BMC Genomics (Jun 2007)

Robust interlaboratory reproducibility of a gene expression signature measurement consistent with the needs of a new generation of diagnostic tools

  • Cardoso Fatima,
  • Ripoche Hugues,
  • Tsalenko Anya,
  • Pover Rob,
  • Glas Annuska M,
  • Lazar Vladimir,
  • Curry Bo,
  • Floore Arno,
  • Ach Robert A,
  • d'Assignies Mahasti,
  • Bruhn Laurakay,
  • Van't Veer Laura J

DOI
https://doi.org/10.1186/1471-2164-8-148
Journal volume & issue
Vol. 8, no. 1
p. 148

Abstract

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Abstract Background The increasing use of DNA microarrays in biomedical research, toxicogenomics, pharmaceutical development, and diagnostics has focused attention on the reproducibility and reliability of microarray measurements. While the reproducibility of microarray gene expression measurements has been the subject of several recent reports, there is still a need for systematic investigation into what factors most contribute to variability of measured expression levels observed among different laboratories and different experimenters. Results We report the results of an interlaboratory comparison of gene expression array measurements on the same microarray platform, in which the RNA amplification and labeling, hybridization and wash, and slide scanning were each individually varied. Identical input RNA was used for all experiments. While some sources of variation have measurable influence on individual microarray signals, they showed very low influence on sample-to-reference ratios based on averaged triplicate measurements in the two-color experiments. RNA labeling was the largest contributor to interlaboratory variation. Conclusion Despite this variation, measurement of one particular breast cancer gene expression signature in three different laboratories was found to be highly robust, showing a high intralaboratory and interlaboratory reproducibility when using strictly controlled standard operating procedures.