USH2A mutational spectrum causing syndromic and non-syndromic retinal dystrophies in a large cohort of Mexican patients

Vianey Ordoñez-Labastida; Oscar F Chacon-Camacho; Victor R Lopez-Rodriguez; Juan C Zenteno

USH2A mutational spectrum causing syndromic and non-syndromic retinal dystrophies in a large cohort of Mexican patients

Mol Vis. 2023 Apr 29:29:31-38. eCollection 2023.

Authors

Vianey Ordoñez-Labastida^{1

2

3}, Oscar F Chacon-Camacho^{2

4}, Victor R Lopez-Rodriguez², Juan C Zenteno^{1

2

5}

Affiliations

¹ Rare Disease Diagnostic Unit, Faculty of Medicine, National Autonomous University of Mexico (UNAM), Mexico City, Mexico.
² Department of Genetics, Institute of Ophthalmology "Conde de Valenciana," Mexico City, Mexico.
³ Faculty of Medicine, Autonomous University of the State of Morelos (UAEM), Morelos, Mexico.
⁴ Carrera Médico Cirujano, Facultad de Estudios Superiores Iztacala, UNAM, Mexico City, Mexico.
⁵ Department of Biochemistry, Faculty of Medicine, UNAM, Mexico City, Mexico.

PMID: 37287646
PMCID: PMC10243674

Abstract

Background: Mutations in the USH2A gene are the leading cause of both non-syndromic autosomal recessive retinitis pigmentosa (RP) and Usher syndrome, a syndromic form of RP characterized by retinal dystrophy and sensorineural hearing loss. To contribute to the expansion of the USH2A-related molecular spectrum, the results of genetic screening in a large cohort of Mexican patients are presented.

Methods: The study population comprised 61 patients with a clinical diagnosis of either non-syndromic RP (n = 30) or Usher syndrome type 2 (USH2; n = 31) who were demonstrated to carry biallelic pathogenic variants in USH2A in a three-year period. Genetic screening was performed either by gene panel sequencing or by exome sequencing. A total of 72 available first- or second-degree relatives were also genotyped for familial segregation of the identified variants.

Results: The USH2A mutational spectrum in RP patients included 39 distinct pathogenic variants, most of them of the missense type. The most common RP-causing variants were p.Cys759Phe (c.2276G>T), p.Glu767Serfs*21 (c.2299delG), and p.Cys319Tyr (c.956G>A), which together accounted for 25% of all RP variants. Novel USH2A mutations included three nonsense, two missense, two frameshift, and one intragenic deletion. The USH2A mutational spectrum in USH2 patients included 26 distinct pathogenic variants, most of them of the nonsense and frameshift types. The most common Usher syndrome-causing variants were p.Glu767Serfs*21 (c.2299delG), p.Arg334Trp (c.1000C>T), and c.12067-2A>G), which together accounted for 42% of all USH2-related variants. Novel Usher syndrome USH2A mutations included six nonsense, four frameshift, and two missense mutations. The c.2299delG mutation was associated with a common haplotype for SNPs located in exons 2-21 of USH2A, indicating a founder mutation effect.

Conclusions: Our work expands the USH2A mutational profile by identifying 20 novel pathogenic variants causing syndromic and non-syndromic retinal dystrophy. The prevalent c.2299delG allele is shown to arise from a founder effect. Our results emphasize the usefulness of molecular screening in underrepresented populations for a better characterization of the molecular spectrum of common monogenic diseases.

MeSH terms

DNA Mutational Analysis
Extracellular Matrix Proteins / genetics
Humans
Mutation
Retinitis Pigmentosa* / genetics
Usher Syndromes* / diagnosis
Usher Syndromes* / genetics

Substances

Extracellular Matrix Proteins
USH2A protein, human

Supplementary concepts

Usher syndrome, type 2A