Abstract
Physiological aging causes motor function decline and anatomical and biochemical changes in the motor cortex. We confirmed that middle-aged mice at 15–18 months old show motor function decline, which can be restored to the young adult level by supplementing with mitochondrial electron transporter coenzyme Q10 (CoQ10) as a water-soluble nanoformula by drinking water for 1 week. CoQ10 supplementation concurrently improved brain mitochondrial respiration but not muscle strength. Notably, we identified an age-related decline in field excitatory postsynaptic potential (fEPSP) amplitude in the pathway from layers II/III to V of the primary motor area of middle-aged mice, which was restored to the young adult level by supplementing with CoQ10 for 1 week but not by administering CoQ10 acutely to brain slices. Interestingly, CoQ10 with high-frequency stimulation induced NMDA receptor-dependent long-term potentiation (LTP) in layer V of the primary motor cortex of middle-aged mice. Importantly, the fEPSP amplitude showed a larger input‒output relationship after CoQ10-dependent LTP expression. These data suggest that CoQ10 restores the motor function of middle-aged mice by improving brain mitochondrial function and the basal fEPSP level of the motor cortex, potentially by enhancing synaptic plasticity efficacy. Thus, CoQ10 supplementation may ameliorate the age-related decline in motor function in humans.
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Introduction
The age-related decrease in motor function can be caused by a loss of muscle mass and strength (sarcopenia), denervation of neuromuscular junctions (NMJs), loss of motor neurons in the spinal cord, and reduced function of the brain motor cortex. In mice, a decline in motor function was observed in middle-aged mice (15 months old); earlier than the drop in survival rate that typically occurs at approximately 24 months of age1,2,3. In the human motor cortex, physiological aging causes cortical atrophy, altered excitability, and decreased neurotransmitter levels 4,5,6. Voluntary activation of skeletal muscles is impaired during aging, especially in elderly individuals who are weak or in poor physical condition5. Elderly individuals show a decrease in the firing rate of lower motor neurons, which may be related, at least in part, to decreased activity of the motor cortex. In rodents, middle-aged mice show motor function impairment and increased phosphorylation of α-synuclein and a decreased level of vesicular glutamate transporter 1 (VGluT1) in motor cortex compared to those of young adult mice1,7. These impairments in the motor cortex may be part of the underlying mechanism that leads to age-related motor function decline.
Brain aging also causes deficits in the mitochondrial oxidative phosphorylation system, producing ATP necessary to fulfill brain neuronal functions8. The basal ganglia putamen of old rhesus monkeys showed decreased mitochondrial functions of ATP synthesis and calcium buffering, which correlated with age-related motor deficits8. Interestingly, mitochondrial function measured by peroxide production was higher in synaptic mitochondria than in nonsynaptic mitochondria in rat brains. Furthermore, mitochondrial respiration function decreased significantly with age only in synaptic mitochondria but not in nonsynaptic mitochondria among 14- and 17-month-old mice compared to those of 3-month-old mice9,10. These data suggest an age-related functional decline of mitochondria located at synapses in the brain. Mechanistically, mitochondrial oxidative phosphorylation requires the electron transporter coenzyme Q. In mice, coenzyme Q9 and Q10 are used to transport electrons from complexes I and II to complex III for ATP synthesis11,12,13. The level of coenzyme Q10 (CoQ10) decreases during aging in rodents and humans1,14,15,16. Interestingly, exogenous administration of CoQ10 ameliorated motor impairment and the brain mitochondrial respiration rate in aged mice1,17.
These studies demonstrate the age-related decline in motor functions, motor cortex functions, and synaptic mitochondrial functions. However, further research is needed to reveal what kind of electrophysiological impairments underlie the age-related decline in motor functions and to develop intervention methods to rescue the motor function and motor cortex neuronal activity of elderly or aged animals. This study tested whether the age-related decline in motor functions could be reversed by supplementing the mitochondrial component that decreases during aging. CoQ10 was supplemented by drinking water in middle-aged mice, which led to motor function improvements. To investigate the mechanism activated by CoQ10, we measured muscle strength, brain mitochondrial function, and electrophysiological activity in the motor cortex of middle-aged mice supplemented with CoQ10.
