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血浆无细胞 DNA(cfDNA)在弥漫性神经胶质瘤中检测 IDH1 R132H 突变的临床效用。

Clinical utility of plasma cell-free DNA (cfDNA) in diffuse gliomas for the detection of IDH1 R132H mutation.

机构信息

Neuropathology Laboratory, All India Institute of Medical Sciences, New Delhi, India.

Department of Neurosurgery, All India Institute of Medical Sciences, New Delhi, India.

出版信息

Pathol Res Pract. 2024 Nov;263:155571. doi: 10.1016/j.prp.2024.155571. Epub 2024 Sep 14.

DOI:10.1016/j.prp.2024.155571
PMID:39298928
Abstract

Liquid biopsy for CNS tumors is in its nascent phase, hindered by the low levels of circulating tumor DNA (ctDNA). Overcoming this challenge requires highly sensitive molecular techniques. DD-PCR emerges as a standout technique due to its ability to identify rare mutations, copy number variations, and circulating nucleic acids, making it one of the best methods for identifying somatic mutations in cell-free DNA (cfDNA). Despite promising results from various studies demonstrating the feasibility of obtaining informative ctDNA profiles from liquid biopsy samples, challenges persist, including the need to standardize sample collection, storage, and processing methods, define clear assay positivity thresholds, and address the overall low assay sensitivity. Our two-phase study began by assessing DD-PCR efficacy in FFPE tissues, revealing robust concordance with immunohistochemistry. In Phase 1 (85 cases), DD-PCR on FFPE tissues demonstrated 100 % sensitivity and specificity for IDH1 R132H mutations. In Phase 2 (100 cases), analysis extended to cfDNA, maintaining high specificity (100 %) with moderate sensitivity (44.2 %). Overall concordance with immunohistochemistry was 61 %, highlighting liquid biopsy's potential in glioma management. The findings emphasized DD-PCR's clinical utility in both tissue and liquid biopsy, underscoring its role in early detection, diagnosis, and therapeutic monitoring of diffuse gliomas.

摘要

液体活检在中枢神经系统肿瘤中的应用尚处于起步阶段,其主要障碍在于循环肿瘤 DNA(ctDNA)的含量较低。克服这一挑战需要高度敏感的分子技术。数字 PCR(DD-PCR)作为一种杰出的技术脱颖而出,因为它能够识别罕见的突变、拷贝数变异和循环核酸,是鉴定游离 DNA(cfDNA)中体细胞突变的最佳方法之一。尽管来自各种研究的有希望的结果表明,从液体活检样本中获得有意义的 ctDNA 图谱是可行的,但仍存在挑战,包括需要标准化样本采集、储存和处理方法,定义明确的检测阳性阈值,并解决总体低检测灵敏度的问题。我们的两阶段研究首先评估了 DD-PCR 在 FFPE 组织中的效果,结果显示其与免疫组织化学具有很强的一致性。在第一阶段(85 例),FFPE 组织上的 DD-PCR 对 IDH1 R132H 突变的检测具有 100%的敏感性和特异性。在第二阶段(100 例),分析扩展到 cfDNA,具有高特异性(100%)和中等敏感性(44.2%)。与免疫组织化学的总体一致性为 61%,这突显了液体活检在神经胶质瘤管理中的潜力。这些发现强调了 DD-PCR 在组织和液体活检中的临床应用价值,突出了其在弥漫性神经胶质瘤的早期检测、诊断和治疗监测中的作用。

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