Abstract
Thalamocortical activity is known to orchestrate sensory gating and consciousness switching. The precise thalamic regions involved, or the firing patterns related to the unconsciousness remain unclear. Interestingly, the highly-expressed thalamic T-type calcium currents have been considered as a candidate for the ionic mechanism for the generation of thalamo-cortically-driven change in conscious state. Here, we tested the hypothesis that Cav3.1 T-type channels in the mediodorsal thalamic nucleus (MD) might control neuronal firing during unconsciousness using Cav3.1 T-type channel knock-out (KO) and knock-down (KD) mice under natural sleep and ethanol-induced unconsciousness. During natural sleep, the MD neurons in KO mice showed general characteristics of sustained firing across sleep stages. We found that KO and MD-specific KD mice showed enhanced resistance to ethanol. During ethanol-induced unconscious state, wild-type (WT) MD neurons showed a significant reduction in neuronal firing from baseline with increased burst firing, whereas Cav3.1 KO neurons showed well sustained neural firing, within the level of wakefulness, and no burst firing. Further, 20 Hz optogenetic and electrical activation of MD neurons mimicked the ethanol resistance behavior in WT mice. These results suggest that maintaining MD neural firing at a wakeful level is sufficient to induce resistance to ethanol-induced hypnosis in WT mice. This work has important implications for the design of treatments for consciousness disorders using thalamic stimulation of deeper nuclei including the targeting of the mediodorsal thalamic nucleus.
Graphical abstract
Introduction
Drug-induced unconsciousness can be achieved using numerous types of anesthetics with varying modes of action 1,2. Ethanol, one of the most frequently abused drugs in human society, can induce sleep-like loss of consciousness at high doses 3. While possible neuropharmacological and neural correlates of ethanol sedation have been proposed using in vitro and in vivo methods 4–7, recent studies have highlighted the slowing of thalamocortical-driven rhythms as a potent marker of unconsciousness 8,9. However, the region and the mechanism linked to the thalamic modulation during ethanol induced unconsciousness remains poorly understood.
Physiological correlates of thalamocortical rhythmic activities and consciousness state of the brain have been studied extensively10–13. T-type calcium channels are known generators of thalamocortical rhythms, through the modulation of cell excitability and rebound burst firing14,15. During sleep, the transition from wakefulness to unconsciousness is associated with membrane hyperpolarization of thalamic neurons 12,16. Similarly, It has been shown that in ethanol sedation, as in natural sleep or absence seizure, the loss of consciousness is characterized by a switch from tonic to burst firing in thalamic neurons, which involves GABAergic inhibition-driven de-inactivation of Cav3.1 T-type channels resulting in slow oscillatory response of the thalamocortical network 7,17–19. Acute intoxication at high doses of ethanol 20,21 induces both slow oscillations in the delta-theta frequency range and a loss of righting reflex (LORR), a classical proxy to assess the loss of consciousness. It has been shown that mice lacking global or thalamic Cav3.1 showed altered slow oscillations and sleep architecture 22,23; delayed sleep induction under several anesthetics (i.e. isoflurane, halothane, sevoflurane and pentobarbital) 24; and increased resistance to drug-induced absence seizure 13. Notably, the absence or blockade of Cav3.1 resulted in an increased preference for ethanol consumption and novelty-seeking behavior 20,21. In the current studies we investigate the role in brain state modulation of Cav3.1-mediated T-currents during ethanol-induced sleep.
The thalamus is one of the major regions expressing Cav3.1 T-type calcium channels 25 and holds a central role in information-transmission and integration 26. In vitro and in vivo studies using genetically modified mice have revealed that Cav3.1 T-type channels play a key role in the genesis of thalamocortical rhythms, such as 3Hz spike-and-wave discharges (SWD), a signature of absence seizures 13,27 and delta waves 16,28,29. Previous investigations on thalamic control of consciousness revealed that nuclei within the dorsal medial thalamus (dMT) hold an important modulatory function in the interaction of attention and arousal 9,30. Particularly, centromedian (CM) thalamic nucleus, and not ventrobasal nucleus (VB), showed rapid shifts in local field potential (LFP) preceding brain state transitions such as NREM and propofol-induced anesthesia 8. The paraventricular thalamic nucleus (PVN) showed critical involvement in wake/sleep cycle regulation 33. The centrolateral (CL) thalamic nucleus has been implicated in the modulation of arousal, behavior arrest 31, and improvement of level of consciousness during seizures 32. Notably, the direct electrical stimulation of the intralaminar nuclei (ILN) and, in particular CL, promoted hallmarks of arousal and awakening in primate under propofol and ketamine propofol anesthesia. The MD, a sub nucleus of dMT, on the other hand, has only recently been implicated in disorders of consciousness 33 and ketamine/ethanol-induced loss of consciousness34 through the alteration of thalamo-cortical functional connectivity. In anesthetized primate, the stimulation of ILN and MD increased arousal and wakefulness score35. However, several key questions still remain to be answered: 1) Is there a specific role for MD Cav3.1 T-type calcium channels in the control of ethanol-induced loss of consciousness? 2) Whether Cav3.1 T-type calcium channel driven neuronal firing pattern has any role in the control of consciousness?
