EQUAL-quant: An International External Quality Assessment Scheme for Real-Time PCR

Author:

Ramsden Simon C1,Daly Sarah2,Geilenkeuser Wolf-Jochen3,Duncan Graeme4,Hermitte Fabienne4,Marubini Ettore5,Neumaier Michael6,Orlando Claudio7,Palicka Vladimir8,Paradiso Angelo9,Pazzagli Mario7,Pizzamiglio Sara10,Verderio Paolo10

Affiliation:

1. National Genetics Reference Laboratory (Manchester), St. Mary’s Hospital, Manchester, UK

2. Molecular Diagnostic Centre, Manchester Royal Infirmary, Manchester, UK

3. DGKL-Reference Institute for Bioanalytics, Bonn, Germany

4. Ipsogen, Luminy Biotech Enterprises, Marseilles, France

5. Institute of Medical Statistics and Biometry, University of Milan, Milan, Italy

6. Institute for Clinical Chemistry, University Hospital Mannheim of the University of Heidelberg, Mannheim, Germany

7. Clinical Biochemistry Unit, Department of Clinical Physiopathology, University of Florence, Florence, Italy

8. Institute for Clinical Biochemistry and Diagnostics, School of Medicine, University Hospital Sokolska, Hradec Králové, Czech Republic

9. National Cancer Institute, Bari, Italy

10. Operative Unit of Medical Statistics and Biometry, Instituto Nazionale per lo Studio e la Cura dei Tumori, Milan, Italy

Abstract

Abstract Background: Quantitative gene expression analysis by real-time PCR is important in several diagnostic areas, such as the detection of minimum residual disease in leukemia and the prognostic assessment of cancer patients. To address quality assurance in this technically challenging area, the European Union (EU) has funded the EQUAL project to develop methodologic external quality assessment (EQA) relevant to diagnostic and research laboratories among the EU member states. We report here the results of the EQUAL-quant program, which assesses standards in the use of TaqMan™ probes, one of the most widely used assays in the implementation of real-time PCR. Methods: The EQUAL-quant reagent set was developed to assess the technical execution of a standard TaqMan assay, including RNA extraction, reverse transcription, and real-time PCR quantification of target DNA copy number. Results: The multidisciplinary EQA scheme included 137 participating laboratories from 29 countries. We demonstrated significant differences in performance among laboratories, with 20% of laboratories reporting at least one result lacking in precision and/or accuracy according to the statistical procedures described. No differences in performance were observed for the >10 different testing platforms used by the study participants. Conclusions: This EQA scheme demonstrated both the requirement and demand for external assessment of technical standards in real-time PCR. The reagent design and the statistical tools developed within this project will provide a benchmark for defining acceptable working standards in this emerging technology.

Publisher

Oxford University Press (OUP)

Subject

Biochemistry (medical),Clinical Biochemistry

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