Results
CoQ10 supplementation reversed age-related decline in motor function
We compared the motor function of young adult mice (6 months old) and middle-aged mice (15–16 months old) by performing the pole test following supplementation with water-soluble nanoformula-type CoQ10 by drinking water (150 μM, 40SP, Petroeuroasia) for 10–13 days or without supplementation (Fig. 1a). The pole test is used to evaluate motor coordination deficit18,19,20 by measuring the time required for mice to orient their body and feet completely downward at the top of a vertical pole (T-turn) and the total time to descend to the floor of the experimental cage (T-total). The 15-month-old middle-aged mice required a significantly longer time for the T-turn than the young adult mice (young adult control, 1.50 ± 0.07 s, middle-aged control, 2.24 ± 0.13 s). CoQ10 supplementation in middle-aged mice improved motor function (T-turn) by 25.76% to a level similar to that of the young adult controls (Fig. 1a left). There was a significant interaction between CoQ10 supplementation and age, a significant main effect of supplementation, and a significant main effect of age (Fig. 1a left; the interaction between supplementation and age p = 0.0296, F (1,76) = 4.919; the main effect of supplementation p = 0.0009, F (1, 76) = 11.95; the main effect of age p < 0.0001, F (1, 76) = 25.77, two-way ANOVA; young adult control compared to middle-aged control p < 0.0001; young adult CoQ10 compared to middle-aged control, p < 0.0001; middle-aged control compared to middle-aged CoQ10, p = 0.0008, Bonferroni’s multiple comparison test). Measurements of the total time (T-total) revealed a significant main effect of supplementation but did not show any main effect of age or a supplementation-age interaction (Fig. 1a right; the interaction between supplementation and age p = 0.1386, F (1,76) = 2.240; the main effect of supplementation p = 0.0043, F (1, 76) = 8.686, two-way ANOVA). The age-dependent decline in motor function in the pole test and recovery by water-soluble nanoformula-type CoQ10 supplementation is consistent with a previous study1.
In this study, we also tested the effect of CoQ10 supplementation in young adult mice to reveal whether the beneficial effect of CoQ10 is an age-specific effect or a general effect. Interestingly, CoQ10 supplementation did not change the T-turn of young adult mice (Fig. 1a left; young adult control compared to young adult CoQ10, p > 0.9999, Bonferroni's multiple comparison test) and revealed the significant main effect of supplementation on the T-total without the main effect of age or the supplementation-age interaction (Fig. 1a right). These results revealed that the beneficial effect of CoQ10 supplementation is stronger in middle-aged mice showing a decline in motor function.
We analyzed whether CoQ10 supplementation for 1 week affects muscle strength by measuring the wire hanging latency of young adult and middle-aged mice with or without CoQ10 supplementation. There was no interaction between CoQ10 supplementation and age or main effect of supplementation. However, there was a significant main effect of age, suggesting an age-related decline in muscle strength (Fig. 1b; the interaction between supplementation and age p = 0.9440, F (1, 76) = 0.0050; the main effect of age p < 0.0001, F (1,76) = 22.42, two-way ANOVA). CoQ10 supplementation did not affect the wire hanging latency of either young adult or middle-aged mice.
Furthermore, we tested the effect of extended CoQ10 supplementation by drinking water for approximately 1 month in middle-aged mice. This longer-term treatment also improved the pole test latency (Fig. 1c; T-turn by 28.62%, p = 0.0002, t (34) = 4.253; T-total by 25.94%, p = 0.0004, t (36.93) = 3.875, Welch's t test), suggesting that the beneficial effect of CoQ10 supplementation is maintained and there is no desensitization during the first month. In addition, there was no significant difference between the wire hanging latency of middle-aged mice with or without CoQ10 supplementation for 1 month (Fig. 1d; p = 0.6387, t (31.63) = 0.4741, Welch's t test). These results suggest no correlation between muscle strength and the improved motor function caused by CoQ10 supplementation.
CoQ10 supplementation improved brain mitochondrial respiration in middle-aged mice
A previous study tested the effect of water-soluble nanoformula-type CoQ10 on motor and brain mitochondrial functions in different sets of animals and did not confirm them concurrently in the same animal1. In the current study, water-soluble nanoformula-type CoQ10 was administered to middle-aged mice for more than 1 month, and behavioral tests and measurements of brain mitochondrial function were performed in the same animals. A brain mitochondrial fraction was purified to measure the NADH-dependent (complex I-mediated) mitochondrial oxygen consumption rate (OCR). The brain mitochondrial OCR increased significantly in the CoQ10-supplemented middle-aged mice compared to that of the age-matched non-drug controls (Fig. 2; p = 0.0459, t (22.23) = 2.115, Welch's t test). These results suggested that brain mitochondrial function and motor function were concurrently restored in middle-aged mice supplemented with CoQ10 by drinking water.
CoQ10 supplementation restored motor cortex neuronal activity
CoQ10 supplementation improved the motor function of middle-aged mice without enhancing muscle strength. Therefore, we investigated whether water-soluble nanoformula-type CoQ10 (Aqua Q10L10-NF) supplementation affects neuronal activity in the motor cortex. Synaptic mitochondria in the brain show age-related functional decline9,10. Brain mitochondrial activity is critical for maintaining normal synaptic function21.
