Abstract
The ventral tegmental area (VTA) contains projection neurons that release the neurotransmitters dopamine, GABA, and/or glutamate from distal synapses. VTA also contains GABA neurons that synapse locally on to VTA dopamine neurons, synapses widely credited to a population of so-called VTA interneurons. Interneurons in cortex, striatum, and elsewhere have well-defined morphological features, physiological properties, and molecular markers, but such features have not been clearly described in VTA. Indeed, there is scant evidence that local and distal synapses originate from separate populations of VTA GABA neurons. In this study we tested whether several markers expressed in non-dopamine VTA neurons are selective markers of interneurons, defined as neurons that synapse locally but not distally. Challenging previous assumptions, we found that VTA neurons genetically defined by expression of parvalbumin, somatostatin, neurotensin, or mu-opioid receptor project to known VTA targets including nucleus accumbens, ventral pallidum, lateral habenula, and prefrontal cortex. Moreover, we provide evidence that VTA GABA and glutamate projection neurons make functional inhibitory or excitatory synapses locally within VTA. These findings suggest that local collaterals of VTA projection neurons could mediate functions prior attributed to VTA interneurons. This study underscores the need for a refined understanding of VTA connectivity to explain how heterogeneous VTA circuits mediate diverse functions related to reward, motivation, or addiction.
Significance statement
GABA neurons in VTA are key regulators of VTA dopamine neurons and considered central to the mechanisms of by which opioids and other drugs of abuse can induce addiction. Conventionally, these VTA GABA neurons are considered interneurons, but GABA projection neurons are also abundant in VTA, and it is unclear if these represent separate populations. We found that several markers enriched in non-dopamine neurons of VTA, including Mu-opioid receptor, are also expressed in projection neurons, and thus are not selective interneuron markers. Moreover, we found that VTA GABA and glutamate projection neurons collateralize within VTA where they make local synapses. These data challenge the notion of a VTA interneuron that synapses only within VTA and suggest that inhibitory projection neurons can serve functions previously attributed to VTA interneurons.
Introduction
The ventral tegmental area (VTA) is a central component of the brain’s reward circuitry, and a common attribute of addictive drugs is their ability to increase dopamine release from VTA projections (Luscher, 2016; Nestler, 2005). The VTA projects to and receives inputs from many brain structures involved in reward-related behavior, including nucleus accumbens (NAc), ventral pallidum (VP), lateral habenula (LHb), and prefrontal cortex (PFC) (Faget et al., 2016; Fields et al., 2007; Morales & Margolis, 2017). The VTA is often simplified as a region containing dopamine (DA) projection neurons and inhibitory GABA ‘interneurons’ that regulate DA neurons (Johnson & North, 1992; Luscher & Malenka, 2011; Nestler, 2005). However, VTA neurons are highly heterogeneous. The VTA contains distinct populations of DA neurons that can be segregated by gene expression, projection target, and function (Azcorra et al., 2023; Poulin et al., 2020; Roeper, 2013). GABA-releasing VTA neurons make local intra-VTA synapses (Bayer & Pickel, 1991; Omelchenko & Sesack, 2009), but also project widely outside the VTA, including dense projections to LHb, VP, and VP-adjacent areas of basal forebrain (Kaufling et al., 2010; Oades & Halliday, 1987; Taylor et al., 2014). Glutamate neurons are also prevalent in VTA and overlap with other populations such that ∼25% of VTA glutamate neurons co-express a DA marker and ∼25% express a GABA marker (Conrad et al., 2024; Ma et al., 2023; Phillips et al., 2022). VTA glutamate neurons release glutamate locally within VTA and from distal axons in medial NAc, PFC, VP, LHb, and elsewhere (Dobi et al., 2010; Gorelova et al., 2012; Hnasko et al., 2012; Root et al., 2014; Taylor et al., 2014; Yamaguchi et al., 2011).
It is now understood that DA signals can induce or correlate with distinct behavioral responses depending on their projection targets (Azcorra et al., 2023; Badrinarayan et al., 2012; de Jong et al., 2019; Faget et al., 2024). This is true also for VTA GABA and glutamate neurons. For example, activating VTA GABA neurons either locally within VTA or from distal processes can drive behavioral avoidance, disrupt reward seeking, or modify opioid reinforcement (Corre et al., 2018; Root et al., 2020; Shields et al., 2021; Soden et al., 2020; Tan et al., 2012; van Zessen et al., 2012; Zhou et al., 2022). On the other hand, stimulation of VTA GABA projections to LHb can be rewarding (Lammel et al., 2015; Stamatakis et al., 2013). Likewise, stimulation of VTA glutamate neurons can drive robust positive reinforcement or behavioral avoidance depending on the projection target and behavioral assay (Root et al., 2018; Root et al., 2014; Wang et al., 2015; Yoo et al., 2016). These responses can depend also on the co-release of distinct transmitters. For example, activation of VTA glutamate projections to NAc drives positive reinforcement through the release of glutamate and avoidance via DA co-release (Warlow et al., 2024; Zell et al., 2020). Thus, VTA neurons can mediate approach or avoidance behaviors through their specific connectivity and neurotransmitter content, and understanding the circuit mechanisms regulating activity in diverse VTA cell types is crucial to understanding the mechanisms by which mesolimbic circuits control motivated behaviors.