In this study, we identified that KO and MD specific silencing of Cav3.1 T-type calcium channels result in increased ethanol resistance in mice. Using single unit recordings, we compared MD activity of WT and KO mice while the mice transitioned from conscious to unconscious state and found that the KO mice showed more sustained MD activity whereas the WT mice showed clearly reduced MD activity. Furthermore and consistently with their resistant phenotype, KO mice showed sustained MD firing, well within the wakefulness level, under ethanol consumption. Finally, we demonstrate that both the optogenetic and electrical stimulations in MD, mimicking the sustained firing pattern of knock-out mice, were sufficient to induce the increased ethanol resistance in WT mice. These results reveal a causal control of brain state by MD during ethanol-induced unconsciousness and with an underlying neural mechanism governed by Cav3.1 T-type calcium channels.
Results
To understand the role of T-type Ca2+ channels in modulating the consciousness level, we compared the ethanol resistance between WT and Cav3.1−/− KO littermates. We used the forced walking task (FWT; Fig. 1-A), an analog to the LORR assay, which enables a continuous and high-temporal resolution assessment of the loss of movement 36 (LOM). Moreover, the FWT objectively measures the latency to and duration of the first LOM, but also the total time spent in LOM using automatized analysis of video confirmed by electromyograms (EMGs) or accelerometer recordings (Fig. 1-B and S1; see Methods). The continuously running treadmill (6 cm/s) ensures a normalized behavior within and between animals before injection (i.e., baseline forced walking) and allows for reduced intervention from experimenters for the monitoring of both electrophysiological (Fig. S1, upper panel) and analyzed behavioral (Fig. S1, lower panel).
The lacking Cav3.1 increases ethanol resistance in mice
Mice lacking Cav3.1 exhibited delayed anesthetic induction 13,24 and impairment in maintenance of low conscious level 22,23 as well as increased ethanol preference 21,34. We tested the sensitivity of Cav3.1 null mutant mice for various acute hypnotic doses of ethanol.
We confirmed that the lack of Cav3.1 resulted in a more delayed and fragmented LOM (Fig. 1-C1 and C2), and a reduction in the total time spent in LOM compared to Cav3.1 WT mice (Fig. 1-C3). We observed that Cav3.1 null mutant mice showed increased latency to and decreased duration of the first episode of loss of motion (fLOM) for ethanol injection doses of 2.0, 3.0 and 4.0 g/Kg (Fig. S2). The total time spent in LOM during one hour of recording was also significantly reduced (Fig. S2-A3 and -B3) compared with WT mice. Two-way analysis of variance (ANOVA) showed a significant effect for the main factor genotype and dose for the latency to and duration of fLOM, and total time in LOM (Table S1), indicating a dose dependency in both wild and mutant mice. In particular, an I.P. Injection of 3.0 g/Kg induced a significant difference between wild and mutant mice in latency to (t(16) =-4.1965, p = 0.002; Student t-test) and duration of fLOM (t(16) =2.3908, p = 0.0294; Student t-test), and total time spent in LOM (t(16) =3.9065, p = 0.0012; Student t-test).
These results indicate that ethanol induces a dose-dependent sedative effect on mice and Cav3.1 mutant mice had an increased resistance to ethanol sedation compared to WT mice.
Cav3.1 silencing in the MD, but not VB, increased ethanol resistance in mice
A great majority of Cav3.1 expression is found in the thalamic region 25 and was shown to specifically correlate with the modulation of thalamocortical-related rhythms and stability of sleep level 22,23. To identify a possible role of the thalamic region in ethanol resistance, we knocked down the expression of Cav3.1 in the MD and a ventral basal nucleus (VB) region, two regions possibly involved in a thalamic control of consciousness 33,34,37, using a lentivirus (LV)-mediated short hairpin (shRNA) delivery.
We found that compared to shControl injected mice, shCav3.1 knock-down of MD resulted in an increased latency to (Fig. 2-A1; t(27) = -3.0045, p = 0.0057; Student t-test) and duration of (Fig. 2-A2; t(27) =2.1448, p = 0.0411; Student t-test) fLOM, and total time spent in LOM (Fig. 2-A3; t(27) =2.6641, p = 0.0128, two-tailed test) for 3.0g/Kg I.P. Injection of ethanol. However, we found that compared to shControl-injected mice, Cav3.1 KD of VB did not change the latency to (t(8) =-1.0093 p = 0.3423, two-tailed test), duration of (t(8) =-0.0983, p = 0.9241, two-tailed test) fLOM and total time spent in LOM (t(8) =- 0.6317, p = 0.5452, two-tailed test) for the same 3.0g/Kg I.P. Injection of ethanol (Fig. S3). Representative traces of mice activity showed that mice with Cav3.1 KD in MD (Fig. S4- A) had a more delayed and fragmented early period of LOM compared to MD LV- shControl and VB injected mice, as in mutant mice.
We then characterized the change in Cav3.1 expression following the shControl and shCav3.1 knock-down injections in three test regions MD (left and right), CM (centromedial nucleus) and CL (centrolateral nuclei, left and right side) and a negative control region SMT (submedial thalamic nuclei, left and right side). The average intensity was obtained from two coronal brain slices for each mice used in the experiment (see Methods sections, Cav3.1 Intensity quantification). Our results show that the targeting of the knock-down was very specific to the bilateral MD (p<0.001; Fig. 2D). We noted that the CM (p<0.05) and a marginal unilateral knock-down of the CL were also observed (p<0.01). Notably, we tested the correlation between the level of knock-down in MD and the total time in LOM and observed a significant association (Fig. 2D inset; R = 0.599, p = 0.018). This result highlights that the Cav3.1 knock-down was specific to MD and with an intensity associated with ethanol-induced loss of motion.
