Your search keyword '"Viljanen MK"' showing total 13 results

1. Application of Bacillus anthracis PCR to simulated clinical samples.

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Author

Rantakokko-Jalava K and Viljanen MK

Subjects

Anthrax blood, Bacillus anthracis genetics, DNA, Bacterial chemistry, DNA, Bacterial genetics, Humans, Nasal Mucosa microbiology, Sensitivity and Specificity, Spores, Bacterial, Stem Cells, Anthrax microbiology, Bacillus anthracis isolation & purification, Polymerase Chain Reaction methods

Abstract

We evaluated PCR for the detection of Bacillus anthracis DNA from simulated clinical specimens relevant for the microbiological diagnosis of anthrax or exposure to B. anthracis spores. In simulated blood specimens, the lowest limit of detection was 400 CFU per mL of blood, which may be sufficient for samples from patients with septic anthrax. Screening nasal swabs by PCR may not be sensitive enough to rule out dangerous exposure to anthrax spores, as a minimum of 2000 spores per sample was required for detectable amplification. As spores survived some standard DNA purification methods, special attention should be paid to laboratory safety when preparing samples possibly containing live spores. more...

Published

2003

2. Semiquantitative detection by real-time PCR of Aspergillus fumigatus in bronchoalveolar lavage fluids and tissue biopsy specimens from patients with invasive aspergillosis.

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Author

Rantakokko-Jalava K, Laaksonen S, Issakainen J, Vauras J, Nikoskelainen J, Viljanen MK, and Salonen J

Subjects

Adolescent, Adult, Aged, Biopsy, DNA, Fungal analysis, DNA, Mitochondrial analysis, Female, Humans, Male, Middle Aged, Sensitivity and Specificity, Aspergillosis diagnosis, Aspergillus fumigatus isolation & purification, Bronchoalveolar Lavage Fluid microbiology, Lung Diseases, Fungal diagnosis, Polymerase Chain Reaction methods

Abstract

A real-time PCR method was developed and used to detect Aspergillus fumigatus mitochondrial DNA (mtDNA) in bronchoalveolar lavage (BAL) fluids and tissue biopsy specimens. The analytical sensitivity of the assay was one A. fumigatus conidium per reaction, and the assay was linear at least over 4 orders of magnitude above the detection limit. BAL fluids from 66 immunocompromised patients at risk of invasive pulmonary aspergillosis (IPA) and 33 immunocompetent controls and tissue biopsy specimens from 10 immunocompromised patients were analyzed. The results were related to the clinical diagnosis established according to recently published consensus criteria. A. fumigatus mtDNA positivity was encountered in 16 of 81 (20%) BAL fluid specimens from patients at risk and 1 of 33 (3%) specimens from immunocompetent controls. PCRs were positive in six of seven, two of four, and four of five of the patients with proven, probable, and possible IPA, respectively, as well as in four patients at risk but without any other evidence of IPA. With qualitative detection, the diagnostic sensitivity of PCR was 73%, specificity was 93%, and predictive values of positive (PPV) and negative (NPV) results were 73 and 95%, respectively. Using a threshold cycle of <35 as a limit for positive PCR, the specificity and PPV of PCR in the diagnosis of invasive aspergillosis were 100%, but its sensitivity was only 45% and NPV was 92%. PCR was positive in tissue biopsy specimens from all patients with invasive aspergillosis caused by A. fumigatus. Semiquantitative detection of A. fumigatus mtDNA in BAL fluid may be helpful in the diagnosis of IPA. PCR is well suited for the verification of the presence of A. fumigatus in tissue biopsy specimens. more...

Published

2003

3. Rapid typing of Bordetella pertussis pertussis toxin gene variants by LightCycler real-time PCR and fluorescence resonance energy transfer hybridization probe melting curve analysis.

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Author

Mäkinen J, Mertsola J, Viljanen MK, Arvilommi H, and He Q

Subjects

Amino Acid Sequence, Bacterial Typing Techniques, Base Sequence, Bordetella pertussis genetics, Bordetella pertussis metabolism, Genetic Variation, Humans, Molecular Sequence Data, Pertussis Vaccine genetics, Spectrometry, Fluorescence, Temperature, Time Factors, Bordetella pertussis classification, Fluorescent Dyes, Nucleic Acid Hybridization methods, Nucleic Acid Probes, Pertussis Toxin, Polymerase Chain Reaction methods, Virulence Factors, Bordetella genetics

Abstract

A LightCycler real-time PCR hybridization probe assay was developed for rapid typing of gene variants of the Bordetella pertussis virulence factor pertussis toxin. The assay correctly identified the ptxS1 alleles of all strains tested, comprising 57 Finnish clinical isolates and 2 vaccine strains. The method is simple, reliable, and suitable for large-scale screening of B. pertussis strains. more...

