Matched Molecular Profiling of Cell-Free DNA and Tumor Tissue in Patients With Advanced Clear Cell Renal Cell Carcinoma

一致性 医学 肾细胞癌 胎儿游离DNA 肾透明细胞癌 基因分型 肿瘤科 生物标志物 队列 病理 内科学 生物 基因型 基因 遗传学 怀孕 胎儿 产前诊断
作者
Ritesh Kotecha,Erika Gedvilaite,Ryan Ptashkin,Andrea Knezevic,Samuel Murray,Ian Johnson,Natalie Shapnik,Darren R. Feldman,Maria I. Carlo,Neil J Shah,Marisa Dunigan,Kety Huberman,Ryma Benayed,Ahmet Zehir,Michael F. Berger,Marc Ladanyi,Dana W.Y. Tsui,Robert J. Motzer,Chung-Han Lee,Martin H. Voss
出处
期刊:JCO precision oncology [American Society of Clinical Oncology]
卷期号: (6) 被引量:1
标识
DOI:10.1200/po.22.00012
摘要

The clinical utility of cell-free DNA (cfDNA) as a biomarker for advanced clear cell renal cell carcinoma (ccRCC) remains unclear. We evaluated the validity of cfDNA-based genomic profiling in a large cohort of patients with ccRCC with matched next-generation sequencing (NGS) from primary tumor tissues.We performed paired NGS of tumor DNA and plasma cfDNA using the MSK-IMPACT platform in 110 patients with metastatic ccRCC. Tissues were profiled for variants and copy number alterations with germline comparison. Manual cross-genotyping between cfDNA and tumor tissue was performed. Deep sequencing with a higher sensitivity platform, MSK-ACCESS, was performed on a subset of cfDNA samples. Clinical data and radiographic tumor volumes were assessed to correlate cfDNA yield with treatment response and disease burden.Tumor tissue MSK-IMPACT testing identified 582 genomic alterations (GAs) across the cohort. Using standard thresholds for de novo variant calling in cfDNA, only 24 GAs were found by MSK-IMPACT in cfDNA in 7 of 110 patients (6%). With manual cross-genotyping, 210 GAs were detectable below thresholds in 74 patients (67%). Intrapatient concordance with tumor tissue was limited, including VHL (31.6%), PBRM1 (24.1%), and TP53 (52.9%). cfDNA profiling did not identify 3p loss because of low tumor fractions. Tumor volume was associated with cfDNA allele frequency, and VHL concordance was superior for patients with greater disease burden.cfDNA-based NGS profiling yielded low detection rates in this metastatic ccRCC cohort. Concordance with tumor profiling was low, even for truncal mutations such as VHL, and some findings in peripheral blood may represent clonal hematopoiesis. Routine cfDNA panel testing is not supported, and its application in biomarker efforts must account for these limitations.
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