During the open field test, Cav3.1 null mutant mice showed significantly increased locomotor activity compared to WT mice as shown by total distance moved (Fig. S4-C; analysis of variance: GROUP F(3) = 8.45, p = 0.0004; Cav3.1+/+ vs Cav3.1-/-: p = 0.0001). The mice with MD-specific Cav3.1 KD, however, did not show any significant difference in total distance moved compared to shControl-injected control mice (MD LV-shControl vs MD LV-shCav3.1: p = 0.868; Holm-Sidak correction), indicating that the ethanol resistance in MD Cav3.1 KD mice was not attributed by hyperlocomotion observed in Cav3.1 KO mice.
Lack of Ca3.1 in MD neurons removes thalamic burst in NREM sleep
Thalamic neurons are known to follow a state-dependent activity 38 ; however, the nature of this state-dependent activity has not been studied for the MD. In order to understand the relationship between MD neuron firing and level of consciousness, we investigated the association between the neural activity in MD and brain states at different levels of consciousness (Fig. 3 and S5).
We observed two major populations of neuronal spike waveform present in MD single unit recordings of Cav3.1 (+/+) mice, also described in previous works 39,40 : 1) a majority of regular spiking (RS) cells characterized by wide spike waveform (36/39 neurons, 92.3%), i.e. spike-to-valley width >250 μsec (Fig. 3B) and high bursting propensity; 2) a minority of narrow spiking (NS; also known as fast spiking) cells showing short spike-to- valley width, i.e. <250 μsec, lower bursting characteristics (Fig. 3 and S6-A3 and -A4) and fast-paced tonic firing (10-50Hz; data not shown). The RS and NS neurons were found in MD of WT and mutant mice; however, MD RS mutant neurons showed an absence of short inter-spike intervals (ISI, i.e. indicative of the absence of burst) in auto cross- correlogram (Fig. S6) and a clear reduction in total bursting represented as bursting index (Fig. 3-B; ratio of spikes count <10 ms and >50 ms based on auto-cross-correlogram). Since RS cells have the profile of the major population of MD, i.e. excitatory neurons, we focused on the analysis of RS neurons mainly in the remainder of this study.
During the deep sleep state non-rapid eye movement (NREM), thalamic neural firing is known to switch from tonic to burst firing 41. We found that a lack of Cav3.1 T-type calcium channels resulted in a near absence of burst (see Methods for definition) in mutant mice (Fig. 3-C1 and C2; 4/44 bursting neurons; Z(77) = 7.20, p < 0.0001, Ranksum test) compared to WT mice (34/34 bursting neurons; 5.76 ± 5.51 burst events/min).
Lack of Ca3.1 reduces neuronal activity across all brain states in MD
In addition, we observed that the mutant mice showed a significant lower total firing rate (main factor group: F(1,186) = 16.5, p = 0.0001; interaction group x brain state: F(3,186) = 4.72, p = 0.0034) and a reduced variability (p <0.0001 for all brain states; Levene’s test) in most brain states compared to the wild type mice, indicating that the lack of Cav3.1 t- type channels results in an overall reduction in neural activity in RS neurons.
RS neurons of MD in Cav3.1 wild type and mutant mice showed a significant change in overall firing across walking, waking (home cage), NREM and REM sleep states as shown by a repeated measure ANOVA (Fig. 3-D; main factor brain state: F(3,186) = 104.96, p <0.0001). In addition, Cav3.1 wild type (R = -0.534, p = 1.6e-10, Spearman ranked correlation) and mutant (R = -0.689, p = 6.8e-20, Spearman ranked correlation) showed a significant negative correlation between neural firing and brain state. Assuming an ordering from higher to lower state of consciousness, these results indicate that MD firing is associated with level of consciousness independently from the Cav3.1 T-type channels in wild type and mutant mice. Importantly, this result indicates that Cav3.1 t-type calcium channels are critical excitatory ion channels that control the overall neural activity along with the brain state. In other words, mutant mice exhibit a less clear distinction in the neural activities associated with wakeful and unconscious states.
Under ethanol, MD neurons lacking Cav3.1 show no burst and a wake state-like neural activity
In order to identify the mechanism linked to Cav3.1 mutant mice ethanol-resistant phenotype, we recorded neural firing of neurons during the FWT and following a hypnotic dose of ethanol (3.0 g/kg, I.P. injection). We focused on the first loss of motion (fLOM) as it is most analogous to the classical LORR and showed the most consistency between animals 36. fLOM also illustrates best the acute effect induced by ethanol before secondary metabolization enters in play.
Under ethanol, we observed that in WT mice a majority of neurons showed burst firing mode (Fig. 4-A1; 20/33 bursting neurons). We found a significant higher burst event rate (Fig. 4-B1; p <0.0001, Ranksum test with Holm-Bonferroni correction) and in the ratio of burst-to-total spike (Fig. 4-B2; p <0.0001, Ranksum test with Holm-Bonferroni correction) comparing walk (awake active) to fLOM (unconscious, unresponsive). Mutant neurons, consistently with NREM data, did not show burst firing during fLOM (0/36 bursting neurons).
Notably, in WT, we observed that ethanol induced a significant decrease in total firing from walking to fLOM states (Fig.4-A1 and -C; p <0.0001, Rank Sum test with Holm- Bonferroni correction) and well below wakefulness level (Home cage awake state). As in sleep, we found that a majority of RS neurons showed decreased tonic firing (total number of spikes) together with an increase in burst firing, indicating a switch in firing mode under ethanol sleep. Interestingly, the mutant mice did not show a significant decrease in total firing (Fig. 4-C; p = 0.130, Ranksum test with Holm-Bonferroni correction) and showed no burst as in sleep.
