Your search keyword '"Wuyts B"' showing total 10 results

1. TRUENESS VERIFICATION OF THE CURRENT CREATININE ASSAYS DEMONSTRATES A DISAPPOINTING VARIABILITY WHICH INSUFFICIENTLY MEETS CHANGING CLINICAL NEEDS

Author

Delanghe, J., Cobbaert, C., Galteau, M.-M., Harmoinen, A., Jansen, R., Kruse, R., Laitinen, P., Panteghini, M., Thienpont, L., Wuyts, B., and Weykamp, C.

Published

2007

2. Compensating for the influence of total serum protein in the Schwartz formula.

Author

Speeckaert MM, Wuyts B, Stove V, Walle JV, and Delanghe JR

Subjects

Adolescent, Blood Proteins metabolism, Child, Child, Preschool, Cohort Studies, Creatinine blood, Female, Glomerular Filtration Rate physiology, Humans, Male, Blood Proteins chemistry, Organometallic Compounds chemistry

Abstract

Background: The Schwartz 2009 creatinine-based revised formula is the only pediatric GFR estimating formula, which is compatible with the recent global creatinine standardization. This formula is only applicable if enzymatic creatinine methods are used. We propose an equation, taking into account the relative bias caused by serum proteins to use Jaffe based creatinine data for GFR estimation., Methods: In a cohort study of 100 pediatric patients, serum creatinine was measured using a kinetic rate-blanked Jaffe assay (modified kinetic alkaline picrate method), a kinetic rate-blanked Jaffe compensated assay for reactive proteins and an enzymatic assay (creatinine plus method). Serum total protein, albumin, urea, uric acid and total bilirubin were measured with the use of commercial agents., Results: The difference in serum creatinine between the enzymatic method and the compensated Jaffe method was mainly dependent on the total protein concentration in serum (r(2)=0.61, p<0.001). After applying the proposed protein correction, corrected compensated Jaffe results and creatinine clearance values became interchangeable with enzymatic serum creatinine results (r(2)=0.99, p<0.001; Deming regression: slope: 0.9787, intercept: -0.351) and with the newly proposed Schwartz formula, respectively (r(2)=0.99, p<0.001; Deming regression: slope 1.004, intercept: 2.16)., Conclusions: In this study, we demonstrated the usability of the alkaline picrate method in the Schwartz formula, taking into account the relative bias caused by serum proteins.

Published

2012

3. Trueness verification of actual creatinine assays in the European market demonstrates a disappointing variability that needs substantial improvement. An international study in the framework of the EC4 creatinine standardization working group.

Author

Delanghe JR, Cobbaert C, Galteau MM, Harmoinen A, Jansen R, Kruse R, Laitinen P, Thienpont LM, Wuyts B, Weykamp C, and Panteghini M

Subjects

Blood Chemical Analysis standards, Europe, International Cooperation, Reference Standards, Reproducibility of Results, Blood Chemical Analysis methods, Creatinine blood

Abstract

Background: The European In Vitro Diagnostics (IVD) directive requires traceability to reference methods and materials of analytes. It is a task of the profession to verify the trueness of results and IVD compatibility., Methods: The results of a trueness verification study by the European Communities Confederation of Clinical Chemistry (EC4) working group on creatinine standardization are described, in which 189 European laboratories analyzed serum creatinine in a commutable serum-based material, using analytical systems from seven companies. Values were targeted using isotope dilution gas chromatography/mass spectrometry. Results were tested on their compliance to a set of three criteria: trueness, i.e., no significant bias relative to the target value, between-laboratory variation and within-laboratory variation relative to the maximum allowable error., Results: For the lower and intermediate level, values differed significantly from the target value in the Jaffe and the dry chemistry methods. At the high level, dry chemistry yielded higher results. Between-laboratory coefficients of variation ranged from 4.37% to 8.74%. Total error budget was mainly consumed by the bias. Non-compensated Jaffe methods largely exceeded the total error budget. Best results were obtained for the enzymatic method. The dry chemistry method consumed a large part of its error budget due to calibration bias., Conclusions: Despite the European IVD directive and the growing needs for creatinine standardization, an unacceptable inter-laboratory variation was observed, which was mainly due to calibration differences. The calibration variation has major clinical consequences, in particular in pediatrics, where reference ranges for serum and plasma creatinine are low, and in the estimation of glomerular filtration rate.