Local intra-VTA GABA modulation of VTA output, particularly DA output, may underlie key aspects of behavioral reinforcement. For example, inhibitory inputs to VTA from lateral hypothalamus, bed nucleus of stria terminalis, or VP can drive positive reinforcement and approach behaviors through inhibition of VTA GABA neurons and disinhibition of VTA DA neurons (Faget et al., 2024; Nieh et al., 2015; Soden et al., 2020; Soden et al., 2023). VTA GABA circuits also appear to be critical for the generation of DA reward prediction error signals (Eshel et al., 2015; Keiflin & Janak, 2015). Moreover, drugs of abuse can induce rapid or plastic changes in DA signaling through mechanisms that depend on intra-VTA GABA transmission (Corre et al., 2018; Gomez et al., 2019; Luscher & Malenka, 2011; Ostroumov & Dani, 2018; Ting & van der Kooy, 2012). Indeed, the observation that Mu-opioid receptor agonists directly inhibit non-DA VTA neurons and produce disinhibitory effects on VTA DA neurons (Johnson & North, 1992) helped establish the notion of VTA interneurons into current models of VTA architecture.
Yet there is scant evidence for the existence of VTA GABA interneurons, defined as neurons that make synapses locally within VTA but that do not make distal connections. Interneurons as so defined in cortex, striatum and other brain regions have characteristic morphological features, physiological properties, and molecular markers (Markram et al., 2004; Pelkey et al., 2017; Tepper et al., 2010). However, no molecular or physiological feature has been described that can clearly distinguish VTA GABA interneurons from GABA projection neurons. Identifying a marker that selectively labels VTA interneurons would enable investigations into distinct roles for VTA interneurons and projection neurons (Bouarab et al., 2019; Paul et al., 2019).
In this study we first sought to test whether several genes that are expressed in a subset of VTA neurons may be selective for interneurons in VTA. We chose markers that are expressed in non-DA neurons, selectively label interneurons in other brain areas, and/or have been widely presumed to label VTA interneurons. We found that these markers labeled neurons that were primarily non-DA neurons, but that made projections to distinct VTA projection targets, and thus did not selectively label VTA interneurons. We thus sought to test the hypothesis that VTA GABA (or glutamate) projection neurons make intra-VTA collaterals. Indeed, we provide both anatomical and physiological evidence that VTA GABA neurons projecting to NAc, VP, or PFC make local synapses within VTA. This work challenges the presumption of GABA interneurons in VTA by providing direct evidence for an alternative model by which GABA projection neurons can regulate the activity of neighboring VTA cells.
Results
PV, SST, MOR, and NTS are not selective interneuron markers in VTA
We selected four genes with well-validated Cre lines to test as putative genetic markers that might selectively label VTA interneurons: Parvalbumin (PV), Somatostatin (SST), Mu-opioid receptor (MOR), or Neurotensin (NTS). We injected adeno-associated virus (AAV) into the VTA for Cre-dependent expression of Channelrhodopsin-2 (ChR2) fused to mCherry that labels distal axons (Figure 1A). To test whether the labeled VTA neurons project distally we assessed expression in known VTA projection sites including nucleus accumbens (NAc), ventral pallidum (VP), prefrontal cortex (PFC), and lateral habenula (LHb).
Parvalbumin (PV) is a marker of interneurons in cortex and striatum (Kawaguchi, 1993; Kawaguchi & Kondo, 2002; Tepper et al., 2018), but is also expressed in VTA GABA neurons (Olson & Nestler, 2007). Injections into VTA of PV-Cre mice labeled neurons located in medial VTA. We also detected a dense concentration of axonal fibers in LHb, with scant labeling in other known VTA projection targets (Figure 1B). These data suggest that PV labels VTA projection neurons and PV is not a selective marker of VTA interneurons.
Like PV, Somatostatin (SST) is an interneuron marker in cortex (Kawaguchi & Kondo, 2002). SST is expressed in VTA GABA neurons that can inhibit neighboring VTA DA neurons (Nagaeva et al., 2020). Injections into SST-Cre mice labeled cell bodies in VTA (Figure 1C). We again identified axons in distal targets, here with notably dense labeling in VP.
MOR is expressed in non-DA VTA GABA neurons, inhibiting GABA release from synapses on to VTA DA neurons, thereby increasing DA neuron firing, and is often described as a marker of VTA interneurons (Gysling & Wang, 1983; Johnson & North, 1992; Luscher & Malenka, 2011; Nestler, 2005; Phillips et al., 2022). Injections into MOR-Cre mice led to the presence of labeled neurons throughout VTA, but also labeled axons in PFC, NAc, LHb, and especially VP (Figure 1D).
