Increased core body temperature exacerbates defective protein prenylation in mouse models of mevalonate kinase deficiency
Marcia A. Munoz, Oliver P. Skinner, Etienne Masle-Farquhar, Julie Jurczyluk, Ya Xiao, Emma K. Fletcher, Esther Kristianto, Mark P. Hodson, Seán I. O’Donoghue, Sandeep Kaur, Robert Brink, David G. Zahra, Elissa K. Deenick, Kristen A. Perry, Avril A.B. Robertson, Sam Mehr, Pravin Hissaria, Catharina M. Mulders-Manders, Anna Simon, Michael J. Rogers
Marcia A. Munoz, Oliver P. Skinner, Etienne Masle-Farquhar, Julie Jurczyluk, Ya Xiao, Emma K. Fletcher, Esther Kristianto, Mark P. Hodson, Seán I. O’Donoghue, Sandeep Kaur, Robert Brink, David G. Zahra, Elissa K. Deenick, Kristen A. Perry, Avril A.B. Robertson, Sam Mehr, Pravin Hissaria, Catharina M. Mulders-Manders, Anna Simon, Michael J. Rogers
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Research Article Inflammation Metabolism

Increased core body temperature exacerbates defective protein prenylation in mouse models of mevalonate kinase deficiency

Abstract

Mevalonate kinase deficiency (MKD) is characterized by recurrent fevers and flares of systemic inflammation, caused by biallelic loss-of-function mutations in MVK. The underlying disease mechanisms and triggers of inflammatory flares are poorly understood because of the lack of in vivo models. We describe genetically modified mice bearing the hypomorphic mutation p.Val377Ile (the commonest variant in patients with MKD) and amorphic, frameshift mutations in Mvk. Compound heterozygous mice recapitulated the characteristic biochemical phenotype of MKD, with increased plasma mevalonic acid and clear buildup of unprenylated GTPases in PBMCs, splenocytes, and bone marrow. The inflammatory response to LPS was enhanced in compound heterozygous mice and treatment with the NLRP3 inflammasome inhibitor MCC950 prevented the elevation of circulating IL-1β, thus identifying a potential inflammasome target for future therapeutic approaches. Furthermore, lines of mice with a range of deficiencies in mevalonate kinase and abnormal prenylation mirrored the genotype-phenotype relationship in human MKD. Importantly, these mice allowed the determination of a threshold level of residual enzyme activity, below which protein prenylation is impaired. Elevated temperature dramatically but reversibly exacerbated the deficit in the mevalonate pathway and the defective prenylation in vitro and in vivo, highlighting increased body temperature as a likely trigger of inflammatory flares.

Authors

Marcia A. Munoz, Oliver P. Skinner, Etienne Masle-Farquhar, Julie Jurczyluk, Ya Xiao, Emma K. Fletcher, Esther Kristianto, Mark P. Hodson, Seán I. O’Donoghue, Sandeep Kaur, Robert Brink, David G. Zahra, Elissa K. Deenick, Kristen A. Perry, Avril A.B. Robertson, Sam Mehr, Pravin Hissaria, Catharina M. Mulders-Manders, Anna Simon, Michael J. Rogers

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Figure 4

MvkVI/Δ91 mice exhibit a lesser defect in prenylation and lack peritoneal inflammation compared with pharmacologic inhibition of the mevalonate pathway.

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MvkVI/Δ91 mice exhibit a lesser defect in prenylation and lack peritone...
(A) Diagram of the mevalonate pathway and points of inhibition in Mvk-mutant mice and in mice treated with alendronate (ALN). (B) Analysis of unprenylated Rab GTPases (uRabs) and unprenylated Rap1A (uRap1A) in peritoneal cells from MvkVI/Δ91 mice, and from wild-type mice 48 hours after i.p. treatment with ALN (6 mg/kg or 13 mg/kg) or saline control. (C) Representative FACS plots of peritoneal cells. Rows show gating of eosinophils, neutrophils, monocytes, and large (LPM) and small (SPM) peritoneal macrophages. Columns 1 and 2 show FACS plots from Mvk+/VI and MvkVI/Δ91 mice, columns 3–5 show FACS plots from wild-type mice treated with saline or 6 mg/kg or 13 mg/kg ALN. Polygons in red depict the population displayed in the proceeding plot (red arrows). (D) Histograms show relative abundance (percentage of live cell singlets) of eosinophils (TCRβB220CD11cSiglec-F+), neutrophils (TCRβB220Siglec-FLy6Ghi), monocytes (TCRβB220Siglec-FLy6GF4/80+Ly6Chi), LPM (TCRβB220Siglec-FLy6GF4/80hiCD11bhi), and SPM (TCRβB220Siglec-FLy6GF4/80+CD11b+). Bars are the mean ± SD, and each symbol represents a single mouse; n = 3 per group for Mvk+/VI and MvkVI/Δ91mice, n = 7 per group for ALN- and saline-treated mice. ****P < 0.0001 by 1-way ANOVA and Dunnett’s post hoc multiple-comparisons test.