Identification of a novel splice-site mutation in the Lebercilin (LCA5) gene causing Leber congenital amaurosis

Vedam Lakshmi Ramprasad; Nagasamy Soumittra; Derek Nancarrow; Parveen Sen; Martin McKibbin; Grange A Williams; Tharigopala Arokiasamy; Praveena Lakshmipathy; Chris F Inglehearn; Govindasamy Kumaramanickavel

Identification of a novel splice-site mutation in the Lebercilin (LCA5) gene causing Leber congenital amaurosis

Mol Vis. 2008 Mar 10:14:481-6.

Authors

Vedam Lakshmi Ramprasad¹, Nagasamy Soumittra, Derek Nancarrow, Parveen Sen, Martin McKibbin, Grange A Williams, Tharigopala Arokiasamy, Praveena Lakshmipathy, Chris F Inglehearn, Govindasamy Kumaramanickavel

Affiliation

¹ Department of Genetics and Molecular Biology, Vision Research Foundation, Sankara Nethralaya Chennai, India.

PMID: 18334959
PMCID: PMC2268850

Abstract

Purpose: Leber congenital amaurosis (LCA) is one of the most common causes of hereditary blindness in infants. To date, mutations in 13 known genes and at two other loci have been implicated in LCA causation. An examination of the known genes highlights several processes which, when defective, cause LCA, including photoreceptor development and maintenance, phototransduction, vitamin A metabolism, and protein trafficking. In addition, it has been known for some time that defects in sensory cilia can cause syndromes involving hereditary blindness. More recently evidence has come to light that non-syndromic LCA can also be a "ciliopathy."

Methods: Here we present a homozygosity mapping analysis in a consanguineous sibship that led to the identification of a mutation in the recently discovered LCA5 gene. Homozygosity mapping was done using Affymetrix 10K Xba I Gene Chip and a 24.5cM region on chromosome 6 (6q12- q16.3) was identified to be significantly homozygous. The LCA5 gene on this region was sequenced and cDNA sequencing also done to characterize the mutation.

Results: A c.955G>A missense mutation in the last base of exon 6 causing disruption of the splice donor site was identified in both the affected sibs. Since there is a second consensus splice donor sequence 5 bp into the adjacent intron, this mutation results in a transcript with a 5 bp insertion of intronic sequence, leading to a frameshift and premature truncation.

Conclusions: We report a missense mutation functionally altering the splice donor site and leading to a truncated protein. This is the second report of LCA5 mutations causing LCA. It may also be significant that one affected child died at eleven months of age due to asphyxia during sleep. To date the only phenotype unambiguously associated with mutations in this gene is LCA. However the LCA5 gene is known to be expressed in nasopharynx, trachea and lungs and was originally identified in the proteome of bronchial epithelium ciliary axonemes. The cause of death in this child may therefore imply that LCA5 mutations can in fact cause a wider spectrum of phenotypes including respiratory disease.

Publication types

Case Reports

MeSH terms

Adult
Aged
Base Sequence
Blindness / genetics*
Child
Child, Preschool
DNA Mutational Analysis
Electroretinography
Exons / genetics
Eye Proteins / genetics*
Female
Fundus Oculi
Humans
Infant
Male
Microtubule-Associated Proteins / genetics*
Middle Aged
Molecular Sequence Data
Mutation / genetics*
Optic Atrophy, Hereditary, Leber / genetics*
RNA Splice Sites / genetics*

Substances

Eye Proteins
LCA5 protein, human
Microtubule-Associated Proteins
RNA Splice Sites