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Cyclophilin D–dependent oligodendrocyte mitochondrial ion leak contributes to neonatal white matter injury
Zoya Niatsetskaya, … , Evgeny Pavlov, Vadim Ten
Zoya Niatsetskaya, … , Evgeny Pavlov, Vadim Ten
Published September 14, 2020
Citation Information: J Clin Invest. 2020;130(10):5536-5550. https://doi.org/10.1172/JCI133082.
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Research Article Development Neuroscience Article has an altmetric score of 2

Cyclophilin D–dependent oligodendrocyte mitochondrial ion leak contributes to neonatal white matter injury

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Abstract

Postnatal failure of oligodendrocyte maturation has been proposed as a cellular mechanism of diffuse white matter injury (WMI) in premature infants. However, the molecular mechanisms for oligodendrocyte maturational failure remain unclear. In neonatal mice and cultured differentiating oligodendrocytes, sublethal intermittent hypoxic (IH) stress activated cyclophilin D–dependent mitochondrial proton leak and uncoupled mitochondrial respiration, leading to transient bioenergetic stress. This was associated with development of diffuse WMI: poor oligodendrocyte maturation, diffuse axonal hypomyelination, and permanent sensorimotor deficit. In normoxic mice and oligodendrocytes, exposure to a mitochondrial uncoupler recapitulated the phenotype of WMI, supporting the detrimental role of mitochondrial uncoupling in the pathogenesis of WMI. Compared with WT mice, cyclophilin D–knockout littermates did not develop bioenergetic stress in response to IH challenge and fully preserved oligodendrocyte maturation, axonal myelination, and neurofunction. Our study identified the cyclophilin D–dependent mitochondrial proton leak and uncoupling as a potentially novel subcellular mechanism for the maturational failure of oligodendrocytes and offers a potential therapeutic target for prevention of diffuse WMI in premature infants experiencing chronic IH stress.

Authors

Zoya Niatsetskaya, Sergey Sosunov, Anna Stepanova, James Goldman, Alexander Galkin, Maria Neginskaya, Evgeny Pavlov, Vadim Ten

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Figure 3

IH or DNP arrests OLs’ maturation.IH or DNP arrests OLs’ maturation.(A) Confocal microscopy of cultured OPCs stained for NG2 and Olig2 (control for OPC purity) and NG2 and CNP-ase before and after 2 days of differentiation under normoxic, IH, or DNP exposures.

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IH or DNP arrests OLs’ maturation.IH or DNP arrests OLs’ maturation.(A) ...
Scale bar: 30 μm. (B) CNP-ase– and NG2-specific fluorescence per Dapi+ cell count in the field after 2 days of the OPC differentiation under IH or DNP exposure. Data expressed as the percentage in relation to the fluorescence in the normoxic controls. *P < 0.0005 (1-way ANOVA, Dunnett’s post hoc); #P < 0.01 (Kruskal-Wallis and Dunn’s post hoc tests). (C and D) Images and analysis of MBP fluorescence per cell in the OPCs before and after 5 days of differentiation under normoxic, IH, or DNP exposure. **P < 0.009 (1-way ANOVA, Dunnett’s post hoc test) compared with controls (NormOx). Blue is DAPI; scale bar: 30 μm.

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