires' Disease microbiology, Legionella pneumophila
Abstract

In Finland, all microbiology laboratories notify Legionella findings and physicians notify Legionnaires' disease (LD) cases to the National Infectious Disease Register. All cases are interviewed, and water samples obtained from potential places of exposure. Legionella isolates from humans and water are compared by whole genome sequencing (WGS). In March 2021, Legionella pneumophila serogroup 1 (Lp 1) pneumonia cases increased in one Finnish city (120,000 inhabitants) where single LD cases are detected annually. We identified 12 LD cases, nine living in different residential buildings and three nosocomial, linked by identical human and/or water isolates. Three of these cases were from January 2020, October 2020 and February 2021 and identified retrospectively. Eleven were diagnosed by urinary antigen test, 10 by PCR and five by culture; age ranged between 52 and 85 years, and 10 had underlying diseases. Nine of 12 homes of LD cases and 15 of 26 water samples from the hospital were positive for Lp 1, with concentrations up to 640,000 cfu/L. Water samples from regional storage tanks were negative. Positivity in homes and the hospital suggested inadequate maintenance measures. Enhanced surveillance combined with WGS was crucial in detecting this unusual LD outbreak related to domestic and hospital water systems.

Published
2023
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27. External quality assessment by European mycobacterial laboratories: results of AFB microscopy and identification rounds.

Author

Mentula S, Paakkanen J, and Hyyryläinen HL

Subjects
Humans, Laboratories, Microscopy, Nontuberculous Mycobacteria, Sputum microbiology, Mycobacterium Infections, Nontuberculous diagnosis, Mycobacterium Infections, Nontuberculous microbiology, Mycobacterium tuberculosis
Abstract

We analyzed mycobacterial stain, culture and identification EQA data from altogether 134 laboratories in 15 mainly European countries over a 4-year period. The aim was to get an overview of the performance and methods and identify diagnostic challenges. The overall success rates for staining and identification were 94% and 91%. The false negative rate for staining was significantly higher for the medium positive than the strong positive slides (11% vs 4%). The false positive rate on negative slides was 10%, indicating contamination issues. The overall success of M. tuberculosis detection was high with error rates ranging from 0.7% to 1.2%. Pre- or postanalytical errors accounted for most of the unsuccessful responses. The detection of nontuberculous mycobacteria (NTM) was less consistent; accurate species identification depended on the assays used. Only 19% of participants performed species level identification for NTMs, 47% detected the presence NTMs while 21% focused on ruling out TB., Competing Interests: Declaration of competing interest The authors have no conflicts of interest to disclose., (Copyright © 2022 The Authors. Published by Elsevier Inc. All rights reserved.)

Published
2022
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28. Emerging source of infection - Mycobacterium tuberculosis in rescue dogs: a case report.

Author

Mentula S, Karkamo V, Skrzypczak T, Seppänen J, Hyyryläinen HL, Haanperä M, and Soini H

Abstract

Rescue dog activity is a heavily increasing form of dog charity. Imported homeless dogs represent a reservoir of zoonotic diseases putting owners, veterinarians and pathologists repeatedly at risk. The clinical signs of tuberculosis in a dog are non-specific and diagnosis is often delayed or dismissed. We present a case of 9 months of possible exposure at home and definite exposure at laparotomy and autopsy to intestinal tuberculosis in a family dog imported from Romania to Finland. Persistent gastrointestinal symptoms started 2 years after the import. Abdominal pain, diarrhoea and vomiting proceeded and led to spontaneous death. Mycobacterium tuberculosis was identified in the liver, lymph nodes and intestine at autopsy. Exposed persons were notified and follow-up was provided, and no further infections were identified within 12 months of follow-up. The heavily increasing import of companion animals presents unexpected public health risks, such as prolonged exposure to tuberculosis, of which the general public is not aware. The dramatic consequences and high costs of tuberculosis could be reduced through accessible information of the risks of imported animals to both the general public and veterinarians, in addition to availability of rapid diagnostics and proper personal protection., Competing Interests: The authors declare that there are no conflicts of interest., (© 2020 The Authors.)

Published
2020
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29. Prospective Evaluation of the mariPOC Test for Detection of Clostridioides difficile Glutamate Dehydrogenase and Toxins A/B.

Author

Savolainen R, Koskinen JM, Mentula S, Koskinen JO, and Kaukoranta SS

Subjects
Bacterial Proteins genetics, Clostridioides, Enterotoxins genetics, Feces, Finland, Glutamate Dehydrogenase genetics, Humans, Prospective Studies, Sensitivity and Specificity, Bacterial Toxins genetics, Clostridioides difficile genetics, Clostridium Infections diagnosis
Abstract

The objective of this study was to evaluate a novel automated random-access test, mariPOC CDI (ArcDia Ltd., Finland), for the detection of Clostridioides difficile glutamate dehydrogenase (GDH) and toxins A and B directly from fecal specimens. The mariPOC test was compared with both the GenomEra C. difficile PCR assay (Abacus Diagnostica Oy, Finland) and the TechLab C. diff Quik Chek Complete (Alere Inc.; now Abbot) membrane enzyme immunoassay (MEIA). Culture and the Xpert C. difficile assay (Cepheid Inc., USA) were used to resolve discrepant results. In total, 337 specimens were tested with the mariPOC CDI test and GenomEra PCR. Of these specimens, 157 were also tested with the TechLab MEIA. The sensitivity of the mariPOC test for GDH was slightly lower (95.2%) than that obtained with the TechLab assay (100.0%), but no toxin-positive cases were missed. The sensitivity of the mariPOC test for the detection of toxigenic C. difficile by analyzing toxin expression was better (81.6%) than that of the TechLab assay (71.1%). The analytical specificities for the mariPOC and the TechLab tests were 98.3% and 100.0% for GDH and 100.0% and 99.2% for toxin A/B, respectively. The analytical specificity of the GenomEra method was 100.0%. The mariPOC and TechLab GDH tests and GenomEra PCR had high negative predictive values of 99.3%, 98.3%, and 99.7%, respectively, in excluding infection with toxigenic C. difficile The mariPOC toxin A/B test and GenomEra PCR had an identical analytical positive predictive value of 100%, providing highly reliable information about toxin expression and the presence of toxin genes, respectively., (Copyright © 2020 American Society for Microbiology.)

