Ying-Jung Huang , Shih-Hsiang Chen , Hsi-Che Liu , Tang-Her Jaing , Ting-Chi Yeh , Ming-Chung Kuo , Tung-Liang Lin , Chiu-Chen Chen , Shih-Chung Wang , Te-Kau Chang , Chih-Cheng Hsiao , Der-Cherng Liang , Lee-Yung Shih
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To validate the NGS approach, NGS-MRD was initially compared with allele-specific oligonucleotide-qPCR-MRD, and the coefficient of determination was good (R<sup>2</sup>=0.8158). A subsequent comparison of NGS-MRD with FT-MRD yielded a good coefficient of determination (R<sup>2</sup>=0.7690), but the coefficient varied by subtype. Specifically, the R<sup>2</sup> was excellent for <em>TCF3::PBX1</em> ALL (R<sup>2</sup>=0.9157), good for <em>ETV6::RUNX1</em> ALL (R<sup>2</sup>=0.8606), and subpar for <em>BCR::ABL1</em> ALL (R<sup>2</sup>=0.5763). The overall concordance between the two methods was 83.7%, and an excellent concordance rate of 95.8% was achieved for <em>TCF3::PBX1</em> ALL. Major discordance, which was defined as a >1 log difference between discordant NGS-MRD and FT-MRD, occurred in 6.7% of the samples, with all but one sample being <em>BCR::ABL1</em> ALL. Among the four non-transplanted patients with <em>BCR::ABL1</em>-MRD (+)/NGS-MRD (−), three did not relapse after long-term follow-up. 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引用次数: 0
摘要
使用下一代测序技术(NGS)监测急性淋巴细胞白血病(ALL)的可测量残留病(MRD)已越来越受到重视。本研究旨在探讨 NGS 在 B 前体 ALL(B-ALL)三大融合转录本(FT)亚型 MRD 监测中的实用性。通过 NGS 和实时定量反转录 PCR(RT-qPCR)分析了 56 例患者 104 份骨髓样本中三种主要 FT 的 MRD 结果:BCR::ABL1、TCF3::PBX1 和 ETV6::RUNX1。为了验证 NGS 方法,最初将 NGS-MRD 与等位基因特异性寡核苷酸-qPCR-MRD 进行了比较,两者的判定系数良好(R2=0.8158)。随后将 NGS-MRD 与 FT-MRD 进行比较,得出了良好的判定系数(R2=0.7690),但系数因亚型而异。具体来说,TCF3::PBX1 ALL 的 R2 非常好(R2=0.9157),ETV6::RUNX1 ALL 的 R2 很好(R2=0.8606),而 BCR::ABL1 ALL 的 R2 不佳(R2=0.5763)。两种方法的总体吻合率为 83.7%,TCF3::PBX1 ALL 的吻合率高达 95.8%。6.7%的样本出现重大不一致,即NGS-MRD和FT-MRD不一致的对数值相差1个对数,除一个样本外,其他样本均为BCR::ABL1 ALL。在 4 例 BCR::ABL1-MRD (+)/NGS-MRD (-) 的非移植患者中,有 3 例在长期随访后没有复发。我们的发现表明,在 ETV6::RUNX1 和 BCR::ABL1 ALL 中,NGS-MRD 比 RT-qPCR-MRD 对预后有更好的影响,而在 TCF3::PBX1 ALL 中,两种方法的疗效相当。
Evaluation of next-generation sequencing for measurable residual disease monitoring in three major fusion transcript subtypes of B-precursor acute lymphoblastic leukaemia
The use of next-generation sequencing (NGS) for monitoring measurable residual disease (MRD) in acute lymphoblastic leukaemia (ALL) has been gaining traction. This study aimed to investigate the utility of NGS in MRD monitoring for the three major fusion transcript (FT) subtypes of B-precursor ALL (B-ALL). The MRD results for 104 bone marrow samples from 56 patients were analysed through NGS and real time quantitative reverse transcription PCR (RT-qPCR) for the three major FTs: BCR::ABL1, TCF3::PBX1, and ETV6::RUNX1. To validate the NGS approach, NGS-MRD was initially compared with allele-specific oligonucleotide-qPCR-MRD, and the coefficient of determination was good (R2=0.8158). A subsequent comparison of NGS-MRD with FT-MRD yielded a good coefficient of determination (R2=0.7690), but the coefficient varied by subtype. Specifically, the R2 was excellent for TCF3::PBX1 ALL (R2=0.9157), good for ETV6::RUNX1 ALL (R2=0.8606), and subpar for BCR::ABL1 ALL (R2=0.5763). The overall concordance between the two methods was 83.7%, and an excellent concordance rate of 95.8% was achieved for TCF3::PBX1 ALL. Major discordance, which was defined as a >1 log difference between discordant NGS-MRD and FT-MRD, occurred in 6.7% of the samples, with all but one sample being BCR::ABL1 ALL. Among the four non-transplanted patients with BCR::ABL1-MRD (+)/NGS-MRD (−), three did not relapse after long-term follow-up. Our finding indicates that NGS-MRD has a better prognostic impact than RT-qPCR-MRD in ETV6::RUNX1 and BCR::ABL1 ALL, whereas in TCF3::PBX1 ALL, both methods exhibit comparable efficacy.
期刊介绍:
Published by Elsevier from 2016
Pathology is the official journal of the Royal College of Pathologists of Australasia (RCPA). It is committed to publishing peer-reviewed, original articles related to the science of pathology in its broadest sense, including anatomical pathology, chemical pathology and biochemistry, cytopathology, experimental pathology, forensic pathology and morbid anatomy, genetics, haematology, immunology and immunopathology, microbiology and molecular pathology.