We quantified the change in activity of individual neurons using Z-score normalized to the home cage wakeful state. Here, we also observed that WT RS neurons showed a significantly reduced Z-score under ethanol fLOM whereas in mutant mice cells did not (Fig. 4-D1; normalized from home cage wake state; t(62) = -5.1400 , p < 0.0001, student t-test). Remarkably, we found that a majority of WT MD neurons (29/31) showed individual significantly decreased Z-scores (Fig. 4-D2; z-threshold defined from a p-value of 0.05). During fLOM, mutant RS neurons subdivided into three populations (Fig. 4-D2) with decreasing (12/33, 36.4%), maintaining (11/33, 30%) and increasing (10/33, 30.3%) activity as measured by the Z-score with respect to wakefulness (i.e. home cage wake state). These results were consistent in individual mice (Fig. S7A) and the distribution of neural population spiking (Fig. S7B), validating that significant drop in neural activity is associated with loss of movement.
Finally, we asked whether the firing modes and properties (tonic firing rate, burst firing rate; see supplementary methods) of single MD neurons would form distinct qualitative representation of “brain stages” using a lowered dimensional UMAP representation (Uniform Manifold Approximation and Projection42 ). We observed that for awake and active (i.e. walk), the brain state representation formed two adjacent clusters that confounded both wild and mutant neurons (Fig. 4E, left panel). The REM and NREM states, the wild type neurons formed 2 additional interconnected clusters, whereas the mutant neurons tend to overlap with the clusters attributed to the “awake” brain state (Fig. 4E, second to left panel). Ethanol induced fLOM, similarly to REM and NREM clusters, was distinct from awake clusters in wild type mice and overlapped with the NREM clusters (Fig. 4E, third to left panel). Here also, mutant MD neurons showed overlap with the awake clusters rather than the “low consciousness” brain states. These results indicate that the firing mode and properties could define a brain state representation that shows distinctions in levels of consciousness. Moreover, the mutant showed a representation of “low consciousness” states overlapping with wild type “awake” states consistent with the hypothesis of resistance to loss of consciousness.
Altogether, these results indicate that, in WT, ethanol induced a strong reduction in neural activity and a switch to bursting firing mode correlated with loss of consciousness. However, under ethanol, MD mutant neurons maintained their activity to a level within home cage wake state without switching to bursting. This indicates that the drop in neural activity under ethanol is modulated by Cav3.1 t-type calcium channels. In its absence, MD mutant neurons display an overall reduced activity in all brain states, however, under ethanol, remain within state wakeful levels.
Under ethanol, 20 Hz neurostimulation of MD induces mutant-like resistance to loss of consciousness in WT mice
We observed that the maintenance of neural activity in MD excitatory neurons might be at the origin of the ethanol resistance in mutant mice. We hypothesized that artificially maintaining MD neural activity within the wakeful level would sustain consciousness under ethanol. In addition, we hypothesized that the triggering of burst firing under ethanol would potentiate loss of consciousness under ethanol. To test this possibility, we used electric and optogenetic stimulations during the FWT in WT mice under a hypnotic dose of ethanol.
MD neurons in WT mice showed a spike firing range 0-50 Hz with an average neural firing around ∼20 Hz during home cage wakefulness (Fig. S7-B). Using the 20 Hz stimulation (Fig. 5-A, inter-pulse interval = 50 msec, pulse width = 6.25 msec) in MD neurons transduced with excitatory channelrhodopsin 43,44 (aav-syn-ChR2-sfGFP; Fig. 5-B and Fig. S9; see Methods), we observed an increase in ethanol resistance, which was demonstrated by a significant increase in latency to fLOM (Fig. 5-D1; Z(13) = -2.372, p = 0.013; Ranksum test). The duration of fLOM (Fig. 5-D2; Z(13) = 2.256, p = 0.020; Ranksum test) and total time spent in LOM (Fig. 5-D3; Z(13) = 2.488, p = 0.009; Ranksum test) were also significantly reduced. We verified that optogenetic stimulation of MD neurons at 20Hz (Fig. S8) induced action potentials at the same frequency with a latency response of about ∼5 ms (Fig. S8-B2; pulse width = 6.25 msec). We also observed that, although marginally higher, optogenetic stimulation did not induce any significant increase in locomotor activity (Fig. S8-C; F(1,12) = 3.6232, p = 0.0812) in the control and stimulated group which indicates that the stimulation-induced increase in ethanol resistance was not due to an increase in locomotor activity.
In order to validate this observation, we then bilaterally implanted mice with twisted wires for bipolar, local electric stimulation of MD (Fig. S11). As in the optogenetics experiment, we used a continuous pulse train of 20Hz electric stimulation (Fig. S10-A; upper panel; inter-pulse interval = 50 msec, pulse width = 1 msec) in addition to a burst-like stimulation (Fig. S10-A; lower pane; 4 pulses at 4 ms interval and interburst interval of 1 sec) that showed, respectively, tonic-like and burst-like entrainment in thalamic neurons 45. We observed that our 20Hz tonic-like stimulation significantly increased the latency to fLOM (Fig. S10-B1; tonic-like vs no stim.: p = 0.008; tonic-like vs burst-like: p = 0.007; Ranksum test with Holm-Bonferroni correction) and significantly decreased the total time spent in LOM (Fig. 5-B3; tonic-like vs no stim.: p = 0.008; tonic-like vs burst-like: p = 0.007, Ranksum test with Holm-Bonferroni correction). No significant changes in the duration of the first LOM were observed (duration of fLOM (Fig. 5-B2; tonic-like vs no stim.: p = 0.917; tonic-like vs burst-like: p = 0.606; Ranksum test with Holm-Bonferroni correction).