NTS is expressed in a subpopulation of VTA GABA neurons (Phillips III et al., 2022) and NTS can stimulate mesolimbic DA cells through activation of NTS receptor 1 (Caceda et al., 2006; Kalivas, 1983). Injections into NTS-Cre mice labeled neurons in VTA, as well as axons in VP, with weaker labeling in other VTA projection sites (Figure 1E).
We also stained VTA sections for Tyrosine hydroxylase (TH) to estimate the rate of ChR2:mCherry colocalization with DA neurons. In all cases only a minority of mCherry-labeled neurons expressed TH, ranging from 2% for PV to 12% for NTS (Figure 1F). In total, our data suggest that these four markers label primarily non-DA neurons in VTA, but that none are selective for interneurons, instead are inclusive of VTA projection neurons.
Anatomical evidence that VTA projection neurons make local synapses
Each of the markers tested are also expressed in neurons proximal to VTA and our injections led to variable spread to neighboring regions, including interpeduncular nucleus (IPN) and red nucleus. While these regions are not known to project to PFC, NAc, VP, or LHb, we nonetheless aimed to validate the above findings with a secondary approach involving a combination of retrograde labeling and intersectional genetics to target VTA projection neurons. We injected AAV-fDIO-mGFP-Synaptophysin:mRuby into VTA of each Cre line, plus retroAAV-DIO-Flp into a projection target receiving dense innervation. This approach allowed for Cre-plus Flp-dependent expression of both membrane-localized GFP and the synaptic vesicle marker Syn:Ruby (Beier et al., 2015). The intersectionality of this approach allows for precise targeting of VTA projection neurons, and Syn:Ruby highlights putative release sites, either local to or distal from VTA.
Using this approach to label PV-Cre projectors to LHb (Figure 2A), or SST-Cre projectors to VP (Figure 2G), revealed GFP-positive soma well-restricted within VTA borders delineated by TH immunolabel (Figure 2B,C,H,I). We also observed GFP-positive axons and Syn:Ruby-positive puncta in LHb of PV-Cre, or VP of SST-Cre mice (Figure 2E,F,K,L). Using high magnification we observed Syn:Ruby puncta proximal to TH-positive cells in VTA (Figure 2D,J), suggesting that these VTA projection neurons collateralize within VTA and synapse on to DA neurons.
The same approach was used to label VTA projectors to VP in MOR-Cre or NTS-Cre mice (Figure 3A). VP-projecting GFP-positive cell bodies in MOR-Cre mice were contained within and throughout VTA (Figure 3B). We also observed axonal fibers densely filling VP, delineated by Substance P immunolabel (Figure 3F-H). Using high magnification, we observed Syn:Ruby puncta proximal to TH-positive VTA neurons, again suggestive of synapses made within VTA by labeled projection neurons (Figure 3C-E). Using the same approach to target VP-projecting neurons in NTS-Cre mice we found similar results, with GFP-positive soma in VTA and Syn:Ruby-positive puncta in both VTA and VP (Figure 3K-J), though signals were notably less dense. These results corroborate the findings in Figure 1 and suggest that multiple markers that had been suggested to label putative interneurons instead label VTA projection neurons that may make local synapses through axon collaterals.
There is evidence indicating that PV, SST, MOR and NTS neurons in VTA express GABA markers or release GABA (Nagaeva et al., 2020; Olson & Nestler, 2007; Phillips et al., 2022). However, some neurons positive for those markers may express VGLUT2 and release glutamate (Miranda-Barrientos et al., 2021). We therefore used VGAT-Cre and VGLUT2-Cre mice to selectively express GFP and Syn:Ruby, here targeting NAc-projecting VTA neurons. In VGAT-Cre mice (Figure 4A) we identified GFP-positive fibers in NAc (Figure 4B-C) and GFP-positive cell bodies were restricted to VTA (Figure 4D). At higher magnification, we observed a pattern of GFP fibers and Syn:Ruby puncta surrounding TH-positive cell bodies (Figure 4E-F), suggesting that NAc-projectors make collaterals on to VTA DA neurons. We observed similar results when using VGLUT2-Cre mice, suggesting that NAc-projecting VTA glutamate neurons can also make local collaterals within VTA (Figure 4G-L). As expected VTA glutamate cell bodies were concentrated in medial VTA, where they are most dense (Conrad et al., 2024; Kawano et al., 2006; Yamaguchi et al., 2011).
Physiological evidence that VTA projection neurons make local synapses
Our anatomical results suggest that multiple types of VTA projection neurons collateralize locally within VTA. Next, to functionally assess whether VTA projection neurons make local synapses in VTA, we used a combination of optogenetics and electrophysiology. We selectively expressed ChR2 in NAc-projecting VTA neurons by injecting retroAAV-Cre into NAc and AAV-DIO-ChR2:mCherry into VTA of wild-type mice (Figure 5A). We then made acute brain slices to record from VTA neurons negative for ChR2:mcherry to test if they received synaptic inputs from NAc-projecting VTA neurons (Figure 5B). Using wild-type mice allowed us to express opsin in both GABA and glutamate projection neurons, and assess for optogenetic-evoked postsynaptic currents (oPSC) that were either inhibitory (oIPSC) or excitatory (oEPSC) from the same cell.
