Abstract 13P
Background
Ovarian cancer (OC) stands as the ninth leading cause of cancer-related deaths in women and represents the most prevalent gynaecological malignancy. Patients with OC are more likely to benefit from iPARP if their tumours present deleterious mutations of BRCA1/2 genes, and if they have a homologous recombination deficiency (HRD). Somatic or germline deleterious mutations of BRCA1/2 occurs in 15 to 20 % of HRD OC. However, not all HRD cases are due to these mutations. Indeed, studies have shown that BRCA1 and RAD51C promoter methylation are responsible for 19% and 2% of HRD cases, respectively.
Methods
Two hundred and twenty-four patients with ovarian cancer were included in the ICL cohort, and 20 in the BOVARY cohort. All of them give their informed consent. DNA was extracted from FFPE tissue and cfDNA from plasma. Low-pass whole-genome sequencing was used to determine HRD status. Methylation of BRCA1 and RAD51C promoters was analysed using droplet digital PCR (ddPCR) after enzymatic conversion. A threshold of 10% was set for defining a sample as methylated.
Results
HRD status was determined for 193 of the 224 patients. A total of 77 patients were identified as HRD. Among the patients with HRD, 25 were found to have a deleterious BRCA1 or 2 mutation. Additionally, 3 patients exhibited a deleterious mutation in the RAD51C gene. After analysis of BRCA1 and RAD51C methylation in all the samples, 32 patients were identified with BRCA1 promoter methylation, while 1 patient had a RAD51C promoter methylation. All patients with promoter methylation were HRD. In the BOVARY cohort, BRCA1 promoter methylation was detected in only one HRD sample, with concordant methylation found in the paired cfDNA sample. No methylation of the RAD51C gene was found.
Conclusions
We demonstrate the feasibility of ddPCR for determining the methylation of BRCA1 and RAD51C promoters to identify patients with HRD. Furthermore, although the number of cfDNA samples analysed remains modest, our findings suggest that liquid biopsy could also be used to determine BRCA1 and RAD51C methylation statuses.
Editorial acknowledgement
Clinical trial identification
NCT03881683.
Legal entity responsible for the study
Institut de Cancérologie de Lorraine.
Funding
Tesaro.
Disclosure
All authors have declared no conflicts of interest.
Resources from the same session
72P - SNCG promotes the malignant progression of hepatocellular carcinoma by activation EGFR signaling and recycling
Presenter: Yue Chen
Session: Cocktail & Poster Display session
Resources:
Abstract
73P - TROP2 amplification is highly present in dedifferentiated liposarcoma: Data from the Cancer Genome Atlas (TCGA) in soft tissue sarcoma
Presenter: Sarah Orlando
Session: Cocktail & Poster Display session
Resources:
Abstract
74P - The influence of genetic phenotype on prognosis of osteosarcoma
Presenter: Nasirov Kamalovich
Session: Cocktail & Poster Display session
Resources:
Abstract
76P - Immune engager compounds screening using CRC patient-derived organoids
Presenter: Claudia Maria A. Pinna
Session: Cocktail & Poster Display session
Resources:
Abstract
77P - Elucidating molecularly stratified single agent, and combination, therapeutic strategies targeting MCL1 for lethal prostate cancer
Presenter: Juan Jiménez-Vacas
Session: Cocktail & Poster Display session
Resources:
Abstract
78P - Exploring ecDNA heterogeneity and evolution in non-small cell lung cancer
Presenter: Jeanette Kittel
Session: Cocktail & Poster Display session
Resources:
Abstract
79P - Targeting galectin-9 in BRCA mutant breast cancer
Presenter: Chun Yan So
Session: Cocktail & Poster Display session
Resources:
Abstract
80P - Suppression of glioblastoma progression by FDA-approved central nervous system-accumulating drugs via autophagy modulation and ER stress-induced apoptosis
Presenter: Smita Dey
Session: Cocktail & Poster Display session
Resources:
Abstract
81P - Evaluating the effect of lenvatinib-resistance in hepatocellular carcinoma cells and in lenvatinib-resistant patient-derived PBMCs
Presenter: Luisa Amato
Session: Cocktail & Poster Display session
Resources:
Abstract
82P - Applying computational approaches to build a predictive protein structure and discover novel inhibitors for mitotic serine/threonine kinase BUB1B
Presenter: Joan Glenny Pescov
Session: Cocktail & Poster Display session
Resources:
Abstract