Objectives: We performed a feasibility study of an FDA-approved commercial ddPCR assay to measure :: in CML patients treated using TKI therapy.

Methods: Assay performance of standard RQ-PCR and commercially available FDA-approved ddPCR were compared to measure :: p210 transcripts in RNA samples from 100 CML patients who received TKI therapy.

Results: %::/ levels obtained from both methods were not statistically significant difference after normalization with batch-specific conversion factor ( = 0.0651). The correlation and agreement of %::/ between the two assays were high. Molecular response stratification data showed 56% concordance between RQ-PCR and ddPCR, and 37% higher residual disease detection using ddPCR. Furthermore, 21.21% (7/33) of RQ-PCR undetectable samples were detected by ddPCR, representing high sensitivity to quantify the low abundance of :: transcripts.

Conclusion: ddPCR was proven to be a highly sensitive method with the potential to overcome some limitations of traditional RQ-PCR, and has the potential of being a valuable tool for monitoring :: transcripts in CML during TKI therapy. (163 words).

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http://dx.doi.org/10.1080/16078454.2023.2256199DOI Listing

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