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核磷蛋白突变的急性髓系白血病临床缓解期出现的 FLT3 ITD 阳性克隆的鉴定及疾病复发的动力学研究

Identification of emerging FLT3 ITD-positive clones during clinical remission and kinetics of disease relapse in acute myeloid leukaemia with mutated nucleophosmin.

机构信息

Department of Biopathology, University of Tor Vergata, Rome, Italy.

出版信息

Br J Haematol. 2013 May;161(4):533-40. doi: 10.1111/bjh.12288. Epub 2013 Mar 11.

DOI:10.1111/bjh.12288
PMID:23480665
Abstract

FLT3 internal tandem duplication (ITD) mutations are frequently detected at diagnosis in cytogenetically normal acute myeloid leukaemia (CN-AML) and predict unfavourable outcome. FLT3 ITD is an unstable aberration and may be lost or acquired at relapse. Recent whole genome sequencing studies have suggested that FLT3 ITD(+)ve AML relapse may evolve from small subclones undetectable at diagnosis by routine polymerase chain reaction (PCR). We developed a patient-specific real-time quantitative-PCR (RQ-PCR) to implement FLT3 ITD detection in six AML patients whose blasts carried wild-type FLT3 at diagnosis and who relapsed with FLT3 ITD by routine PCR. Patient-specific forward primers were designed after cloning and sequencing the FLT3 ITD in each case. The assay allowed retrospective detection of FLT3 ITD in diagnostic samples of 4/6 cases and to establish the kinetics of clonal evolution preceding relapse. After conventional chemotherapy, all patients had early relapse despite having been classified as NPM1(+)ve/FLT3 ITD(-)ve at presentation, with shorter remissions being observed in four patients re-classified as FLT3 ITD(+)ve by the new assay. Notably, FLT3 ITD clone became detectable by conventional PCR in three patients tested during remission after initial treatment. Our data underscore the need of identifying low FLT3 ITD levels, which are probably associated with relapse in otherwise good prognosis CN-AML.

摘要

FLT3 内部串联重复(ITD)突变在细胞遗传学正常的急性髓系白血病(CN-AML)的诊断中经常被检测到,并预测预后不良。FLT3 ITD 是一种不稳定的畸变,可能在复发时丢失或获得。最近的全基因组测序研究表明,FLT3 ITD(+) AML 复发可能是由常规聚合酶链反应(PCR)在诊断时无法检测到的小亚克隆演变而来。我们开发了一种患者特异性实时定量 PCR(RQ-PCR),用于检测 6 名患者的 FLT3 ITD,这些患者在诊断时的blasts 携带野生型 FLT3,并且通过常规 PCR 复发时带有 FLT3 ITD。在每个病例中克隆和测序 FLT3 ITD 后,设计了患者特异性的正向引物。该检测方法允许在 4/6 例病例的诊断样本中进行回顾性检测 FLT3 ITD,并确定复发前克隆进化的动力学。尽管在最初治疗后检测到的缓解期患者中,所有患者均出现早期复发,4 例患者通过新检测方法重新分类为 FLT3 ITD(+),缓解期较短,但所有患者在接受常规化疗后均出现早期复发。值得注意的是,在最初治疗后缓解期检测到的 3 例患者中,常规 PCR 可检测到 FLT3 ITD 克隆。我们的数据强调了需要确定低水平的 FLT3 ITD,这可能与细胞遗传学正常的 AML 患者的复发有关。

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