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102. Reliable analysis of the single nucleotide polymorphism of lactase persistence LPH(-13910) C/T from saliva derived DNA: validation of a standardized saliva collection system

Author

Brigitte Zahel, Dietmar Enko, Joerg Berg, Christian Paar, and Roland Mayr

Subjects
Adult, Male, Saliva, Single-nucleotide polymorphism, Real-Time Polymerase Chain Reaction, Polymorphism, Single Nucleotide, General Biochemistry, Genetics and Molecular Biology, White People, Specimen Handling, chemistry.chemical_compound, Saliva collection, Lactose Intolerance, Predictive Value of Tests, Genotype, Humans, Genetic Predisposition to Disease, Lactase, Automation, Laboratory, Reproducibility of Results, DNA, Equipment Design, Middle Aged, Molecular biology, Lactase persistence, genomic DNA, Phenotype, chemistry, Female, Spectrophotometry, Ultraviolet, SNP array
Abstract

BACKGROUND The purpose of this study was to investigate the applicability of the Greiner Saliva Collection System (SCS) to obtain human genomic DNA for the analysis of single nucleotide polymorphisms (SNP) in the clinical routine laboratory. METHODS Saliva and EDTA-blood were collected pair-wise from 112 participants. DNA was prepared by two automated procedures (MagNA Pure LC or MagNa Pure compact) and analyzed by UV-spectrophotometry and real-time PCR. RESULTS Mean saliva derived DNA concentration was 52.7 ng/μL ± 36.4 (1000 μL, MagNA Pure LC) and 9.2 ng/μL ± 5.6 (200 μL, MagNA Pure compact) with A260/A280 ratios of 1.9 ± 0.1 and 2.1 ± 0.3 for MagNA Pure LC and MagNA Pure compact, respectively. SNP analysis for caucasian adult type lactase persistence showed a 100% success rate from saliva derived DNA and as reference from blood derived DNA. Matching genotypes were obtained in each sample pair. CONCLUSIONS Saliva obtained with the standardized SCS yielded sufficient amounts of DNA in high purity and was found to represent a suitable and reliable source of human DNA for SNP analysis in the clinical routine laboratory.

Published
2015

104. Method evaluation study of a new generation of vitamin D assays

Author

Robert Stolba, Elfriede Worf, Dietmar Enko, Gernot Kriegshäuser, and Gabriele Halwachs-Baumann

Subjects
Male, Chromatography, Chemiluminescence immunoassay, Chemistry, Biochemistry (medical), Clinical Biochemistry, Chromatography liquid, vitamin D, Mass spectrometry, Mass Spectrometry, Method evaluation, quality improvement, immunoassays, Deming regression, Method comparison, Liquid chromatography–mass spectrometry, reference standards, liquid chromatography-tandem mass spectrometry, Vitamin D and neurology, Humans, Female, Chromatography, Liquid, Research Article
Abstract

Introduction: Recently several diagnostic manufacturers have launched new 25-hydroxy-vitamin D (25[OH]D) assays, which are aligned to the National Institute of Standards and Technology (NIST) Standard Reference Materials (SRM) (NIST, Gaithersburg, Maryland). The aim of this study was to compare the performance of one liquid chromatography-tandem mass spectrometry (LC-MS/MS) method, one enzyme linked immunosorbent assay (ELISA), and one recalibrated and previous version of a chemiluminescence immunoassay (CLIA). Material and methods: Serum-aliquots of 198 patient samples from routine 25(OH)D analysis were measured by the ClinMass® LC-MS/MS Complete Kit (RECIPE Chemicals + Instruments GmbH, Munich, Germany), the ORGENTEC 25(OH)D 3 /D 2 ELISA (ORGENTEC Diagnostika GmbH, Mainz, Germany), the recalibrated Immunodiagnostic Systems (IDS)-iSYS 25(OH)D S and the previous used IDS-iSYS 25(OH)D CLIA (Immunodiagnostic Systems Ltd, Boldon, United Kingdom). Bland-Altman and Deming regression analyses were calculated for methods comparison of all tested 25(OH)D assays. The LC-MS/MS method was defined as the reference method. Within-run and between-run precision measurements were performed for all met hods with three different concentration levels. Results: Compared to the LC-MS/MS method, the new IDS-iSYS 25(OH)D S and ORGENTEC 25(OH)D 3 /D 2 assay demonstrated mean relative biases of 16.3% and 17.8%. The IDS-iSYS 25(OH)D assay showed the lowest mean bias of 1.5%. Deming regression analyses of the recalibrated IDS-iSYS 25(OH) D S and the ORGENTEC 25(OH)D 3 /D 2 assay showed proportional differences, when compared to the reference method. All assays showed a within-run and between-run imprecision of ≤ 20% at each of the evaluated concentration levels. Conclusions: The evaluated standardized immunoassays and LC-MS/MS are useful methods for measuring 25(OH)D serum-levels in clinical labora

Published
2014

105. Frequencies and Specificities of 'Enzyme-Only' Detected Erythrocyte Alloantibodies in Patients Hospitalized in Austria: Is an Enzyme Test Required for Routine Red Blood Cell Antibody Screening?