Published
2020
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30. The recognition and characterisation of Finnish Clostridium difficile isolates resembling PCR-ribotype 027.

Author

Krutova M, Nyc O, Matejkova J, Kuijper EJ, Jalava J, and Mentula S

Subjects
ADP Ribose Transferases genetics, Adult, Aged, Aged, 80 and over, Anti-Bacterial Agents pharmacology, Bacterial Proteins genetics, Bacterial Toxins analysis, Bacterial Toxins genetics, Base Sequence, Clostridioides difficile classification, Clostridioides difficile drug effects, Clostridium Infections epidemiology, Clostridium Infections microbiology, DNA Gyrase genetics, DNA, Bacterial analysis, Drug Resistance, Bacterial, Enterotoxins genetics, Female, Finland, Fluoroquinolones pharmacology, Genotype, Humans, Male, Microbial Sensitivity Tests, Middle Aged, Minisatellite Repeats genetics, Molecular Epidemiology, Moxifloxacin, Multilocus Sequence Typing methods, Repressor Proteins genetics, Young Adult, Bacterial Typing Techniques, Clostridioides difficile genetics, Clostridioides difficile isolation & purification, Polymerase Chain Reaction methods, Ribotyping methods
Abstract

Purpose: To characterise and compare twenty-eight Finnish Clostridium difficile RT027-like isolates, selected based on the presence of 18 bp deletion in the tcdC gene and toxin gene profile (A, B, binary), with eleven RT027 isolates from different Finnish geographical areas and time periods., Methods: Twenty-eight C. difficile RT027-like isolates and 11 RT027 comparative strains were characterised by capillary-electrophoresis (CE) ribotyping, multi-locus variable tandem-repeats analysis (MLVA), multi-locus sequence typing (MLST), and sequencing of tcdC and gyrA gene fragments. Susceptibility to moxifloxacin was determined by E-test., Results: Of 28 RT027-like isolates, seven RTs (016, 034, 075, 080, 153, 176 and 328), three WEBRIBO types (411, 475, AI-78) and three new profiles (F1-F3) were identified. MLVA revealed six clonal complexes (RTs 016, 027, 176 and F3). MLST showed eleven sequence types (1, 41, 47, 67, 95, 191,192, 223, 229, 264 and new ST). Twenty-two isolates (RTs 016, 080, 176, 328, F1, F2, F3 and WRTAI-78) carried Δ117 in the tcdC gene. Isolates of RTs 016, 027 and 176 were moxifloxacin resistant and harboured Thr82Ile in the GyrA., Conclusion: Our results show a high diversity within 28 Finnish RT027-like C. difficile isolates, with twelve CE-ribotyping profiles and eleven STs. MLVA revealed the regional spread of RTs 016, 027, 176 and F3. The presence of Δ117 in the tcdC gene in eight non-027 RTs highlights the importance of careful interpretation of the results from molecular systems targeting this site in the genome of C. difficile and the need of strain typing for epidemiological purposes., (Copyright © 2017. Published by Elsevier B.V.)

Published
2018
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31. Lactobacillus reuteri to Treat Infant Colic: A Meta-analysis.

Author

Sung V, D'Amico F, Cabana MD, Chau K, Koren G, Savino F, Szajewska H, Deshpande G, Dupont C, Indrio F, Mentula S, Partty A, and Tancredi D

Subjects
Abdominal Pain diagnosis, Abdominal Pain etiology, Administration, Oral, Crying, Double-Blind Method, Female, Humans, Infant, Infant, Newborn, Male, Prognosis, Randomized Controlled Trials as Topic, Severity of Illness Index, Treatment Outcome, Colic diagnosis, Colic therapy, Limosilactobacillus reuteri, Probiotics therapeutic use
Abstract

Context: Lactobacillus reuteri DSM17938 has shown promise in managing colic, but conflicting study results have prevented a consensus on whether it is truly effective., Objective: Through an individual participant data meta-analysis, we sought to definitively determine if L reuteri DSM17938 effectively reduces crying and/or fussing time in infants with colic and whether effects vary by feeding type., Data Sources: We searched online databases (PubMed, Medline, Embase, the Cumulative Index to Nursing and Allied Health Literature, the Database of Abstracts of Reviews of Effects, and Cochrane), e-abstracts, and clinical trial registries., Study Selection: These were double-blind randomized controlled trials (published by June 2017) of L reuteri DSM17398 versus a placebo, delivered orally to infants with colic, with outcomes of infant crying and/or fussing duration and treatment success at 21 days., Data Extraction: We collected individual participant raw data from included studies modeled simultaneously in multilevel generalized linear mixed-effects regression models., Results: Four double-blind trials involving 345 infants with colic (174 probiotic and 171 placebo) were included. The probiotic group averaged less crying and/or fussing time than the placebo group at all time points (day 21 adjusted mean difference in change from baseline [minutes] -25.4 [95% confidence interval (CI): -47.3 to -3.5]). The probiotic group was almost twice as likely as the placebo group to experience treatment success at all time points (day 21 adjusted incidence ratio 1.7 [95% CI: 1.4 to 2.2]). Intervention effects were dramatic in breastfed infants (number needed to treat for day 21 success 2.6 [95% CI: 2.0 to 3.6]) but were insignificant in formula-fed infants., Limitations: There were insufficient data to make conclusions for formula-fed infants with colic., Conclusions: L reuteri DSM17938 is effective and can be recommended for breastfed infants with colic. Its role in formula-fed infants with colic needs further research., Competing Interests: POTENTIAL CONFLICT OF INTEREST: Dr Sung reports personal fees from Mead Johnson Nutrition outside the submitted work; Dr Tancredi reports personal fees from Pfizer Consumer Healthcare outside the submitted work; Dr Cabana reports personal fees from BioGaia outside the submitted work; Dr Szajewska reports personal fees from BioGaia outside the submitted work; and Dr Dupont reports on the following outside the submitted work: Nutricia Research’s Scientific Advisory Board, Nestle Health Science Scientific Advisory Board, Sodilac Consulting, and Novalac clinical trials. Dr Savino reports the following outside the submitted work: received fees for scientific consultancy from Nestlé Italia (Assago, Milan), HiPP GmbH & Company Vertrieb KG (Germany), and Danone Trading BV (Amsterdam); he receives royalties from Springer for the book Nutrizione Parenterale in Pediatria and declares that the book does not cover any interventions investigated in the article and is outside the submitted work; he has received travel grants, accommodations, and meeting expenses from Cana Pharmaceutical Laboratories (Iraklio, Attica), Radiotelevisione Italiana (Rome), Nestlé Italy, and Nestlé France; he has received personal fees from Mead Johnson Nutrition Italy, Cana Laboratories (Thessaloniki, Greece), Nutricia (part of Groupe Danone; Dubai, United Arab Emirates, and Kuwait); HiPP GmbH & Company Vertrieb KG (Germany), and Menarini Farmaceutica Internazionale (Firenze); and he declares that none of these companies had any input or involvement in any aspect of the manuscript conducted by him or have a real or vested interest in the findings of the article. Dr Indrio reports, outside of the submitted work, being a consultant for BioGaia for an educational program for its Web site and being a speaker for the bureaus for the Nestle Nutrition Institute, Abbot Danone, and BioGaia at scientific events and lectures; and the other authors have indicated they have no potential conflicts of interest to disclose., (Copyright © 2018 by the American Academy of Pediatrics.)