The motor cortex is anatomically and functionally divided into the primary motor (M1) and the secondary motor (M2) cortices. In this study, we analyzed the two motor regions separately. We prepared cortical slices, stimulated layers II/III, and recorded the responses from layer V neurons to analyze the major intralaminar excitatory connection between layers II/III and V in the motor cortex22,23,24,25,26,27,28. fEPSP amplitudes were significantly reduced on average by 35.30 ± 1.85% in the M1 region of middle-aged mice compared to young adult mice in the tested range of 20–80 μA current stimuli (Fig. 3a left). The field excitatory postsynaptic potential (fEPSP) amplitude of young adult mice and middle-aged mice, both without CoQ10 supplementation, showed no interaction but a significant effect of age by two-way repeated-measures ANOVA (Fig. 3a left; the interaction between stimulus intensity and age p = 0.2778, F (6, 246) = 1.257; the main effect of age p = 0.0231, F (1, 41) = 5.572). These results suggested that physiological aging altered neuronal activity in the connection between layers II/III and V in the motor cortex. However, there was no significant interaction or main effect of age by two-way repeated-measures ANOVA in the fEPSP amplitude in the M2 region between young adult and middle-aged mice (Fig. 3a right; the interaction between stimulus intensity and age p = 0.0941, F (6, 198) = 1.835; the main effect of age p = 0.1107, F (1, 33) = 2.687, two-way repeated-measures ANOVA). These results suggest an age-dependent decline in neuronal activity in a motor cortex region-specific manner.
Next, we tested whether CoQ10 supplementation affects the age-related decline in fEPSP amplitude in middle-aged mice. Cortical slices were prepared from the brains of middle-aged mice supplemented with CoQ10 for 1 week and compared to those of age-matched controls without CoQ10 supplementation. fEPSP amplitudes were significantly increased on average by 61.51 ± 1.12% in the M1 region of CoQ10-supplemented middle-aged mice compared to middle-aged control mice in the range of 50–80 μA current stimuli (Fig. 3a left; Middle-aged compared to Middle-aged CoQ10, 50–80 μA: p = 0.0076–0.0464, Bonferroni's multiple comparison test). The fEPSP amplitude in the layer V of M1 region of the CoQ10-supplemented middle-aged mice and that of the age-matched controls showed a significant interaction and a significant difference between mice with and without CoQ10 supplementation (Fig. 3b left; the interaction between stimulus intensity and supplementation p < 0.0001, F (6, 228) = 5.064; the main effect of supplementation p = 0.0127, F (1, 38) = 6.843, two-way repeated-measures ANOVA). On the other hand, there was no significant interaction or difference in the fEPSP amplitude in the layer V of M2 region between mice with and without CoQ10 supplementation (Fig. 3b right; the interaction between stimulus intensity and supplementation p = 0.9032, F (6, 240) = 0.3607; the main effect of supplementation p = 0.9095, F (1, 40) = 0.0131, two-way repeated-measures ANOVA). In summary, the connection between layers II/III and layer V in the mouse motor cortex showed an age-related decline in fEPSP amplitude in the layer V of M1 region, which was restored by CoQ10 supplementation by drinking water for 1 week. There was no significant interaction or difference in the fEPSP amplitude in the layer V of M1 region between young adult mice without CoQ10 supplementation and middle-aged mice with CoQ10 supplementation (Data shown in Fig. 3a left and 3b left; the interaction between stimulus intensity and age p = 0.5174, F (6, 138) = 0.8719; the main effect of age p = 0.8316, F (1, 23) = 0.0463, two-way repeated-measures ANOVA).
CoQ10 supplementation did not affect short-term plasticity in the motor cortex
We assessed short-term synaptic plasticity of the major intralaminar excitatory connection from layers II/III to layer V in the motor cortex22,28 using cortical slices and measuring paired-pulse ratios (PPRs) following paired stimulation at 25- to 500-ms intervals. There was no significant interaction or main effect of age group and stimulus interval on PPRs in the M1 region (Fig. 4a left; the interaction between interval and age p = 0.8607, F (4, 156) = 0.3252; the main effect of age p = 0.7295, F (1, 39) = 0.1213, two-way repeated-measures ANOVA). In the M2 region, there was a significant interaction between age group and stimulus interval but there was not a significant main effect of age, and Bonferroni's multiple comparison showed no significant differences in PPRs between young adult and middle-aged mice among all stimulus intervals (Fig. 4a right; the interaction between interval and age p = 0.0293, F (4, 124) = 2.790; the main effect of age p = 0.4784, F (1, 31) = 0.5150, two-way repeated-measures ANOVA). In addition, there were no significant interactions or differences in PPRs in the M1 and M2 regions of middle-aged mice with and without CoQ10 supplementation for 1 week (Fig. 4b; M1, the interaction between interval and supplementation p = 0.6793, F (4, 132) = 0.5777; the main effect of supplementation p = 0.7833, F (1, 33) = 0.0769; M2, the interaction between interval and supplementation p = 0.1694, F (4, 136) = 1.633; the main effect of supplementation p = 0.1640, F (1, 34) = 2.023, two-way repeated-measures ANOVA). These results suggested that physiological aging and CoQ10 supplementation did not affect the short-term plasticity of the layers II/III to V connection in the motor cortex in these preparations.
Acute CoQ10 treatment induced NMDA receptor-dependent LTP
Mitochondria have effects on age-related synaptic plasticity29. Therefore, we studied the involvement of plasticity enhancement as a mechanism that augmented the fEPSP amplitude in the motor cortex of CoQ10-supplemented middle-aged mice. A larger fEPSP amplitude is recorded after long-term potentiation (LTP) induction30,31, and LTP can be induced in the motor cortex by motor-skill learning or several induction methods30,32. Furthermore, a larger fEPSP amplitude can be retained for months in the motor cortex after motor-skill learning33.