Published

2008

4. Quantitative measurement of ketone bodies in urine using reflectometry.

Author

Penders J, Fiers T, Giri M, Wuyts B, Ysewyn L, and Delanghe JR

Subjects

3-Hydroxybutyric Acid urine, Acetoacetates urine, Acetone urine, Adult, Diabetes Mellitus drug therapy, Female, Humans, Insulin Infusion Systems, Male, Middle Aged, Reproducibility of Results, Urinalysis statistics & numerical data, Diabetes Mellitus urine, Ketone Bodies urine, Urinalysis methods

Abstract

Background: Recently, automated urine test strip readers became available that can report quantitative data. We explored the possibility of measuring all ketone bodies (acetone, acetoacetate, 3-hydroxybutyrate) in urine with these test strips. Monitoring urinary ketone concentrations could offer the advantages of measuring higher values (due to the low renal thresholds) and being less sensitive to fluctuations., Methods: We evaluated URISYS 2400 (Roche) quantitative reflectance data for the ketone reflectance field and compared it with biochemical data from urine samples. Using an easy sample pre-treatment with 3-hydroxybutyrate dehydrogenase, we were able to assay 3-hydroxybutyrate as well, which normally does not react on urine test strips., Results: Within- and between-run reproducibility of the reflectance signal for high- and low-concentration urine pools was 11.0-3.6% and 11.0-5.8% for aceto-acetate, 8.2-9.2% and 10.4-16.1% for acetone, and 5.1-3.0% and 5.6-3.5% for 3-hydroxybutyrate, respectively. The lower limit of detection for acetoacetate was 0.13 mmol/L (CV=3.6%). Fair agreement was obtained between test strip data for ketones andcolorimetrically determined acetoacetate values (r=0.90)., Conclusions: In urine test strip analysis, quantitative ketone reflectance data allow a simple and fast analysis, offering affordable screening for the detection of ketone body production in diabetes, especially in emergency settings.

Published

2005

5. Prohepcidin accumulates in renal insufficiency.

Author

Taes YE, Wuyts B, Boelaert JR, De Vriese AS, and Delanghe JR

Subjects

Aged, Creatinine blood, Cystatin C, Cystatins blood, Enzyme-Linked Immunosorbent Assay, Female, Ferritins blood, Hepcidins, Humans, Intramolecular Oxidoreductases blood, Lipocalins, Male, Metabolic Clearance Rate, Protein Precursors, Transferrin metabolism, Antimicrobial Cationic Peptides metabolism, Iron metabolism, Renal Insufficiency blood

Abstract

Background: The understanding of iron metabolism has increased substantially during the last decade. Several new transporters and iron regulating molecules have been described. Hepcidin, a small hepatic peptide has recently been proposed as a central mediator of dietary iron absorption. We have investigated the relationship between prohepcidin, the prohormone of hepcidin, and renal function and iron status., Methods: Forty six patients, referred for 51Cr-EDTA clearance were included in this study. Renal function was assessed by determination of serum creatinine, creatinine clearance, serum cystatin C and serum beta-trace protein. Iron status was evaluated by determination of serum iron, transferrin, transferrin saturation and serum ferritin. All determinations were performed using commercial reagents (Roche Diagnostics, Dade Behring). Serum prohepcidin was determined using an ELISA kit., Results: Serum prohepcidin was found to correlate with 51Cr-EDTA clearance (r = -0.44; p = 0.005), creatinine clearance, serum creatinine, beta-trace protein and cystatin C. No significant relationship was observed between serum prohepcidin concentrations and red cell count, hemoglobin concentration or hematocrit. No significant correlation was found in this population between prohepcidin concentrations and iron status., Conclusion: Increased serum prohepcidin concentrations were observed with declining kidney function. We observed no relationship between red cell indices or iron status and serum prohepcidin concentrations.

