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Different rate of retinal degenerations in mice with two distinct mutations in the Mitf gene
Author(s) -
Eysteinsson Thor,
Jónasdóttir Ingunn,
GarcíaLlorca Andrea,
Björg Gudmundsdóttir Thorunn,
Ögmundsdóttir Margrét Helga,
Steingrímsson Eiríkur
Publication year - 2019
Publication title -
acta ophthalmologica
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.534
H-Index - 87
eISSN - 1755-3768
pISSN - 1755-375X
DOI - 10.1111/j.1755-3768.2019.5309
Subject(s) - microphthalmia associated transcription factor , hypopigmentation , retinal , retinal degeneration , microphthalmia , erg , biology , retinal pigment epithelium , endocrinology , ophthalmology , genetics , medicine , gene , transcription factor
Purpose The microphthalmia‐associated transcription factor (Mitf) gene is crucial for development of the retinal pigment epithelium (RPE) and photoreceptors. Loss of function mutations in this gene can cause ocular hypopigmentation, microphthalmia and blindness. Mice heterozygous for the Mitf mi‐wh/+ mutation have been used as a model for Waardenburg and Tietz syndromes in humans. The compound heterozygote Mitf mi‐wh/ Mitf mi has two different mutant alleles in the Mitf gene each of which have quite severe effects on the phenotype. The purpose of this study was to examine changes over time in retinal function and structure in these mice, between 1 and 5 months of age, to elucidate the rate of progression of the retinal degenerations. Methods B6‐Mitf mi‐wh/+ and B6‐Mitf mi‐wh/ Mitf mi mice were examined and compared to C5BL/6J mice as control. Mice were anesthetized by an intraperitoneal injection of 40 mg/kg ‐1 Ketamine and 4 mg/kg ‐1 Xylazine. Fundus and optical coherence tomography (OCT) images were obtained with a Micron IV. Flash electroretinography (ERG) from mice with a corneal electrode was used to determine retinal function. Results Fundus images from all mutant mice show hypopigmentation at 1 month, with large non‐pigmented areas forming at later stages. Mitf mi‐wh/+ mice are either blind or not at 1 month, with the ERG normal in amplitude in some animals and absent in others. The Mitf mi‐wh/+ mice with ERG responses at 1 month show slow retinal degeneration, with reduced responses at 5 months. Mitf mi‐wh/ Mitf mi mice show either abnormal ERG responses at 1 month, or a flat ERG. The ERG responses in some of the Mitf mi‐wh/ Mitf mi mice decrease with time, and at 4 months is flat. OCT images reveal that retinal layers in animals with flat ERG are thinner than in mice showing reduced ERG, but abnormally thin in both. Conclusions We conclude that Mitf mi‐wh/ Mitf mi mutant mice show evidence of fast retinal degeneration. The Mitf mi‐wh/+ mutant mice are either blind at 1 month or show evidence of slow degeneration. Mice with these Mitf mutations may serve as models of retinal degenerations progressing at different rates, due to mutations in a gene expressed in the RPE.