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Novel ADGRG2 truncating variants in patients with X‐linked congenital absence of vas deferens
Author(s) -
Pagin Adrien,
Bergougnoux Anne,
Girodon Emmanuelle,
Reboul MariePierre,
Willoquaux Christelle,
Kesteloot Maryse,
Raynal Caroline,
Bienvenu Thierry,
Humbert Mathilde,
Lalau Guy,
Bieth Eric
Publication year - 2020
Publication title -
andrology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.947
H-Index - 43
eISSN - 2047-2927
pISSN - 2047-2919
DOI - 10.1111/andr.12744
Subject(s) - vas deferens , cystic fibrosis , exon , mutation , medicine , exome sequencing , allele , ivacaftor , obstructive azoospermia , population , genetics , biology , gene , pathology , azoospermia , cystic fibrosis transmembrane conductance regulator , infertility , pregnancy , environmental health
Background Congenital absence of vas deferens (CAVD) represents a major cause of obstructive azoospermia and is mainly related to biallelic alteration of the CFTR gene, also involved in cystic fibrosis. Using whole exome sequencing, we recently identified hemizygous loss‐of‐function mutations in the Adhesion G Protein‐coupled Receptor G2 gene ( ADGRG2 ) as responsible of isolated CAVD in the absence of associated unilateral renal agenesis. Objectives The objective of this study was to retrospectively perform ADGRG2 sequencing on a large cohort of patients with CAVD, and 0 or only 1 CFTR defective allele identified after comprehensive testing in order to (a) define more precisely the spectrum and the frequency of ADGRG2 mutations within Caucasian population (b) explore the possibility of co‐occurrence of CFTR and ADGRG2 mutations. Materials and methods We collected 53 DNA samples from CAVD patients with 0 (n = 23) or 1 (n = 30) alteration identified after comprehensive CFTR testing in order to perform ADGRG2 sequencing. Twenty patients had normal ultrasonographic renal examination, and renal status was not documented for 33 patients. Results We identified six new truncating ADGRG2 mutations in 8 patients including two twin brothers: c.251C > G (p.Ser84*), c.1013delC (p.Pro338Hisfs*4), c.1460delG (p.Gly487Alafs*9), c.2096dupT (p.Phe700Ilefs*29), c.2473C > T (p.Arg825*), and c.1731_1839 + 373del (p.Asn578Thrfs*12), which is a 596 base pair deletion affecting the last five bases of exon 21 and the whole exon 22. Five of the eight patients also harbored an heterozygous CFTR mutation which we consider as incidental regarding the high penetrance expected for ADGRG2 truncating variants. The frequency of ADGRG2 truncating mutation was 26% (5/19 unrelated patients) when presence of both kidneys was attested by ultrasonography and 6.1% (2/33) among patients with unknown renal status. Discussion & Conclusion Our results confirm the interest of ADGRG2 sequencing in patients with CAVD not formerly related to CFTR dysfunction, especially in the absence of associated unilateral renal agenesis.