Published

2004

6. The analysis of carbohydrate-deficient transferrin, marker of chronic alcoholism, using capillary electrophoresis.

Author

Wuyts B and Delanghe JR

Subjects

Biomarkers blood, Chromatography, High Pressure Liquid methods, Chromatography, Ion Exchange methods, Electrophoresis, Capillary instrumentation, Humans, Isoelectric Focusing methods, Time Factors, Alcoholism blood, Electrophoresis, Capillary methods, Transferrin analogs & derivatives, Transferrin analysis

Abstract

Carbohydrate-deficient transferrin (CDT) is currently considered to be the best available marker for the diagnosis of chronic alcoholism. A large variety of methods have been developed, demonstrating the need for standardisation. Commercially available anion-exchange chromatographic-based assays are easy to use and require no specialised, expensive instruments. However, these methods cannot identify genetic transferrin variants or the carbohydrate-deficient glycoprotein syndrome. In 1989, a capillary isoelectric focusing method was developed for quantitative measurement of CDT. Despite the optimal resolution, this method is not easily applied in a clinical routine environment due to the complexity of analysis. Capillary electrophoresis in a polymer network using coated capillaries allowed full resolution of the sialoforms of human transferrin. The drawbacks due to an expensive and time-consuming sample preparation were eliminated when a method in neat serum was developed. Capillary zone electrophoresis allowed full resolution of the transferrin isoforms with a high analytical performance in a short analysis time thanks to a strong electroosmotic flow. Genetic transferrin variants were easily detected, avoiding false-positive results. Also, using capillary zone electrophoresis, it was shown that CDT is a suitable marker of chronic alcohol abuse detection in transferrin CD (common/cathodal) variants.

Published

2003

7. Novel haptoglobin insertion/deletion polymorphism is associated with the lipid profile and C-reactive protein (CRP) concentration.

Author

Wuyts B, Hetet G, Grandchamp B, and Delanghe JR

Subjects

Adult, Belgium, Female, Gene Frequency, Genetic Heterogeneity, Genetic Testing methods, Genotype, Humans, Introns, Male, Middle Aged, Mutagenesis, Insertional, Phenotype, Sequence Deletion, Carrier Proteins blood, Haptoglobins genetics, Lipids blood, Polymorphism, Genetic

Abstract

We discovered a hitherto undescribed insertion/deletion (I/D) polymorphism of 7 base pairs in intron 4 of the HP1 allele and intron 4 and 6 of the HP2 allele. Genotyping was performed in 311 Belgian subjects. The association between serum haptoglobin (Hp) and lipid concentrations and the Hp I/D genotypes was investigated. Genotype distribution in 103 Hp 1-1 phenotypes (50.5% DD, 39.8% DI, 9.7% II) and D allele frequency (0.70) were in close agreement with the Hardy-Weinberg equilibrium. No association between Hp concentrations and the Hp I/D genotypes could be found. Apolipoprotein (apo)A2, apoB and cholesterol concentrations were slightly lower in Hp II compared to DI and DD. Low-density lipoprotein (LDL)-cholesterol and ultrasensitive C-reactive protein (CRP) concentrations and the apoA1/apoA2 ratios differed significantly between Hp D/I genotypes. We added a further component to the molecular heterogeneity of Hp by the detection of an I/D polymorphism. Studies on the Hp I/D polymorphism in various populations open perspectives for further investigation of the distribution pattern of the human Hp gene. The association of the Hp I/D polymorphism with various lipid parameters might add a further component to the complex and multifaceted lipid metabolism.

Published

2002

8. Carbohydrate-deficient transferrin and chronic alcohol ingestion in subjects with transferrin CD-variants.

Author

Wuyts B, Delanghe JR, Kasvosve I, Gordeuk VR, Gangaidzo IT, and Gomo ZA

Subjects

Adult, Aged, Alcoholism genetics, Biomarkers blood, Blood Chemical Analysis methods, Chromatography, High Pressure Liquid, Electrophoresis, Capillary methods, False Positive Reactions, Female, Humans, Male, Middle Aged, Phenotype, Temperance, Alcoholism blood, Alcoholism diagnosis, Genetic Variation, Transferrin analogs & derivatives, Transferrin analysis, Transferrin genetics