As expected, the medial shell of NAc showed dense mCherry-positive fibers (Figure 5C), and mCherry-positive cell bodies were restricted to VTA (Figure 5D). We patched ChR2:mCherry-negative VTA neurons (Supplemental Figure 5), flashed 2-ms blue light pulses, and observed oPSCs in 60% of neurons; 42% displayed short-latency oIPSCs (mean 86 ± 17 pA), 14% had short-latency oEPSCs (mean −24 ± 4 pA), 40% had no response (responses less than 5 pA were considered unconnected), and 10% had oPSCs with long-latency to onset (>5 ms) (Figure 5E-F). Note that unconnected and long-latency cells are not included in Figures 5F, I. The GABAA receptor antagonist picrotoxin (PTX) blocked oIPSCs while oEPSCs were blocked by the AMPA receptor antagonist DNQX (Figure 5G,H), confirming that these responses are mediated by evoked GABA or glutamate release, respectively.
Most responses displayed onset latencies less than 5 ms, consistent with monosynaptic connectivity (3.2 ± 0.1 ms and 3.5 ± 0.2 ms for oIPSCs and oEPSCs, respectively) (Figure 5I). To confirm connections are monosynaptic we performed additional pharmacology. We found that the amplitude of oPSCs was diminished following the application of the voltage-gated sodium channel blocker tetrodotoxin (TTX, voltage-gated sodium channel are necessary for the propagation of action potentials), and that oPSCs recovered with bath application of the inhibitor of voltage-sensitive potassium channels 4-aminopyridine (4AP). When this strategy was applied to oIPSCs (Figure 5J), 8 out of 9 TTX diminished currents were restored by the application of 4AP (Figure 5J,K). Similarly, 6 of 9 oEPSCs were recovered by 4AP (Figure 5L,M). We plotted the latency of oPSC onset against the percent oPSC recovery mediated by 4AP and found that 3 of 4 neurons that failed to recover had a latency >5ms, whereas only 1 of 15 neurons that had a latency <5 ms failed to recover (Figure 5N). Therefore, we used 5 ms as a ‘short latency’ cutoff to consider an oPSC as monosynaptic. In total we recorded ten cells with oPSC latency >5 ms (identified as long latency on Figure 5E). Out of these 10 long-latency oPSCs, 8 were oEPSCs and 2 oIPSCs. This proportion (8:2) of neurons with oEPSCs versus oIPSCs was strikingly greater than that for short-latency responses (13:41), suggesting that in some cells/slices optogenetic stimulation of projection neurons recruited a more extensive intra-VTA excitatory network.
We used a similar approach to assess whether VTA neurons projecting to VP or PFC also made local collaterals in VTA. We used the same combination of viruses but here injected retroAAV-Cre into VP of wild-type mice (Figure 6A), again recording from mCherry-negative VTA neurons (Figure 6B). As expected, we observed dense mCherry-positive fibers in VP and mCherry-positive cell bodies restricted to VTA (Figure 6C-D). We found that 54% of mCherry-negative neurons were connected (14 of 26), 31% displayed short-latency oIPSCs, 12% had short-latency oEPSCs, and 19% were connected but with long latency (>5 ms) (Figure 6E-G). We also patched from postsynaptic neurons in VP and found 89% displayed oPSCs, with a mix of oIPSCs and oEPSCs (Figure 6H-K).
Finally, we repeated the same approach but for PFC-projecting VTA neurons (Figure 6L-M). We observed mCherry-positive fibers in PFC (Figure 6O) arising from sparse cell bodies found exclusively within the bounds of VTA (Figure 6P). In VTA, we found that 36% of ChR2:mCherry-negative neurons were connected, all of which displayed oIPSCs, with 2 of the 12 connected cells also showing oEPSCs (Figure 6N-R). Altogether our data indicate that both GABAergic and glutamatergic VTA projection neurons make functional synapses within VTA.
Discussion
The VTA plays consequential roles in the orchestration of motivated behaviors and is composed of heterogeneous populations of DA, GABA, and glutamate neurons that send dense projections to diverse forebrain regions (Fields et al., 2007; Morales & Margolis, 2017). Yet VTA DA, GABA, and glutamate neurons also release their neurotransmitters locally within VTA. DA is released from somatodendritic compartments, activating DA autoreceptors (Ford, 2014). Multiple lines of evidence indicate that GABA and glutamate neurons resident to VTA synapse locally on to VTA DA and non-DA neurons (Beier, 2022; Dobi et al., 2010; Omelchenko & Sesack, 2009; Soden et al., 2020; Tan et al., 2012). VTA GABA neurons that make local synapses within VTA have frequently been described as interneurons (Bonci & Williams, 1996; Johnson & North, 1992; Luscher & Malenka, 2011; O’Brien & White, 1987). But there is scant evidence that VTA GABA interneurons and projection neurons represent distinct cell types. In this study we used retroAAV to target VTA neurons that project to NAc, VP, PFC, or LHb for recombinase-dependent expression of synaptic tags to image putative release sites, or opsin for optogenetic stimulation of projection neurons while recording synaptic events in neighboring VTA neurons. Both approaches point to the same conclusion, that at least a subset of GABA and glutamate projection neurons collateralize locally and make intra-VTA synapses.