Published
2018
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32. Community- and Healthcare-Associated Clostridium difficile Infections, Finland, 2008-2013

Author

Kotila SM, Mentula S, Ollgren J, Virolainen-Julkunen A, and Lyytikäinen O

Subjects
Adolescent, Adult, Aged, Aged, 80 and over, Child, Child, Preschool, Clostridium Infections mortality, Female, Finland epidemiology, Humans, Incidence, Infant, Male, Middle Aged, Young Adult, Clostridioides difficile, Clostridium Infections epidemiology, Community-Acquired Infections epidemiology, Cross Infection epidemiology
Abstract

We evaluated incidence, case-fatality rate, and trends of community-associated (CA) and healthcare-associated (HA) Clostridium difficile infections (CDIs) in Finland during 2008-2013. CDIs were identified in the National Infectious Disease Register, deaths in the National Population Information System, hospitalizations to classify infections as CA or HA in the National Hospital Discharge Register, and genotypes in a reference laboratory. A total of 32,991 CDIs were identified: 10,643 (32.3%) were CA (32.9 cases/100,000 population) and 22,348 (67.7%) HA (69.1/100,000). Overall annual incidence decreased from 118.7/100,000 in 2008 to 92.1/100,000 in 2013, which was caused by reduction in HA-CDI rates (average annual decrease 8.1%; p<0.001). The 30-day case-fatality rate was lower for CA-CDIs than for HA-CDIs (3.2% vs. 13.3%; p<0.001). PCR ribotypes 027 and 001 were more common in HA-CDIs than in CA-CDIs. Although the HA-CDI incidence rate decreased, which was probably caused by increased awareness and improved infection control, the CA-CDI rate increased.

Published
2016
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33. Standardised surveillance of Clostridium difficile infection in European acute care hospitals: a pilot study, 2013.

Author

van Dorp SM, Kinross P, Gastmeier P, Behnke M, Kola A, Delmée M, Pavelkovich A, Mentula S, Barbut F, Hajdu A, Ingebretsen A, Pituch H, Macovei IS, Jovanović M, Wiuff C, Schmid D, Olsen KE, Wilcox MH, Suetens C, and Kuijper EJ

Subjects
Adolescent, Adult, Aged, Aged, 80 and over, Clinical Laboratory Techniques methods, Clostridioides difficile isolation & purification, Europe, Female, Humans, Male, Middle Aged, Pilot Projects, Polymerase Chain Reaction methods, Young Adult, Clinical Laboratory Techniques standards, Clostridioides difficile genetics, Clostridium Infections diagnosis, Polymerase Chain Reaction standards, Population Surveillance methods, Ribotyping standards
Abstract

Clostridium difficile infection (CDI) remains poorly controlled in many European countries, of which several have not yet implemented national CDI surveillance. In 2013, experts from the European CDI Surveillance Network project and from the European Centre for Disease Prevention and Control developed a protocol with three options of CDI surveillance for acute care hospitals: a 'minimal' option (aggregated hospital data), a 'light' option (including patient data for CDI cases) and an 'enhanced' option (including microbiological data on the first 10 CDI episodes per hospital). A total of 37 hospitals in 14 European countries tested these options for a three-month period (between 13 May and 1 November 2013). All 37 hospitals successfully completed the minimal surveillance option (for 1,152 patients). Clinical data were submitted for 94% (1,078/1,152) of the patients in the light option; information on CDI origin and outcome was complete for 94% (1,016/1,078) and 98% (294/300) of the patients in the light and enhanced options, respectively. The workload of the options was 1.1, 2.0 and 3.0 person-days per 10,000 hospital discharges, respectively. Enhanced surveillance was tested and was successful in 32 of the hospitals, showing that C. difficile PCR ribotype 027 was predominant (30% (79/267)). This study showed that standardised multicountry surveillance, with the option of integrating clinical and molecular data, is a feasible strategy for monitoring CDI in Europe., (This article is copyright of The Authors, 2016.)

Published
2016
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34. Survey of diagnostic and typing capacity for Clostridium difficile infection in Europe, 2011 and 2014.

