Inflammatory priming predisposes mice to age-related retinal degeneration
Debarshi Mustafi, … , Joseph H. Nadeau, Krzysztof Palczewski
Debarshi Mustafi, … , Joseph H. Nadeau, Krzysztof Palczewski
Published August 1, 2012; First published July 17, 2012
Citation Information: J Clin Invest. 2012;122(8):2989-3001. https://doi.org/10.1172/JCI64427.
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Categories: Research Article Ophthalmology

Inflammatory priming predisposes mice to age-related retinal degeneration

Abstract

Disruption of cellular processes affected by multiple genes and accumulation of numerous insults throughout life dictate the progression of age-related disorders, but their complex etiology is poorly understood. Postmitotic neurons, such as photoreceptor cells in the retina and epithelial cells in the adjacent retinal pigmented epithelium, are especially susceptible to cellular senescence, which contributes to age-related retinal degeneration (ARD). The multigenic and complex etiology of ARD in humans is reflected by the relative paucity of effective compounds for its early prevention and treatment. To understand the genetic differences that drive ARD pathogenesis, we studied A/J mice, which develop ARD more pronounced than that in other inbred mouse models. Although our investigation of consomic strains failed to identify a chromosome associated with the observed retinal deterioration, pathway analysis of RNA-Seq data from young mice prior to retinal pathological changes revealed that increased vulnerability to ARD in A/J mice was due to initially high levels of inflammatory factors and low levels of homeostatic neuroprotective factors. The genetic signatures of an uncompensated preinflammatory state and ARD progression identified here aid in understanding the susceptible genetic loci that underlie pathogenic mechanisms of age-associated disorders, including several human blinding diseases.

Authors

Debarshi Mustafi, Tadao Maeda, Hideo Kohno, Joseph H. Nadeau, Krzysztof Palczewski

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Figure 1

A/J mice display a pronounced age-dependent decline in vision.

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A/J mice display a pronounced age-dependent decline in vision. (A) Light...
(A) Light microscopy of A/J mouse retinas revealed a marked decrease in ONL and inner nuclear layer (INL) thickness in 8- versus 1-month-old animals, as well as pathological changes in the RPE layer at 8 months of age, as shown by the higher-magnification view of the boxed region (arrow, pyknotic cell). These changes were minimal in B6 mice. (B) ONL thickness, plotted as a function of distance from the optic nerve head (ONH), showed the most pronounced decline occurred between 3 and 8 months of age, a finding that was absent in B6 mice. (C) Cone cell sheaths were imaged by PNA staining at 1, 3, and 8 months of age. Average numbers of cone cells in both the superior and inferior retina in a 100-μm range located 500 μm from the optic nerve head were plotted (red, A/J; black, B6). A/J mice showed a marked decline between 3 and 8 months of age. (D) Representative ERG responses at 1.6 log cd•s•m–2, and functional a-wave and b-wave amplitudes, obtained from A/J (red) and B6 (black) mice at 1, 3, and 8 months of age. ERG responses were more attenuated with age in A/J versus B6 mice under both scotopic and photopic conditions (P < 0.001). Scale bars: 20 μm (A and C).