The genetic modifier Rpe65Leu(450): effect on light damage susceptibility in c-Fos-deficient mice

The genetic modifier Rpe65Leu(450): effect on light damage susceptibility in c-Fos-deficient mice

To test whether introduction of the Rpe65Leu(450) variant can overcome protection against light-induced photoreceptor apoptosis in mice without the activator protein (AP)-1 constituent c-Fos. c-Fos-deficient mice (c-fos(-/-)) carrying the Leu(450) variant of RPE65 were compared with c-fos(-/-) mice...

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Veröffentlicht in:Investigative ophthalmology & visual science 2003-06, Vol.44 (6), p.2798
Hauptverfasser: Wenzel, Andreas, Grimm, Christian, Samardzija, Marijana, Remé, Charlotte E
Format: Artikel
Sprache:eng
Schlagworte:
Animals
Blotting, Western
Carrier Proteins
cis-trans-Isomerases
Dexamethasone - pharmacology
Disease Susceptibility
DNA-Binding Proteins - metabolism
Electrophoretic Mobility Shift Assay
Eye Proteins
Fos-Related Antigen-2
Glucocorticoids - pharmacology
Leucine
Light
Mice
Mice, Inbred C57BL
Mice, Knockout
Proteins - genetics
Proteins - metabolism
Proto-Oncogene Proteins c-fos - deficiency
Radiation Injuries, Experimental - etiology
Radiation Injuries, Experimental - metabolism
Radiation Injuries, Experimental - pathology
Retina - metabolism
Retina - radiation effects
Retinal Degeneration - etiology
Retinal Degeneration - metabolism
Retinal Degeneration - pathology
Rhodopsin - physiology
Transcription Factor AP-1 - antagonists & inhibitors
Transcription Factor AP-1 - genetics
Transcription Factor AP-1 - metabolism
Transcription Factors - metabolism
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Zusammenfassung:To test whether introduction of the Rpe65Leu(450) variant can overcome protection against light-induced photoreceptor apoptosis in mice without the activator protein (AP)-1 constituent c-Fos. c-Fos-deficient mice (c-fos(-/-)) carrying the Leu(450) variant of RPE65 were compared with c-fos(-/-) mice with Rpe65Met(450). Expression of RPE65 was analyzed by Western blot analysis. Rhodopsin regeneration was determined by measuring rhodopsin after different times in darkness after bleaching. Susceptibility to light-induced damage was tested by exposure to white light and subsequent morphologic analysis. Activation of AP-1 and its complex composition was analyzed by electromobility shift assay (EMSA) and antibody interference. The contribution of AP-1 to apoptosis was tested by pharmacological inhibition of AP-1, using dexamethasone. Compared with RPE65Met(450), introduction of the RPE65Leu(450) variant led to increased levels of RPE65 protein, accelerated rhodopsin regeneration, loss of protection against light-induced damage, and AP-1 responsiveness to toxic light doses, despite the absence of c-Fos. c-Fos was mainly replaced by Fra-2. Application of dexamethasone restored resistance to light-induced damage. Increasing retinal photon catch capacity by introducing the Rpe65Leu(450) variant overcomes light damage resistance provided by c-fos deficiency. Thus, a variation of RPE65 at position 450 is a strong genetic modifier of susceptibility to light-induced damage in mice. Under conditions of high rhodopsin availability during exposure to light, Fra-2 and, to a minor degree, FosB substitute for c-Fos and enable light-induced AP-1 activity and thus photoreceptor apoptosis. Regardless of the AP-1 complex's composition, glucocorticoid receptor activation inhibits AP-1 and prevents apoptosis. Thus, not the absence of c-Fos per se, but rather impairment of AP-1 DNA binding is protective against light-induced damage. This impairment may result from the absence of c-Fos or glucocorticoid receptor-mediated transrepression.
ISSN:0146-0404
DOI:10.1167/iovs.02-1134