Your search keyword '"Myrtennäs K"' showing total 9 results

1. Phenotypic and genotypic discrimination of Francisella tularensis ssp. holarctica clades.

Author

Köppen K, Rydzewski K, Doellinger J, Myrtennäs K, Forsman M, Appelt S, Scholz H, and Heuner K

Subjects

Animals, Phylogeny, Zoonoses microbiology, Phenotype, Francisella tularensis genetics, Tularemia microbiology

Abstract

Francisella tularensis is the causative agent of tularemia, a zoonotic disease with a wide host range. F. tularensis ssp. holarctica (Fth) is of clinical relevance for European countries, including Germany. Whole genome sequencing methods, including canonical Single Nucleotide Polymorphism (canSNP) typing and whole genome SNP typing, have revealed that European Fth strains belong to a few monophyletic populations. The majority of German Fth isolates belong to two basal phylogenetic clades B.6 (biovar I) and B.12 (biovar II). Strains of B.6 and B.12 seem to differ in their pathogenicity, and it has been shown that strains of biovar II are resistant against erythromycin. In this study, we present data corroborating our previous data demonstrating that basal clade B.12 can be divided into clades B.71 and B.72. By applying phylogenetic whole genome analysis as well as proteome analysis, we could verify that strains of these two clades are distinct from one another. This was confirmed by measuring the intensity of backscatter light on bacteria grown in liquid media. Strains belonging to clades B.6, B.71 or B.72 showed clade-specific backscatter growth curves. Furthermore, we present the whole genome sequence of strain A-1341, as a reference genome of clade B.71, and whole proteomes comparison of Fth strains belonging to clades B.6, B.71 and B.72. Further research is necessary to investigate phenotypes and putative differences in pathogenicity of the investigated different clades of Fth to better understand the relationship between observed phenotypes, pathogenicity and distribution of Fth strains., Competing Interests: Declaration of Competing Interest All authors declare no conflict of interest., (Copyright © 2023 The Authors. Published by Elsevier GmbH.. All rights reserved.)

Published

2023

2. Genomic characterization of Francisella tularensis and other diverse Francisella species from complex samples.

Author

Wagner DM, Birdsell DN, McDonough RF, Nottingham R, Kocos K, Celona K, Özsürekci Y, Öhrman C, Karlsson L, Myrtennäs K, Sjödin A, Johansson A, Keim PS, Forsman M, and Sahl JW

Subjects

Animals, DNA, Bacterial genetics, Genomics, Humans, Phylogeny, RNA, Anti-Infective Agents, Francisella tularensis genetics, Tularemia microbiology

Abstract

Francisella tularensis, the bacterium that causes the zoonosis tularemia, and its genetic near neighbor species, can be difficult or impossible to cultivate from complex samples. Thus, there is a lack of genomic information for these species that has, among other things, limited the development of robust detection assays for F. tularensis that are both specific and sensitive. The objective of this study was to develop and validate approaches to capture, enrich, sequence, and analyze Francisella DNA present in DNA extracts generated from complex samples. RNA capture probes were designed based upon the known pan genome of F. tularensis and other diverse species in the family Francisellaceae. Probes that targeted genomic regions also present in non-Francisellaceae species were excluded, and probes specific to particular Francisella species or phylogenetic clades were identified. The capture-enrichment system was then applied to diverse, complex DNA extracts containing low-level Francisella DNA, including human clinical tularemia samples, environmental samples (i.e., animal tissue and air filters), and whole ticks/tick cell lines, which was followed by sequencing of the enriched samples. Analysis of the resulting data facilitated rigorous and unambiguous confirmation of the detection of F. tularensis or other Francisella species in complex samples, identification of mixtures of different Francisella species in the same sample, analysis of gene content (e.g., known virulence and antimicrobial resistance loci), and high-resolution whole genome-based genotyping. The benefits of this capture-enrichment system include: even very low target DNA can be amplified; it is culture-independent, reducing exposure for research and/or clinical personnel and allowing genomic information to be obtained from samples that do not yield isolates; and the resulting comprehensive data not only provide robust means to confirm the presence of a target species in a sample, but also can provide data useful for source attribution, which is important from a genomic epidemiology perspective., Competing Interests: The authors have declared that no competing interests exist.

