Prosaposin gene expression in normal and dystrophic RCS rat retina

To identify proteins secreted by the retinal pigment epithelium (RPE) and to analyze their cellular distribution in normal and pathologic rat retinas at various stages of eye development. A cDNA library was constructed with RNA isolated from porcine RPE sheets and screened by using the yeast signal...

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Published inInvestigative ophthalmology & visual science Vol. 45; no. 5; pp. 1297 - 1305
Main Authors VAN DEN BERGHE, Loïc, SAINTON, Karine, GOGAT, Karïn, MARCBANT, Dominique, DUFOUR, Eric, BONNEL, Sébastien, GADIN, Stéphanie, MENASCHE, Maurice, ABITBOL, Marc
Format Journal Article
LanguageEnglish
Published Rockville, MD Association for Research in Vision and Ophtalmology 01.05.2004
Subjects
Amino Acid Sequence
Animals
Base Sequence
Biological and medical sciences
Gene Expression
Gene Library
Glycoproteins - genetics
Immunohistochemistry
In Situ Hybridization
Medical sciences
Molecular Sequence Data
Ophthalmology
Rats
Rats, Mutant Strains
Retina - metabolism
Retinal Degeneration - metabolism
Retinal Degeneration - pathology
Retinopathies
Reverse Transcriptase Polymerase Chain Reaction
RNA, Messenger - metabolism
Saposins
Swine
Vertebrata
Mammalia
Rat
Animal
Rodentia
Retina
Dystrophy
Ophthalmology
Gene expression
Normal
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Summary:To identify proteins secreted by the retinal pigment epithelium (RPE) and to analyze their cellular distribution in normal and pathologic rat retinas at various stages of eye development. A cDNA library was constructed with RNA isolated from porcine RPE sheets and screened by using the yeast signal sequence trap system. In situ hybridization, immunohistochemistry, and semiquantitative RT-PCR analysis were performed on rat retinas. The cDNA encoding prosaposin was isolated. This is the first time this gene has been shown to be expressed in the retina. Prosaposin mRNA was detected in the rat RPE cell monolayer and in ganglion cells 14, 21, and 45 days after birth. The amount of prosaposin mRNA increased between days 14 and 45 after birth in normal retinas (rdy+), but not in the pathologic retinas (rdy-) of RCS rats. Several techniques were used to determine the localization of prosaposin in rat retinas. The increase in the amount of prosaposin mRNA in normal retinas coincided with the maturation of photoreceptor cells and the beginning of the phagocytosis process. In addition, the RCS rdy- RPE cells, characterized by the abrogation of the ingestion phase of the photoreceptor outer segments, are deficient in prosaposin expression.
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ISSN:0146-0404
1552-5783
DOI:10.1167/iovs.03-1048