循环游离DNA的浓度和完整性指数作为儿科B-ALL患者的生物标志物。

Jessica Fabiola Rodriguez-Ortiz, Anilú Margarita Saucedo-Sariñana, Mónica Alejandra Rosales-Reynoso, Janet Soto Padilla, Rocío Ortíz-López, Ana Rebeca Jaloma-Cruz, César de Jesús Tovar-Jácome, Patricio Barros-Núñez
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引用次数: 0

摘要

本研究的目的是评估循环无细胞DNA (ccf-DNA)的浓度和完整性指数作为检测和监测儿童b细胞急性淋巴细胞白血病(B-ALL)患者微量残留病(MRD)的生物标志物。与一种有效的方法进行了比较,用于定量的单克隆重排的IGH基因。收集了10例B-ALL患儿在诊断、缓解和维持期的外周血和骨髓样本。使用Qubit®荧光法估计ccf-DNA总浓度,并通过ALU247/ALU115片段的qPCR扩增获得完整性指数。采用多重PCR定量分析单克隆重排,毛细管电泳检测单克隆重排。结果显示,诊断时ccf-DNA平均浓度为5607 ng/mL,完整性指数为0.38;缓解诱导期分别为968 ng/mL和0.35 ng/mL;维持期分别为748 ng/mL和0.33 ng/mL。治疗期间差异有统计学意义(p=0.02)。对照组ccf-DNA平均浓度为247 ng/mL,完整性指数为0.20,与患者组比较差异有统计学意义(p=0.01)。单克隆分析显示诊断和缓解之间(p=0.022)以及诊断和维持之间(p=0.001)存在显著差异。治疗期间的线性回归分析显示ccf-DNA浓度和单克隆性的趋势相似。综上所述,ccf-DNA浓度和完整性指数可以作为监测B-ALL患者MRD的有用生物标志物,其疗效与检测IGH基因单克隆相当。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Concentration and integrity index of circulating cell-free DNA as a biomarker in pediatric patients with B-ALL.

The objective of this study was to evaluate the concentration and integrity index of circulating cell-free DNA (ccf-DNA) as biomarkers for the detection and monitoring of minimal residual disease (MRD) in pediatric patients with B-cell acute lymphoblastic leukemia (B-ALL). Comparison with a validated methodology for the quantification of monoclonal rearrangements of the IGH gene was made. Peripheral blood and bone marrow samples were collected from 10 pediatric patients with B-ALL at diagnosis, remission, and maintenance phases. Total ccf-DNA concentration was estimated using Qubit® fluorometry, and the integrity index was obtained through qPCR amplification of ALU247/ALU115 fragments. Monoclonal rearrangements of the IGH gene were quantified by multiplex PCR and detected by capillary electrophoresis. Results showed that at diagnosis, the mean ccf-DNA concentration was 5,607 ng/mL with an integrity index of 0.38; during remission induction, they were 968 ng/mL and 0.35; and during the maintenance phase, 748 ng/mL and 0.33, respectively. Differences between treatment phases were significant (p=0.02). The reference group had a mean ccf-DNA concentration of 247 ng/mL and an integrity index of 0.20, showing significant differences compared to the patient group (p=0.01). Monoclonality analysis showed significant differences between diagnosis and remission (p=0.022) and between diagnosis and maintenance (p=0.001). Linear regression analysis during treatment demonstrated a similar trend for ccf-DNA concentration and monoclonality. In conclusion, ccf-DNA concentration and integrity index could be useful biomarkers for monitoring MRD in patients with B-ALL, showing comparable efficacy to the detection of monoclonality in the IGH gene.

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