A Novel Next-Generation Sequencing Assay for the Identification of BCR::ABL1 Transcript Type and Accurate and Sensitive Detection of TKI-Resistant Mutations.

IF 1.8 Q3 MEDICAL LABORATORY TECHNOLOGY Journal of Applied Laboratory Medicine Pub Date : 2024-11-04 DOI:10.1093/jalm/jfae096
Zhenyu Yan, Lin Shi, Wei Li, Weihua Liu, Chad Galderisi, Cynthia Spittle, Jin Li
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Abstract

Background: The clinical management of chronic myeloid leukemia (CML) patients requires the identification of the type of BCR::ABL1 transcript at diagnosis and the monitoring of its expression and potential tyrosine kinase inhibitor (TKI) resistance mutations during treatment. Detection of resistant mutation requires transcript type-specific amplification of BCR::ABL1 from RNA.

Methods: In this study, a custom RNA-based next-generation sequencing (NGS) assay (Dup-Seq BCR::ABL1) that enables (a) the identification of BCR::ABL1 transcript type and (b) the detection of resistance mutations from common and atypical BCR::ABL1 transcript types was developed and validated. The assay design covers BCR exon 1 to ABL1 exon 10 and employs duplicate PCR amplification for error correction. The custom data analysis pipeline enables breakpoint determination and overlapped mutation calling from duplicates, which minimizes the low-level mutation artifacts.

Results: This study demonstrates that this novel assay achieves high accuracy (positive percent agreement (PPA) for fusion: 98.5%; PPA and negative percent agreement (NPA) for mutation at 97.8% and 100.0%, respectively) and sensitivity (limit of detection (LOD) for mutation detection at 3% from 10 000 copies of BCR::ABL1 input).

Conclusions: The Dup-Seq BCR::ABL1 assay not only allows for the identification of BCR::ABL1 typical and atypical transcript types and accurate and sensitive detection of TKI-resistant mutations but also simplifies molecular testing work flow for the clinical management of CML patients.

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一种用于鉴定 BCR::ABL1 转录本类型并准确灵敏地检测 TKI 抗性突变的新型下一代测序分析法。
背景:慢性髓性白血病(CML)患者的临床治疗需要在诊断时确定BCR::ABL1转录本的类型,并在治疗过程中监测其表达和潜在的酪氨酸激酶抑制剂(TKI)耐药突变。检测耐药突变需要从 RNA 中扩增 BCR::ABL1 的转录本类型特异性:本研究开发并验证了一种基于 RNA 的定制下一代测序(NGS)检测方法(Dup-Seq BCR::ABL1),该检测方法可(a)识别 BCR::ABL1 转录本类型,(b)从常见和非典型 BCR::ABL1 转录本类型中检测耐药突变。检测设计涵盖 BCR 外显子 1 至 ABL1 外显子 10,并采用重复 PCR 扩增进行纠错。定制的数据分析管道可确定断点并从重复序列中进行重叠突变调用,从而最大限度地减少低水平突变伪影:结果:这项研究表明,这种新型检测方法具有很高的准确性(融合的阳性一致率(PPA)为 98.5%;突变的阳性一致率(PPA)和阴性一致率(NPA)分别为 97.8% 和 100.0%)和灵敏度(突变检测的检测限(LOD)为 3%,BCR::ABL1 的输入量为 10,000 拷贝):结论:Dup-Seq BCR::ABL1检测不仅能鉴定BCR::ABL1典型和非典型转录本类型,准确灵敏地检测TKI耐药突变,还能简化CML患者临床管理的分子检测工作流程。
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来源期刊
Journal of Applied Laboratory Medicine
Journal of Applied Laboratory Medicine MEDICAL LABORATORY TECHNOLOGY-
CiteScore
3.70
自引率
5.00%
发文量
137
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