Published

2002

4. Rapid differentiation of Borrelia garinii from Borrelia afzelii and Borrelia burgdorferi sensu stricto by LightCycler fluorescence melting curve analysis of a PCR product of the recA gene.

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Author

Pietilä J, He Q, Oksi J, and Viljanen MK

Subjects

Animals, Borrelia genetics, Borrelia burgdorferi Group genetics, Fluorescence, Humans, Ixodes microbiology, Temperature, Borrelia classification, Borrelia burgdorferi, Borrelia burgdorferi Group classification, Lyme Disease microbiology, Polymerase Chain Reaction methods, Rec A Recombinases genetics

Abstract

To differentiate the Borrelia burgdorferi sensu lato genospecies, LightCycler real-time PCR was used for the fluorescence (SYBR Green I) melting curve analysis of borrelial recA gene PCR products. The specific melting temperature analyzed is a function of the GC/AT ratio, length, and nucleotide sequence of the amplified product. A total of 32 DNA samples were tested. Of them three were isolated from B. burgdorferi reference strains and 16 were isolated from B. burgdorferi strains cultured from Ixodes ricinus ticks; 13 were directly isolated from nine human biopsy specimens and four I. ricinus tick midguts. The melting temperature of B. garinii was 2 degrees C lower than that of B. burgdorferi sensu stricto and B. afzelii. Melting curve analysis offers a rapid alternative for identification and detection of B. burgdorferi sensu lato genospecies. more...

Published

2000

5. Line probe assay in the rapid detection of rifampin-resistant Mycobacterium tuberculosis directly from clinical specimens.

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Author

Marttila HJ, Soini H, Vyshnevskaya E, Vyshnevskiy BI, Otten TF, Vasilyef AV, and Viljanen MK

Subjects

DNA, Bacterial analysis, Drug Resistance, Microbial genetics, Humans, Microbial Sensitivity Tests, Mycobacterium tuberculosis genetics, Mycobacterium tuberculosis isolation & purification, Reagent Kits, Diagnostic, Sensitivity and Specificity, Antibiotics, Antitubercular pharmacology, Mycobacterium tuberculosis drug effects, Polymerase Chain Reaction methods, Rifampin pharmacology, Tuberculosis microbiology

Abstract

The sensitivity of a PCR-based line probe assay (Inno-LiPA Rif. TB Assay; Innogenetics NV Zwijndrecht, Belgium) was studied by using nested-PCR technique. A total of 75 specimens, representing various body locations from 70 suspected tuberculosis patients were obtained. LiPA yielded 30 Mycobacterium tuberculosis complex positive results (sensitivity 58.8%, compared with final diagnoses) whereas culture for M. tuberculosis was positive in 18 specimens (sensitivity 35.3%). Genotypic rifampin resistance testing by LiPA showed that 7 specimens contained rpoB mutations associated with RMP resistance, and sequencing data of the rpoB gene and LiPA patterns agreed in 29 of 30 M. tuberculosis positive specimens (96.7%). This indicates reliable performance, which makes the test suitable for the rapid determination of resistance to rifampin directly in clinical samples. However, the best results are obtained if LiPA is combined with conventional staining and culture methods. more...

Published

1999

6. Rapid detection of rifampin-resistant Mycobacterium tuberculosis by sequencing and line probe assay.

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Author

Marttila HJ, Soini H, Vyshnevskiy BI, Otten TF, Vasilyef AV, Huovinen P, and Viljanen MK

Subjects

Base Sequence, Drug Resistance, Microbial, Humans, Microbial Sensitivity Tests, Molecular Sequence Data, Mycobacterium tuberculosis drug effects, Sensitivity and Specificity, Antibiotics, Antitubercular pharmacology, DNA, Bacterial analysis, Mycobacterium tuberculosis isolation & purification, Polymerase Chain Reaction, Rifampin pharmacology

Abstract

Resistance to rifampin (RMP) is associated with mutations in the rpoB gene. Disk elution method, direct DNA sequencing and line probe assay were compared in rapid detection of rpoB mutations from 30 Mycobacterium tuberculosis isolates. Concordance between LiPA and culture was 93.3%, whereas sequencing yielded 100% concordance with culture. These results indicate that line probe assay is nearly as sensitive a method as sequencing in rapid detection of RMP-resistance of M. tuberculosis isolates, and can be applied in laboratories working with standard PCR equipment. more...