Interestingly, we observed that burst-like electrical stimulation (Fig. S10-A; lower panel; inter-spike interval = 4 msec, inter-burst interval = 1 sec, pulse width = 1 msec) did not induce any significant change in ethanol sensitivity compared to the no stimulation group (Latency to fLOM: p = 0.365; duration of fLOM: p = 0.835; total time spent in LOM: p = 1; Ranksum test with Holm-Bonferroni correction). This result suggests that burst firing alone might not have a role in ethanol resistance.
Altogether, these results suggest that the maintenance of MD firing at wakefulness level (20Hz) causally drives resistance to loss of consciousness after a hypnotic dose of ethanol. Burst-like stimulation alone did not promote or reduce loss of consciousness. This result supports the idea that neural activity maintenance in MD promotes the maintenance of consciousness even under heavy sedatives.
Discussion
In this work, we identified that the neural activity in MD plays a causal role in the maintenance of consciousness. Whole body Cav3.1 KO and MD-specific Cav3.1 KD mice showed resistance to loss of consciousness induced by hypnotic dose of ethanol. In WT mice, MD neurons demonstrated a reduced firing rate in natural (sleep) and ethanol- induced unconscious states compared to awake states. This neural activity reduction was impaired in KO mice. In particular, transition to an unconscious state was accompanied with a switch of firing mode from tonic firing to burst firing in WT mice whereas this mode- shift disappeared in KO mice. Finally, optogenetic or electric stimulations of the MD after ethanol injection were sufficient to induce a resistance to loss of motion, supporting that the level of neural firing in the MD is critical to maintain conscious state and delay unconscious state. We showed that the expression of Cav3.1 t-type calcium channels in MD is a cellular modulator associated with this effect.
MD is a modulator of consciousness
The role of mediodorsal (MD) thalamic nucleus in perception, attention 46 and emotional control 45,47 has been the dominant focus thus far. The recent investigations on thalamic control of consciousness revealed that nuclei within dMT holds an important modulatory function in the interaction of attention and arousal 9,30. Particularly, centromedian thalamic nucleus, and not VB, showed rapid shifts in LFP preceding brain state transitions such as NREM and propofol-induced anesthesia 8. The centrolateral thalamic nucleus was implicated in the modulation of arousal and improvement of consciousness during seizure32 and paraventricular thalamic nucleus showed critical involvement in wake/sleep cycle regulation 48 . The mediodorsal thalamic nucleus, however, has rarely been included as a possible pathway in the direct modulation of consciousness 33. The MD receives projections from various parts of the basal forebrain 9 and brainstem nuclei such as the pedunculopontine nucleus that control the ascending pathway of arousal and attention 49. The MD is known to innervate limbic region, basal ganglia and medial prefrontal cortex 50 and increased activity in MD might modulate the stability of cortical UP states (e.g. awaken, aroused and attentive states) and synchronization 9,26. Thus, MD might be a major hub involved in cortical state control and brain state stabilization.
Supporting the brain state stabilization theory and the ethanol resistance of Cav3.1 mutants, Choi et al.34 demonstrated that the loss of Cav3.1 T-type calcium channel reduced the bilateral coherence between PFC and MD under ketamine anesthesia and ethanol hypnosis, especially in the delta frequency bands. More importantly, under propofol anesthesia, Bastos et al.35 showed that intralaminar nucleus and MD stimulation lead to increased wake-up subscore and arousal, together with an increased in cortico- cortico and thalamo-cortical slow (delta) frequency power.
In the present study, we observed that MD KD (Fig. 2A), but not VB KD (Fig. S3) of Cav3.1 increased and is associated (Fig. 2D) with ethanol resistance in mice. We found that MD neurons in Cav3.1 mutant mice exhibited tonic firing within range of wakefulness (Fig. 3 and 4), indicative of resistance to ethanol and wake-like brain state. In addition, we found a strong association between the normalized tonic firing in MD and the arousal through brain states (i.e. walk to wake to sleep states), supporting that MD tonic firing could be interpreted both as a thalamic readout and a modulator of the brain state 11 (Fig. 3). Finally, direct optogenetic and electric MD stimulation increased resistance to loss of consciousness in WT mice (Fig.5 and Fig. S10). To our knowledge, this is the first report demonstrating the causal involvement of mediodorsal thalamic nucleus in the modulation of wakefulness and the resistance to ethanol-induced loss of consciousness in mice.
Cav3.1 T-type calcium channels drive thalamic firing mode and activity
The decrease of absolute firing rate observed in thalamic neurons of Cav3.1 mutant mice supports the polyvalent role of Cav3.1 in controlling both burst and tonic firing in the thalamus. Cav3.1 channels are major contributors of excitability, and in their absence or blockade, leads to a reduced neural excitability and stability and lower tonic relay of thalamocortical cells under wake-like state 51,52. The burst and tonic firing-mediated response of thalamic neurons under sensory stimulation and under the control of thalamocortical layer 6 projecting neurons was found to recruit Cav3.1 t-type calcium channels to differentiate salient novel stimuli versus complex coded information 53. Therefore, the nonlinear amplification and regularization of excitatory postsynaptic potentials (EPSPs) by Cav3.1 T-type calcium channels through complexes such as with metabotropic-glutamatergic receptor 1 (mGluR1) 54 or the role of a “T window” 55 would explain how the lack of T-current in mutant mice could result in an overall reduced excitation of thalamic neurons. Cav3.1 T-type is therefore a major excitatory ion channel of the central thalamic neurons.