In cortex, hippocampus and other areas dominated by glutamate projection neurons the term interneuron is often used to describe inhibitory GABA neurons that synapse on to neurons within the same structure as their soma reside. However, the limbic basal ganglia circuits in which VTA neurons are embedded include many GABAergic projection neurons, at least subsets of which are understood to make both distal and local synapses. For example, DA D2 receptor-expressing medium spiny neurons are GABA projection neurons that also make extensive local collaterals that laterally inhibit and regulate other striatal neurons (Dobbs et al., 2016; Tunstall et al., 2002). Thus, a meaningful definition of the term in the context of mesolimbic circuitry, and the definition of interneuron we use in this study, is a neuron that synapses locally but not distally. Indeed, this definition captures many well characterized populations of neurons throughout the cortex, hippocampus, striatum, or cerebellum (Lim et al., 2018; Maccaferri & Lacaille, 2003; Pelkey et al., 2017; Petilla Interneuron Nomenclature et al., 2008). For example, cortical or striatal interneurons that express PV, SST, or cholinergic markers can be readily distinguished at the molecular level, but also by physiological properties that distinguish them from projection neurons or other cell types (Huang & Paul, 2019; Markram et al., 2004; Tepper et al., 2018).
The VTA has been known to contain non-DA GABA neurons since at least the early 1980’s (Gysling & Wang, 1983; Oertel & Mugnaini, 1984; Waszczak & Walters, 1980; Yim & Mogenson, 1980). Moreover, VTA GABA neurons were demonstrated to make inhibitory synapses on to VTA DA neurons (Bayer & Pickel, 1991; Johnson & North, 1992). VTA DA neurons may be distinguished from non-DA neurons (at least in lateral VTA) based on firing rate and other physiological and pharmacological features (Bunney et al., 1973; German et al., 1980; Waszczak & Walters, 1980). These observations serve as the primary basis for the notion of a VTA interneuron. However, those observations could instead be explained by VTA GABA projection neurons that collateralize locally. Indeed, one notable study used in vivo electrophysiology to identify a population of non-DA projection neurons and showed that they were reliably activated by antidromic stimulation of the internal capsule (Steffensen et al., 1998). This suggests that the population of non-DA VTA neurons they were able to identify through in vivo recordings were projection neurons.
If GABA interneurons represent one or more bona fide VTA cell types, then it is reasonable to suppose that they would be distinguishable by a molecular marker (or a constellation of markers). Markers that confer a GABAergic identity label VTA GABA projection neurons, and thus could not distinguish putative interneurons from projection neurons. However, several other markers have been shown to co-localize with a subset of VTA GABA but not DA neurons and thus represent potential interneuron markers (Bouarab et al., 2019; Nagaeva et al., 2020; Olson & Nestler, 2007; Phillips et al., 2022). We selected four of these markers that had well-validated Cre lines: PV, SST, MOR, and NTS. Using two different tracing strategies we confirmed that these markers are expressed in a subset of VTA neurons that are primarily non-dopaminergic. We found that PV+ VTA neurons project densely to LHb (and weakly to other projection targets), while SST+, NTS+, and especially MOR+ VTA neurons project densely to VP (and other projection targets). Thus, while it is possible that there exists a subset of VTA interneurons that express one or more of these markers, none of these markers can be used on its own to discriminate between VTA projection neurons and VTA interneurons.
While the retroAAV approach resulted in strong labeling of projection neurons, including GABA and glutamate-releasing neurons, it is likely that the intrinsic tropism of retroAAV influenced the population of projection cells that we labeled. Indeed, prior work showed that midbrain DA neurons are not efficiently targeted by the retroAAV vector we used (Tervo et al., 2016). Thus, populations of neurons that release DA and co-release GABA or glutamate may not contribute to the signals we measured.
In addition to GABA projection neurons, our experiments revealed that glutamate projection neurons in VTA make local synapses. Therefore, the local excitatory synaptic events observed in prior studies (Dobi et al., 2010; McGovern et al., 2023; Yoo et al., 2016) may be driven by collaterals made by VTA glutamate projection neurons rather than a population of glutamate interneurons. Interestingly, we found that optogenetic activation of unspecified VTA projection neurons induced intra-VTA oEPSCs more rarely than intra-VTA oIPSCs. However, we also observed long-latency oPSCs, that were likely the result of activating VTA glutamate projection neurons that make intra-VTA excitatory collaterals and drive feed-forward recruitment of other VTA cells that also make local synapses.