Author

van Dorp SM, Notermans DW, Alblas J, Gastmeier P, Mentula S, Nagy E, Spigaglia P, Ivanova K, Fitzpatrick F, Barbut F, Morris T, Wilcox MH, Kinross P, Suetens C, and Kuijper EJ

Subjects
Clinical Laboratory Information Systems, Clostridioides difficile isolation & purification, Clostridium Infections epidemiology, Clostridium Infections microbiology, Diarrhea epidemiology, Europe epidemiology, Humans, Laboratories, Surveys and Questionnaires, Clinical Laboratory Techniques methods, Clostridioides difficile genetics, Clostridium Infections diagnosis, Polymerase Chain Reaction methods, Population Surveillance methods, Ribotyping
Abstract

Suboptimal laboratory diagnostics for Clostridium difficile infection (CDI) impedes its surveillance and control across Europe. We evaluated changes in local laboratory CDI diagnostics and changes in national diagnostic and typing capacity for CDI during the European C. difficile Infection Surveillance Network (ECDIS-Net) project, through cross-sectional surveys in 33 European countries in 2011 and 2014. In 2011, 126 (61%) of a convenience sample of 206 laboratories in 31 countries completed a survey on local diagnostics. In 2014, 84 (67%) of these 126 laboratories in 26 countries completed a follow-up survey. Among laboratories that participated in both surveys, use of CDI diagnostics deemed 'optimal' or 'acceptable' increased from 19% to 46% and from 10% to 15%, respectively (p  < 0.001). The survey of national capacity was completed by national coordinators of 31 and 32 countries in 2011 and 2014, respectively. Capacity for any C. difficile typing method increased from 22/31 countries in 2011 to 26/32 countries in 2014; for PCR ribotyping from 20/31 countries to 23/32 countries, and specifically for capillary PCR ribotyping from 7/31 countries to 16/32 countries. While our study indicates improved diagnostic capability and national capacity for capillary PCR ribotyping across European laboratories between 2011 and 2014, increased use of 'optimal' diagnostics should be promoted., (This article is copyright of The Authors, 2016.)

Published
2016
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35. Regional differences in Clostridium difficile infections in relation to fluoroquinolone and proton pump inhibitor use, Finland, 2008-2011.

Author

Kanerva M, Ollgren J, Voipio T, Mentula S, and Lyytikäinen O

Subjects
Anti-Bacterial Agents adverse effects, Clostridioides difficile classification, Clostridioides difficile genetics, Clostridioides difficile isolation & purification, Clostridium Infections prevention & control, Cross Infection epidemiology, Drug Utilization, Finland epidemiology, Humans, Incidence, Models, Statistical, Ribotyping, Risk Factors, Time Factors, Clostridium Infections epidemiology, Fluoroquinolones adverse effects, Proton Pump Inhibitors adverse effects
Abstract

Background: Several antimicrobial agents and proton pump inhibitors (PPIs) have been identified as risk factors for Clostridium difficile infections (CDIs). Nationwide laboratory-based surveillance of CDIs in Finland since 2008 has shown variation in regional CDI rates. We evaluated whether regional differences in CDI rates were associated with antibacterial and PPI use., Methods: Data on mean annual incidence rates of CDIs during 2008-2011 in 21 healthcare districts (HDs) were obtained from the National Infectious Disease Register, consumption (median annual use) of antimicrobials and PPIs from the Finnish Medical Agency, availability of molecular diagnostics by a laboratory survey and data on ribotypes from the national reference laboratory. The association over the 4 years was measured by incidence rate ratio (IRR) and we performed both bivariate and multivariate analyses., Results: During 2008-2011, PPI use increased 27% but fluoroquinolone use was stable. The level of fluoroquinolone use was strongly associated with the mean annual CDI incidence rate in different HDs over the 4-year period, but PPI use had less effect. The molecular diagnostics methodology and PCR ribotype 027 were not independently associated with CDI rate. The final multivariable model only included fluoroquinolone and PPI use; IRR for fluoroquinolones was 2.20 (95% confidence interval (CI), 1.32-3.67; p = 0.003)., Conclusions: Fluoroquinolone use may play a role in regional differences in CDI rates. Although the use has not recently increased, regionally targeted antimicrobial stewardship campaigns promoting appropriate use of fluoroquinolones should still be encouraged since they may decrease the incidence of CDIs.

Published
2015
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36. Differentiating virulent 027 and non-027 Clostridium difficile strains by molecular methods.

Author

Mentula S, Laakso S, Lyytikäinen O, and Kirveskari J

Subjects
Clostridium Infections diagnosis, Clostridium Infections microbiology, Genes, Bacterial, Humans, Polymerase Chain Reaction methods, Clostridioides difficile genetics, Clostridioides difficile pathogenicity, Ribotyping methods, Virulence genetics
Abstract

Objective: Hypervirulent Clostridium difficile clade has been shown to include several lineages of ribotype 027 and also other ribotypes. We present data on additional non-027 strains, identified as presumptive 027 by two commercial molecular C. difficile assays., Methods: The tested clinical isolates were selected from the national reference laboratory collection on the basis of toxin gene profile similarities with ribotype 027 and tested with XpertC. difficile/Epi and Amplidiag C. difficile+027 assay., Result: Xpert misclassified five ribotypes (016, 019, 080, 176 and variant of type 046) as presumptive 027 and Amplidiag two ribotypes (016, 176). The misclassified strains were rare, covering 1.6% of reference laboratory strain collection., Conclusion: Our findings confirm the concept that there are closely related outliers to hypervirulent 027 clones that can be misclassified as 027, and that these comprise numerous ribotypes, including previously reported four ribotypes (198, 176, 244, 019), and additional three (016, v046, 080) identified in the present study.

Published
2015
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37. Lactobacillus reuteri DSM 17938 for managing infant colic: protocol for an individual participant data meta-analysis.

