Targeting energy metabolism via the mitochondrial pyruvate carrier as a novel approach to attenuate neurodegeneration

The adverse effects associated with PPARγ activation and the discovery that the beneficial effects of TZDs do not require PPARγ prompted the development of novel drugs with little affinity for PPARγ. Two such drugs are MSDC-0602 and MSDC-0160. Several studies have shown that MSDC-0160 is an excellent insulin-sensitizer, despite the drug and its major hydroxymetabolite having extremely low affinities for PPARγ (over 250- and 50-fold lower, respectively) compared to rosiglitazone (Table 1) [30], making it a ‘PPARγ-sparing’ drug. Instead MSDC-0160 enhances insulin sensitivity by inhibiting the MPC complex. In a Drosophila model of insulin resistance, treatment with MSDC-0160 significantly enhanced insulin sensitivity [47]. This beneficial effect of the drug was suggested to be mediated by the MPC complex, as deletion of the Mpc1 orthologue resulted in a loss of the drug effect in the Drosophila model [47]. Further evaluations indicated that the drug’s action was, at least in part, related to the alterations in pyruvate, a key substrate in the citric acid cycle. These findings place insulin sensitizers such as MSDC-0160 at the heart of the metabolism of carbohydrates, amino acids and fatty acids [47]. Notably, dysfunctions of such cellular metabolic pathways are implicated in the pathophysiology of insulin resistance [57, 58].

Based on the attractive pharmacological profile of MSDC-0160 in preclinical models, it was entered into clinical trials. A double-blind, randomized phase II b clinical trial over three months in individuals with type 2 diabetes explored three exposures of MSDC-0160 as compared to pioglitazone. In this trial, MSDC-0160 reduced plasma glucose and elicited similar beneficial effects as pioglitazone, but without the undesirable side effects [52]. Importantly, the trial with MSDC-0160 also demonstrated that the drug can be dosed to a 50% higher circulating exposure. The highest MSDC-0160 dose explored produced an area under the curve (AUC) of 90,000 ng.hr/ml as compared to 60,000 ng.hr/ml for 45 mg pioglitazone (parent and active metabolites). Table 1 compares the IC₅₀ for the effects of the compounds on binding to PPARγ versus MPC, along with the C_max. Based on these data, a phase II a clinical trial was conducted in subjects with Alzheimer’s disease.

A phase IIa study in non-diabetic subjects with mild to moderate Alzheimer’s disease demonstrated that treatment with 150 mg/day MSDC-0160 for three months resulted in significant changes in the pattern of ¹⁸F-2deoxyglucose uptake on positron emission tomography (PET) scans as compared to the placebo-treated subjects [59]. Analysis of these PET scans suggested increased glucose uptake in brain regions known to be affected in Alzheimer’s disease suggesting that oral treatment was having central (possibly neuroprotective) effects. Attention was then turned to the study of MSDC-0160 in models of PD where the mechanisms involved could be probed in more detail [60].

Recently, we demonstrated that MSDC-0160 attenuated neurodegeneration in multiple cell and animal models of PD by a process that includes autophagy augmentation and inflammation reduction [60]. These effects occurred both in genetic and neurotoxin-based PD models. These actions of MSDC-0160 involved effects on both neurons and glial cells (Fig. 1) [60].

Specifically, the effect of MSDC-0160 was evaluated in models induced by 1-methyl-4-phenyl-1,2,3,6-tetrahydropyridine/1-methyl-4-phenylpyridinium (MPTP/ MPP⁺) and in genetic models with hemizygous loss of Engrailed 1 (En1) in mice or neuronal overexpression of α-synuclein in Caenorhabditis elegans (C. elegans) [60]. MSDC-0160 treatment protected against MPTP-induced loss of tyrosine hydroxylase (TH)-immunoreactive neurons, both in those derived from Lund human mesencephalic (LUHMES) cells and in TH-immunoreactive mouse primary mesencephalic neurons. In addition to protecting dopamine neurons in cell culture, the drug also reduced MPP⁺ induced dopaminergic neuron loss in vivo in C. elegans. Further, the effect of the drug was evaluated in mammalian models. In this regard, MPTP was utilized to induce PD-like features in mice including loss of nigral dopaminergic neurons and dopaminergic terminals in the striatum. When evaluated using multiple methods (e.g. cell counts, western blotting and neurochemistry), the toxic effects of MPTP were significantly reduced through pretreatment with MSDC-0160. A similar protective effect of the drug was observed even when it was delivered 2 days after MPTP toxicity had been induced in mice. Behaviorally, MPTP injections caused the expected impairments in locomotion (reductions in distance traveled, speed, mobility time in an open field and time spent on a rotating rod), akin to the hypokinetic syndrome of PD. MSDC-0160 treatment mitigated these behavioral impairments. Experiments in En1 hemizygous null mice, that normally exhibit a protracted 40% loss of nigral dopamine neurons, showed that MSDC-0160 could significantly reduce nigrostriatal degeneration and attenuate the development of motor deficits [60]. Similar to the protective effect of MPC inhibition using MSDC-0160 on dopaminergic neurons, other studies have shown that MPC inhibition using UK-5099 protects cortical neurons against excitotoxic injury by modulating glutamate abundance and release [31, 61]. Given that MSDC-0160 attenuated MPC in both neurons and microglia in the PD models, it is still not clear whether the neuroprotective effect of the drug was due primarily to its action on MPC in either one of these two cell types or both. The individual far-reaching effects of MPC modulation in microglia and neurons are depicted in Fig. 1.

