OMA1 mediates local and global stress responses against protein misfolding in CHCHD10 mitochondrial myopathy
Mario K. Shammas, … , Joanna Poulton, Derek P. Narendra
Mario K. Shammas, … , Joanna Poulton, Derek P. Narendra
Published June 14, 2022
Citation Information: J Clin Invest. 2022;132(14):e157504. https://doi.org/10.1172/JCI157504.
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OMA1 mediates local and global stress responses against protein misfolding in CHCHD10 mitochondrial myopathy

Abstract

Mitochondrial stress triggers a response in the cell’s mitochondria and nucleus, but how these stress responses are coordinated in vivo is poorly understood. Here, we characterize a family with myopathy caused by a dominant p.G58R mutation in the mitochondrial protein CHCHD10. To understand the disease etiology, we developed a knockin (KI) mouse model and found that mutant CHCHD10 aggregated in affected tissues, applying a toxic protein stress to the inner mitochondrial membrane. Unexpectedly, the survival of CHCHD10-KI mice depended on a protective stress response mediated by the mitochondrial metalloendopeptidase OMA1. The OMA1 stress response acted both locally within mitochondria, causing mitochondrial fragmentation, and signaled outside the mitochondria, activating the integrated stress response through cleavage of DAP3-binding cell death enhancer 1 (DELE1). We additionally identified an isoform switch in the terminal complex of the electron transport chain as a component of this response. Our results demonstrate that OMA1 was critical for neonatal survival conditionally in the setting of inner mitochondrial membrane stress, coordinating local and global stress responses to reshape the mitochondrial network and proteome.

Authors

Mario K. Shammas, Xiaoping Huang, Beverly P. Wu, Evelyn Fessler, Insung Y. Song, Nicholas P. Randolph, Yan Li, Christopher K.E. Bleck, Danielle A. Springer, Carl Fratter, Ines A. Barbosa, Andrew F. Powers, Pedro M. Quirós, Carlos Lopez-Otin, Lucas T. Jae, Joanna Poulton, Derek P. Narendra

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Figure 7

OMA1 is critical for C10 G58R pup survival.

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OMA1 is critical for C10 G58R pup survival. (A) Immunoblot of OPA1 and O...
(A) Immunoblot of OPA1 and OMA1 levels in 14-week-old littermates of the C10WT OMA1–/– and C10G58R OMA1+/– cross. m, mouse (n = 4 mice per genotype). (B) Survival curves for pups from the C10WT and C10G58R cross and the C10WT OMA1–/– and C10G58R OMA1+/– cross. All 6 dead pups genotyped from the latter cross were C10G58R OMA1–/– (n = 18 pups from the C10WT and C10G58R cross; n = 46 pups from C10WT OMA1–/– and C10G58R OMA1+/– cross). (C) Top: 14-week-old littermates from the C10WT OMA1–/– and C10G58R OMA1+/– cross. Middle: Masson’s trichrome (MT) stainings of mouse hearts. Bottom: Magnified MT stainings of heart showing prominent vacuolation in C10G58R OMA1–/– hearts (n = 3 mice per genotype). Scale bars: 1 mm (middle) and 100 μm (bottom). (D) Immunoblot of OPA1 levels in hearts from C10WT or C10G58R mice on the OMA1+/– background, on P1 and P5. Loading controls are shown in Supplemental Figure 9G (n = 3 mice per genotype). (E) Quantification of OMA-cleaved OPA1 bands (c+e/total) from immunoblot data in D. Error bars represent the SEM. **P < 0.01 and ****P < 0.0001, by log-rank test (B) and 2-way ANOVA with Sidak’s multiple comparisons (E). See also Supplemental Figure 9.