RNA assay identifies a previous misclassification of BARD1 c.1977A>G variant

Paula Rofes,Marta Pineda,Carolina Gómez,Rafael De Cid,Gabriel Capellá,Jesús Del Valle,Joan Brunet,Mireia Menéndez,Lídia Feliubadaló,Eva Montes,Conxi Lázaro

doi:10.1038/s41598-021-02465-y

Abstract

Case–control studies have shown an association of BARD1 with hereditary breast and/or ovarian cancer (HBOC) predisposition. BARD1 alternatively spliced isoforms are abundant and some are highly expressed in different cancer types. In addition, a number of BARD1 germline pathogenic variants have been reported among HBOC patients. In previous reports, BARD1 c.1977A>G variant has been classified as pathogenic since it produces a frameshift transcript lacking exons 2 to 9. In the present study, we sought to validate the mRNA splicing results previously published and to contribute with new evidence to refine the classification of this substitution according to ACMG/AMP guidelines. The presence of the variant was screened in patients and controls. RT-PCR was performed in order to compare the transcriptional profiles of two variant carriers and ten non-carrier controls. In addition, allele-specific expression was assessed. No differences in variant frequency were detected between patients and controls. The RNA assay confirmed the presence of the shorter transcript lacking exons 2–9, but it was detected both in carriers and non-carriers. Furthermore, allelic imbalance was discarded and no significant differences in the proportion of full-length and shorter transcript were detected between carriers and controls. The shorter transcript detected corresponds to BARD1 isoform η, constituted by exons 1, 10 and 11. Our results support that this transcript is a constitutive splicing product rather than an aberrant transcript caused by BARD1 c.1977A>G variant, and for this reason this variant should be considered as likely benign following ACMG/AMP guidelines.

Highlights

Case–control studies have shown an association of BRCA1-associated RING domain 1 (BARD1) with hereditary breast and/or ovarian cancer (HBOC) predisposition
Multi-gene panel testing was performed in a total of 4168 hereditary cancer (HC) patients, and BARD1 carrier status was retrieved from all individuals in a research context for this study
BARD1 was postulated as a hereditary breast and ovarian cancer (HBOC) predisposing gene shortly after it was first described, due to its relationship with BRCA1 in terms of shared structural homology and functional association for the development of their tumor-suppressor r oles[1]

Summary

Introduction

Case–control studies have shown an association of BARD1 with hereditary breast and/or ovarian cancer (HBOC) predisposition. The RNA assay confirmed the presence of the shorter transcript lacking exons 2–9, but it was detected both in carriers and non-carriers. The shorter transcript detected corresponds to BARD1 isoform η, constituted by exons 1, 10 and 11. Fulllength (FL) BARD1 transcript comprises 11 exons and encodes a 777 amino acid protein that consists of one N-terminal RING-finger domain, four ankyrin (Ank) repeats and two C-terminal tandem BRCT domains[2,3] It is through their RING domains that BARD1 and BRCA1 directly interact, mediating double-strand break (DSB) repair as a heterodimer[1,4]. The synonymous BARD1 c.1977A>G has been previously reported as a pathogenic variant that affects splicing[14], generating an aberrant transcript characterized by the skipping of exons 2 to 9, coinciding with isoform η. P: sample treated with puromycin prior to RNA extraction; NP: sample not treated with puromycin; cDNA-FL: cDNA analysis on the full-length excised band

Objectives

Methods

Results

Conclusion