Measurement of islet cell antibodies in the Type 1 Diabetes Genetics Consortium: efforts to harmonize procedures among the laboratories

Author:

Bingley Polly J1,Williams Alistair JK1,Colman Peter G2,Gellert Shane A2,Eisenbarth George3,Yu Liping3,Perdue Letitia H4,Pierce June J4,Hilner Joan E5,Nierras Concepcion6,Akolkar Beena7,Steffes Michael W8,

Affiliation:

1. Department of Clinical Science at North Bristol, University of Bristol, Bristol, UK

2. Departments of Diabetes and Endocrinology and Pathology, Royal Melbourne Hospital, Melbourne, Victoria, Australia

3. Barbara Davis Center for Childhood Diabetes, University of Colorado Health Sciences, Denver, CO, USA

4. Division of Public Health Sciences, Wake Forest University Health Sciences, Winston-Salem, NC, USA

5. Department of Biostatistics, School of Public Health, University of Alabama at Birmingham, Birmingham, AL, USA

6. Juvenile Diabetes Research Foundation International, New York, NY, USA

7. Division of Diabetes, Endocrinology and Metabolic Diseases, National Institute of Diabetes and Digestive and Kidney Diseases, National Institutes of Health, Bethesda, MD, USA

8. Department of Laboratory Medicine and Pathology, University of Minnesota Medical School, Minneapolis, MN, USA, steff001@umn.edu

Abstract

Background and Purpose Three network laboratories measured antibodies to islet autoantigens. Antibodies to glutamic acid decarboxylase (GAD65 [GADA]) and the intracellular portion of protein tyrosine phosphatase (IA-2ic [IA-2A]) were measured by similar, but not identical, methods in samples from participants in the Type 1 Diabetes Genetics Consortium (T1DGC). Methods All laboratories used radiobinding assays to detect antibodies to in vitro transcribed and translated antigen, but with different local standards, calibrated against the World Health Organization (WHO) reference reagent. Using a common method to calculate WHO units/mL, we compared results reported on samples included in the Diabetes Autoantibody Standardization Program (DASP), and developed standard methods for reporting in WHO units/mL. We evaluated intra-assay and inter-assay coefficient of variation (CV) in blind duplicate samples and assay comparability in four DASP workshops. Results Values were linearly related in the three laboratories for both GADA and IA-2A, and intra-assay technical errors for values within the standard curve were below 13% for GADA and below 8.5% for IA-2A. Correlations in samples tested 1—2 years apart were >97%. Over the course of the study, internal CVs were 10—20% with one exception, and the laboratories concordantly called samples GADA or IA-2A positive or negative in 96.7% and 99.6% of duplicates within the standard curve. Despite acceptable CVs and general concordance in ranking samples, the laboratories differed markedly in absolute values for GADA and IA-2A reported in WHO units/mL in DASP over a large range of values. Limitations With three laboratories using different assay methods (including calibrators), consistent values among them could not be attained. Conclusions Modifications in the assays are needed to improve comparability of results expressed as WHO units/mL across laboratories. It will be essential to retain high intra- and inter-assay precision, sensitivity and specificity and to confirm the accuracy of harmonized methods. Clinical Trials 2010; 7: S56—S64. http:// ctj.sagepub.com

Publisher

SAGE Publications

Subject

Pharmacology,General Medicine

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