Author

Sung V, Cabana MD, D'Amico F, Deshpande G, Dupont C, Indrio F, Mentula S, Partty A, Savino F, Szajewska H, and Tancredi D

Subjects
Humans, Infant, Treatment Outcome, Colic therapy, Limosilactobacillus reuteri, Probiotics therapeutic use
Abstract

Introduction: Infant colic, or excessive crying of unknown cause in infants less than 3 months old, is common and burdensome. Its aetiology is undetermined, and consensus on its management is still lacking. Recent studies suggest a possible link between infant colic and gut microbiota, indicating probiotics to be a promising treatment. However, only a few strains have been tested, and results from randomised controlled trials are conflicting. It is important to clarify whether probiotics are effective for treating infant colic in general, and to identify whether certain subgroups of infants with colic would benefit from particular strains of probiotics., Methods and Analysis: Through an individual participant data meta-analysis (IPDMA), we aim to identify whether the probiotic Lactobacillus reuteri DSM 17938 is effective in the management of infant colic, and to clarify whether its effects differ according to feeding method (breast vs formula vs combined), proton pump inhibitor exposure, and antibiotic exposure. The primary outcomes are infant crying duration and treatment success (at least 50% reduction in crying time from baseline) at 21 days postintervention. Individual participant data from all studies will be modelled simultaneously in multilevel generalised linear mixed-effects regression models to account for the nesting of participants within studies. Subgroup analyses of participant-level and intervention-level characteristics will be undertaken on the primary outcomes to assess if the intervention effect differs between certain groups of infants., Ethics and Dissemination: Approved by the Royal Children's Hospital Human Research Ethics Committee (HREC 34081). Results will be reported in a peer-reviewed journal in 2015., Trial Registration Number: PROSPERO CRD42014013210., (Published by the BMJ Publishing Group Limited. For permission to use (where not already granted under a licence) please go to http://group.bmj.com/group/rights-licensing/permissions.)

Published
2014
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38. Legionella longbeachae infection in a persistent hand-wound after a gardening accident.

Author

Mentula S, Pentikäinen J, Perola O, and Ruotsalainen E

Abstract

Introduction: Unlike other Legionella species, Legionella longbeachae has been associated with soil and potting composts instead of water systems, and it has caused pneumonia in gardeners., Case Presentation: We report, to our knowledge, the first case of prolonged localized L. longbeachae infection in an accidental wound on the back of a hand caused by a broken flowerpot., Conclusion: Identification of L. longbeachae requires awareness and expertise, since commercial tests are most often specific for L. pneumophila .

Published
2014
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39. Underdiagnosis of Clostridium difficile across Europe: the European, multicentre, prospective, biannual, point-prevalence study of Clostridium difficile infection in hospitalised patients with diarrhoea (EUCLID).

Author

Davies KA, Longshaw CM, Davis GL, Bouza E, Barbut F, Barna Z, Delmée M, Fitzpatrick F, Ivanova K, Kuijper E, Macovei IS, Mentula S, Mastrantonio P, von Müller L, Oleastro M, Petinaki E, Pituch H, Norén T, Nováková E, Nyč O, Rupnik M, Schmid D, and Wilcox MH

Subjects
Adolescent, Adult, Aged, Aged, 80 and over, Europe epidemiology, False Negative Reactions, Female, Health Services Research, Humans, Male, Middle Aged, Prospective Studies, Surveys and Questionnaires, Young Adult, Clostridioides difficile isolation & purification, Clostridium Infections diagnosis, Clostridium Infections epidemiology, Diagnostic Errors statistics & numerical data
Abstract

Background: Variations in testing for Clostridium difficile infection can hinder patients' care, increase the risk of transmission, and skew epidemiological data. We aimed to measure the underdiagnosis of C difficile infection across Europe., Methods: We did a questionnaire-based study at 482 participating hospitals across 20 European countries. Hospitals were questioned about their methods and testing policy for C difficile infection during the periods September, 2011, to August, 2012, and September, 2012, to August, 2013. On one day in winter, 2012-13 (December, 2012, or January, 2013), and summer, 2013 (July or August), every hospital sent all diarrhoeal samples submitted to their microbiology laboratory to a national coordinating laboratory for standardised testing of C difficile infection. Our primary outcome measures were the rates of testing for and cases of C difficile infection per 10 000 patient bed-days. Results of local and national C difficile infection testing were compared with each other. If the result was positive at the national laboratory but negative at the local hospital, the result was classified as undiagnosed C difficile infection. We compared differences in proportions with the Mann-Whitney test, or McNemar's test if data were matched., Findings: During the study period, participating hospitals reported a mean of 65·8 tests (country range 4·6-223·3) for C difficile infection per 10 000 patient-bed days and a mean of 7·0 cases (country range 0·7-28·7) of C difficile infection per 10 000 patient-bed days. Only two-fifths of hospitals reported using optimum methods for testing of C difficile infection (defined by European guidelines), although the number of participating hospitals using optimum methods increased during the study period, from 152 (32%) of 468 in 2011-12 to 205 (48%) of 428 in 2012-13. Across all 482 European hospitals on the two sampling days, 148 (23%) of 641 samples positive for C difficile infection (as determined by the national laboratory) were not diagnosed by participating hospitals because of an absence of clinical suspicion, equating to about 74 missed diagnoses per day., Interpretation: A wide variety of testing strategies for C difficile infection are used across Europe. Absence of clinical suspicion and suboptimum laboratory diagnostic methods mean that an estimated 40 000 inpatients with C difficile infection are potentially undiagnosed every year in 482 European hospitals., Funding: Astellas Pharmaceuticals Europe., (Copyright © 2014 Elsevier Ltd. All rights reserved.)

Published
2014
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40. Evaluation of a new automated homogeneous PCR assay, GenomEra C. difficile, for rapid detection of Toxigenic Clostridium difficile in fecal specimens.

