Deacetylation via SIRT2 prevents keratin-mutation-associated injury and keratin aggregation
Jingyuan Sun, Pei Li, Honglian Gui, Laure Rittié, David B. Lombard, Katrin Rietscher, Thomas M. Magin, Qing Xie, Li Liu, M. Bishr Omary
Jingyuan Sun, Pei Li, Honglian Gui, Laure Rittié, David B. Lombard, Katrin Rietscher, Thomas M. Magin, Qing Xie, Li Liu, M. Bishr Omary
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Research Article Dermatology Hepatology

Deacetylation via SIRT2 prevents keratin-mutation-associated injury and keratin aggregation

Abstract

Keratin (K) and other intermediate filament (IF) protein mutations at conserved arginines disrupt keratin filaments into aggregates and cause human epidermolysis bullosa simplex (EBS; K14-R125C) or predispose to mouse liver injury (K18-R90C). The challenge for more than 70 IF-associated diseases is the lack of clinically utilized IF-targeted therapies. We used high-throughput drug screening to identify compounds that normalized mutation-triggered keratin filament disruption. Parthenolide, a plant sesquiterpene lactone, dramatically reversed keratin filament disruption and protected cells and mice expressing K18-R90C from apoptosis. K18-R90C became hyperacetylated compared with K18-WT and treatment with parthenolide normalized K18 acetylation. Parthenolide upregulated the NAD-dependent SIRT2, and increased SIRT2-keratin association. SIRT2 knockdown or pharmacologic inhibition blocked the parthenolide effect, while site-specific Lys-to-Arg mutation of keratin acetylation sites normalized K18-R90C filaments. Treatment of K18-R90C–expressing cells and mice with nicotinamide mononucleotide had a parthenolide-like protective effect. In 2 human K18 variants that associate with human fatal drug-induced liver injury, parthenolide protected K18-D89H– but not K8-K393R–induced filament disruption and cell death. Importantly, parthenolide normalized K14-R125C–mediated filament disruption in keratinocytes and inhibited dispase-triggered keratinocyte sheet fragmentation and Fas-mediated apoptosis. Therefore, keratin acetylation may provide a novel therapeutic target for some keratin-associated diseases.

Authors

Jingyuan Sun, Pei Li, Honglian Gui, Laure Rittié, David B. Lombard, Katrin Rietscher, Thomas M. Magin, Qing Xie, Li Liu, M. Bishr Omary

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Figure 5

Keratin deacetylation by lysine point mutation normalizes K18-R90C–induced keratin filament disruption.

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Keratin deacetylation by lysine point mutation normalizes K18-R90C–induc...
(A) Double mutants of K18 (R90C/acetylation) and K18-R90C/K8 acetylation mutants, WT K8 and WT K18, or WT K8 and K18-R90C were cotransfected into NIH-3T3 cells (which do not express endogenous keratins) followed by double staining (green = keratins, blue = nuclei). Scale bars: 50 μm. (B) Quantification of the percentage cells with dots using pooled counts from 3 separate experiments. Data are presented as the mean ± SD. *P < 0.05, **P < 0.01, ***P < 0.001, ****P < 0.0001 when comparing each of the double mutant constructs with cells transfected with WT K8 and K18-R90C. One-way ANOVA was used for comparison between treatment groups, and Tukey’s post hoc test was used for comparing multiple groups with the R90C/WT group.