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Mitochondrial membrane dynamics is increasingly implicated in various human diseases. Numerous studies show that the protein OPA1 plays a central role in determining mitochondrial ultrastructure and apoptotic remodeling of the inner mitochondrial membrane during Cytochrome c release and apoptosis. Crista junctions are crucial for the regulation of apoptotic Cytochrome c release. Previous publications suggest that OPA1 is required to maintain a normal structure of the inner mitochondrial membrane. The protein MIC60 (Mitofilin) appears to be an essential physical constituent of crista junctions and is also crucial for the general determination of mitochondrial ultrastructure. Furthermore, recent studies suggest that MIC60 is also implicated in Cytochrome c release during apoptosis.
In this regard, the question whether OPA1 is essential for crista junction formation was investigated. In addition to that, the interplay between OPA1 and MIC60 and its physiological role were analyzed. Electron microscopy of OPA1+/- and OPA1+/+ mice, as well as of OPA1-/- and OPA1+/+ MEFs clearly showed that OPA1 plays a role but is not essential for crista junction formation. In contrast to that, the results indicate that OPA1 is crucial to maintain a normal structure of the inner mitochondrial membrane. Immunogold experiments fit well to these observations as OPA1 was found equally distributed throughout the cristae membrane with only a minor part located at crista junctions. MIC60 localization studies showed a clear enrichment at crista junctions. Interaction studies revealed that endogenous OPA1 and MIC60 physically interact with each other. Analysis of protein levels upon OPA1 or MIC60 depletion indicate that both proteins play a dual role in cristae- and crista junction formation in which MIC60 is a physical constituent of crista junctions essential for their formation while OPA1 primarily has a regulatory impact on MIC60 function. Finally, apoptosis assays and cell viability measurements showed that knockout of OPA1 in MEFs leads to increased cellular resistance suggesting that the interplay of these proteins is important for the regulation of crista junction remodeling during apoptosis.
Besides its role in determining mitochondrial ultrastructure, OPA1 mediates inner membrane fusion of mitochondria thereby contributing to mitochondrial quality control. Additionally, proteolytic processing is crucial for the ability of OPA1 to distinguish between functional and dysfunctional mitochondria. Functional mitochondria are fused while dysfunctional mitochondria are not, a process termed selective mitochondrial fusion. Dysfunctional mitochondria were shown to be degraded by mitophagy in a fission-dependent manner. Numerous studies suggest that OPA1 and mitophagy are directly linked. However, this idea is still under debate. Mitophagy is also crucial for mitochondrial quality control, which directly impacts mitochondrial integrity. Furthermore, mitochondrial quality control has been linked to neurodegeneration as demonstrated by the observation that mutations in OPA1 cause the disorder ADOA-1.
In order to analyze a potential link between OPA1 and mitophagy, mitochondrial colocalization with LC3 was analyzed microscopically in primary adult skin fibroblasts isolated from OPA1+/- and OPA1+/+ mice in an age-dependent manner. Fibroblasts from young OPA1+/- mice showed increased colocalization of mitochondria with autophagosomes compared to fibroblasts from young wild type mice suggesting that OPA1 exerts an inhibitory role in mitophagy. This effect was even more pronounced in old mice, which also displayed higher mitophagy levels in general than young mice, consistent with the finding that old mice had higher Parkin levels than young mice. Mitochondrial fragmentation was elevated in fibroblasts from young and old OPA1+/- mice compared to control fibroblasts. However, extensive mitochondrial fusion, which occurred in fibroblasts from old wild type mice, was prevented in old OPA1+/- mice. Furthermore, old wild type mice had decreased numbers of crista junctions compared to young wild type mice, an effect that was not observed in OPA1+/- mice. Despite the observed age-dependent phenotypes in mitochondrial quality control and mitochondrial integrity, deletion of one allele of OPA1 had no influence on the life span in vivo. Analysis of the OPA1-dependent proteome of aging mice, which was performed in collaboration with Ansgar Poetsch and Carina Ramallo-Guevara from Bochum, showed that OPA1-dependent aging is accompanied by a reduction of proteins involved in autophagy. In contrast to that, a switch from glucose to fatty acid metabolism and alterations in apoptotic proteins were observed in both OPA1+/- and OPA1+/+ mice in an age-dependent manner indicating that the changes in proteins implicated in autophagy could be a compensatory response to the diminished inhibitory effect of OPA1 on mitophagy. On the other hand, increased mitochondrial degradation by mitophagy could be a cellular response to itself compensating for the loss of OPA1 mediated fusion thereby contributing to the observation that OPA1+/- and OPA1+/+ mice had no differences in life span. Furthermore, analysis of the OPA1-dependent proteome of aging mice revealed that OPA1, besides its role in mitochondrial fusion, could interact with the fission machinery: MFF and Neuronal pentraxin 1, two proteins involved in mitochondrial fission, were up-regulated in 12-month-old OPA1+/- mice suggesting that a reduced fission activity could contribute to mitochondrial hyperfusion in aged wild- type mice. Nonetheless, the exact nature of the possible interplays between OPA1 and these candidates remains to be investigated.