Inhibition of ceramide accumulation in AdipoR1–/– mice increases photoreceptor survival and improves vision
Dominik Lewandowski, Andrzej T. Foik, Roman Smidak, Elliot H. Choi, Jianye Zhang, Thanh Hoang, Aleksander Tworak, Susie Suh, Henri Leinonen, Zhiqian Dong, Antonio F.M. Pinto, Emily Tom, Jennings Luu, Joan Lee, Xiuli Ma, Erhard Bieberich, Seth Blackshaw, Alan Saghatelian, David C. Lyon, Dorota Skowronska-Krawczyk, Marcin Tabaka, Krzysztof Palczewski
Dominik Lewandowski, Andrzej T. Foik, Roman Smidak, Elliot H. Choi, Jianye Zhang, Thanh Hoang, Aleksander Tworak, Susie Suh, Henri Leinonen, Zhiqian Dong, Antonio F.M. Pinto, Emily Tom, Jennings Luu, Joan Lee, Xiuli Ma, Erhard Bieberich, Seth Blackshaw, Alan Saghatelian, David C. Lyon, Dorota Skowronska-Krawczyk, Marcin Tabaka, Krzysztof Palczewski
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Research Article Ophthalmology

Inhibition of ceramide accumulation in AdipoR1–/– mice increases photoreceptor survival and improves vision

Abstract

Adiponectin receptor 1 (ADIPOR1) is a lipid and glucose metabolism regulator that possesses intrinsic ceramidase activity. Mutations of the ADIPOR1 gene have been associated with nonsyndromic and syndromic retinitis pigmentosa. Here, we show that the absence of AdipoR1 in mice leads to progressive photoreceptor degeneration, significant reduction of electroretinogram amplitudes, decreased retinoid content in the retina, and reduced cone opsin expression. Single-cell RNA-Seq results indicate that ADIPOR1 encoded the most abundantly expressed ceramidase in mice and one of the 2 most highly expressed ceramidases in the human retina, next to acid ceramidase ASAH1. We discovered an accumulation of ceramides in the AdipoR1–/– retina, likely due to insufficient ceramidase activity for healthy retina function, resulting in photoreceptor death. Combined treatment with desipramine/L-cycloserine (DC) lowered ceramide levels and exerted a protective effect on photoreceptors in AdipoR1–/– mice. Moreover, we observed improvement in cone-mediated retinal function in the DC-treated animals. Lastly, we found that prolonged DC treatment corrected the electrical responses of the primary visual cortex to visual stimuli, approaching near-normal levels for some parameters. These results highlight the importance of ADIPOR1 ceramidase in the retina and show that pharmacological inhibition of ceramide generation can provide a therapeutic strategy for ADIPOR1-related retinopathy.

Authors

Dominik Lewandowski, Andrzej T. Foik, Roman Smidak, Elliot H. Choi, Jianye Zhang, Thanh Hoang, Aleksander Tworak, Susie Suh, Henri Leinonen, Zhiqian Dong, Antonio F.M. Pinto, Emily Tom, Jennings Luu, Joan Lee, Xiuli Ma, Erhard Bieberich, Seth Blackshaw, Alan Saghatelian, David C. Lyon, Dorota Skowronska-Krawczyk, Marcin Tabaka, Krzysztof Palczewski

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Figure 5

Accumulation of ceramides in the retina and RPE eyecup of AdipoR1–/– mice, and the ceramidase activity of ADIPOR1.

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Accumulation of ceramides in the retina and RPE eyecup of AdipoR1–/– mic...
(AC) Ceramides were quantified by LC-MS in the retina (A and B) and RPE eyecup (C) of 4-week-old AdipoR1+/+ and AdipoR1–/– mice. Data represent the mean ± SEM; n = 4 for each genotype. The statistical significance was determined by the 2-tailed unequal variance (Welch) t test; *P < 0.05, **P < 0.01, ***P < 0.001. (D) En face images of ceramide staining (green) in RPE flatmounts of 4-week-old AdipoR1+/+ and AdipoR1–/– mice. The tight junction protein ZO-1 (purple) demarcates cell boundaries. Scale bar: 20 μm. (E) Cross sections of the AdipoR1+/+ and AdipoR1–/– mouse retinas stained with ceramide Ab (red). Cones were stained with PNA-fluorescein (green), and cell nuclei were stained with DAPI (blue). Scale bar: 50 μm. (F) Enzymatic assay performed on the whole eye lysates from AdipoR1+/+ and AdipoR1–/– mice, using ceramide C2, C18, or C24:1 as substrates. (G) The enzymatic assay was performed with purified mouse ADIPOR1 (WT) or with the H191A,H337A-mutant (M) of ADIPOR1, using ceramide C18 as a substrate. The ceramidase activity was compared with or without adding high-molecular-weight fractions of recombinant mouse adiponectin, recombinant human C1QTNF5, or native mouse C1Q. Detected sphingosine (d18:1) values were normalized to internal standard (sphingosine-d7). The data (mean ± SEM) in F and G are representative of 3 independent experiments performed in 3 or 4 replicates. (H) Coomassie-stained reducing SDS-PAGE analysis of the proteins used in the assay shown in G. In F and G, statistical significance was determined by 1-way ANOVA followed by Sidak’s post hoc test; *P < 0.05, **P < 0.01, ***P < 0.001, ****P < 0.0001.