Multimodal detection of molecular residual disease in high-risk locally advanced squamous cell carcinoma of the head and neck

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作者
Enrique Sanz-Garcia
Jinfeng Zou
Lisa Avery
Anna Spreafico
John Waldron
David Goldstein
Aaron Hansen
B. C. John Cho
John de Almeida
Andrew Hope
Ali Hosni
Ezra Hahn
Bayardo Perez-Ordonez
Zhen Zhao
Christopher Smith
Yangqiao Zheng
Nitthusha Singaravelan
Scott V. Bratman
Lillian L. Siu
机构
[1] University of Toronto,Division of Medical Oncology and Hematology, Princess Margaret Cancer Centre, University Health Network
[2] University of Toronto,Princess Margaret Cancer Research Institute, University Health Network
[3] University of Toronto,Department of Biostatistics, Princess Margaret Cancer Centre, University Health Network
[4] University of Toronto,Department of Radiation Oncology, Princess Margaret Cancer Centre, University Health Network
[5] University of Toronto,Department of Surgical Oncology, Division of ENT, Princess Margaret Cancer Centre, University Health Network
[6] University of Toronto,Department of Pathology, Princess Margaret Cancer Centre, University Health Network
[7] Babraham Research Park,Neogenomics
[8] University of Toronto,Cancer Genomics Program, Princess Margaret Cancer Center, University Health Network
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Up to 30% of patients with locally advanced head and neck squamous cell carcinoma (LA-HNSCC) relapse. Molecular residual disease (MRD) detection using multiple assays after definitive therapy has not been reported. In this study, we included patients with LA-HNSCC (stage III Human Papilloma virus (HPV)-positive, III-IVB HPV-negative) treated with curative intent. Plasma was collected pre-treatment, at 4–6 weeks (FU1) and 8-12 weeks (FU2) post-treatment. Circulating tumor DNA (ctDNA) was analyzed using a tumor-informed (RaDaR®) and a tumor-naïve (CAPP-seq) assay. HPV DNA was measured using HPV-sequencing (HPV-seq) and digital PCR (dPCR). A total of 86 plasma samples from 32 patients were analyzed; all patients with at least 1 follow-up sample. Most patients were stage III HPV-positive (50%) and received chemoradiation (78%). No patients had radiological residual disease at FU2. With a median follow-up of 25 months, there were 7 clinical relapses. ctDNA at baseline was detected in 15/17 (88%) by RaDaR and was not associated with recurrence free survival (RFS). Two patients relapsed within a year after definitive therapy and showed MRD at FU2 using RaDaR; detection of ctDNA during follow-up was associated with shorter RFS (p < 0.001). ctDNA detection by CAPP-seq pre-treatment and during follow-up was not associated with RFS (p = 0.09). HPV DNA using HPV-seq or dPCR during follow-up was associated with shorter RFS (p < 0.001). Sensitivity and specificity for MRD at FU2 using RaDaR was 40% and 100% versus 20 and 90.5% using CAPP-seq. Sensitivity and specificity for MRD during follow-up using HPV-seq was 100% and 91.7% versus 50% and 100% using dPCR. In conclusion, HPV DNA and ctDNA can be detected in LA-HNSCC before definitive therapy. The RaDaR assay but not CAPP-seq may detect MRD in patients who relapse within 1 year. HPV-seq may be more sensitive than dPCR for MRD detection.
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页码:460 / 468
页数:8
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