Published

1998

7. Impact of polymerase chain reaction on clinical pertussis research: Finnish and Swiss experiences.

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Author

He Q, Schmidt-Schläpfer G, Just M, Matter HC, Nikkari S, Viljanen MK, and Mertsola J

Subjects

Adolescent, Adult, Age Factors, Aged, Antibodies, Bacterial analysis, Bacterial Outer Membrane Proteins immunology, Bacteriological Techniques, Bordetella pertussis immunology, Child, Child, Preschool, Disease Outbreaks, Finland epidemiology, Hemagglutinins immunology, Humans, Immunoenzyme Techniques, Immunoglobulin A analysis, Immunoglobulin G analysis, Immunoglobulin M analysis, Incidence, Infant, Middle Aged, Seroepidemiologic Studies, Switzerland epidemiology, Vaccination statistics & numerical data, Virulence Factors, Bordetella immunology, Whooping Cough immunology, Bordetella pertussis isolation & purification, Polymerase Chain Reaction methods, Whooping Cough diagnosis, Whooping Cough epidemiology

Abstract

Since April 1993 in Finland and March 1994 in Switzerland, polymerase chain reaction (PCR) has been used routinely nationwide for the diagnosis of pertussis. Nasopharyngeal specimens from 3794 patients suspected of having pertussis and 1125 controls were tested. Finnish and Swiss assays found 23% and 36% of clinical specimens positive, respectively. PCR showed a higher incidence of pertussis infection among 1- to 6-year-old children in Switzerland than in Finland (P < .001). This difference may be due to the booster dose of vaccine given at 2 years of age in Finland but not in Switzerland. In Finland, PCR-confirmed asymptomatic cases were more common among children <7 years old than in older children (P < .001), whereas older children tended to have symptomatic infection. The use of PCR markedly improves the diagnosis of pertussis and opens new perspectives for epidemiologic and vaccine efficacy studies. more...

Published

1996

8. Comparison of amplicor and 32-kilodalton PCR for detection of Mycobacterium tuberculosis from sputum specimens.

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Author

Soini H, Agha SA, El-Fiky A, and Viljanen MK

Subjects

DNA, Bacterial genetics, DNA, Bacterial isolation & purification, Egypt, Evaluation Studies as Topic, Humans, Polymerase Chain Reaction statistics & numerical data, Sensitivity and Specificity, Tuberculosis, Pulmonary diagnosis, Tuberculosis, Pulmonary microbiology, Mycobacterium tuberculosis genetics, Mycobacterium tuberculosis isolation & purification, Polymerase Chain Reaction methods, Sputum microbiology

Abstract

The commercial PCR test Amplicor was compared with the 32-kDa PCR for detection of Mycobacterium tuberculosis from 76 sputum specimens from Egyptian patients. Both tests performed with rather equal efficacy (resolved sensitivity of 88.9% for both tests; specificity of 98.0% for Amplicor and 93.9% for 32-kDa PCR). PCR was found to be useful in detection of auramine fluorescent stain-positive, culture-negative specimens. more...

Published

1996

9. Primers are decisive for sensitivity of PCR.

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Author

He Q, Marjamäki M, Soini H, Mertsola J, and Viljanen MK

Subjects

Base Sequence, Bordetella pertussis genetics, Borrelia burgdorferi Group genetics, Molecular Sequence Data, Mycobacterium tuberculosis genetics, Sensitivity and Specificity, DNA Primers genetics, Polymerase Chain Reaction

Abstract

A sufficient sensitivity of PCR is a prerequisite for its use in the diagnosis of infectious diseases. We have used PCR for detecting gene elements of Borrelia burgdorferi, mycobacteria and Bordetella pertussis. With all these microbe groups, difficulties were encountered in achieving the demanded sensitivity with the primer pairs primarily selected. An extensive testing of various reaction parameters did not improve the sensitivity. Subsequently, we synthesized more primers derived from slightly different positions of the original target sequences. When the original and new primers were tested in possible combinations, some primer pairs reached 100-fold to 1000-fold higher sensitivity than the primary pairs. We conclude that in optimizing the sensitivity of PCR, more emphasis should be put on testing of several primer pairs than on the extensive screening of reaction parameters. Thus far, a trial-and-error approach has to be used, because there is no means to predict the sensitivity properties of a selected primer pair. more...

Published

1994

10. Effects of thermocyclers and primers on the reproducibility of banding patterns in randomly amplified polymorphic DNA analysis.