Author

Hirvonen JJ, Mentula S, and Kaukoranta SS

Subjects
Adolescent, Adult, Aged, Aged, 80 and over, Bacteriological Techniques methods, Child, Clostridioides difficile genetics, Female, Finland, Humans, Male, Middle Aged, Predictive Value of Tests, Sensitivity and Specificity, Time Factors, Young Adult, Automation, Laboratory methods, Bacterial Toxins genetics, Clostridioides difficile isolation & purification, Clostridium Infections diagnosis, Feces microbiology, Molecular Diagnostic Techniques methods, Polymerase Chain Reaction methods
Abstract

We evaluated a new automated homogeneous PCR assay to detect toxigenic Clostridium difficile, the GenomEra C. difficile assay (Abacus Diagnostica, Finland), with 310 diarrheal stool specimens and with a collection of 33 known clostridial and nonclostridial isolates. Results were compared with toxigenic culture results, with discrepancies being resolved by the GeneXpert C. difficile PCR assay (Cepheid). Among the 80 toxigenic culture-positive or GeneXpert C. difficile assay-positive fecal specimens, 79 were also positive with the GenomEra C. difficile assay. Additionally, one specimen was positive with the GenomEra assay but negative with the confirmatory methods. Thus, the sensitivity and specificity were 98.8% and 99.6%, respectively. With the culture collection, no false-positive or -negative results were observed. The analytical sensitivity of the GenomEra C. difficile assay was approximately 5 CFU per PCR test. The short hands-on (<5 min for 1 to 4 samples) and total turnaround (<1 h) times, together with the high positive and negative predictive values (98.8% and 99.6%, respectively), make the GenomEra C. difficile assay an excellent option for toxigenic C. difficile detection in fecal specimens.

Published
2013
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41. Two Legionnaires' disease cases associated with industrial waste water treatment plants: a case report.

Author

Kusnetsov J, Neuvonen LK, Korpio T, Uldum SA, Mentula S, Putus T, Tran Minh NN, and Martimo KP

Subjects
Finland epidemiology, Humans, Industrial Waste, Legionella pneumophila classification, Legionnaires' Disease epidemiology, Male, Middle Aged, Pneumonia, Bacterial epidemiology, Waste Disposal, Fluid, Water Microbiology, Legionnaires' Disease diagnosis, Occupational Exposure, Pneumonia, Bacterial diagnosis
Abstract

Background: Finnish and Swedish waste water systems used by the forest industry were found to be exceptionally heavily contaminated with legionellae in 2005., Case Presentation: We report two cases of severe pneumonia in employees working at two separate mills in Finland in 2006. Legionella serological and urinary antigen tests were used to diagnose Legionnaires' disease in the symptomatic employees, who had worked at, or close to, waste water treatment plants. Since the findings indicated a Legionella infection, the waste water and home water systems were studied in more detail. The antibody response and Legionella urinary antigen finding of Case A indicated that the infection had been caused by Legionella pneumophila serogroup 1. Case A had been exposed to legionellae while installing a pump into a post-clarification basin at the waste water treatment plant of mill A. Both the water and sludge in the basin contained high concentrations of Legionella pneumophila serogroup 1, in addition to serogroups 3 and 13. Case B was working 200 meters downwind from a waste water treatment plant, which had an active sludge basin and cooling towers. The antibody response indicated that his disease was due to Legionella pneumophila serogroup 2. The cooling tower was the only site at the waste water treatment plant yielding that serogroup, though water in the active sludge basin yielded abundant growth of Legionella pneumophila serogroup 5 and Legionella rubrilucens. Both workers recovered from the disease., Conclusion: These are the first reported cases of Legionnaires' disease in Finland associated with industrial waste water systems.

Published
2010
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42. Diagnostic trends in Clostridium difficile detection in Finnish microbiology laboratories.

Author

Könönen E, Rasinperä M, Virolainen A, Mentula S, and Lyytikäinen O

Subjects
Bacterial Proteins analysis, Bacterial Proteins genetics, Bacterial Toxins analysis, Bacterial Toxins genetics, Bacteriological Techniques, Clinical Laboratory Techniques statistics & numerical data, Clostridioides difficile genetics, Clostridioides difficile pathogenicity, Clostridium Infections epidemiology, Clostridium Infections microbiology, Culture Media, Enterocolitis, Pseudomembranous microbiology, Enterotoxins analysis, Enterotoxins genetics, Feces chemistry, Feces microbiology, Finland, Humans, Polymerase Chain Reaction, Reagent Kits, Diagnostic, Surveys and Questionnaires, Clinical Laboratory Techniques trends, Clostridioides difficile isolation & purification, Clostridium Infections diagnosis, Enterocolitis, Pseudomembranous diagnosis, Microbiology
Abstract

Due to increased interest directed to Clostridium difficile-associated infections, a questionnaire survey of laboratory diagnostics of toxin-producing C. difficile was conducted in Finland in June 2006. Different aspects pertaining to C. difficile diagnosis, such as requests and criteria used for testing, methods used for its detection, yearly changes in diagnostics since 1996, and the total number of investigations positive for C. difficile in 2005, were asked in the questionnaire, which was sent to 32 clinical microbiology laboratories, including all hospital-affiliated and the relevant private clinical microbiology laboratories in Finland. The situation was updated by phone and email correspondence in September 2008. In June 2006, 28 (88%) laboratories responded to the questionnaire survey; 24 of them reported routinely testing requested stool specimens for C. difficile. Main laboratory methods included toxin detection (21/24; 88%) and/or anaerobic culture (19/24; 79%). In June 2006, 18 (86%) of the 21 laboratories detecting toxins directly from feces, from the isolate, or both used methods for both toxin A (TcdA) and B (TcdB), whereas only one laboratory did so in 1996. By September 2008, all of the 23 laboratories performing diagnostics for C. difficile used methods for both TcdA and TcdB. In 2006, the number of specimens processed per 100,000 population varied remarkably between different hospital districts. In conclusion, culturing C. difficile is common and there has been a favorable shift in toxin detection practice in Finnish clinical microbiology laboratories. However, the variability in diagnostic activity reported in 2006 creates a challenge for national monitoring of the epidemiology of C. difficile and related diseases.

Published
2009
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43. Detection of virulence genes of Clostridium difficile by multiplex PCR.