We tested whether acute CoQ10 administration (50 μM) to brain slices could enhance fEPSP amplitude in the connection between layers II/III and layer V in the motor cortex. Figure 5a shows normalized fEPSP amplitudes in the presence of CoQ10 and during CoQ10 washout. Acute CoQ10 administration alone did not augment fEPSP amplitude in the layer V of M1 region after the treatment (Fig. 5a; middle-aged without stimulation, averaged fEPSP, between − 2 and 0 min and 25–27 min p = 0.5931, t (4) = 0.5799, paired t test). The combination of CoQ10 administration (50 μM, 20–25 min before and during LTP induction) and high-frequency stimulation induced an LTP of 122.39 ± 7.15% of baseline in middle-aged mice (Fig. 5a; middle-aged with stimulation, averaged fEPSP, between − 2 and 0 min and 25–27 min p = 0.0061, t (17) = 3.133, paired t test). The mean normalized fEPSP amplitude at 25–27 min after CoQ10 administration was significantly higher with high-frequency stimulation than without stimulation (Fig. 5b, without stimulation, n = 5; with stimulation, n = 18; p = 0.0107, t (19.67) = 2.819, Welch's t test).
Next, we evaluated the magnitude of LTP in slices taken from young adult and middle-aged mice by measuring changes in normalized fEPSP amplitude before and after LTP induction with high-frequency stimulation with and without acute CoQ10 administration. High-frequency stimulation with acute CoQ10 administration induced LTP in slices of young adult and middle-aged mice (Fig. 5c; CoQ10: young adult, p = 0.0051, t (18) = 3.187; middle-aged, p = 0.0061, t (17) = 3.133, paired t test). The high-frequency stimulation without CoQ10 administration induced LTP in slices of young adult and middle-aged mice similarly (Fig. 5d; Control, young adult: 108.1 ± 1.98% of baseline, p = 0.0006, t (19) = 4.092; Middle-aged: 108.03 ± 1.35% of baseline, p < 0.0001, t (15) = 5.962, paired t test). The fEPSP amplitude in slices of young adult and middle-aged mice after LTP induction with or without acute CoQ10 administration showed a significant interaction and a significant difference of age by two-way ANOVA. The magnitude of LTP was significantly greater in CoQ10-treated slices of middle-aged mice than CoQ10-treated slices of young adult mice (Fig. 5d; the interaction between treatment and age p = 0.0355, F (1, 69) = 4.598; the main effect of treatment p = 0.0371, F (1, 69) = 4.519, two-way ANOVA; young adult CoQ10 compared to middle-aged CoQ10, p = 0.0195, Bonferroni’s multiple comparison test). These results suggested that exogenous CoQ10 and increased neuronal activity enhanced the synaptic plasticity efficacy of middle-aged mice.
An age-related increase in NMDA receptor-dependent LTP has been observed in rat hippocampal slices34. Therefore, the NMDA receptor selective antagonist 2-amino-5-phosphonovaleric acid (APV) was applied with CoQ10 during LTP induction in the motor cortex to examine the role of NMDA receptors in the age-related LTP induction described in Fig. 5. The high-frequency stimulation in the presence of CoQ10 (50 μM, 23–25 min before and during LTP induction) induced an LTP of on average 110.88 ± 1.77% of baseline in the M1 region of middle-aged mice (Fig. 6a, CoQ10; averaged fEPSP, between − 2 to 0 min and 58 to 60 min p = 0.0001, t (10) = 6.139, paired t test). However, the high-frequency stimulation in the presence of CoQ10 and APV (each 50 μM, 23–25 min before and during LTP induction) failed to induce LTP in slices taken from the same mice (Fig. 6a, CoQ10 + APV: 102.94 ± 2.65% of baseline; averaged fEPSP, between − 2 to 0 min and 58 to 60 min p = 0.2924, t (10) = 1.111, paired t test). APV significantly blocked CoQ10-dependent LTP induction to a level similar to that of the control (Fig. 6b; p = 0.0167, F (2, 30) = 4.703, one-way ANOVA; control compared to CoQ10, p = 0.0343; CoQ10 compared to CoQ10 + APV, p = 0.0414, Bonferroni's multiple comparison test). These results suggested that CoQ10-dependent LTP of the M1 region in middle-aged mice was dependent on NMDA receptors.