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Author

He Q, Viljanen MK, and Mertsola J

Subjects

Base Sequence, Bordetella pertussis genetics, Chromosome Banding, Gene Amplification, Molecular Sequence Data, Reproducibility of Results, Temperature, DNA Primers, DNA, Bacterial genetics, Polymerase Chain Reaction instrumentation, Polymorphism, Genetic, Thermometers

Abstract

The effects of thermocyclers and primers on the reproducibility of banding patterns in randomly amplified polymorphic DNA analysis were tested. Purified Bordetella pertussis DNA was analysed with four primers (12-mer), which did not differ from each other in their GC-content. Three different thermocycler models from two manufacturers were tested. Three of the primers produced consistent banding patterns in separate wells of the reaction plates of individual thermocyclers, and in different thermocycler models. In contrast, the fourth primer showed extensive between-instrument variation, and the within-instrument variation with this primer was acceptable only when the most advanced thermocycler model was used. We conclude that only primers that provide consistent banding patterns in different environments should be chosen for interlaboratory use in randomly amplified polymorphic DNA analysis. The primers showing variability in banding patterns can only be used if they produce consistent results in the thermocycler used. more...

Published

1994

11. Sensitive and specific polymerase chain reaction assays for detection of Bordetella pertussis in nasopharyngeal specimens.

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Author

He Q, Mertsola J, Soini H, and Viljanen MK

Subjects

Adult, Bacteriological Techniques, Base Sequence, Bordetella pertussis genetics, Child, DNA, Bacterial analysis, Humans, Molecular Sequence Data, Sensitivity and Specificity, Whooping Cough microbiology, Bordetella pertussis isolation & purification, Nasopharynx microbiology, Polymerase Chain Reaction, Whooping Cough diagnosis

Abstract

Polymerase chain reaction (PCR) assays that amplify segments of a repeated gene element and a toxin promoter gene of Bordetella pertussis were compared with a culture established for the diagnosis of pertussis. Of 44 nasopharyngeal (NP) aspirates collected during a pertussis outbreak, repeated gene element PCR showed a positive result in 21 (48%), including all three patients with positive culture results. Results of toxin promoter gene PCR were positive in eight (18%) cases, and the pathogen was not detected in one patient with a positive culture result. A more sensitive nested PCR assay, based on repeated gene element PCR, was then developed. During a second outbreak two different transportation systems were tested in 146 duplicate NP swabs. Transportation of swabs in empty tubes proved to be better than in transport media for PCR. A total of 190 NP specimens from the two outbreaks were tested, and in 56 the results were shown to be positive by PCR, including all 16 cases confirmed as positive by culture. We conclude that the PCR assay is more sensitive than culture in the diagnosis of pertussis; NP swabbing is a simple, practical, and reliable method of collecting clinical specimens for PCR assays and cultures. more...

Published

1994

12. Comparison of polymerase chain reaction with culture and enzyme immunoassay for diagnosis of pertussis.

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Author

He Q, Mertsola J, Soini H, Skurnik M, Ruuskanen O, and Viljanen MK

Subjects

Adolescent, Adult, Aged, Base Sequence, Bordetella pertussis growth & development, Child, Child, Preschool, Female, Finland epidemiology, Humans, Infant, Male, Microbiological Techniques, Middle Aged, Molecular Sequence Data, Disease Outbreaks, Immunoenzyme Techniques, Polymerase Chain Reaction, Whooping Cough diagnosis

Abstract

A polymerase chain reaction (PCR) assay amplifying a segment of a repeated gene element of Bordetella pertussis was compared with culture and enzyme immunoassay (EIA) for the diagnosis of pertussis. The PCR assay was specific for B. pertussis in tests with a panel of other bacteria and with an extensive collection of specimen material from healthy persons and children with respiratory infections other than pertussis. The PCR assay was used in the analysis of 117 nasopharyngeal swabs collected from children at an elementary school at which a pertussis outbreak occurred. Fifty-six (48%) of the 117 swabs were positive, including those for all six culture-positive cases. The PCR method was then applied to analyze another pertussis outbreak. Of 40 nasopharyngeal aspirates taken from 37 clinically susceptible pertussis patients and from three asymptomatic contacts, the PCR identified 18 (45%), including all 3 culture-positive and 5 (35%) of the 14 seropositive patients. The most consistent and reliable diagnosis by positive PCR result was observed with those patients experiencing symptoms within 1 to 6 weeks of sample collection. We conclude that PCR is a rapid, sensitive, and specific means of diagnosing pertussis, especially during the first weeks of disease. The assay can be performed with both nasopharyngeal swabs and aspirates. more...

Published

1993

13. Misdiagnosis of Mycobacterium avium-intracellulare by rapid PCR/DNA probe tests.

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Author

Viljanen MK and Olkkonen L

Subjects

Diagnostic Errors, Humans, DNA Probes, Mycobacterium avium-intracellulare Infection diagnosis, Polymerase Chain Reaction

Published

1993