Abstract
Most diagnostic laboratories are confronted with the increasing demand for molecular diagnosis from patients and families and the ever-increasing genetic heterogeneity of visual disorders. Concerning Retinal Dystrophies (RD), almost 200 causative genes have been reported to date, and most families carry private mutations. We aimed to approach RD genetic diagnosis using all the available genetic information to prioritize candidates for mutational screening, and then restrict the number of cases to be analyzed by massive sequencing. We constructed and optimized a comprehensive cosegregation RD-chip based on SNP genotyping and haplotype analysis. The RD-chip allows to genotype 768 selected SNPs (closely linked to 100 RD causative genes) in a single cost-, time-effective step. Full diagnosis was attained in 17/36 Spanish pedigrees, yielding 12 new and 12 previously reported mutations in 9 RD genes. The most frequently mutated genes were USH2A and CRB1. Notably, RD3–up to now only associated to Leber Congenital Amaurosis– was identified as causative of Retinitis Pigmentosa. The main assets of the RD-chip are: i) the robustness of the genetic information that underscores the most probable candidates, ii) the invaluable clues in cases of shared haplotypes, which are indicative of a common founder effect, and iii) the detection of extended haplotypes over closely mapping genes, which substantiates cosegregation, although the assumptions in which the genetic analysis is based could exceptionally lead astray. The combination of the genetic approach with whole exome sequencing (WES) greatly increases the diagnosis efficiency, and revealed novel mutations in USH2A and GUCY2D. Overall, the RD-chip diagnosis efficiency ranges from 16% in dominant, to 80% in consanguineous recessive pedigrees, with an average of 47%, well within the upper range of massive sequencing approaches, highlighting the validity of this time- and cost-effective approach whilst high-throughput methodologies become amenable for routine diagnosis in medium sized labs.
Highlights
Retinal dystrophies (RD) are a group of more than 25 genetic visual disorders [1]
Analysis of Usher Syndrome Cases Usher syndrome is characterized by specific phenotypic traits that allow a clear clinical characterization in three main forms, being USH II the most frequent type, and USH2A the major causative gene (75–80% of USH II cases) [27]
Twelve new and 12 previously reported pathological variants have been identified in 9 RD genes, adding to the high genetic diversity in retinal disorders
Summary
Retinal dystrophies (RD) are a group of more than 25 genetic visual disorders [1]. RDs rank among mendelian rare diseases, taken together, they occur at an estimated prevalence of 1–2 patients per 1000 individuals. More than 5000 mutations in almost 200 genes are causative of retinal dystrophies so far [1,5,6]. The extreme heterogeneity of RDs at the clinical and genetic levels hinders the accurate clinical assessment, patient management, and genetic counseling. Within this context, molecular diagnosis, challenging, is instrumental to improve the diagnosis and prognosis of RDs and guide future therapies [7,8,9]
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