Acute CoQ10 treatment augmented basal fEPSP amplitude
We hypothesized that CoQ10-dependent LTP might be part of the mechanism augmenting the basal fEPSP amplitude in middle-aged mice supplemented with CoQ10 by drinking water. Figure 6c shows the average amplitude of fEPSPs recorded from 5 trials of each current stimulus in 1 brain slice before the LTP experiment and 1 h after the high-frequency stimulation shown in Fig. 6a, b. In the control condition, there was no significant main effect between the fEPSP amplitudes before/after the high-frequency stimulation, but there was a significant interaction between the fEPSP amplitudes before/after stimulation and the stimulus intensity (the interaction between the fEPSP amplitudes before/after stimulation and the stimulus intensity p < 0.0001, F (8, 80) = 5.145; the main effect of the fEPSP amplitudes before/after stimulation p = 0.4513, F (1, 10) = 0.6145, the main effect of the stimulus intensity p < 0.0001, F (8, 80) = 102.2; two-way repeated-measures ANOVA). Bonferroni's multiple comparison showed significant differences between the fEPSP amplitudes before/after the high-frequency stimulation among stimulus intensities between 60 and 90 μA (Fig. 6c left; Before compared to After, 60–90 μA: p = 0.001 to 0.0279). However, when CoQ10-dependent LTP expression was observed, there was a significant interaction between the fEPSP amplitudes before/after stimulation and the stimulus intensity and a significant difference between the fEPSP amplitudes before/after stimulation. The fEPSP amplitudes increased significantly at an average of 115.95 ± 1.61% between the two recording time points (Fig. 6c center; the interaction between the fEPSP amplitudes before/after stimulation and the stimulus intensity p = 0.0067, F (8, 80) = 2.912; the main effect of the fEPSP amplitudes before/after stimulation p = 0.0031, F (1, 10) = 14.92, two-way repeated-measures ANOVA; Before compared to After, 10–90 μA: p < 0.0001 to p = 0.0031, Bonferroni's multiple comparison test). In contrast, when coadministration of CoQ10 and APV occluded LTP expression, there was a significant interaction between the fEPSP amplitudes before/after stimulation and the stimulus intensity by two-way repeated-measures ANOVA and a significant difference between the fEPSP amplitudes before/after stimulation. The fEPSP amplitudes were significantly smaller among 20–50 μA stimuli (Fig. 6c right; the interaction between the fEPSP amplitudes before/after stimulation and the stimulus intensity p = 0.0057, F (8, 80) = 2.980; the main effect of fEPSP amplitudes before/after stimulation p = 0.0076, F (1, 10) = 11.09, the main effect of the stimulus intensity p < 0.0001, F (8, 80) = 88.42; two-way repeated-measures ANOVA; Before compared to After, 20–50 μA: p = 0.0001 to 0.0359, Bonferroni's multiple comparison test). These results suggested that basal fEPSP amplitudes were augmented when LTP expression was observed; therefore, CoQ10-dependent LTP may have improved the fEPSP amplitudes of the M1 region motor cortex of the CoQ10-supplemented middle-aged mice.
Discussion
The middle-aged mice showed an age-related decline in motor function (Fig. 1a, c). Concomitantly, the M1 region of the middle-aged mice showed an age-related decline in fEPSP amplitude in the pathway from layers II/III to layer V neurons (Fig. 3a). The decreased motor function and fEPSP amplitude were reverted to the young adult level by supplementing CoQ10 by drinking water for 1 week (Figs. 1a, 3b). Furthermore, acute CoQ10 treatment of brain slices induced LTP in the layer V of M1 region of middle-aged mice (Fig. 5a, c). This LTP induction depended on exogenous CoQ10, high-frequency stimulation, and NMDA receptors; however, acute CoQ10 administration alone did not alter the fEPSP amplitude (Fig. 5a). Coadministration of CoQ10 and APV reduced basal synaptic transmission (Fig. 6c, right), which also indicates the contribution of NMDA receptors in the pathway from layers II/III to layer V neurons at LTP induction. These results suggested that a change in the efficacy of plasticity may be the underlying mechanism for the fEPSP amplitude recovery by CoQ10 treatment. Indeed, we demonstrated that CoQ10-dependent LTP in the layer V of M1 region translates to enhanced fEPSP amplitude (Fig. 6c). To our knowledge, this report is the first to demonstrate that the pathway from layers II/III to V of the M1 region shows (a) an age-related decrease in fEPSP amplitude and (b) LTP in middle-aged mice. We identified an age-related alteration and CoQ10 and NMDA receptor dependency of LTP induction in the M1 region.
The efficacy of CoQ10 depends on its formulation35. Nanoformulations of CoQ10 have higher bioavailability than regular CoQ10 and have been reported to increase brain CoQ10 content and protect neurons by oral administration7,36. A previous study by Takahashi et al.1 used the water-soluble nanoformula product of Nisshin Pharma (Aqua Q10L10). To test whether the beneficial effect of CoQ10 supplementation could be generalized, we used a water-soluble nanoformula-type CoQ10 from Petroeuroasia (40SP) in the behavioral and OCR analyses of this study. CoQ10 (40SP) showed a beneficial effect on motor function and the oxygen consumption rate of brain mitochondria in middle-aged mice, similar to Aqua Q10L10. These results demonstrated that the beneficial effect of CoQ10 supplementation could be confirmed in water-soluble nanoformula-type CoQ10 from at least two different sources and suggested that the beneficial effect of CoQ10 could be generalized.
