Residual Complex I activity and amphidirectional Complex II operation support glutamate catabolism through mtSLP in anoxia

Author:

Ravasz Dora,Bui David,Nazarian Sara,Pallag Gergely,Karnok Noemi,Roberts Jennie,Marzullo Bryan P.,Tennant Daniel A.,Greenwood Bennett,Kitayev Alex,Hill Collin,Komlódi Timea,Doerrier Carolina,Cunatova Kristyna,Fernandez-Vizarra Erika,Gnaiger Erich,Kiebish Michael A.,Raska Alexandra,Kolev Krasimir,Czumbel Bence,Narain Niven R.,Seyfried Thomas N.,Chinopoulos Christos

Abstract

AbstractAnoxia halts oxidative phosphorylation (OXPHOS) causing an accumulation of reduced compounds in the mitochondrial matrix which impedes dehydrogenases. By simultaneously measuring oxygen concentration, NADH autofluorescence, mitochondrial membrane potential and ubiquinone reduction extent in isolated mitochondria in real-time, we demonstrate that Complex I utilized endogenous quinones to oxidize NADH under acute anoxia. 13C metabolic tracing or untargeted analysis of metabolites extracted during anoxia in the presence or absence of site-specific inhibitors of the electron transfer system showed that NAD+ regenerated by Complex I is reduced by the 2-oxoglutarate dehydrogenase Complex yielding succinyl-CoA supporting mitochondrial substrate-level phosphorylation (mtSLP), releasing succinate. Complex II operated amphidirectionally during the anoxic event, providing quinones to Complex I and reducing fumarate to succinate. Our results highlight the importance of quinone provision to Complex I oxidizing NADH maintaining glutamate catabolism and mtSLP in the absence of OXPHOS.

Funder

Nemzeti Kutatási Fejlesztési és Innovációs Hivatal

Horizon 2020 Framework Programme

Semmelweis University

Publisher

Springer Science and Business Media LLC

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