Author

Franz Wallner, Gabriele Halwachs-Baumann, Barbara Mayr, Claudia Habres, and Dietmar Enko

Subjects
chemistry.chemical_classification, Article Subject, biology, business.industry, Enzyme test, Papain, chemistry.chemical_compound, Red blood cell, Enzyme, medicine.anatomical_structure, chemistry, Immunology, biology.protein, Medicine, In patient, Antibody, Indirect Antiglobulin Test, business, Antibody screening, Research Article
Abstract

The aim of this study was to determine the frequencies and specificities of “enzyme-only” detected red blood cell (RBC) alloantibodies in the routine antibody screening and antibody identification in patients hospitalized in Austria. Routine blood samples of 2420 patients were investigated. The antibody screening was performed with a 3-cell panel in the low-ionic strength saline- (LISS-) indirect antiglobulin test (IAT) and with an enzyme-pretreated (papain) 3-cell panel fully automated on the ORTHO AutoVue Innova System. The antibody identification was carried out manually with an 11-cell panel in the LISS-IAT and with an enzyme-pretreated (papain) 11-cell panel. In total 4.05% (n=98) of all patients (n=2420) had a positive RBC antibody screening result. Of them 25.51% (25/98) showed “enzyme-only” detected specific or nonspecific RBC alloantibodies. Rhesus and Lewis system antibodies were found the only specificities of “enzyme-only” RBC alloantibodies: all in all 4.8% (4/98) were detected with anti-E, 3.06% (3/98) with anti-Lea, 3.06% (3/98) with anti-D after anti-D prophylaxis and 1.02% (1/98) with anti-e. In total, 14.29% (14/98) showed a nonspecific RBC alloantibody result with the enzyme test. The results of the present study demonstrate that a high number of unwanted positive reactions with the enzyme technique overshadows the detection of “enzyme-only” RBC alloantibodies. (Trial Registration: K-37-13).

Published
2014

106. 25-Hydroxy-Vitamin D Status: Limitations in Comparison and Clinical Interpretation of Serum-Levels Across Different Assay Methods

Author

Leo Fridrich, Gabriele Halwachs-Baumann, Juliane Ernst, Robert Stolba, Erwin Rezanka, Iris Wendler, Daniel K. Fabian, Susanne Hauptlorenz, and Dietmar Enko

Subjects
Quality Control, Vitamin, Analyte, Radioimmunoassay, High-performance liquid chromatography, General Biochemistry, Genetics and Molecular Biology, law.invention, Matrix (chemical analysis), chemistry.chemical_compound, Predictive Value of Tests, Tandem Mass Spectrometry, law, Vitamin D and neurology, Humans, ADVIA Centaur, Prospective Studies, Vitamin D, Chromatography, High Pressure Liquid, Chemiluminescence, Chromatography, Reproducibility of Results, Vitamin D Deficiency, chemistry, Austria, Luminescent Measurements, Total Vitamin D, Biomarkers, Blood Chemical Analysis
Abstract

Background: Over the last decade, clinical interest to evaluate human 25-hydroxy-vitamin D (25[OH]D) serum levels has increased exponentially. In the present study, four chemiluminescence immunoassays (CLIA), one radioimmunoassy (RIA), and one high performance liquid chromatography (HPLC) method were compared and also with the liquid chromatography-tandem mass spectrometry (LC-MS/MS) method in view of 25(OH)D serum level determination. Methods: For the method comparison, blood samples from 133 consecutive patients were prospectively collected. All participants gave written informed consent for their blood samples to be used in this study. They came to the Department of Nuclear Medicine of the Central Hospital Steyr (Austria) for osteodensidometric measurement as part of their preventive medical check-up. Pearson's correlation coefficients, Bland-Altman plots, and paired t-tests were calculated. Assay-specific reference ranges were considered using blood samples from persons with normal parathormone, calcium, and total-protein values (n = 97). Results: The highest correlation was between the HPLC and the LC-MS/MS method (r = 0.96). The lowest correlation was between the cobas Vitamin D3 assay (Roche) and any of the evaluated assays (r = 0.46 - 0.63). Bland-Altman plots revealed a big negative mean bias in three assays (cobas Vitamin D3 assay [Roche]: -22.8; DiaSorin LIAISON [25[OH]D total CLIA [Diasorin]: -18.4; Diasorin 25[OH]D125 I RIA [Diasorin]: -23.8 [nmol/L]) and a much smaller positive mean bias in the other assays (ClinRep complete 25[OH]D2/D3 HPLC kit [Recipe]: 2.7; ADVIA Centaur Vitamin D total assay [Siemens]: 8.2; IDS total vitamin D assay [Immunodiagnostic Systems]: 12.1 [nmol/L]) compared to the LC-MS/MS method. Meanwhile, the manufacturer has withdrawn the cobas Vitamin D3 assay from the market. Conclusions: Poor antibody specificity with cross-reactivity to other vitamin D metabolites, incomplete extraction of the 25(OH)D analyte from the vitamin D-binding protein (DBP), and confounding matrix substances such as lipids could be potential reasons for the unacceptable performance of the cobas Vitamin D3 assay (Roche) and also the significant differences in the 25(OH)D determination between various assays. Standardization and harmonization of 25(OH)D measurements are therefore urgently needed. The widespread introduction of well standardized assays in clinical laboratories is the challenge in the next years. (Clin. Lab. 2014;60:1541-1550. DOI: 10.7754/Clin.Lab.2014.131114)

