Abstract
We recently reported a previously unrecognized mitochondrial respiratory phenomenon. When [ADP] was held constant ("clamped") at sequentially increasing concentrations in succinate-energized muscle mitochondria in the absence of rotenone (commonly used to block complex I), we observed a biphasic, increasing then decreasing, respiratory response. Here we investigated the mechanism. We confirmed decades-old reports that oxaloacetate (OAA) inhibits succinate dehydrogenase (SDH). We then used an NMR method to assess OAA concentrations (known as difficult to measure by MS) as well as those of malate, fumarate, and citrate in isolated succinate-respiring mitochondria. When these mitochondria were incubated at varying clamped ADP concentrations, respiration increased at low [ADP] as expected given the concurrent reduction in membrane potential. With further increments in [ADP], respiration decreased associated with accumulation of OAA. Moreover, a low pyruvate concentration, that alone was not enough to drive respiration, was sufficient to metabolize OAA to citrate and completely reverse the loss of succinate-supported respiration at high [ADP]. Further, chemical or genetic inhibition of pyruvate uptake prevented OAA clearance and preserved respiration. In addition, we measured the effects of incremental [ADP] on NADH, superoxide, and H2O2 (a marker of reverse electron transport from complex II to I). In summary, our findings, taken together, support a mechanism (detailed within) wherein succinate-energized respiration as a function of increasing [ADP] is initially increased by [ADP]-dependent effects on membrane potential but subsequently decreased at higher [ADP] by inhibition of succinate dehydrogenase by OAA. The physiologic relevance is discussed.
Highlights
We recently reported a previously unrecognized mitochondrial respiratory phenomenon
We provide compelling evidence for the role of OAA in regulating biphasic complex II–supported respiration. We describe how this process is related to changes in reverse electron transport (RET), reactive oxygen species (ROS), membrane potential (⌬⌿), and the oxidation/reduction state of NADϩ and NADH
Respiration and metabolite concentrations in succinate (10 mM) -energized mouse hind limb skeletal muscle mitochondria isolated from the mitochondrial pyruvate carrier 1 knock out (MCP1 KO) and littermate control mice incubated in the presence of 32 M ADP
Summary
We used ADP clamp methodology, 2-deoxyglucose plus hexokinase [5], combined with sensitive NMR technology to detect TCA cycle metabolites This includes quantification of oxaloacetic acid (OAA), a metabolite that is very difficult to measure by MS because of instability [6, 7]. We describe how this process is related to changes in reverse electron transport (RET), reactive oxygen species (ROS), membrane potential (⌬⌿), and the oxidation/reduction state of NADϩ and NADH. These findings advance our understanding of complex II– energized respiration and, suggest that we may need to re-think how complex II respiration is studied, i.e. that we might best do this at intermediate degrees of ADP availability without rotenone.
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