To understand the mechanism by which MSDC-0160 protects against neurodegeneration, we turned to the C. elegans PD model [60]. In this worm model, modulation of the function of the MPC1 orthologue rescued dopaminergic neurons overexpressing A53T α-synuclein (a mutation that causes autosomal dominant PD in humans). Downstream of MPC activity and crucial for autophagy is the mammalian target of rapamycin (mTOR) and its signaling pathway. Thus, we knocked down key players in the MPC and mTOR pathways using RNA interference in these worm models and then evaluated if the effect of MSDC-0160 was maintained. Using this approach, knockdown of the MPC1 orthologue, and the mTOR orthologue or its regulators such as AKT-1 and RHEB-1 prevented the neuroprotection induced by MSDC-0160, implicating the mTOR pathway as a mediator of MSDC-0160 effects. These effects were similar to what was previously published in flies, where knockdown of MPC1 or its modulation with MSDC-0160 altered AKT phosphorylation status [47]. In contrast, knockdown of the orthologue of the cellular energy sensor AMPK (AMP-activated protein kinase which is an upstream regulator of mTOR-mediated autophagy following changes in cellular energy state) did not prevent the neuroprotection induced by MSDC-0160 [60].

Complete pharmacological inhibition of MPC using UK-5099 has been shown not to affect cell viability or oxygen consumption significantly and maintains a degree of ‘metabolic flexibility’ in healthy cortical neurons and astrocytes [61]. To define the effects of MPC inhibition on oxygen consumption in a setting potentially more relevant to PD, we measured the effects of MSDC-0160 on oxygen consumption in cultured dopaminergic neurons exposed to the mitochondrial complex inhibitor MPP⁺. Under these stressful conditions, the drug normalized oxygen consumption in cells exposed to MPP⁺, indicating a direct metabolic effect of MSDC-0160 on mitochondrial respiration, upstream of the mTOR pathway. Importantly, we also established the effects of MSDC-0160 on autophagy in vivo. In our in vivo studies using the MPTP and En1 models, there were abnormalities in mTOR signaling and autophagy, reflected by increases in ratios of p-mTOR/mTOR ratio and the downstream substrate pS6/S6, as well as changes in DNA damage responses (REDD1)/β-actin ratios. The abnormally high mTOR activation in these two mouse PD models were inhibited by MSDC-0160. Most interestingly, in no case did the treatment with MSDC-0160 reduce the activity of mTOR under control additions. In other words, rather than inhibiting mTOR activation, treatment prevented the over-activation of mTOR caused by the various manipulations. In addition, the En1 mouse PD model exhibited abnormally low ratios of the autophagy markers LC3b/β-actin and p62/β-actin, which was corrected by MSDC-0160 [60]. Together, our study revealed that MPC inhibition by MSDC-0160 leads to normalization of oxygen consumption in compromised cells and it protects against neuronal loss by inhibiting mTOR and enhancing autophagy. Notably, the onset of the aforementioned effects on mitochondrial respiration was within a few minutes of exposure to MSDC-0160, while changes in autophagy pathways took more than 24 h to be apparent. Thus, it remains to be established precisely how mTOR inhibition is achieved following MPC inhibition, and the metabolic events that follow the immediate effects on mitochondrial respiration and that precede changes in the mTOR pathway still need to be elucidated. A greater understanding of these changes will solidify the MPC as a therapeutic target in PD and might reveal new molecular targets for intervention.

Neuroinflammation is considered to play a major role in the pathophysiology of PD [62, 63]. Therefore, we further assessed the effect of MSDC-0160 on neuroinflammatory markers in different PD models [60]. In both mouse models (MPTP and En1^+/−), MSDC-0160 reduced the microglial marker ionized calcium-binding adapter molecule 1 (Iba-1), the astrocyte marker glial fibrillary acidic protein (GFAP), and the expression of the inducible nitric oxide synthase (iNOS) in the midbrain, indicative of reductions in microgliosis and astrogliosis. Further experiments using a microglial cell line (BV2 cell line) and mouse primary microglial cells revealed that MSDC-0160 prevented lipopolysaccharide (LPS)-induced nitrite production and iNOS expression. Moreover, while phosphorylated p65 were found to accumulate in the nucleus of BV2 cells exposed to LPS, MSDC-0160 prevented this nuclear accumulation, perhaps as a result of the inhibition of NFκB (a transcription factor involved in inflammatory responses). As expected from the decreases in inflammatory markers, there were also reductions in the release of proinflammatory cytokines from LPS-stimulated BV2 cells that were exposed to MSDC-0160. Specifically, MSDC-0160 reduced LPS-induced release of the cytokines IL-1β, TNF-α and IL-6, consistent with an inhibition of neuroinflammation (Fig. 1b-c).

From a mechanistic point of view, it is clear that glial cells and neurons communicate in vivo, and it is possible that MSDC-0160 could have influenced either neuronal survival or glial activation states indirectly. However, in vitro experiments where neurons and glia are cultured separately, like those discussed above, indicate that MSDC-0160 has direct effects on both cell types. In addition, application of MSDC-0160 to LPS-treated BV2 cells also restored mitochondrial oxygen consumption back to normal levels within minutes of the drug being added to the culture [60]. Notably, in the absence of cell stressors or genetic changes we observed no measurable effects of MSDC-0160 on the different markers we monitored in either neurons or BV2 cells, or in the mouse models in vivo. This strongly suggest that modulation of the activity of MPC, a pharmacology that also improves insulin sensitivity [53], directly impacts the pathophysiology relevant to PD in both glial cells and neurons without significantly altering their normal biology. Therefore, MPC appears to be a particularly attractive molecular target for disease modification in PD.