Droplet Digital PCR for BCR–ABL1 Monitoring in Diagnostic Routine: Ready to Start?

Author:

Bochicchio Maria TeresaORCID,Petiti JessicaORCID,Berchialla PaolaORCID,Izzo Barbara,Giugliano Emilia,Ottaviani Emanuela,Errichiello Santa,Rege-Cambrin Giovanna,Venturi Claudia,Luciano Luigiana,Daraio Filomena,Calistri DanieleORCID,Rosti Gianantonio,Saglio Giuseppe,Martinelli GiovanniORCID,Pane Fabrizio,Cilloni DanielaORCID,Gottardi Enrico M.,Fava Carmen

Abstract

BCR–ABL1 mRNA levels represent the key molecular marker for the evaluation of minimal residual disease (MRD) in chronic myeloid leukemia (CML) patients and real-time quantitative PCR (RT-qPCR) is currently the standard method to monitor it. In the era of tyrosine kinase inhibitors (TKIs) discontinuation, droplet digital PCR (ddPCR) has emerged to provide a more precise detection of MRD. To hypothesize the use of ddPCR in clinical practice, we designed a multicentric study to evaluate the potential value of ddPCR in the diagnostic routine. Thirty-seven RNA samples from CML patients and five from healthy donors were analyzed using both ddPCR QXDxTMBCR-ABL %IS Kit and LabNet-approved RT-qPCR methodologies in three different Italian laboratories. Our results show that ddPCR has a good agreement with RT-qPCR, but it is more precise to quantify BCR–ABL1 transcript levels. Furthermore, we did not find differences between duplicate or quadruplicate analysis in terms of BCR–ABL1% IS values. Droplet digital PCR could be confidently introduced into the diagnostic routine as a complement to the RT-qPCR.

Funder

University of Turin

Publisher

MDPI AG

Subject

Cancer Research,Oncology

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