Published

2022

3. Antibiotic susceptibility in vitro of Francisella tularensis subsp. holarctica isolates from Germany.

Author

Tomaso H, Hotzel H, Otto P, Myrtennäs K, and Forsman M

Subjects

Animals, Animals, Wild, Ciprofloxacin pharmacology, Doxycycline pharmacology, Foxes microbiology, Francisella tularensis classification, Francisella tularensis genetics, Genotype, Germany epidemiology, Humans, Microbial Sensitivity Tests methods, Raccoons microbiology, Real-Time Polymerase Chain Reaction, Rodentia microbiology, Tetracycline pharmacology, Ticks microbiology, Tularemia drug therapy, Tularemia epidemiology, Anti-Bacterial Agents pharmacology, Francisella tularensis drug effects, Tularemia microbiology

Abstract

Background: Tularaemia is a zoonotic disease caused by the bacterium Francisella tularensis. In Germany, the disease is still rare (e.g. 34 human cases reported in 2015). There is a lack of data about the susceptibility of F. tularensis strains to antibiotics, because many cases are diagnosed using serological assays only., Objectives: The antibiotic susceptibility in vitro of F. tularensis subsp. holarctica strains isolated in Germany was assessed to determine whether the currently recommended empirical therapy is still adequate., Methods: A total of 128 F. tularensis strains were investigated that were collected between 2005 and 2014 in Germany from wild animals, ticks and humans. All isolates were genotyped using real-time PCR assays targeting canonical SNPs, and antibiotic susceptibility was tested using MIC test strips on agar plates. MIC values were interpreted using CLSI breakpoints., Results: The strains were susceptible to antibiotics commonly recommended for tularaemia therapy, i.e. aminoglycosides (MIC90 values: gentamicin 1 mg/L; streptomycin 4.0 mg/L), tetracyclines (MIC90 values: tetracycline 0.5 mg/L; doxycycline 1.5 mg/L) and quinolones (MIC90 value: ciprofloxacin 0.064 mg/L). Chloramphenicol (MIC90 value: 3.0 mg/L) may be of value in treatment of tularaemia meningitis. Ninety-four isolates were susceptible to erythromycin, which defines biovar I (genotypes B.4 and B.6); 34 were resistant (biovar II; genotype B.12)., Conclusions: The F. tularensis isolates investigated in this study showed the typical antibiotic susceptibility pattern that was previously observed in other countries. Therefore, recommendations for empirical antibiotic therapy of tularaemia can remain unchanged. However, antibiotic susceptibility testing of clinical isolates should be performed whenever possible., (© The Author 2017. Published by Oxford University Press on behalf of the British Society for Antimicrobial Chemotherapy. All rights reserved. For Permissions, please email: journals.permissions@oup.com.)

Published

2017

4. High and novel genetic diversity of Francisella tularensis in Germany and indication of environmental persistence.

Author

Schulze C, Heuner K, Myrtennäs K, Karlsson E, Jacob D, Kutzer P, GROßE K, Forsman M, and Grunow R

Subjects

Animals, Germany epidemiology, Male, Phylogeny, Real-Time Polymerase Chain Reaction veterinary, Sequence Analysis, DNA veterinary, Tularemia epidemiology, Tularemia microbiology, Carnivora, Francisella tularensis genetics, Genetic Variation, Genome, Bacterial, Rodentia, Sus scrofa, Tularemia veterinary

Abstract

In Germany tularemia is a re-emerging zoonotic disease. Therefore, we investigated wild animals and environmental water samples for the presence and phylogenetic diversity of Francisella tularensis in the poorly studied Berlin/Brandenburg region. The phylogenomic analysis of three isolates from wild animals revealed three new subclades within the phylogenetic tree of F. tularensis [B.71 from a raccoon dog (Nyctereutes procyonoides); B.74 from a red fox (Vulpes vulpes), and B.75 from a Eurasian beaver (Castor fiber albicus)]. The results from histological, PCR, and genomic investigations on the dead beaver showed that the animal suffered from a systemic infection. Indications were found that the bacteria were released from the beaver carcass into the surrounding environment. We demonstrated unexpectedly high and novel phylogenetic diversity of F. tularensis in Germany and the fact that the bacteria persist in the environment for at least one climatic season. These findings support a broader host species diversity than previously known regarding Germany. Our data further support the assumption derived from previous serological studies of an underestimated frequency of occurrence of the pathogen in the environment and in wild animals. F. tularensis was isolated from animal species not previously reported as natural hosts in Germany.

Published

2016

5. Genomic analyses of Francisella tularensis strains confirm disease transmission from drinking water sources, Turkey, 2008, 2009 and 2012.