Author

Antikainen J, Pasanen T, Mero S, Tarkka E, Kirveskari J, Kotila S, Mentula S, Könönen E, Virolainen-Julkunen AR, Vaara M, and Tissari P

Subjects
Clostridioides difficile genetics, DNA, Bacterial analysis, Enterocolitis, Pseudomembranous microbiology, Humans, Sensitivity and Specificity, Bacterial Proteins genetics, Bacterial Toxins genetics, Clostridioides difficile isolation & purification, Clostridioides difficile pathogenicity, Enterocolitis, Pseudomembranous diagnosis, Enterotoxins genetics, Polymerase Chain Reaction methods, Repressor Proteins genetics
Abstract

Clostridium difficile strains belonging to the PCR ribotype 027, pulse-field gel electrophoresis (PFGE) type NAP1, toxinotype III and restriction endonuclease analysis group BI harbouring mutations in the tcdC gene and possessing binary toxin components A and B have been described to cause epidemics with increased morbidity and mortality. In the present study we developed a conventional multiplex PCR designed to detect selected virulence associated markers of the hypervirulent C. difficile PCR ribotype 027. The multiplex PCR assay detected the major toxins A and B, binary toxin components A and B as well as a possible deletion in the tcdC gene: a characteristic pattern of amplification products for the PCR ribotype 027 strains was detected. This rather simple method was specific for the screening of this hypervirulent C. difficile strain. The correlation between the multiplex PCR and PCR ribotyping methods was excellent. The sensitivity and specificity were 100% in our epidemiological situation. In conclusion, this multiplex PCR was found useful in the preliminary screening for the hypervirulent C. difficile PCR ribotype 027.

Published
2009
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44. P1A recombinant beta-lactamase prevents emergence of antimicrobial resistance in gut microflora of healthy subjects during intravenous administration of ampicillin.

Author

Tarkkanen AM, Heinonen T, Jõgi R, Mentula S, van der Rest ME, Donskey CJ, Kemppainen T, Gurbanov K, and Nord CE

Subjects
Adolescent, Adult, Ampicillin administration & dosage, Ampicillin Resistance, Drug Resistance, Bacterial, Female, Humans, Infusions, Intravenous, Male, Recombinant Proteins pharmacology, Ampicillin pharmacology, Anti-Bacterial Agents pharmacology, Intestines microbiology, beta-Lactamases pharmacology
Abstract

Ipsat P1A is a recombinant beta-lactamase which degrades antibiotic residue in the gastrointestinal tract. In an open-label, single-center controlled trial, 36 healthy subjects were randomized to receive (i) ampicillin (1 g intravenously [i.v.] every 6 h [q6h]), (ii) oral P1A recombinant beta-lactamase (8.2 mg q6h), or (iii) ampicillin (1 g i.v. q6h) in combination with oral P1A recombinant beta-lactamase (8.2 mg q6h) for 5 days. Fecal samples were collected before treatment, during treatment (days 3 to 5), and at follow-up (day 12). The primary end points were (i) changes in gastrointestinal microflora (determined by temperature gradient gel electrophoresis [TGGE]) and (ii) emergence of bacterial resistance (determined by conventional microbiology and PCR of TEM beta-lactamase genes). Thirty-five subjects completed the study. The mean similarity percentages of TGGE profiles between baseline and each treatment day sample were significantly lower for the ampicillin group than for the group receiving ampicillin plus P1A recombinant beta-lactamase on days 3, 4, and 5 (P < 0.001). Compared with the ampicillin group, subjects receiving ampicillin plus P1A recombinant beta-lactamase had significantly fewer ampicillin-resistant coliforms on days 3, 4, and 5 and at follow-up (P < or = 0.001) and fewer TEM beta-lactamase genes on days 3, 4, and 5 (P < 0.02). P1A recombinant beta-lactamase was safe and well tolerated. In healthy subjects, P1A recombinant beta-lactamase prevents ampicillin-induced alterations in intestinal microflora, emergence of resistance, and the number of TEM genes.

Published
2009
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45. First isolation of Clostridium difficile PCR ribotype 027 in Finland.

Author

Lyytikäinen O, Mentula S, Könönen E, Kotila S, Tarkka E, Anttila VJ, Mattila E, Kanerva M, Vaara M, and Valtonen V

Subjects
Adult, Aged, Clostridioides difficile genetics, Finland epidemiology, Humans, Male, Polymerase Chain Reaction, Ribotyping, Clostridioides difficile classification, Clostridioides difficile isolation & purification, Enterocolitis, Pseudomembranous diagnosis, Enterocolitis, Pseudomembranous epidemiology, Enterocolitis, Pseudomembranous microbiology
Published
2007
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46. Relatedness of Escherichia coli strains with different susceptibility patterns isolated from beagle dogs during ampicillin treatment.

Author

Mentula S, Virtanen T, Kanervo-Nordström A, Harmoinen J, Westermarck E, Rautio M, Huovinen P, and Könönen E

Subjects
Ampicillin pharmacology, Animals, Dogs, Electrophoresis, Gel, Pulsed-Field, Escherichia coli isolation & purification, Feces microbiology, Jejunum microbiology, Selection, Genetic, Ampicillin Resistance, Escherichia coli drug effects, Escherichia coli physiology
Abstract

The aim of this study was to investigate the effects of ampicillin treatment on selection and diversity of ampicillin-resistant intestinal Escherichia coli in beagles treated with ampicillin, ampicillin + beta-lactamase (targeted to degrade antibiotic residues in the gut) or placebo. Selected faecal (n = 339) and jejunal (n = 63) E. coli isolates with known resistance patterns were typed using pulsed-field gel electrophoresis (PFGE). Among the 25 detected PFGE types, ampicillin resistance was detected in 6, none of which was dominant over others among the dogs. The resistant types increased especially in the ampicillin group, whilst beta-lactamase inhibited their emergence. Selection of genetically unrelated resistant strains rather than emerging resistance among previously susceptible strains accounts for increasing resistance rates during ampicillin treatment.

Published
2006
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47. Comparison between cultured small-intestinal and fecal microbiotas in beagle dogs.

