Metabolic rerouting via SCD1 induction impacts X-linked adrenoleukodystrophy
Quentin Raas, … , Joshua L. Bonkowsky, Stephan Kemp
Quentin Raas, … , Joshua L. Bonkowsky, Stephan Kemp
Published March 9, 2021
Citation Information: J Clin Invest. 2021;131(8):e142500. https://doi.org/10.1172/JCI142500.
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Research Article Metabolism Neuroscience

Metabolic rerouting via SCD1 induction impacts X-linked adrenoleukodystrophy

Abstract

X-linked adrenoleukodystrophy (ALD) is a progressive neurodegenerative disease caused by mutations in ABCD1, the peroxisomal very long–chain fatty acid (VLCFA) transporter. ABCD1 deficiency results in accumulation of saturated VLCFAs. A drug screen using a phenotypic motor assay in a zebrafish ALD model identified chloroquine as the top hit. Chloroquine increased expression of stearoyl-CoA desaturase-1 (scd1), the enzyme mediating fatty acid saturation status, suggesting that a shift toward monounsaturated fatty acids relieved toxicity. In human ALD fibroblasts, chloroquine also increased SCD1 levels and reduced saturated VLCFAs. Conversely, pharmacological inhibition of SCD1 expression led to an increase in saturated VLCFAs, and CRISPR knockout of scd1 in zebrafish mimicked the motor phenotype of ALD zebrafish. Importantly, saturated VLCFAs caused ER stress in ALD fibroblasts, whereas monounsaturated VLCFA did not. In parallel, we used liver X receptor (LXR) agonists to increase SCD1 expression, causing a shift from saturated toward monounsaturated VLCFA and normalizing phospholipid profiles. Finally, Abcd1–/y mice receiving LXR agonist in their diet had VLCFA reductions in ALD-relevant tissues. These results suggest that metabolic rerouting of saturated to monounsaturated VLCFAs may alleviate lipid toxicity, a strategy that may be beneficial in ALD and other peroxisomal diseases in which VLCFAs play a key role.

Authors

Quentin Raas, Malu-Clair van de Beek, Sonja Forss-Petter, Inge M.E. Dijkstra, Abigail Deschiffart, Briana C. Freshner, Tamara J. Stevenson, Yorrick R.J. Jaspers, Liselotte Nagtzaam, Ronald J.A. Wanders, Michel van Weeghel, Joo-Yeon Engelen-Lee, Marc Engelen, Florian Eichler, Johannes Berger, Joshua L. Bonkowsky, Stephan Kemp

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Figure 2

Zebrafish phenotypic secondary screening to identify CQ.

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Zebrafish phenotypic secondary screening to identify CQ. (A) Heatmap of ...
(A) Heatmap of results of a secondary screen performed on the 15 compounds with the highest z scores, comparing control (0.1% DMSO) versus compound (2.5 μm in 0.1% DMSO) homozygous abcd1sa509/sa509, heterozygous abcd1sa509/+ mutants (n = 48), or their WT relatives (n = 48). (B) Rescreening of the 2 top hits. Heatmap of z scores for distance and time-moving values of 5 to 7 dpf abcd1sa509 mutants treated with 1, 2.5, or 10 μM CQ or prednisolone (n = 70–150). Right panel; effect of CQ (10 μM) on the distance swum by 7 dpf abcd1sa509, abcd1zc92, or WT larvae (n = 90–130 per group); 2-way ANOVA, followed by Bonferroni’s multiple comparison test. **P < 0.01; ****P < 0.0001.