Author

Karadenizli A, Forsman M, Şimşek H, Taner M, Öhrman C, Myrtennäs K, Lärkeryd A, Johansson A, Özdemir L, and Sjödin A

Subjects

Disease Outbreaks, Francisella tularensis genetics, Humans, Polymerase Chain Reaction, Tularemia epidemiology, Turkey epidemiology, Water Microbiology, DNA, Bacterial genetics, Drinking Water microbiology, Francisella tularensis classification, Francisella tularensis isolation & purification, Genomics, Tularemia transmission

Abstract

Waterborne epidemics of tularaemia caused by Francisella tularensis are increasingly reported in Turkey. We have used whole genome sequencing to investigate if F. tularensis isolated from patients could be traced back to drinking water sources. Tonsil swabs from 33 patients diagnosed with oropharyngeal tularaemia in three outbreaks and 140 water specimens were analysed. F. tularensis subsp. holarctica was confirmed by microagglutination and PCR in 12 patients and five water specimens. Genomic analysis of three pairs of patient and water isolates from outbreaks in Sivas, Çorum, and Kocaeli showed the isolates to belong to two new clusters of the F. tularensis B.12 genetic clade. The clusters were defined by 19 and 15 single nucleotide polymorphisms (SNPs) in a multiple alignment based on 507 F. tularensis genomes. One synonymous SNP was chosen as a new canonical SNP (canSNP) for each cluster for future use in diagnostic assays. No SNP was identified between the genomes from the patient–water pair of isolates from Kocaeli, one SNP between the pair of isolates from Sivas, whereas the pair from Çorum differed at seven SNPs. These results illustrate the power of whole genome sequencing for tracing F. tularensis patient isolates back to their environmental source.

Published

2015

6. Phylogeography of Francisella tularensis subspecies holarctica in Finland, 1993-2011.

Author

Sissonen S, Rossow H, Karlsson E, Hemmilä H, Henttonen H, Isomursu M, Kinnunen PM, Pelkola K, Pelkonen S, Tarkka E, Myrtennäs K, Nikkari S, and Forsman M

Subjects

Animals, Bacterial Typing Techniques, DNA, Bacterial, Europe, Finland epidemiology, Francisella tularensis classification, Genome, Bacterial, Genotype, Humans, Phylogeny, Phylogeography, Polymerase Chain Reaction, Polymorphism, Single Nucleotide, Tularemia epidemiology, Francisella tularensis genetics, Francisella tularensis isolation & purification, Genetic Variation, Tularemia microbiology

Abstract

Background: Finland repeatedly reports some of the highest incidences of tularaemia worldwide. To determine genetic diversity of the aetiologic agent of tularaemia, Francisella tularensis, a total of 76 samples from humans (n = 15) and animals (n = 61) were analysed., Methods: We used CanSNPs and canINDEL hydrolysis or TaqMan MGB probes for the analyses, either directly from the clinical tissue samples (n = 21) or from bacterial isolates (n = 55)., Results: The genotypes of the strains were assigned to three previously described basal subspecies holarctica clades. The majority of strains (n = 67) were assigned to B.12, a clade reported to dominate in Scandinavia and Eastern Europe. A single strain was assigned to clade B.4, previously reported from North America, Europe and China. The remaining strains (n = 8) were members of clade B.6. Importantly, new diversity was discovered in clade B.6. We describe two newly designed TaqMan MGB probe assays for this new B.6 subclade B.70, and its previously identified sister clade B.11, a clade dominantly found in Western Europe., Conclusions: The high genetic diversity of F. tularensis subspecies holarctica present in Finland is consistent with previous findings in Sweden. The results suggest a northern and southern division of the B.6 subclade B.10, where B.11 predominates in Western and Central Europe and B.70 is found in Fennoscandia. Further research is required to define whether the vast diversity of genotypes found is related to different habitats or reservoir species, their different postglacial immigration routes to Fennoscandia, or dynamics of the reservoir species.

Published

2015

7. Hare-to-human transmission of Francisella tularensis subsp. holarctica, Germany.

Author

Otto P, Kohlmann R, Müller W, Julich S, Geis G, Gatermann SG, Peters M, Wolf PJ, Karlsson E, Forsman M, Myrtennäs K, and Tomaso H

Subjects

Animals, Genes, Bacterial, Germany, Humans, Polymorphism, Single Nucleotide, Tularemia microbiology, Zoonoses, Francisella tularensis genetics, Hares microbiology, Tularemia transmission

Abstract

In November 2012, a group of 7 persons who participated in a hare hunt in North Rhine-Westphalia, Germany, acquired tularemia. Two F. tularensis subsp. holarctica isolates were cultivated from human and hare biopsy material. Both isolates belonged to the FTN002-00 genetic subclade (derived for single nucleotide polymorphisms B.10 and B.18), thus indicating likely hare-to-human transmission.

