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Literature DB >> 35908105

Droplet digital PCR for the detection of second-generation tyrosine kinase inhibitor-resistant BCR::ABL1 kinase domain mutations in chronic myeloid leukemia.

Sara De Santis¹, Margherita Martelli¹, Cecilia Monaldi¹, Simona Soverini², Fausto Castagnetti³, Gabriele Gugliotta⁴, Cristina Papayannidis⁴, Manuela Mancini⁴, Samantha Bruno¹, Claudia Venturi⁴, Katerina Machova Polakova⁵, Thomas Ernst⁶, Dianna Maar⁷, Adam Corner⁸, Michele Cavo³.

Abstract

One of the indications for BCR::ABL1 mutation testing in chronic myeloid leukemia (CML) is when tyrosine kinase inhibitor therapy (TKI) needs to be changed for unsatisfactory response. In this study, we evaluated a droplet digital PCR (ddPCR)-based multiplex strategy for the detection and quantitation of transcripts harbouring mutations conferring resistance to second-generation TKIs (2GTKIs). Parallel quantitation of e13a2, e14a2 and e1a2 BCR::ABL1 fusion transcripts enables to express results as percentage of mutation positive- over total BCR::ABL1 transcripts. We determined the limit of blank in 60 mutation-negative samples. Accuracy was demonstrated by further analysis of 48 samples already studied by next generation sequencing (NGS). Mutations could be called down to 0.5% and across 3-logs of BCR::ABL1 levels. Retrospective review of BCR::ABL1 NGS results in 513 consecutive CML patients with non-optimal response to first- or second-line TKI therapy suggested that a ddPCR-based approach targeted against 2GTKI-resistant mutations would score samples as mutation-negative in 22% of patients with warning response to imatinib but only in 6% of patients with warning response to 2GTKIs. We conclude ddPCR represents an attractive method for easy, accurate and rapid screening for 2GTKI-resistant mutations impacting on TKI selection, although ddPCR cannot identify compound mutations.

Entities: Chemical

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Year: 2022 PMID： 35908105 DOI： 10.1038/s41375-022-01660-8

Source DB: PubMed Journal: Leukemia ISSN： 0887-6924 Impact factor: 12.883

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