Evaluating personalized circulating tumor DNA detection for early‐stage lung cancer

Author:

Huang Haihua1,Kai Zhentian2ORCID,Wang Yuchen1,Zhang Xiaomiao1,Wang Jin1,Zhang Wei1,Xue Qian1,Zhang Hang1,Jin Hansong1,Meng Peize1,Zhang Shuilong2,Yang Yueyue2,Yang Honghua2,Liang Wanning2,Zha Guangbing2,Luo Peng2,Xu Yan2,Shi Weiwei2,Ruan Zheng1

Affiliation:

1. Department of Thoracic Surgery Shanghai First People's Hospital Shanghai China

2. Department of research and Development, Zhejiang Shaoxing Topgen Biomedical Technology Co., Ltd. Shanghai China

Abstract

AbstractCirculating tumor DNA (ctDNA) has been widely used as a minimally invasive biomarker in clinical routine. However, a number of factors such as panel design, sample quality, patients' disease stages are known to influence ctDNA detection sensitivity. In this study, we systematically evaluated common factors associated with the variability of ctDNA detection in plasma and investigated ctDNA abundance in bronchoalveolar lavage (BAL). Whole exome profiling was conducted on 61 tumor tissue samples to identify tumor‐specific variants, which were then used to design personalized assay MarRyDa® for ctDNA detection. DNA extracted from BAL fluid and plasma were genotyped using MarRyDa® platform. Our analysis showed that histological subtypes and disease stages had significant differences in ctDNA detection rate. Furthermore, we found that DNA purified from BAL supernatants contains the highest levels of ctDNA compared with BAL precipitates and plasma; therefore, utilizing BAL supernatants for tumor detection might provide additional benefits. Finally, we demonstrated that tumor cellularity played significant roles in the design of personalized ctDNA panel which eventually impacts ctDNA detection sensitivity. We suggest setting a flexible criteria for sample quality control and utilization of BAL might benefit more patients in clinics.

Publisher

Wiley

Subject

Cancer Research,Radiology, Nuclear Medicine and imaging,Oncology

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