Author

Mentula S, Harmoinen J, Heikkilä M, Westermarck E, Rautio M, Huovinen P, and Könönen E

Subjects
Animals, Bacteria, Aerobic classification, Bacteria, Aerobic growth & development, Bacteria, Anaerobic classification, Bacteria, Anaerobic growth & development, Colony Count, Microbial, Culture Media, Dogs, Intestine, Small microbiology, Male, Bacteria, Aerobic isolation & purification, Bacteria, Anaerobic isolation & purification, Feces microbiology, Jejunum microbiology
Abstract

The microbiota of the small intestine is poorly known because of difficulties in sampling. In this study, we examined whether the organisms cultured from the jejunum and feces resemble each other. Small-intestinal fluid samples were collected from 22 beagle dogs with a permanent jejunal fistula in parallel with fecal samples. In addition, corresponding samples from seven of the dogs were collected during a 4-week period (days 4, 10, 14, and 28) to examine the stability of the microbiota. In the jejunal samples, aerobic/facultative and anaerobic bacteria were equally represented, whereas anaerobes dominated in the fecal samples. Despite lower numbers of bacteria in the jejunum (range, 10(2) to 10(6) CFU/g) than in feces (range, 10(8) to 10(11) CFU/g), some microbial groups were more prevalent in the small intestine: staphylococci, 64% versus 36%; nonfermentative gram-negative rods, 27% versus 9%; and yeasts, 27% versus 5%, respectively. In contrast, part of the fecal dominant microbiota (bile-resistant Bacteroides spp., Clostridium hiranonis-like organisms, and lactobacilli) was practically absent in the jejunum. Many species were seldom isolated simultaneously from both sample types, regardless of their overall prevalence. In conclusion, the small intestine contains a few bacterial species at a time with vastly fluctuating counts, opposite to the results obtained for the colon, where the major bacterial groups remain relatively constant over time. Qualitative and quantitative differences between the corresponding jejunal and fecal samples indicate the inability of fecal samples to represent the microbiotas present in the upper gut.

Published
2005
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48. Inhibition of ampicillin-induced emergence of resistance in intestinal coliforms by targeted recombinant beta-lactamase.

Author

Mentula S, Harmoinen J, Koski P, Westermarck E, Rautio M, Huovinen P, and Könönen E

Subjects
Administration, Oral, Ampicillin administration & dosage, Ampicillin pharmacology, Ampicillin Resistance genetics, Ampicillin Resistance physiology, Animals, Dogs, Feces microbiology, Hydrogen-Ion Concentration, Jejunum drug effects, Jejunum microbiology, Recombinant Proteins administration & dosage, Recombinant Proteins pharmacology, Tablets, Enteric-Coated, beta-Lactamases administration & dosage, beta-Lactamases genetics, Ampicillin metabolism, Ampicillin Resistance drug effects, Digestive System enzymology, beta-Lactamases pharmacology
Abstract

The aim of the present study was to determine whether oral targeted recombinant beta-lactamase (TRBL) administration could overcome the development of ampicillin-induced resistance in the gut microbiota. Eighteen laboratory beagles with permanent jejunal fistula were randomised to receive ampicillin + placebo, ampicillin + TRBL or placebo. A total of 982 coliform isolates, collected from jejunal and faecal samples before, during and after the treatment were tested against nine antimicrobials. The proportion of ampicillin resistance (multi-resistance) among coliform isolates increased from 20 to 36% in the ampicillin + placebo group but far less, 20-36%, in the ampicillin + TRBL group. These results indicate that TRBL may prevent the emergence of beta-lactam-associated resistance in coliforms in the gut.

Published
2004
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49. Orally administered targeted recombinant Beta-lactamase prevents ampicillin-induced selective pressure on the gut microbiota: a novel approach to reducing antimicrobial resistance.

Author

Harmoinen J, Mentula S, Heikkilä M, van der Rest M, Rajala-Schultz PJ, Donskey CJ, Frias R, Koski P, Wickstrand N, Jousimies-Somer H, Westermarck E, and Lindevall K

Subjects
Administration, Oral, Ampicillin administration & dosage, Ampicillin pharmacokinetics, Ampicillin Resistance genetics, Animals, Digestive System drug effects, Dogs, Escherichia coli drug effects, Escherichia coli enzymology, Feces microbiology, Infusions, Parenteral, Jejunum microbiology, Male, Penicillins administration & dosage, Penicillins pharmacokinetics, Recombinant Proteins pharmacology, Tablets, Enteric-Coated, beta-Lactamases administration & dosage, beta-Lactamases genetics, Ampicillin pharmacology, Ampicillin Resistance physiology, Digestive System microbiology, Penicillins pharmacology, beta-Lactamases pharmacology
Abstract

Antibiotics that are excreted into the intestinal tract promote antibiotic resistance by exerting selective pressure on the gut microbiota. Using a beagle dog model, we show that an orally administered targeted recombinant beta-lactamase enzyme eliminates the portion of parenteral ampicillin that is excreted into the small intestine, preventing ampicillin-induced changes to the fecal microbiota without affecting ampicillin levels in serum. In dogs receiving ampicillin, significant disruption of the fecal microbiota and the emergence of ampicillin-resistant Escherichia coli and TEM genes were observed, whereas in dogs treated with ampicillin in combination with an oral beta-lactamase, these did not occur. These results suggest a new strategy for reducing antimicrobial resistance in humans.

Published
2004
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50. A newborn with domestically acquired legionnaires disease confirmed by molecular typing.

Author

Skogberg K, Nuorti JP, Saxen H, Kusnetsov J, Mentula S, Fellman V, Mäki-Petäys N, and Jousimies-Somer H

Subjects
DNA, Bacterial analysis, Environment, Female, Humans, Infant, Newborn, Legionella genetics, Legionnaires' Disease epidemiology, Legionella isolation & purification, Legionnaires' Disease microbiology
Abstract

Legionella pneumophila serogroup 6 was recovered from a bronchoalveolar lavage specimen from a 1-week-old, full-term newborn with pneumonia, as well as from water samples from the maternity hospital and the newborn's home (an apartment). Amplified fragment-length polymorphism typing revealed that the strains isolated from the newborn and her home were indistinguishable from each other but were clearly different from the hospital and control strains. To our knowledge, this is the first report of domestic acquisition of legionnaires disease in a newborn to have been confirmed by molecular typing.

Published
2002
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