Elderly individuals suffer a progressive loss of muscle mass and strength (sarcopenia) and motor function37,38,39,40,41. However, the motor deficit in middle-aged mice is less likely to be due to motor neuron loss, NMJ denervation, or muscle atrophy. NMJ denervation is not detected significantly at or earlier than 18 months of age in mice42,43. Similarly, the maintenance of NMJ number suggests that spinal motor neurons are preserved in middle-aged mice44. A decline in muscle contractility is less prominent earlier than 20 months of age in mice44, and we also confirmed that muscle strength did not change significantly with CoQ10 supplementation (Fig. 1b, d).
Age-related changes in electrophysiological activity in layer V have been linked to motor function deficits in humans and animals. Middle-aged humans (between the late 50 s and early 60 s) showed more intracortical inhibition and less intracortical facilitation in the motor cortex than young adults when examined using transcranial magnetic stimulation45. Elderly individuals in their 70 s exhibited similar but more profound intracortical inhibition and less intracortical facilitation46. These data suggested an age-related decline in neuronal activity in the motor cortex of humans due to an altered balance of excitatory and inhibitory circuits. The correlation of hypoexcitability in the motor cortex and behavioral defects has also been implicated in chronic obstructive pulmonary disease (COPD) and amyotrophic lateral sclerosis (ALS) patients 47,48. In contrast, motor function improved when the activity of motor cortex layer V neurons was increased using optogenetic stimulation in Parkinson's disease model mice49. Layer V pyramidal neurons directly evoke or control the rhythm of whisker movements in rodents50. These observations suggest that the excitability level of layer V neurons of the motor cortex is important to maintain motor functions.
Neuronal plasticity enhancers augment motor-skill learning or accelerate rehabilitation after brain damage51,52. In the rat motor cortex, the LTP-like plasticity of M1 region augments motor-skill learning and rehabilitation effects53. LTP can be induced in the motor cortex by motor-skill learning32,33, and a larger fEPSP amplitude can be stabilized for months in the motor cortex after motor-skill learning33. LTP is also naturally induced by the environment or sensory stimuli. Enriched environmental exposure changed cellular excitability and synaptic transmission, induced NMDA-dependent LTP54,55 and enhanced learning56. Sensory stimulation, such as rhythmic stimulation of whiskers, also induced NMDA-dependent LTP57,58. An age-related increase in NMDA receptor-dependent LTP has been observed in rat hippocampal slices34. These types of LTP may have been induced in the middle-aged mice supplemented with CoQ10 by drinking water and contributed to recovering fEPSP amplitude and motor function.
CoQ10 supplementation by drinking water in middle-aged mice enhanced complex I activity in the brain mitochondria (Fig. 2). Considering that oxidative phosphorylation is associated with oxidative stress59,60, CoQ10 supplementation might induce higher oxidative stress, and excessive oxidative stress impairs cognitive function61,62. However, CoQ10 supplementation by drinking water reduces oxidative stress and improves cognitive function63. Furthermore, exogenous CoQ10 administration is protective against age-related and pathological oxidative stress64,65. Therefore, the antioxidant status in the brain of the CoQ10-supplemented middle-aged mice may be beneficial overall for the behavioral outcome of these mice in the current study.
CoQ10 supplementation had a beneficial effect on the motor function of the middle-aged mice and rescued their behavior to the young adult level (Fig. 1a). The beneficial effect of CoQ10 was partially achieved by enhancing the excitability level of layer V neurons in the M1 region. We hypothesized that the basal fEPSP amplitude level was enhanced in the middle-aged mice during CoQ10 supplementation (Fig. 3) by the continuation and retention of LTP-like plasticity33,66, such as CoQ10-dependent LTP (Figs. 5, 6). The enhanced LTP induction efficacy augments the rehabilitation-like effect to improve the pole test latency (Fig. 1a, b). These effects might be similar to the recovery of motor function after stroke and nervous system damage by rehabilitation training, which makes use of the plasticity and recovery function of the central nervous system. Therefore, these results suggest the possibility of translational application of CoQ10 supplementation in the following circumstances: (1) oral CoQ10 administration as preventive care for age-related motor decline and (2) the enhancement of plasticity of the primary motor cortex to improve motor function in elderly individuals.
Methods
Animals
All experimental procedures were approved by the Animal Care and Use Committee of the Tokyo Metropolitan Institute for Geriatrics and Gerontology. All experiments were carried out in accordance with the approved animal care and use protocol and the Guidelines for Care and Use of Laboratory Animals. The authors complied with the ARRIVE 2.0 guidelines67,68. C57BL/6NCr male mice were purchased from Japan SLC Inc. (Shizuoka, Japan) at 4 weeks old. The mice were housed in groups of two to five per cage and maintained in a temperature- and humidity-controlled environment with a 12-h light/dark cycle. We used a total of 56 young adult mice (6–8 months old) and 86 middle-aged mice (15–18 months old) given ad libitum food and water. For details of animal numbers, see Supplementary Table 1.
