Establishment and validation of analytical reference panels for the standardization of quantitative BCR-ABL1 measurements on the international scale

White, H.; Hedges, J.; Bendit, I.; Branford, S.; Colomer, D.; Hochhaus, A.; Hughes, T.; Kamel-Reid, S.; Kim, D.; Modur, V.; Muller, M.; Pagnano, K.; Pane, F.; Radich, J.; Cross, N.; Labourier, E.

Please use this identifier to cite or link to this item: https://hdl.handle.net/2440/79137

Scopus	Web of Science®	Altmetric
Citations
?	?

Type:	Journal article
Title:	Establishment and validation of analytical reference panels for the standardization of quantitative BCR-ABL1 measurements on the international scale
Author:	White, H. Hedges, J. Bendit, I. Branford, S. Colomer, D. Hochhaus, A. Hughes, T. Kamel-Reid, S. Kim, D. Modur, V. Muller, M. Pagnano, K. Pane, F. Radich, J. Cross, N. Labourier, E.
Citation:	Clinical Chemistry (Washington, DC): international journal of molecular diagnostics and laboratory medicine, 2013; 59(6):938-948
Publisher:	Amer Assoc Clinical Chemistry
Issue Date:	2013
ISSN:	0009-9147 1530-8561
Statement of Responsibility:	Helen E. White, John Hedges, Israel Bendit, Susan Branford, Dolors Colomer, Andreas Hochhaus, Timothy Hughes, Suzanne Kamel-Reid, Dong-Wook Kim, Vijay Modur, Martin C. Müller, Katia B. Pagnano, Fabrizio Pane, Jerry Radich, Nicholas C.P. Cross and Emmanuel Labourier
Abstract:	BACKGROUND: Current guidelines for managing Philadelphia-positive chronic myeloid leukemia include monitoring the expression of the BCR-ABL1 (breakpoint cluster region/c-abl oncogene 1, non-receptor tyrosine kinase) fusion gene by quantitative reverse-transcription PCR (RT-qPCR). Our goal was to establish and validate reference panels to mitigate the interlaboratory imprecision of quantitative BCR-ABL1 measurements and to facilitate global standardization on the international scale (IS). METHODS: Four-level secondary reference panels were manufactured under controlled and validated processes with synthetic Armored RNA Quant molecules (Asuragen) calibrated to reference standards from the WHO and the NIST. Performance was evaluated in IS reference laboratories and with non–IS-standardized RT-qPCR methods. RESULTS: For most methods, percent ratios for BCR-ABL1 e13a2 and e14a2 relative to ABL1 or BCR were robust at 4 different levels and linear over 3 logarithms, from 10% to 0.01% on the IS. The intraassay and interassay imprecision was <2-fold overall. Performance was stable across 3 consecutive lots, in multiple laboratories, and over a period of 18 months to date. International field trials demonstrated the commutability of the reagents and their accurate alignment to the IS within the intra- and interlaboratory imprecision of IS-standardized methods. CONCLUSIONS: The synthetic calibrator panels are robust, reproducibly manufactured, analytically calibrated to the WHO primary standards, and compatible with most BCR-ABL1 RT-qPCR assay designs. The broad availability of secondary reference reagents will further facilitate interlaboratory comparative studies and independent quality assessment programs, which are of paramount importance for worldwide standardization of BCR-ABL1 monitoring results and the optimization of current and new therapeutic approaches for chronic myeloid leukemia.
Keywords:	Severity of Illness Index Reverse Transcriptase Polymerase Chain Reaction Genes, abl Reference Standards Leukemia, Myelogenous, Chronic, BCR-ABL Positive Genetic Testing
Rights:	© 2013 The American Association for Clinical Chemistry
DOI:	10.1373/clinchem.2012.196477
Published version:	http://dx.doi.org/10.1373/clinchem.2012.196477
Appears in Collections:	Aurora harvest 4 Molecular and Biomedical Science publications

Files in This Item:

There are no files associated with this item.

Show full item record

Adelaide Research & Scholarship