Comparison of cross-platform flow cytometry minimal residual disease evaluation in multiple myeloma using a common antibody combination and analysis strategy.
Fiche publication
Date publication
octobre 2014
Auteurs
Membres identifiés du Cancéropôle Est :
Pr MAYNADIE Marc
Tous les auteurs :
Mathis S, Chapuis N, Borgeot J, Maynadie M, Fontenay M, Bene MC, Guy J, Bardet V
Lien Pubmed
Résumé
Background: A seven-color/eight-antibody approach has recently been proposed for the minimal residual disease (MRD) determination in multiple myeloma (MM), which was developed on FACSCantoII instruments. This strategy should be also applicable on different multiparameter flow cytometers (MFC), but this needs to be demonstrated before moving MRD assessment to local flow cytometry core facilities, nearer to patients, thereby reducing the risk of cell losses induced by sample transportation and delays in cell processing. Methods: To evaluate the comparability of testing the same 7-color/8-antibody single-tube on any instruments, MRD was evaluated concomitantly on two distinct MFC in a cohort of 80 bone marrow MM samples (ie. 73 patients including 7 with 2 MRD evaluations) in two French centers, Paris-Cochin and Dijon. Results: No significant difference in the MM residual plasma-cells (MM-PCs) quantification was observed. Calculated on the basis of the whole amount of leukocytes assessed, the mean MRD percentage was respectively 0.1661% and 0.1458% using FACSCantoII or Navios instruments, with a very high correlation between instruments (r2 = 0.9798) and a very minimal bias (-0.02). Moreover, there was no difference in MRD interpretation at 10-4 threshold; whereas 3 MRD interpretation discordances were observed at 2.5x10-5 threshold. Conclusion: This study demonstrates that this MRD-detection strategy is transposable between harmonized >/=7-color instruments. This shows that a homogeneous rapid MRD evaluation can be performed in most MFC platforms, in the near vicinity of clinical wards. However, the clinical validation of this approach needs to be strengthened, as well as its relevance compared to molecular approaches. (c) 2014 Clinical Cytometry Society.
Référence
Cytometry B Clin Cytom. 2014 Oct 28