CoQ10-supplemented mouse experiments
CoQ10-supplemented mice were analyzed by behavioral experiments, measurement of brain mitochondrial respiration, and electrophysiological recording with a multi-electrode array. Drinking water containing 150 μM water-soluble nanoformula-type CoQ10 (Figs. 1, 2, Coenzyme Q10 40% Water-dispersive Powder 40SP, Petroeuroasia Co. Ltd., Shizuoka, Japan; Figs. 3, 4, Aqua Q10L10-NF, Nisshin Pharma Inc., Tokyo, Japan) were prepared in light-protected bottles twice weekly and given ad libitum to mice until sacrifice based on the preceding studies1,17. An overview of the mouse experiments is shown in Fig. 7.
Behavioral experiments
We performed a priori power analysis using G-Power software69 to estimate the required sample size for behavioral experiments. The experiments aimed to analyze the effects of aging and CoQ10 supplementation with 95% actual power using a two-way analysis of variance (ANOVA) with four groups, a significance level of p < 0.05 and an effect size of f = 0.4. The required total sample size was 84 mice, 21 mice per group. We decided to use 20 mice in each group and house five mice per cage for social housing. The middle-aged mouse group had one less data point due to death (Fig. 1c, d). Mice were handled by the experimenter for three consecutive days for habituation and then sequentially tested on the wire hanging and pole tests. The behavior tests were performed by personnel blinded to the treatment group and the animals were randomized.
Wire hanging test
The four-limb wire hanging test (O'Hara & Co., Ltd., Tokyo, Japan) was performed as described previously70. The latency to fall from the grid was recorded from two trials with a 30 min intertrial interval. The longer latency was considered the representative value for the mice.
Pole test
The pole test was first designed to evaluate bradykinesia in a Parkinson's disease murine model and has been used to measure motor coordination deficits18,19,20. Initially, mice were habituated to an experimental cage and the pole (length 45 cm, diameter 1 cm). The day before the test, four training trials were conducted. During the test, the time required for mice to turn their body and feet completely downward (T-turn) and the total time to descend to the floor of the experimental cage (T-total) were measured with 15 min intertrial intervals. The average of five test trials was used as the representative value.
Measurement of mitochondrial respiration
After the behavioral experiments (16 months old; control, n = 20; CoQ10, n = 19), mitochondrial fractions from one brain hemisphere were isolated as previously described17. We measured NADH-linked (Complex I) respiration of brain mitochondrial fractions, which declined with age1. The OCRs of mitochondrial fractions in mitochondrial respiration medium (MiR05; 0.5 mM EGTA, 3 mM MgCl2, 60 mM lactobionic acid, 20 mM taurine, 10 mM KH2PO4, 20 mM HEPES, 110 mM D-sucrose, 1 g/l bovine serum albumin; pH 7.1) containing 10 mM cytochrome c were determined at 37 °C using high-resolution respirometry (Oxygraph-2k; Oroboros Instruments, Innsbruck, Austria). NADH-linked respiration was assessed by adding 2.5 mM ADP in the presence of 5 mM malate and 10 mM glutamate, as previously described17,71. The data were normalized to total protein of the mitochondrial fraction in the high-resolution respirometry chamber (1.23–2.00 mg of protein). The respiration rates were analyzed by pairing the control and CoQ10-supplemented groups in each measurement by personnel blinded to the treatment group. Three samples in the control group were not measurable due to insufficient sample volume caused by a human error. Two samples in the CoQ10 group were not measurable due to an equipment failure of the Oxygraph-2k.
Brain slice preparation for electrophysiology
Mouse brains were cut at a 15°–20° angle inclined rostrally against the coronal plane of the cortex yielding slices with apical dendrites of layer V neurons parallel to the cut surface22. Brains were cut into 300 μm thick slices using a Pro 7 Linear Microslicer (Dosaka, Kyoto, Japan) in chilled artificial cerebrospinal fluid (ACSF, 124 mM NaCl, 3 mM KCl, 1 mM NaH2PO4, 1.2 mM MgCl2, 2.4 mM CaCl2, and 10 mM glucose) with 26 mM NaHCO3 bubbled with 95% O2 and 5% CO2 for oxygenation and pH adjustment to pH 7.4. The slices were incubated in 30 °C ACSF for 1 h for recovery and then maintained in room temperature (23–25 °C) ACSF until recordings. We selected a small but empirically adequate sample size for all electrophysiological experiments because this was the first evaluation.
Multi-electrode array recording
We separately analyzed the primary motor (M1) and secondary motor (M2) cortices in the motor cortex (approximately + 0.8 to + 1.2 mm from bregma based on the mouse brain atlas by Paxinos and Franklin72). Evoked field excitatory postsynaptic potentials (fEPSPs) were recorded with a multi-electrode array (60pMEA200/30iR-Ti; Multi Channel Systems, Reutlingen, Germany) at room temperature by placing the multiple electrodes in the layer V of M1 or M2 regions. A stimulating glass electrode filled with 1 M NaCl (resistance < 1 MΩ) was placed in layers II/III of the motor cortex. Signals were sampled at room temperature at 50 kHz using a multi-electrode array 1060 amplifier with a band pass filter (3 kHz) (Multi Channel Systems), digitized with a Digidata 1440 series acquisition interface (Molecular Devices, San Jose, USA), and analyzed with pCLAMP10 software (Molecular Devices). Among the electrodes in layer V, we analyzed data from one electrode that recorded the largest fEPSP amplitude at 80 µA current stimuli. A paired-pulse ratio (PPR) was calculated as the ratio of fEPSPs (second amplitude/first amplitude) recorded during paired stimulation (60 μA) in 25- to 500-ms intervals. At the end of the recordings, an AMPA and kainate receptor antagonist, 6-cyano-7-nitroquinoxa-line-2,3-dione (CNQX, 10 μM), and an NMDA receptor antagonist, 2-amino-5-phosphonovaleric acid (APV, 25 μM), were bath-applied to block synaptic transmission and to confirm the disappearance of fEPSPs (data not shown). We used a total of 20 mice (young adult: n = 5; middle-aged control: n = 10; middle-aged supplemented with CoQ10: n = 5). The recordings were performed on brain slices in randomized order.
Single glass electrode recording
Evoked fEPSPs were recorded at 30 °C with a borosilicate glass electrode (3.0–4.5 MΩ resistance) filled with ACSF and placed in the layer V of M1 region. A stimulating glass electrode filled with 1 M NaCl was placed in layers II/III of the M1 region in the radial direction from the recording electrode. Signals were sampled at 10 kHz and filtered at 1 kHz using an EPC 10 amplifier (HEKA Elektronik, Lambrecht/Pfalz, Germany) and analyzed offline with FITMASTER software (version 2 × 90.2, HEKA Elektronik). Baseline fEPSPs were evoked with short pulses (100 μs at 0.067 Hz) and recorded for at least 10 min preceding CoQ10 administration. The stimulus intensity was adjusted to a level where 65–80% of the maximal fEPSP amplitude was evoked. We used slices prepared from the same animals and recorded using alternating stimulus and pharmacological treatments on the same day. The experiment was discarded if the baseline variation was greater than 10% in the first 20 min of recording. LTP was induced with three trains of high-frequency stimulation consisting of 100 pulses at 100 Hz applied at 15-s intervals. The magnitude of LTP was expressed as the % change in the average fEPSP amplitude obtained from 25 to 27 min (Fig. 5) or 58 to 60 min (Fig. 6) after LTP induction to the average amplitude of baseline fEPSP measured during the 2 min before the high-frequency stimulation. We used a total of 26 mice (young adult: n = 11; middle-aged: n = 15) in Fig. 5.
For the APV experiments, water-soluble nanoformula-type CoQ10 and APV (each 50 μM) dissolved in ACSF were bath-applied to the chamber from 23 to 25 min before LTP induction and then washed out after high-frequency stimulation. Immediately before and after the LTP experiments, the input‒output relationship was examined by varying the stimulus intensity. Three conditions (ACSF, CoQ10, CoQ10 + APV) were tested in each mouse, and data from mice that showed more than 5% CoQ10-dependent LTP were analyzed (Fig. 6, 11 mice were analyzed among 16 mice tested at 15–18 months old with the same birthdate). The recordings were performed on brain slices prepared from the same animals and treated in randomized order with three experimental conditions.
Drugs
APV was purchased from Tocris Bioscience (Bristol, UK). All other drugs were purchased from Sigma‒Aldrich (St. Louis, USA).
Statistics
Statistical differences of three or more groups were assessed using one-way analysis of variance (ANOVA) or two-way repeated-measures ANOVA with a multiple comparison test with Bonferroni's correction (Prism version 8.4.3, GraphPad Software, La Jolla, USA). Statistical differences between the two groups or conditions were assessed using the two-tailed Welch's t test or paired t test. All values are expressed as the mean ± SEM. Statistical significance was set at p < 0.05. For details of the statistical analyses, see Supplementary Table 2.
Data availability
The datasets generated in this study are available from the corresponding author upon reasonable request.
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Acknowledgements
We thank Nisshin Pharma Inc. and Petroeuroasia Co., Ltd. for providing water-soluble nano-formula type CoQ10. The authors are grateful to Drs. Mayumi Takahashi and Kazuhide Takahashi for their suggestions and preceding studies that lead to this project. We also thank Drs. Shogo Endo and Yasunori Fujita for valuable discussions and MS. Tomoko Arasaki for technical assistance with the experiments. This work was supported by a grant from the Japan Society for the Promotion of Science (19K11407 for RI).
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R.I., M.M., S.Y. designed the experiments; R.I. performed the experiments; R.I., M.M., S.Y., H.N. analyzed the data and prepared the figures; R.I., H.N. wrote the paper. All authors reviewed the manuscript.
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Inoue, R., Miura, M., Yanai, S. et al. Coenzyme Q10 supplementation improves the motor function of middle-aged mice by restoring the neuronal activity of the motor cortex. Sci Rep 13, 4323 (2023). https://doi.org/10.1038/s41598-023-31510-1
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DOI: https://doi.org/10.1038/s41598-023-31510-1
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