The VTA integrates a large number of inhibitory inputs from a multitude of brain regions. However, recent studies indicate that neurons local to VTA preferentially inhibit DA neurons compared to GABAergic afferents from distal sources (Beier, 2022; Soden et al., 2020). Yet these studies cannot determine whether the local neurons synapsing on to VTA DA neurons are interneurons versus collaterals made by projection neurons. Moreover, VTA has been shown to receive an important GABAergic input from the rostral medial tegmental nucleus (RMTg) (Jhou, 2005; Perrotti et al., 2005). While VTA and RMTg are considered separate structures, the boundary between caudal VTA and rostral RMTg is ambiguous, and this area is dominated by GABA neurons (Smith et al., 2019). Interestingly, RMTg inhibitory synapses on to VTA DA neurons are strongly inhibited by MOR activation, and thus some of the functions classically attributed to VTA interneurons may be mediated by these short-range projection neurons (Jhou, 2021; Jhou et al., 2009; Kaufling & Aston-Jones, 2015; Matsui et al., 2014; St Laurent et al., 2020).
Within VTA, we found that MOR and several other potential interneuron markers were instead expressed in projection neurons. Other interneuron marker candidates have been suggested but, to our knowledge, no other VTA marker has been shown to be expressed selectively within a VTA interneuron population (Bouarab et al., 2019; Paul et al., 2019). One promising candidate is neuronal nitric oxide synthase (nNOS) which labels a subset of VTA GABA neurons in the parabrachial pigmented area of VTA that may not project distally, but also labels DA and glutamate neurons in adjacent areas of VTA and substantia nigra (Paul et al., 2018). Future work, for example using intersectional labeling, may resolve whether nNOS selectively labels bona fide GABA interneurons in VTA. Another candidate marker of interest is prepronociceptin (PNOC). A recent report showed that PNOC labels a population of paranigral non-DA neurons that make dense intra-VTA synapses without projecting to NAc (Parker et al., 2019). However, VTA PNOC neurons express GABA and/or glutamate markers, and it is not clear whether they project to other VTA projection targets, such as VP or LHb.
In sum, we provide multiple lines of evidence that VTA GABA (and glutamate) neurons that project to distal targets also collateralize locally and make intra-VTA synapses. We also demonstrate that several candidate markers, including MOR, are expressed in VTA projection neurons. Future efforts may reveal positive evidence for the existence of VTA interneurons, for example through the identification of a marker, or a combinatorial set of markers, that labels VTA neurons that make local but not distal connections. At present, however, there is little evidence to support the notion of a VTA interneuron. We suggest that some functions prior attributed to VTA interneurons, such as MOR-mediated disinhibition of DA neurons, may instead be mediated by VTA projection neurons that make synaptic collaterals on to DA neurons. In this way the actions of opioids on VTA neurons would not only disinhibit DA neurons, but simultaneously inhibit GABA (or glutamate) release from distal VTA projections to VP and elsewhere. Indeed, given our increasing understanding for the roles of VTA GABA and glutamate projections in processes underlying behavioral reinforcement, their direct effects on distal targets may contribute to opioid-induced behaviors or adaptations relevant to drug addiction distinct from their effects on VTA DA neurons.
Methods
Animals
Mice were group-housed (up to 5 mice/cage), bred at the University of California, San Diego (UCSD), kept on a 12h light-dark cycle, and had access to food and water ad libitum. Initial breeders were acquired from The Jackson Laboratory (Table 1), except for the MOR-Cre (Bailly et al., 2020) obtained from the lab of Brigitte Kieffer (University of Strasbourg). All mice were bred with a C57Bl/6 background and used as a mix of heterozygotes and homozygotes). Male and female mice were used in all experiments. All experiments were performed in accordance with protocols approved by the UCSD Institutional Animal Care and Use Committee.
Stereotaxic surgery
Mice >5 weeks (and up to 6months old) were deeply anesthetized with Isoflurane (502017, Primal Critical Care) and placed on a stereotaxic frame (Kopf 1900) for microinjection into discrete brain areas (Table 2). After ensuring the skull is flat small holes were drilled (1911-C Kopf) and AAVs (Table 3) infused with Nanoject (3-000-207, Drummond) using glass injectors (3-000-203-G/X, Drummond) pulled on a horizontal pipette puller (P-1000 Sutter Instrument). After infusion the injector was left for 3 to 5 min then withdrawn. Analgesia was provided via injections with 5mg/kg S.C. Carprofen (510510 Vet One). Electrophysiology was performed >3 weeks after surgery, histolgy >5 weeks.