The lower variability in MD Firing reflects Ethanol Resistance in Cav3.1 mutant mice
Under acute hypnotic dose of ethanol, two mechanisms might favor the reduction in firing in MD: 1) an increase in synaptic and extra synaptic GABAergic inhibition 17 and/or 2) reduced NMDA synaptic transmission 7. The presence of burst firing during fLOM, and during LOM in general, supports that MD neurons might have been subject to GABA receptor-mediated hyperpolarization, a necessary condition for the de-inactivation of Cav3.1 T-type burst. However, considering the dramatic difference in tonic firing observed during the FWT following I.P. injection of ethanol, the change in tonic firing in MD was the focus of our analysis.
We observed a reduction in neural firing under ethanol sleep conditions in WT mice (Fig. 4-C, -D1 and -D2) suggesting that low firing level should be associated with a state of low consciousness as observed during NREM sleep. Mutant RS neurons in MD showed an overall lower excitability and variability of firing in various natural conscious and unconscious states compared to wild type mice. Remarkably, Cav3.1 mutant mice exhibited a clear increased locomotor activity and an increased resistance to ethanol. The general lower firing rate and the high “arousal” observed in mutant mice suggests that the relative change from state to state in tonic firing in MD, and not the absolute value of firing, might be a better correlate of change in brain state in the mice. Our optogenetic and electrical stimulation showed that a sustained tonic-like stimulation in the MD at 20Hz (Fig. 5-A), a physiological relevant firing rate in wake state (Fig. 4), could increase ethanol resistance in WT mice. Reducing MD firing using phasic inhibition under ethanol, potentially leading to inhibition and rebound burst 56, could also increase the duration of the fLOM in WT mice injected with a lower dose of ethanol (Figure S12; 2.0 g/kg). We propose that the relative change in firing rate in MD RS neurons might be an important driver and indicator of the change of transition in and out of consciousness as demonstrated for other nuclei of the dMT 8,9,32,48. Therefore, the low variability in firing of MD in Cav3.1 mutant mice might be the driving force for the higher resistance to loss of motion under ethanol. In mutants, brain states might be less distinguishable leading to frequent sleep stages switch23 or resistance to unconsciousness34.
Cav3.1 T-type Calcium and Burst during Low Conscious State
Burst, as a result of Cav3.1 T-type calcium channel de-inactivation/activation, is thought to control the gating of sensory-motor stimuli 57,58 and modulate attention towards novel stimuli rather than the transmission of details 53,57,59. Previous reports highlighted the importance of burst in the stabilization of low level of consciousness 13,22,23 suggesting a direct role for burst, while no mention of the importance of tonic firing was made. We found that the propensity for burst during ethanol-induced LOM (Fig. 4-A1, -B1 and -B2; fLOM: 20/33 bursting neurons; 0.79±1.63 Burst event/min) was lower than in NREM (NREM: 34/34 bursting neurons; 5.76 ± 5.51 burst events/min) and higher than during wakefulness (Wake: 5/36 bursting neurons; 0.16±0.31 Burst event/min). In addition, burst-like electrical stimulation of MD did not significantly affect ethanol resistance (Fig. S10). Although burst-like stimulations are highly artificial and do not recruit T-current and associated mechanisms following low-threshold burst, they allow for the reproduction of the influence of TC burst firing on target centers45, including thalamo-cortical and thalamo- thalamic efferents.
Interestingly, under lower doses of ethanol (I.P. injection of 2.0g/kg of ethanol) mutant and WT alike showed similar levels of resistance to ethanol. We observed a phasic inhibition of MD neurons in WT, capable of inducing partial silencing 60 and rebound bursts 61 (Fig. S12; 1sec ON-OFF using archaerhodopsin-mediated inhibition), did increase fLOM duration mostly (Z(13) = -2.214, p = 0.022, Ranksum test). This result supports that in the context of hypnotic dose of ethanol, the apparition of burst might correlate with unconscious state stability rather than induction. Burst stimulation without inhibition did not have this effect (Fig. S10 and S11). Currently, our data does not allow us to formulate any clear conclusion on the direct role of burst events during fLOM. We propose that the absence of burst and an accompanying effect of maintenance of tonic firing under ethanol in MD was responsible for the observed increase in resistance and maintenance of activity in Cav3.1 mutant mice.
A bidirectional modulation of Cav3.1 expression and alcoholism
In human mutation of Cav3.1 T-type channels exhibit mental disorders including cerebellar ataxia, absence seizure, schizophrenia and autism62. Remarkably, mutation in voltage-gated calcium channels, including Cav3.1 leads to ethanol resistance and alcohol- seeking behavior 21. Reversibly, chronic exposure to ethanol intake is known to impair sleep 63 and increase ethanol resistance. Previous studies have found an alteration in T- type calcium channel expression following chronic exposure to ethanol in non-human primates 64 suggesting that a reduced T-current and the resulting sustained thalamic tonic firing could be a possible mechanism for early stage ethanol resistance in alcoholic subjects, which increases the conversion probability from casual to compulsive consumption of ethanol. The lack of burst and sustained tonic firing might impair the stabilization of sleep, and in turn chronic sleep impairments might engage addiction related networks. Mechanisms such as adenosine receptor depreciation 65,66 or GABA- receptor potentiation 18,67,68 would enhance ethanol resistance and addiction 69,70 spiraling into further sleep fragmentation, memory consolidation deficit, impulsivity and other impairments associated with alcoholism.
