Validation of a novel NGS based BCR::ABL1 kinase domain mutation detection assay in Indian cohort

Author:

Chaudhary Pooja,Chaudhary Spandan,Patel Falguni,Patel Shiv,Vaishnani Toral,Trivedi Nikha,Patel Dhiren,Sonagara Tushar,Hirapara Ashish,Vyas Kavisha,Patel Lokesh,Kumar Raja,Chakraborty Nikkan,Sharma Divya,Suthar Jigar,Kamdar Payal,Jajodia Ekta,Ahmad Firoz,Arora Neeraj

Abstract

AbstractThe efficacy and treatment outcome of a CML patient are heavily dependent on BCR::ABL1 kinase domain (KD) mutation status. Next-generation sequencing technology is a bright alternative to the previously used sanger sequencing method due to its global presence in diagnostic setups, massive parallel sequencing ability, and far better sensitivity. In the present study, we have demonstrated a new protocol for kinase domain mutation analysis using the next-generation sequencing (NGS) method using the ion torrent sequencing platform. This protocol uses RNA as the starting material, followed by nested PCR to amplify the fusion transcript, which is subsequently used as a template for NGS. Initial validation and comparison of this assay with the sanger sequencing (SS) method yielded 95.23% agreement. CML samples (n = 121) with a failure to TKI response were subjected to this newly developed NGS-based assay to detect KD mutations, from which samples were found to have mutations with a sensitivity ranging from 2.32 to 93.41%. A total of 34.71% of samples (n = 42) were found to be positive for one or more KD mutations, whereas 65.29% of samples (n = 81) were found to be negative. Nine samples out of 42 positive samples, i.e., 21.42%, were found to have compound mutations. This is one of the first studies from India, which includes more than 160 samples and is analyzed by the NGS approach for KD mutation analysis.

Publisher

Springer Science and Business Media LLC

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