Abstract 2223P
Background
RET rearrangements have emerged as a new actionable alteration in papillary thyroid cancers (PTC). These fusions may involve many partner genes, are thought to be mutually exclusive with other oncogenic drivers and their screening is recommended based on fluorescence in situ hybridization (FISH), RT-PCR or next-generation sequencing (NGS). The aim of this study is to evaluate the use of NGS as a standard molecular technique to characterize RET gene fusions.
Methods
Sixty PTC cases without the BRAF p.V600E and/or TERT promoter mutations were selected retrospectively in two institutions. Molecular alterations were evaluated using the Oncomine Focus Assay, and all samples were analyzed by RT-PCR using the Idylla GeneFusion Assay. Fusion positive samples were confirmed with FISH with break-apart probes.
Results
All DNA samples were acceptable for analysis, whereas 4 RNA samples failed quality control NGS parameters. RET fusions were detected in 11 cases (18%): CCDC6::RET (C1:R12) in 8 samples, NCOA4::RET (N6:R12) in 2 samples, and 1 RET expression imbalance positive sample without gene partner characterization. All 11 cases were validated by both FISH and RT-PCR. Besides, 4 more cases presented NGS RET expression imbalance but none of them were confirmed neither by RT-PCR nor by FISH and considered false positive results. There were no false negative NGS cases identified in parallel by RT-PCR. Overall, a positive predictive value of 89% and a negative predictive value of 90% were estimated, reaching a concordance of 89% compared to NGS. Regarding DNA analysis, NRAS p.Q61R/K was the most prevalent alteration in 13 cases (22%) followed by 2 cases with KRAS mutations (p.G12S and p.Q61R). Other potentially actionable fusions found in our series were 2 ETV6::NTRK3 (E4:N14), 2 STRN::ALK (S3:A20) and 1 EML4::ALK (E6:A20).
Conclusions
Molecular screening in non-BRAF PTC patients is useful to identify patients harboring RET fusions who may benefit from targeted therapies. As other potentially actionable gene fusions are also found in these patients, routine implementation of NGS analysis warrants a comprehensive biomarker study.
Clinical trial identification
Editorial acknowledgement
Legal entity responsible for the study
The authors.
Funding
Lilly.
Disclosure
All authors have declared no conflicts of interest.
Resources from the same session
2326P - Circulating tumor DNA (ctDNA) dynamics and clinical outcome in metastatic colorectal cancer (mCRC) patients (pts) undergoing front-line chemotherapy
Presenter: Michele Ghidini
Session: Poster session 16
2327P - The impact of the microenvironment on the intratumoral cellular heterogeneity in colorectal cancer
Presenter: Idan Carmi
Session: Poster session 16
2328P - Alternative molecular mechanisms underpinning breast invasive lobular carcinoma identified by genomics-driven artificial intelligence model
Presenter: Fresia Pareja
Session: Poster session 16
2329P - Evidence for the utility of artificial intelligence and image analysis in Ki-67 quantification in solid tumors
Presenter: Xavier Pichon
Session: Poster session 16
2331P - Interest of next generation sequencing (NGS) for integrated molecular diagnosis of HER2-low breast cancer
Presenter: Jean Louis Merlin
Session: Poster session 16
2332P - Overall survival in breast cancer patients with HER2-low status single- center experience
Presenter: Joanna Huszno
Session: Poster session 16
2333P - Associating BRCA1 hypermethylation with clinicopathological and molecular variables in triple-negative breast cancers
Presenter: Anna Karlsson
Session: Poster session 16
2334P - Pathologic patterns following different neoadjuvant therapies in non-small cell lung cancer (NSCLC)
Presenter: Annikka Weissferdt
Session: Poster session 16
2335P - Spatial whole exome sequencing reveals the genetic features of highly-aggressive components in lung adenocarcinoma
Presenter: Jianfu Li
Session: Poster session 16