Histology
Mice were deeply anesthetized with pentobarbital (200 mg.kg-1, i.p., 200-071, Virbac) and transcardially perfused with 30mL of PBS (BP399, Fisher bioreagents) followed by 50mL of 4% PFA (18210, Electron Microscopy Sciences) in PBS. Brains were removed, post-fixed in 4% PFA overnight, and dehydrated in 30% sucrose (S0389, Sigma-Aldrich) in PBS for 48h then flash-frozen in isopentane. Brains were cut in 30µm sections on a cryostat (CM3050S, Leica). Sections were selected to encompass the VTA and efferents to PFC, NAc, VP, and LHb. Sections were blocked in 5% normal donkey serum/0.4% Triton X-100 in PBS for 1h at room temperature and incubated with primary antibodies (Table 4) overnight at 4°C in the blocking buffer. Next day, slides were washed three times in 0.4% Triton X-100 in PBS for 5 min and incubated with secondary antibodies for two hours at room temperature shielded from the light. Finally, sections were washed three times in 0.4% Triton X-100 in PBS for 5 min and coverslipped with Fluoromount-G (Southern Biotech) containing 0.5µg/mL of DAPI (Roche). Images were taken using a Zeiss Axio Observer Epifluorescence microscope.
Colocalization with TH and counting
For each genetic marker, 3-4 mice and 4 sections through VTA per mouse were stained with antibodies against TH and DsRed. All sections were imaged at 10X with the same exposure parameters, using a Zeiss AxioObserver equipped with apotome2 for structured illumination. The same display settings were applied to all images within condition. TH signal was used to define the boundaries of VTA and align to Bregma point. Cells expressing mCherry were identified first, then scored for presence or absence of TH expression. The counts were done independently by two experimenters and a high correlation was observed between the experimenters (R2=0.77 p<0.001, 60 total sections). Each cell that was only identified by one observer was reassessed for inclusion in final dataset.
Single injection tracing
For evaluation of projection targets following a single AAV injection into VTA, we excluded subjects that had <30% of labeled cell bodies outside the VTA (Table 5). We also excluded subjects that had mCherry labeled cell bodies in supramammillary nucleus. But we did not exclude mice with spread to red nucleus or IPN because these regions are not known to project to NAc, PFC, VP, or LHb (Liang et al., 2011; McLaughlin et al., 2017).
Electrophysiology
Mice were deeply anesthetized using pentobarbital (200 mg/kg, i.p., Virbac) and transcardially perfused with 30 ml cold N-methyl D-glucamine (NMDG)-artificial Crebro-Spinal Fluid (aCSF, containing in mM: 92 NMDG, 2.5 KCl, 1.25 NaH2PO4, 30 NaHCO3, 20 HEPES, 25 D-glucose, 5 sodium ascorbate, 2 thiourea, 3 sodium pyruvate, 10 MgSO4, 0.5 CaCl2, pH 7.3) saturated with carbogen (95% O2–5% CO2). Sections (coronal, 200µm) were cut through VTA while immersed in cold NMDG-aCSF using a vibratome (VT1200S, Leica). Slices were incubated at 33°C for 25-30 min in a holding chamber containing NMDG-aCSF saturated with carbogen. During the incubation NaCl concentration was slowly increased in 5 min increments by spiking the holding-aCSF with a 2M NaCl solution diluted with the NMDG-aCSF (Ting et al., 2018). Slices were incubated at 25°C for 30-45 min in a holding chamber containing holding-aCSF (containing in mM: 115 NaCl, 2.5 KCl, 1.23 NaH2PO4, 26 NaHCO3, 10 D-glucose, 5 sodium ascorbate, 2 Thiourea, 3 sodium pyruvate, 2 MgSO4, 2 CaCl2, pH7.3) saturated with carbogen. While recording, slices were superfused with 31°C recording-aCSF (containing in mM: 125 NaCl, 2.5 KCl, 1.20 NaH2PO4, 26 NaHCO3, 12.5 D-glucose, 2 MgSO4, 2 CaCl2) using an in-line heater (TC-324B, Warner) at 1.5 ml/min. Whole-cell patch-clamp recordings from mCherry-negative VTA neurons were performed under visual guidance with infrared illumination and differential interference contrast using a Zeiss Axiocam MRm, Examiner.A1, Zeiss equipped with a 40X objective. 6-7MΩ patch pipettes were pulled from borosilicate glass (Sutter Instruments) and filled with internal solution (containing in mM: 133.4 cesium-methanesulfonate, 22.7 HEPES, 0.45 EGTA, 3.2 NaCl, 5.7 tetraethylammonium-chloride, 0.48 NA-GTP, 4.5 Na2-ATP, pH to 7.3 with Cesium-OH). Postsynaptic currents were recorded in whole-cell voltage clamp (Multiclamp 700B amplifier, Axon Instruments), filtered at 2 kHz, digitized at 20 kHz (Axon Digidata 1550, Axon Instruments), and collected using pClamp 10 software (Molecular Device). Neurons were first held at −65mV to record excitatory currents and then at 0mV to record inhibitory currents. Optogenetic-evoked postsynaptic currents (oPSCs) were induced by flashing blue light (two 10Hz 2ms pulses, every 15s) through the light path of the microscope using a light-emitting diode (UHP-LED460, Prizmatix) under computer control. We discarded likely ChR2+ cells, displaying photocurrent (Supplemental Figure 5), identified as starting within 1 ms of the light pulse, as well as cells where the series resistance varied by more than 20%. After breaking-in we waited 2-3 minutes before beginning optogenetic stimulation. For each cell we first recorded a baseline period (4-6 min) and for some cells baseline was followed by 4-6 min bath application of drug: 1µM TTX, 50-100µM 4AP, 10µM DNQX, 100µM PTX (Table 6). For each condition we averaged the last 10 sweeps; amplitude represented the peak current, and latency calculated as the duration from light onset to current onset.