Acknowledgements
This work was supported by the grant IBS-R001-D1 and IBS-R001-D2 from the Institute for Basic Science, Korea. We would like to thank Dr. Gireesh Gangadharan for his precious help in the editing of this manuscript.
Data Sharing
Part of the analyzed data and codes are available on the open access platform, mendeley:
Latchoumane, Charles-francois (2024), “Mediodorsal thalamic nucleus mediates resistance to ethanol through Cav3.1 T-type Ca2+ regulation of neural activity”, Mendeley Data, V1, doi: 10.17632/7fr427426m.1
Additional data (heavy recording and images) can be provided upon reasonable requests.
Methods
Animals
Cav3.1 heterozygous mice (Cav3.1+/−) were maintained in two genetic backgrounds, 129/svjae and C57BL/6J. All experiments used Cav3.1-/− mice and their WT littermates in the F1 hybrid generated by mating CaV3.1+/− mice from these two genetic backgrounds. Mice were maintained with free access to food and water under a 12-h light/12-h dark cycle, with the light cycle beginning at 8:00 AM. Animal care was provided and all experiments were conducted in accordance with the ethical guidelines of the Institutional Animal Care and Use Committee of the Institute of Basic Science and the Korean Institute of Science and Technology. All experiments were conducted using 12- to 16-wk-old male mice.
Surgery for electrophysiological recordings and neurostimulation
The surgical implantation of electrodes (EEG, EMG and/or tetrode Microdrive) and virus injection procedures were performed under 0.2% tribromoethanol (Avertin) anesthesia (20 mL/kg i.p.). Following anesthetic administration, mice (11-week-old for electrode implantation; 10 weeks for virus injection) were fixed in a stereotaxic device (David Kopf Instruments). For chronic recording of EEG and EMG, a stainless-steel screw electrode was fixed into the skull over the right parietal hemisphere and an uncoated stainless-steel wire was tied to the nuchal muscle, respectively. For in vivo freely moving single unit recording, we used a Harlan 4 Drive (Neuralynx inc.) mounted with 3 to 4 tetrode wires inserted to the caudal region of the right mediodorsal thalamic nucleus (anteroposterior, −1.4; lateral, +0.4; depth: 3.2 mm). Single tetrode wires were prepared from 4 twisted nichrome- formvar/PAC wires (Kanthal precision technology, OD 0.0127 mm) and gold plated to achieve an impedance range of 150-400kΩ (1kHz, in saline solution). A period of 7 days was given to allow a complete recovery from the surgical procedure. For all chronic implantation of electrodes, an additional screw was positioned over the occipital region and used as a reference.
Optogenetic neurostimulation
For optogenetic experiment, 16 mice were bilaterally injected with aav9-syn-ChR2-sfGFP virus in the mediodorsal thalamus and implanted with optic fiber guides (125 μm core diameter, Doric Lenses inc.) positioned at 30 degree angle from the transverse plane. The mice were given 2∼3 weeks to recover and to allow for the viral expression. These mice were then randomly assigned to a no stimulation (n = 8) and a 20 Hz stimulation group (n = 6). The mice received the stimulation immediately after being placed in the treadmill, then received the i.p. injection of 3.0 g/kg of ethanol as in other experiments. We discarded 2 mice due to a low viral expression found after histological analysis.
In order to measure the neural response to optogenetic stimulation, we implanted one mouse unilaterally (right MD) with a Harlan 4 Drive (4 tetrodes) converging with a single optic fiber (right side, 30 deg inclination). This mouse received optogenetic stimulation in a home cage resting condition and at frequency 1-5-10-20-40 Hz with a fixed stimulation pulse of 6.5 ms (Fig. S8). Using these recordings, we verified the fidelity between the triggered laser stimulation and the single unit response in the vicinity of the laser illumination. The spike per stimulation trial, spike initiation success rate and the delayed triggered spiking (jittering) were estimated from these recordings. For all simulations, we used a high stability 473 nm (blue, MFB-III-473-AOM; Changchun New Industries Optoelectronics Technology Co., Ltd.) fiber coupled (FC) at an intensity of 6.0 mW. Laser triggering was performed using a Pulsepal pulse generator (gen1, open-source; https://open-ephys.org/pulsepal) or Master-8 (A.M.P. Instruments, Israel) pulse stimulator. Electric neurostimulation. For experiments using electrical stimulation, 18 mice were implanted with bilateral twisted dual stainless-steel wires (A-M systems, PFA coated, 50 um diameter) targeting MD (anteroposterior, −1.4; lateral, +/-0.4; depth: 3.2 mm; from bregma). The wires were minted on a custom made 4x1 pin header connector and cemented. As in the optogenetic experiment, the mice received the stimulation immediately after being placed in the treadmill, then received the i.p. injection of 3.0 g/kg of ethanol. The mice were randomly distributed into 3 groups, Sham no stimulation (n = 6), 20 Hz tonic stimulation (n = 5; 100 μsec pulse duration with inter pulse interval of 50 msec), and Burst stimulation (n = 7; 4x pulses of 100 μsec duration at 250 Hz; inter burst interval of 1 sec). All stimulation were performed in a bipolar configuration (twisted wire, bilateral implants) and biphasic pulse (100 μA, current stimulation) using a 2100 isolated pulse stimulator (A-M Systems, inc.).