Published
2014
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107. Method evaluation study of a new generation of vitamin D assays

Author

Dietmar Enko, Gernot Kriegshäuser, Robert Stolba, Elfriede Worf, Gabriele Halwachs-Baumann, Dietmar Enko, Gernot Kriegshäuser, Robert Stolba, Elfriede Worf, and Gabriele Halwachs-Baumann

Abstract

Introduction: Recently several diagnostic manufacturers have launched new 25-hydroxy-vitamin D (25[OH]D) assays, which are aligned to the National Institute of Standards and Technology (NIST) Standard Reference Materials (SRM) (NIST, Gaithersburg, Maryland). The aim of this study was to compare the performance of one liquid chromatography-tandem mass spectrometry (LC-MS/MS) method, one enzyme linked immunosorbent assay (ELISA), and one recalibrated and previous version of a chemiluminescence immunoassay (CLIA). Material and methods: Serum-aliquots of 198 patient samples from routine 25(OH)D analysis were measured by the ClinMass® LC-MS/MS Complete Kit (RECIPE Chemicals + Instruments GmbH, Munich, Germany), the ORGENTEC 25(OH)D3/D2 ELISA (ORGENTEC Diagnostika GmbH, Mainz, Germany), the recalibrated Immunodiagnostic Systems (IDS)-iSYS 25(OH)DS and the previous used IDS-iSYS 25(OH)D CLIA (Immunodiagnostic Systems Ltd, Boldon, United Kingdom). Bland-Altman and Deming regression analyses were calculated for methods comparison of all tested 25(OH)D assays. The LC-MS/MS method was defined as the reference method. Within-run and between-run precision measurements were performed for all methods with three different concentration levels. Results: Compared to the LC-MS/MS method, the new IDS-iSYS 25(OH)DS and ORGENTEC 25(OH)D3/D2 assay demonstrated mean relative biases of 16.3% and 17.8%. The IDS-iSYS 25(OH)D assay showed the lowest mean bias of 1.5%. Deming regression analyses of the recalibrated IDS-iSYS 25(OH)DS and the ORGENTEC 25(OH)D3/D2 assay showed proportional differences, when compared to the reference method. All assays showed a within-run and between-run imprecision of ≤ 20% at each of the evaluated concentration levels. Conclusions: The evaluated standardized immunoassays and LC-MS/MS are useful methods for measuring 25(OH)D serum-levels in clinical laboratories.

Published
2015

109. Performance evaluation of a rapid whole-blood immunoassay for the detection of IgG antibodies against Helicobacter pylori in daily clinical practice

Author

Gabriele Halwachs-Baumann, Dietmar Enko, Gernot Kriegshäuser, Ortrun Rössler, and Robert Stolba

Subjects
Adult, Microbiology (medical), medicine.medical_specialty, Adolescent, Bacteremia, Drug resistance, Gastroenterology, Sensitivity and Specificity, Helicobacter Infections, 03 medical and health sciences, 0302 clinical medicine, Medical microbiology, Internal medicine, Germany, medicine, Humans, Urea, Aged, Breath test, Aged, 80 and over, Immunoassay, Carbon Isotopes, biology, medicine.diagnostic_test, Helicobacter pylori, Research, General Medicine, Gold standard (test), Middle Aged, biology.organism_classification, Antibodies, Bacterial, Confidence interval, Anti-Bacterial Agents, Infectious Diseases, Breath Tests, 030220 oncology & carcinogenesis, Immunoglobulin G, Laboratory diagnosis, Immunology, biology.protein, 030211 gastroenterology & hepatology, Antibody
Abstract

A growing number of rapid Helicobacter pylori antibody tests are commercially available now, however, some of these tests are often used without sufficient evaluation. The aim of this study was to evaluate the performance of a commercially available rapid whole-blood immunoassay (gabControl® H. pylori; gabmed GmbH, Koln, Germany), for the qualitative detection of IgG antibodies against H. pylori with the 13C-urea breath test (13C-UBT) serving as a reference method. A total of 108 consecutive outpatients, who were referred for 13C-UBT by general practitioners and specialists, were also tested for H. pylori infection by the gabControl® H. pylori immunoassay. The clinical performance of this rapid whole-blood test was evaluated by determining the sensitivity, specificity, positive predictive value (PPV), and negative predictive value (NPV) compared to the 13C-UBT. The agreement between the two tests was calculated using Cohen’s Kappa (κ) with 95 % confidence intervals (CI). The agreement between the gabControl® H. pylori assay and the 13C-UBT was 0.62 [95 % confidence intervals (CIs) 0.47–0.76; P

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