An intronic deletion in the PROM1 gene leads to autosomal recessive cone-rod dystrophy

Osnat Eidinger; Rina Leibu; Hadas Newman; Leah Rizel; Ido Perlman; Tamar Ben-Yosef

An intronic deletion in the PROM1 gene leads to autosomal recessive cone-rod dystrophy

Mol Vis. 2015 Dec 8:21:1295-306. eCollection 2015.

Authors

Osnat Eidinger¹, Rina Leibu², Hadas Newman³, Leah Rizel¹, Ido Perlman⁴, Tamar Ben-Yosef¹

Affiliations

¹ Ruth and Bruce Rappaport Faculty of Medicine, Technion-Israel Institute of Technology, Haifa, Israel.
² Alberto Moscona Department of Ophthalmology, Rambam Health Care Center, Haifa, Israel.
³ Department of Ophthalmology, Tel-Aviv Souraski Medical Center, Tel-Aviv, Israel ; Sackler Faculty of Medicine, Tel Aviv University, Tel Aviv, Israel.
⁴ Ruth and Bruce Rappaport Faculty of Medicine, Technion-Israel Institute of Technology, Haifa, Israel ; Department of Ophthalmology, Tel-Aviv Souraski Medical Center, Tel-Aviv, Israel.

PMID: 26702251
PMCID: PMC4676936

Abstract

Purpose: To investigate the genetic basis for autosomal recessive cone-rod dystrophy (CRD) in a consanguineous Israeli Jewish family.

Methods: Patients underwent a detailed ophthalmic evaluation, including eye examination, visual field testing, optical coherence tomography (OCT), and electrophysiological tests, electroretinography (ERG) and visual evoked potential (VEP). Genome-wide homozygosity mapping using a single nucleotide polymorphism (SNP) array was performed to identify homozygous regions shared among two of the affected individuals. Mutation screening of the underlying gene was performed with direct sequencing. In silico and in vitro analyses were used to predict the effect of the identified mutation on splicing.

Results: The affected family members are three siblings who have various degrees of progressive visual deterioration, glare, color vision abnormalities, and night vision difficulties. Visual field tests revealed central scotomas of different extension. Cone and rod ERG responses were reduced, with cones more severely affected. Homozygosity mapping revealed several homozygous intervals shared among two of the affected individuals. One included the PROM1 gene. Sequence analysis of the 26 coding exons of PROM1 in one affected individual revealed no mutations in the coding sequence or in intronic splice sites. However, in intron 21, proximate to the intron-exon junction, we observed a homozygous 10 bp deletion between positions -26 and -17 (c.2281-26_-17del). The deletion was linked to a known SNP, c.2281-6C>G. The deletion cosegregated with the disease in the family, and was not detected in public databases or in 101 ethnically-matched control individuals. In silico analysis predicted that this deletion would lead to altered intron 21 splicing. Bioinformatic analysis predicted that a recognition site for the SRSF2 splicing factor is located within the deleted sequence. The in vitro splicing assay demonstrated that c.2281-26_-17del leads to complete exon 22 skipping.

Conclusions: A novel and unique intronic mutation of PROM1, underlying autosomal recessive CRD in a consanguineous Israeli family, was found. This report expands the spectrum of pathogenic mutations of PROM1 and further demonstrates the importance of intronic mutations.

Publication types

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

MeSH terms

AC133 Antigen
Adolescent
Amino Acid Sequence
Antigens, CD / chemistry
Antigens, CD / genetics*
Base Sequence
Child
Consanguinity
DNA / genetics
Electroretinography
Evoked Potentials, Visual
Female
Genes, Recessive
Glycoproteins / chemistry
Glycoproteins / genetics*
Homozygote
Humans
Introns
Israel
Jews / genetics
Male
Models, Molecular
Molecular Sequence Data
Pedigree
Peptides / chemistry
Peptides / genetics*
Retinitis Pigmentosa / genetics*
Retinitis Pigmentosa / pathology
Retinitis Pigmentosa / physiopathology
Sequence Deletion*
Sequence Homology, Amino Acid
Twins, Dizygotic

Substances

AC133 Antigen
Antigens, CD
Glycoproteins
PROM1 protein, human
Peptides
DNA