Virus Injection
WT mice (10-week-old) were placed in the stereotaxic device following 0.2% tribomoethanol anesthesia (20 mL/kg i.p.). Custom elongated (Sutter Instrument Co.) borosilicate pipette (ID: 0.05 mm, OD: 0.07mm, World Precision Instruments, inc.) was used to inject 0.2 to 0.5 μL of virus solution at a rate of 0.1μL/min (Hamilton syringe, pump) bilaterally in to the mediodorsal thalamic nuclei (anteroposterior, −1.4; lateral, +/- 0.4; depth: 3.2 mm). The injection pipette was then removed slowly after a diffusion period of 10min. A period of 2 to 3 weeks was given to allow viral infection to settle and a complete recovery from the surgical procedure.
Cav3.1 knock-down virus
For genetic knock-down of Cav3.1 T-type calcium channels in the MD and VB in vivo, we used a lentivirus-mediated knockdown injection43. High-titer, concentrated lentiviral vectors (107 TU/μl) expressing shCav3.1(target sequence: 5’- CGGGAAGATCGTAGATAGCAAA-3’) or control shRNA (non-human or mouse shRNA : 5’-AATCGCATAGCGTATGCCGTT-3’) were prepared.
Channelrhodopsin virus
Channelrhodopsin fused with superfolder GFP (ChR2-sfGFP) was designed and synthesized from published sequences using codon optimization for M. musculus (DNA 2.0). To express ChR2-sfGFP in the mouse brain, the AAV vector under a control of the human Synapsin promoter (aav-Syn) was generated using PCR- amplified human Synapsin promoter. Viruses were produced with Serotype 1 or DJ (Cell Biolabs, Inc.) and purified by CsCl gradients 71. The virus was injected at a volume of 0.5 μL in each side of the MD, followed by a bilateral implantation of optical fibers (100/125 μm, DP, Doric lens). The mice were given a period of 3 weeks to allow a strong expression of the channelrhodopsin channel following viral infection, as well as to recover from the surgical procedures.
Cav3.1 Intensity quantification
For the quantification of Cav3.1 expression in the MD, we defined ROIs centered to the left and right of the MD (2x ROIs), CL/PCN (centrolateral, pericentral nucleus; 2x ROIs), and SMT (submedial thalamic nucleus; 1x ROIs; used as a control region of high Cav3.1 intensity, far from lentivirus injection). We added the CM (centromedial region; 1x ROI central only). All ROIs were predefined using a custom script in FIJI (ImageJ, doi:10.1038/nmeth.2019) and manually rectified to match anatomical position within the nuclei. We then run a custom MATLAB script to estimate the average intensity per area for all ROIs (11 ROIs defined in total per animal for each side, left and right). All intensities were then normalized to the average intensity of the SMT (highest expression region). We then compared the normalized Cav3.1 intensity for each animal for the factors side (left, right) and knock-down conditions (shRNA, shCAv3.1).
Drugs
Tribromoethanol (Avertin) and Ethanol were purchased from Sigma-Aldrich. All drugs were administered by i.p. injection. The surgical implantation and virus injection procedures were performed under 0.2% tribromoethanol (Avertin) anesthesia (20 mL/kg i.p.). Ethanol injections were based from a prepared stock mixture of ethanol (26%) and saline and dosage were adjusted according to the experiments and the animal body weight (i.e. 2.0 g/Kg, 3.0 g/Kg and 4.0 g/Kg).
Statistical Analysis
All statistical analyses were performed using Matlab and SPSS 17.0 (Statistical Package for the Social Sciences). Group differences were assessed using the Student t-test. In the case of low sample number (i.e. n<7) or distribution comparison of non-normal and/or non-equal variance number group difference were additionally confirmed using a nonparametric test (i.e. Wilcoxon Ranksum test/Signrank test). Multiple comparison p-value corrections were performed using a Holm-Bonferroni method. General longitudinal and group difference analysis were performed using repeated measures analysis of variance (ANOVA) and one/two-way ANOVA when advised. Linear correlation was performed using Pearson’s correlation coefficient.
Mouse activity classification
Mouse activity was obtained using a video analysis and alternatively using an accelerometer placed on the head stage of the mouse when video wasn’t available. For video analysis, after histogram filtering of the mouse’s body color, the instantaneous activity was estimated as the frame-by-frame intensity difference followed by a 2D median filtering (3x3 pixel) and summed as the number of displaced pixels on camera. For the accelerometer, a zero-phase 5th order Butterworth band-pass filter with cut off frequency of 0.5-20 Hz was used in order to remove the DC component; the instantaneous activity was derived as the root mean square (RMS) of x-, y- and z-axis filtered signals. The mean and standard deviation of the mean (STD) of the instantaneous activity was estimated in moving windows of 4sec duration (50% overlap).
The normalized activity index was obtained from the product of MEAN x STD (i.e. sustained activity and variability). Normalization was performed so that 1) complete cessation of activity approximate a value of 0 and 2) the 10 min walking baseline prior I.P. injection average a value of 1. A mouse was classified as not walking if its normalized activity was lower than the 95% confidence interval of baseline activity for a duration of at least 60 sec, and classified as walking otherwise. Non-walking states were reclassified as loss of motion (LOM) if the mouse’s normalized activity was maintained below 0.25 (lower quartile) for a duration of at least 30 sec. Adjustments were performed after manual video verification.
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