Clinical Utility of a Novel Triplex Digital PCR Assay for Clone Monitoring in Sequential and Relapsed Pediatric B-Cell Acute Lymphoblastic Leukemia Patients.

IF 2.4 3区医学 Q2 HEMATOLOGY Pediatric Blood & Cancer Pub Date : 2024-11-24 DOI:10.1002/pbc.31443

Prateek Bhatia, Rozy Thakur, Sreejesh Sreedharanunni, Minu Singh, Meenakshi Malhotra, Swati Arora, Ashish George, Amita Trehan

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Abstract

Introduction: Digital polymerase chain reaction (PCR) studies for clonal disease monitoring in B-acute lymphoblastic leukemia patients are currently limited due to the heterogeneous nature of mutations, which limit cost-effective assay designs.

Materials and methods: In this study, 70 samples (14 relapse and 56 sequential therapy samples) were tested for 13 recurrent mutations identified on deep sequencing in our published cohort (KRAS, NRAS, NT5C2, PMS2, UHRF1, KMT2D, and TP53 genes) via a novel triplex digital PCR assay.

Results and discussion: A total of seven major clones of NRAS [five] and NT5C2 [two] were noted in six out of 14 (43%) relapse patients, accounting for 44% of early relapses. In addition, 10 minor clones (PMS2 [two], NRAS [four], NT5C2 [three], and TP53 [one]) were noted in five out of 14 (36%) patients. In the 56 sequential therapy samples, six major clones were noted (NRAS [five], KRAS [one]) in four out of 14 (28.5%) patients, with two increasing in size in maintenance samples, leading to subsequent relapse in both cases. In addition, therapy-acquired minor clones in NT5C2 [four] and PMS2 [one] were seen to emerge in maintenance samples in four out of 14 (28.5%) patients, with concordant detection of such major and minor clones in unpaired relapse samples, indicating the need for their active surveillance during therapy. Overall, digital PCR validated NRAS and NT5C2 major clones in one-third (10 out of 27; 37%) of cases, driving nearly half of early relapses.

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新型三重数字 PCR 检测法对连续性和复发性小儿 B 细胞急性淋巴细胞白血病患者克隆监测的临床实用性

导言：由于突变的异质性，目前用于监测B型急性淋巴细胞白血病患者克隆性疾病的数字聚合酶链反应（PCR）研究非常有限，这限制了具有成本效益的检测设计：在这项研究中，我们通过一种新型三重数字 PCR 检测法对 70 份样本（14 份复发样本和 56 份连续治疗样本）进行了检测，以检测我们已发表的队列中通过深度测序发现的 13 种复发突变（KRAS、NRAS、NT5C2、PMS2、UHRF1、KMT2D 和 TP53 基因）：在14例复发患者中，有6例（43%）发现了NRAS（5个）和NT5C2（2个）共7个主要克隆，占早期复发患者的44%。此外，14 名患者中有 5 名（36%）发现了 10 个小克隆（PMS2 [2]、NRAS [4]、NT5C2 [3] 和 TP53 [1]）。在 56 份连续治疗样本中，14 位患者中有 4 位（28.5%）发现了 6 个主要克隆（NRAS [5个]、KRAS [1个]），其中 2 个克隆在维持样本中增大，导致两个病例随后复发。此外，在 14 例（28.5%）患者中，有 4 例（28.5%）的维持样本中出现了治疗获得的 NT5C2 [4 例] 和 PMS2 [1 例] 小克隆，在未配对的复发样本中也同时检测到了此类主要和次要克隆，这表明在治疗期间需要对其进行积极监测。总体而言，数字 PCR 验证了三分之一病例（27 例中有 10 例，占 37%）的 NRAS 和 NT5C2 主要克隆，导致近一半的早期复发。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

Pediatric Blood & Cancer 医学-小儿科

CiteScore

4.90

自引率

9.40%

发文量

546

审稿时长

1.5 months

期刊介绍： Pediatric Blood & Cancer publishes the highest quality manuscripts describing basic and clinical investigations of blood disorders and malignant diseases of childhood including diagnosis, treatment, epidemiology, etiology, biology, and molecular and clinical genetics of these diseases as they affect children, adolescents, and young adults. Pediatric Blood & Cancer will also include studies on such treatment options as hematopoietic stem cell transplantation, immunology, and gene therapy.