Evaluation of a Four-Gene Panel for Hereditary Cancer Risk Assessment

Angela Secondino; Flavio Starnone; Iolanda Veneruso; Maria Antonietta Di Tella; Serena Conato; Carmine De Angelis; Sabino De Placido; Valeria D'Argenio

doi:10.3390/genes13040682

Evaluation of a Four-Gene Panel for Hereditary Cancer Risk Assessment

Genes (Basel). 2022 Apr 13;13(4):682. doi: 10.3390/genes13040682.

Authors

Angela Secondino^{1

2}, Flavio Starnone², Iolanda Veneruso^{1

2}, Maria Antonietta Di Tella², Serena Conato², Carmine De Angelis³, Sabino De Placido³, Valeria D'Argenio^{2

4}

Affiliations

¹ Department of Molecular Medicine and Medical Biotechnologies, Federico II University, Via Sergio Pansini 5, 80131 Napoli, Italy.
² CEINGE-Biotecnologie Avanzate, Via G. Salvatore 486, 80145 Napoli, Italy.
³ Department of Clinical Medicine and Surgery, Federico II University, Via Sergio Pansini 5, 80131 Napoli, Italy.
⁴ Department of Human Sciences and Quality of Life Promotion, San Raffaele Open University, Via di Val Cannuta 247, 00166 Roma, Italy.

Abstract

BRCA1/2 are tumor suppressor genes involved in DNA double-strand break repair. They are the most penetrant genes for hereditary breast and ovarian cancers, but pathogenic variants in these two genes can be identified only in a fraction of hereditary cases. Following the diffusion of BRCA molecular testing and the availability of specific therapeutic strategies for the management of pathogenic variant carriers, the demand for the analysis of additional predisposing genetic factors has increased. Indeed, there is accumulating evidence regarding the role of other genes, including CHEK2 and PALB2. Both of them are involved in the same molecular pathway as BRCA genes, with CHEK2 being responsible for cell cycle stopping to allow the repair of DNA double-strand breaks and PALB2 being able to interact with BRCA1 and activate BRCA2. Thus, their role as additional hereditary cancer predisposing factors is intriguing. Accordingly, guidelines for hereditary cancer risk assessment have been updated to include the criteria for additional genes testing. In this context, we validated a commercially available kit allowing for the simultaneous analysis of BRCA1, BRCA2, CHEK2 and PALB2. Forty-eight patients, already tested for BRCA mutational status, were re-analyzed in the present study. Results comparison showed that the tested method was able to correctly identify all the variants previously detected in the same patients. In particular, all single-nucleotide variants and small indels were correctly identified. Moreover, two copy number variants, included to assess the software's performance in detecting this kind of gene alteration, were also detected. Even if copy number variant estimation still requires confirmation by a molecular technique to avoid false positive results, it is able to reduce the number of patients requiring multiplex ligation probe amplification analysis, positively impacting the test's turnaround time. Finally, since the time and costs of the analysis are similar to those required just for BRCA genes, this strategy may be affordable for providing a more comprehensive test for hereditary cancer risk assessment.

Keywords: BRCA1; BRCA2; CHEK2; PALB2; breast cancer; hereditary cancers; multigene panel testing; next generation sequencing; ovarian cancer.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Female
Genes, BRCA2
Genetic Predisposition to Disease*
Humans
Mutation
Ovarian Neoplasms* / genetics
Risk Assessment