Targeted Analysis of Cell-free Circulating Tumor DNA is Suitable for Early Relapse and Actionable Target Detection in Patients with Neuroblastoma

神经母细胞瘤 液体活检 医学 间变性淋巴瘤激酶 微小残留病 肿瘤科 脑脊液 数字聚合酶链反应 靶向治疗 病理 癌症研究 生物标志物 内科学 癌症 生物 聚合酶链反应 肺癌 基因 细胞培养 白血病 生物化学 遗传学 恶性胸腔积液
作者
Marco Lodrini,Josefine Graef,Theresa M. Thole-Kliesch,Kathy Astrahantseff,Annika Sprüssel,Maddalena Grimaldi,Constantin Peitz,Rasmus B. Linke,Jan F. Hollander,Erwin Lankes,Annette Künkele,Lena Oevermann,Georg C. Schwabe,Jörg Fuchs,Annabell Szymansky,Johannes H. Schulte,Patrick Hundsdörfer,Cornelia Eckert,Holger Amthauer,Angelika Eggert
出处
期刊:Clinical Cancer Research [American Association for Cancer Research]
卷期号:28 (9): 1809-1820 被引量:40
标识
DOI:10.1158/1078-0432.ccr-21-3716
摘要

Abstract Purpose: Treating refractory or relapsed neuroblastoma remains challenging. Monitoring body fluids for tumor-derived molecular information indicating minimal residual disease supports more frequent diagnostic surveillance and may have the power to detect resistant subclones before they give rise to relapses. If actionable targets are identified from liquid biopsies, targeted treatment options can be considered earlier. Experimental Design: Droplet digital PCR assays assessing MYCN and ALK copy numbers and allelic frequencies of ALK p.F1174L and ALK p.R1275Q mutations were applied to longitudinally collected liquid biopsies and matched tumor tissue samples from 31 patients with high-risk neuroblastoma. Total cell-free DNA (cfDNA) levels and marker detection were compared with data from routine clinical diagnostics. Results: Total cfDNA concentrations in blood plasma from patients with high-risk neuroblastoma were higher than in healthy controls and consistently correlated with neuron-specific enolase levels and lactate dehydrogenase activity but not with 123I-meta-iodobenzylguanidine scores at relapse diagnosis. Targeted cfDNA diagnostics proved superior for early relapse detection to all current diagnostics in 2 patients. Marker analysis in cfDNA indicated intratumor heterogeneity for cell clones harboring MYCN amplifications and druggable ALK alterations that were not detectable in matched tumor tissue samples in 17 patients from our cohort. Proof of concept is provided for molecular target detection in cerebrospinal fluid from patients with isolated central nervous system relapses. Conclusions: Tumor-specific alterations can be identified and monitored during disease course in liquid biopsies from pediatric patients with high-risk neuroblastoma. This approach to cfDNA surveillance warrants further prospective validation and exploitation for diagnostic purposes and to guide therapeutic decisions.
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