Published

2015

8. Francisella tularensis subsp. tularensis group A.I, United States.

Author

Birdsell DN, Johansson A, Öhrman C, Kaufman E, Molins C, Pearson T, Gyuranecz M, Naumann A, Vogler AJ, Myrtennäs K, Larsson P, Forsman M, Sjödin A, Gillece JD, Schupp J, Petersen JM, Keim P, and Wagner DM

Subjects

Francisella tularensis genetics, Genome, Viral, Humans, Phylogeny, Phylogeography, Polymorphism, Single Nucleotide, Tularemia microbiology, United States epidemiology, Francisella tularensis classification, Tularemia epidemiology

Abstract

We used whole-genome analysis and subsequent characterization of geographically diverse strains using new genetic signatures to identify distinct subgroups within Francisella tularensis subsp. tularensis group A.I: A.I.3, A.I.8, and A.I.12. These subgroups exhibit complex phylogeographic patterns within North America. The widest distribution was observed for A.I.12, which suggests an adaptive advantage.

Published

2014

9. German Francisella tularensis isolates from European brown hares (Lepus europaeus) reveal genetic and phenotypic diversity.

Author

Müller W, Hotzel H, Otto P, Karger A, Bettin B, Bocklisch H, Braune S, Eskens U, Hörmansdorfer S, Konrad R, Nesseler A, Peters M, Runge M, Schmoock G, Schwarz BA, Sting R, Myrtennäs K, Karlsson E, Forsman M, and Tomaso H

Subjects

Animal Structures microbiology, Animals, Anti-Bacterial Agents pharmacology, Cluster Analysis, DNA, Bacterial genetics, DNA, Bacterial isolation & purification, Drug Resistance, Bacterial, Erythromycin pharmacology, Francisella tularensis isolation & purification, Genotype, Germany, Microbial Sensitivity Tests, Minisatellite Repeats, Molecular Typing, Phylogeography, Polymerase Chain Reaction, Tularemia microbiology, Francisella tularensis classification, Francisella tularensis genetics, Genetic Variation, Hares microbiology, Rodent Diseases microbiology, Tularemia veterinary

Abstract

Background: Tularemia is a zoonotic disease caused by Francisella tularensis that has been found in many different vertebrates. In Germany most human infections are caused by contact with infected European brown hares (Lepus europaeus). The aim of this study was to elucidate the epidemiology of tularemia in hares using phenotypic and genotypic characteristics of F. tularensis., Results: Cultivation of F. tularensis subsp. holarctica bacteria from organ material was successful in 31 of 52 hares that had a positive PCR result targeting the Ft-M19 locus. 17 isolates were sensitive to erythromycin and 14 were resistant. Analysis of VNTR loci (Ft-M3, Ft-M6 and Ft-M24), INDELs (Ftind33, Ftind38, Ftind49, RD23) and SNPs (B.17, B.18, B.19, and B.20) was shown to be useful to investigate the genetic relatedness of Francisella strains in this set of strains. The 14 erythromycin resistant isolates were assigned to clade B.I, and 16 erythromycin sensitive isolates to clade B.IV and one isolate was found to belong to clade B.II. MALDI-TOF mass spectrometry (MS) was useful to discriminate strains to the subspecies level., Conclusions: F. tularensis seems to be a re-emerging pathogen in Germany. The pathogen can easily be identified using PCR assays. Isolates can also be identified within one hour using MALDI-TOF MS in laboratories where specific PCR assays are not established. Further analysis of strains requires genotyping tools. The results from this study indicate a geographical segregation of the phylogenetic clade B.I and B.IV, where B.I strains localize primarily within eastern Germany and B.IV strains within western Germany. This phylogeographical pattern coincides with the distribution of biovar I (erythromycin sensitive) and biovar II (erythromycin resistance) strains. When time and costs are limiting parameters small numbers of isolates can be analysed using PCR assays combined with DNA sequencing with a focus on genetic loci that are most likely discriminatory among strains found in a specific area. In perspective, whole genome data will have to be investigated especially when terrorist attack strains need to be tracked to their genetic and geographical sources.

Published

2013