Statistics
Data values are presented as means ± SEM. Effects of drug application were subjected to Friedman’s test (nonparametric ANOVA) followed by a Dunn’s posthoc test (GraphPad Prism). Statistical significance was set at p<0.05.
Acknowledgements
This work was supported by funds from the National Institutes of Health (R01DA036612), Veterans Affairs (I01BX005782). We thank Karl Deisseroth and Liqun Luo for AAV vectors provided through Addgene (see methods), and Sarah Uran for technical assistance.
References
- Unique functional responses differentially map onto genetic subtypes of dopamine neuronsNat Neurosci 26:1762–1774https://doi.org/10.1038/s41593-023-01401-9
- Aversive stimuli differentially modulate real-time dopamine transmission dynamics within the nucleus accumbens core and shellJ Neurosci 32:15779–15790https://doi.org/10.1523/JNEUROSCI.3557-12.2012
- Targeting Morphine-Responsive Neurons: Generation of a Knock-In Mouse Line Expressing Cre Recombinase from the Mu-Opioid Receptor Gene LocuseNeuro 7https://doi.org/10.1523/ENEURO.0433-19.2020
- GABA-labeled terminals form proportionally more synapses with dopaminergic neurons containing low densities of tyrosine hydroxylase-immunoreactivity in rat ventral tegmental areaBrain Res 559:44–55https://doi.org/10.1016/0006-8993(91)90285-4
- Modified viral-genetic mapping reveals local and global connectivity relationships of ventral tegmental area dopamine cellsElife 11https://doi.org/10.7554/eLife.76886
- A common mechanism mediates long-term changes in synaptic transmission after chronic cocaine and morphineNeuron 16:631–639https://doi.org/10.1016/s0896-6273(00)80082-3
- VTA GABA Neurons at the Interface of Stress and RewardFront Neural Circuits 13https://doi.org/10.3389/fncir.2019.00078
- Dopaminergic neurons: effect of antipsychotic drugs and amphetamine on single cell activityJ Pharmacol Exp Ther 185:560–571
- Neurotensin: role in psychiatric and neurological diseasesPeptides 27:2385–2404https://doi.org/10.1016/j.peptides.2006.04.024
- Proportion and distribution of neurotransmitter-defined cell types in the ventral tegmental area and substantia nigra pars compactabioRxiv https://doi.org/10.1101/2024.02.28.582356
- Dopamine neurons projecting to medial shell of the nucleus accumbens drive heroin reinforcementElife 7https://doi.org/10.7554/eLife.39945
- A Neural Circuit Mechanism for Encoding Aversive Stimuli in the Mesolimbic Dopamine SystemNeuron 101:133–151https://doi.org/10.1016/j.neuron.2018.11.005
- Dopamine Regulation of Lateral Inhibition between Striatal Neurons Gates the Stimulant Actions of CocaineNeuron 90:1100–1113https://doi.org/10.1016/j.neuron.2016.04.031
- Glutamatergic and nonglutamatergic neurons of the ventral tegmental area establish local synaptic contacts with dopaminergic and nondopaminergic neuronsJ Neurosci 30:218–229https://doi.org/10.1523/JNEUROSCI.3884-09.2010
- Arithmetic and local circuitry underlying dopamine prediction errorsNature 525:243–246https://doi.org/10.1038/nature14855
- Ventral pallidum GABA and glutamate neurons drive approach and avoidance through distinct modulation of VTA cell typesNat Commun 15https://doi.org/10.1038/s41467-024-48340-y
- Afferent Inputs to Neurotransmitter-Defined Cell Types in the Ventral Tegmental AreaCell Rep 15:2796–2808https://doi.org/10.1016/j.celrep.2016.05.057
- Ventral tegmental area neurons in learned appetitive behavior and positive reinforcementAnnu Rev Neurosci 30:289–316https://doi.org/10.1146/annurev.neuro.30.051606.094341
- The role of D2-autoreceptors in regulating dopamine neuron activity and transmissionNeuroscience 282:13–22https://doi.org/10.1016/j.neuroscience.2014.01.025
- Electrophysiological examination of the ventral tegmental (A10) area in the ratBrain Res 181:191–197https://doi.org/10.1016/0006-8993(80)91269-x
- