Your search keyword '"Dutly, F."' showing total 5 results

1. Lymphogranuloma venereum variant L2b-specific polymerase chain reaction: insertion used to close an epidemiological gap.

Author

Verweij SP, Catsburg A, Ouburg S, Lombardi A, Heijmans R, Dutly F, Frei R, Morré SA, and Goldenberger D

Subjects

Bacterial Outer Membrane Proteins genetics, Base Sequence, Chlamydia trachomatis genetics, Cross Reactions, DNA Primers genetics, Europe, Humans, Male, Molecular Sequence Data, Sensitivity and Specificity, Sequence Alignment, Sequence Analysis, DNA, Bacteriological Techniques methods, Chlamydia trachomatis classification, Chlamydia trachomatis isolation & purification, Lymphogranuloma Venereum diagnosis, Lymphogranuloma Venereum microbiology, Molecular Diagnostic Techniques methods, Polymerase Chain Reaction methods

Abstract

The management of the ongoing lymphogranuloma venereum epidemic in industrialized Western countries caused by Chlamydia trachomatis variant L2b still needs improvements in diagnosis, therapy and prevention. We therefore developed the first rapid C. trachomatis variant L2b-specific polymerase chain reaction to circumvent laborious ompA gene sequencing., (© 2011 The Authors. Clinical Microbiology and Infection © 2011 European Society of Clinical Microbiology and Infectious Diseases.)

Published

2011

2. Analysis of 721 Chlamydia trachomatis-positive urogenital specimens from men and women using lymphogranuloma venereum L2-specific real-time PCR assay.

Author

Goldenberger D, Dutly F, and Gebhardt M

Subjects

Adult, Bacteriuria epidemiology, Bacteriuria microbiology, Chlamydia Infections microbiology, Chlamydia Infections transmission, Chlamydia trachomatis classification, Chlamydia trachomatis genetics, Computer Systems, Disease Outbreaks, Europe epidemiology, Female, Heterosexuality, Homosexuality, Male, Humans, Lymphogranuloma Venereum epidemiology, Male, Proctitis epidemiology, Proctitis microbiology, Retrospective Studies, Sensitivity and Specificity, Serotyping, Switzerland epidemiology, Urethra microbiology, Urethritis epidemiology, Urethritis microbiology, Chlamydia Infections epidemiology, Chlamydia trachomatis isolation & purification, Genitalia, Female microbiology, Genitalia, Male microbiology, Lymphogranuloma Venereum microbiology, Polymerase Chain Reaction methods, Porins genetics, Urine microbiology

Published

2006

3. Detection of Tropheryma whipplei DNA in feces by PCR using a target capture method.

Author

Maibach RC, Dutly F, and Altwegg M

Subjects

Bacteriological Techniques, Base Sequence, Case-Control Studies, Feces microbiology, Humans, RNA, Bacterial genetics, RNA, Ribosomal, 16S genetics, RNA, Ribosomal, 23S genetics, Actinobacteria genetics, Actinobacteria isolation & purification, DNA, Bacterial genetics, DNA, Bacterial isolation & purification, Polymerase Chain Reaction methods, Whipple Disease diagnosis, Whipple Disease microbiology

Abstract

Whipple's disease is a rare multisystemic bacterial infection with variable clinical manifestations. For decades, the laboratory diagnosis was based on the demonstration of periodic acid Schiff-positive inclusions in macrophages of gastrointestinal biopsies. PCR has improved the diagnosis of Whipple's disease due to its increased sensitivity compared to histopathological analysis. To avoid invasive procedures for taking specimens, we have investigated the possibility of detecting Tropheryma whipplei DNA in feces rather than in biopsies or gastric aspirate of patients with and without Whipple's disease. Total bacterial DNA was isolated from stool specimens using Qiagen columns followed by a T. whipplei-specific hybridization step with a biotinylated capture probe and streptavidin-coated magnetic particles. The captured DNA was then amplified using the same seminested PCR targeting the 16S rRNA gene of the organism that had been applied to other specimens without capturing. For five of eight patients with Whipple's disease, duodenal biopsies and stool samples were PCR positive, whereas for the three other patients, both specimens were PCR negative. Of 84 patients without Whipple's disease, 75 tested negative in the duodenal biopsy and in the stool sample. For four, both specimens were positive. Five patients tested positive in the stool sample but not in the biopsy. However, for three of these five patients, the gastric aspirate had been PCR positive, indicating that the stool PCR result was true rather than false positive. Compared to PCR from duodenal biopsies, stool PCR has a sensitivity of 100% and a specificity of 97.3%. Additionally, 15 PCR-positive and 22 PCR-negative stool samples were extracted using the Invisorb Spin Stool DNA kit. The simplified stool extraction showed 93.3% sensitivity and 95.5% specificity compared to the target capture method. We conclude that PCR with stool specimens with either extraction method is a sensitive and specific diagnostic tool for the detection of T. whipplei DNA and one not requiring invasive sampling procedures.

Published

2002

4. Cloning and sequencing of a part of the heat shock protein 65 gene (hsp65) of "Tropheryma whippelii" and its use for detection of "T. whippelii" in clinical specimens by PCR.

Author

Morgenegg S, Dutly F, and Altwegg M

Subjects

Chaperonin 60, Cloning, Molecular, Heart Valves microbiology, Humans, Molecular Sequence Data, Peptide Fragments genetics, Sequence Analysis, DNA, Actinobacteria genetics, Actinomycetales Infections diagnosis, Bacterial Proteins, Chaperonins genetics, Polymerase Chain Reaction methods, Whipple Disease microbiology

Abstract

Using broad-spectrum primers, we have amplified, cloned, and sequenced a 620-bp fragment of the "Tropheryma whippelii" heat shock protein 65 gene (hsp65) from the heart valve of a patient with Whipple's endocarditis. The deduced amino acid sequence shows high similarity to those from actinobacteria, confirming that "T. whippelii" is indeed a member of this phylum. Based on the nucleotide sequence, we have developed a "T. whippelii"-specific seminested PCR. Seventeen patients shown to be positive by 16S ribosomal DNA (rDNA) PCR and/or internal transcribed spacer (ITS) PCR were also positive by hsp65 PCR. All 33 control specimens from patients without Whipple's disease and negative for "T. whippelii" by both seminested 16S rDNA and ITS PCR remained negative. All amplicons digested with XhoI revealed an identical restriction pattern. Eight of the 17 hsp65 amplicons representing all three previously described ITS types were sequenced. Three of the amplicons showed slight differences, but none of the mutations detected affected the amino acid sequence of the corresponding protein. We conclude that the hsp65 gene is a suitable target for the specific detection of "T. whippelii." Its product represents a putative antigen for a future serodiagnostic assay.

Published

2000

5. Evaluation of a specific nested PCR targeting domain III of the 23S rRNA gene of "Tropheryma whippelii" and proposal of a classification system for its molecular variants.

Author

Hinrikson HP, Dutly F, and Altwegg M

Subjects

Actinobacteria genetics, Actinobacteria isolation & purification, DNA, Ribosomal analysis, Evaluation Studies as Topic, Genetic Variation, Humans, RNA, Ribosomal, 16S genetics, Sequence Analysis, DNA, Actinobacteria classification, Genes, rRNA, Polymerase Chain Reaction methods, RNA, Ribosomal, 23S genetics, Whipple Disease microbiology

Abstract

"Tropheryma whippelii"-associated infections are usually confirmed histopathologically by using light microscopy. PCR assays targeting the 16S rRNA gene (16S rDNA) of "T. whippelii" are increasingly being applied for this purpose. Compared to microscopic analysis, PCR seems to be more sensitive, as indicated by the fact that several cases of Whipple's disease with negative histopathological findings but positive PCR results have been reported. Considering the lack of pathognomonic clinical features for this disease and the fact that "T. whippelii" DNA has repeatedly been found in patients without clinical Whipple's disease, such PCR results should be confirmed by additional tests. We have, therefore, evaluated a "T. whippelii"-specific nested PCR targeting domain III of the 23S rDNA with 41 clinical specimens known to contain "T. whippelii" 16S rDNA. All of these specimens were also positive for "T. whippelii" 23S rDNA. The specificity of the test was shown by sequencing of the amplicons and by the absence of amplicons in 38 negative controls. We consider this PCR test to be a suitable tool for confirming the presence of "T. whippelii" DNA in specimens with inconclusive histopathological findings. The information derived from sequencing of the partial "T. whippelii" 23S rDNA was then combined with our recent data of the 16S-23S rDNA spacer region of this organism. Overall, four different rDNA types are recognized in our proposed classification system for molecular variants of "T. whippelii." This preliminary scheme may provide a basis for further epidemiological and clinical studies with "T. whippelii" and associated diseases.

Published

2000