Abstract

Carbohydrate-deficient transferrin (CDT) is widely accepted as screening test for excessive alcohol consumption. However, results from subjects with transferrin variants must be interpreted with caution since chromatography-based methods may give false-positive results. Furthermore, due to the co-elution in HPLC or the co-migration in capillary zone electrophoresis (CZE) of the di- and trisialylated C transferrins with the tetrasialylated D peak, exact measurement of CDT is impossible in CD-variants. Therefore, in this study, we tried to offer a different solution, including only the asialo-D, asialo-C, monosialo-D, monosialo-C, disialo-D and trisialo-D transferrins in the CDT calculation and referring to a different cut-off value for CDT in transferrin CD-variants. Comparison of alcohol consumers with teetotalers demonstrated area under the receiver operating characteristic curve of 0.79 and 0.76 for carbohydrate-deficient transferrin, 0.71 and 0.71 for mean corpuscular volume and 0.51 and 0.68 for gamma-glutamyltransferase in 43 subjects with transferrin CD-variants and 225 subjects with CC-phenotypes, respectively. Since false-positive carbohydrate-deficient transferrin results due to a transferrin CD-variant have major social implications, capillary electrophoresis-based or similar methods (HPLC, FPLC) should be preferred in populations carrying a high D-allele frequency.

Published

2001

9. A new method for fast haptoglobin phenotyping and hemoglobin binding capacity calculation based on capillary zone electrophoresis.

Author

Wuyts B, Delanghe JR, Kasvosve I, Langlois MR, De Buyzere ML, and Janssens J

Subjects

Electrophoresis, Capillary methods, Electrophoresis, Starch Gel, Haptoglobins chemistry, Haptoglobins genetics, Hemoglobins chemistry, Hemoglobins genetics, Humans, Isoelectric Focusing, Nephelometry and Turbidimetry methods, Neuraminidase metabolism, Phenotype, Polymorphism, Genetic, Protein Binding, Sensitivity and Specificity, Haptoglobins classification, Haptoglobins metabolism, Hemoglobins classification, Hemoglobins metabolism

Abstract

A capillary zone electrophoresis method was developed for haptoglobin (Hp) phenotyping in hemoglobin (Hb) supplemented serum. The method allows a complete resolution of the major haptoglobin phenotypes Hp 1-1, Hp 2-1, and Hp 2-2 based on the difference in charge-to-mass ratio of their Hb-Hp complexes. Identification of these phenotypes was achieved by their significant differences in migration times and their marked difference in electrophoretic pattern. Our method showed full agreement with starch gel electrophoresis. Furthermore, following neuraminidase treatment of the serum, the Hp subtypes Hp1-1FF, FS and SS could be resolved, based on the same criteria as the phenotyping. The new electrophoretic method allowed typing of the rare phenotypes Hp 2-1 modified (Hp 2-1M) and Hp Johnson. The calculated hemoglobin binding capacity of serum correlates well with the nephelometrically determined haptoglobin concentration. The new method for typing haptoglobin gives prospectives for fast haptoglobin typing and Hp 1-1 subtyping.

Published

2000

10. Effect of haptoglobin phenotypes on growth of Streptococcus pyogenes.

Author

Delanghe J, Langlois M, Ouyang J, Claeys G, De Buyzere M, and Wuyts B

Subjects

Antigens, Bacterial immunology, Ferric Compounds blood, Humans, Phenotype, Streptococcus pyogenes immunology, Haptoglobins genetics, Streptococcus pyogenes growth & development

Abstract

The haptoglobin (Hp) 2-1 and 2-2 phenotypes have been shown to agglutinate Streptococcus pyogenes carrying the membrane antigen T4. In this study, the growth rate of two strains of Streptococcus pyogenes (T1 and T4) in human serum was compared among haptoglobin phenotypes in vitro. During incubation for 16 hours in serum of different haptoglobin types, only Hp 2-1 and Hp 2-2 sera showed an inhibitory effect on growth, Hp 2-2 being 1.85 times more potent than Hp 2-1. Growth of Streptococcus pyogenes T4 negatively correlated with the serum concentration of Hp 2-1 (r = -0.908) and Hp 2-2 (r = -0.953). Haptoglobin-depleted serum had no inhibitory effect on bacterial growth. Addition of haemoglobin and ferric citrate to the serum accelerated the growth of Streptococcus pyogenes T4 (P <0.05) but not in Hp 2-2 serum. Haptoglobin types 2-1 and 2-2 can be regarded as inhibitors of Streptococcus pyogenes growth in vitro. These data point towards a potential protective role of Hp 2-2 in Streptococcus pyogenes infection in vivo, independently of iron uptake.

Published

1998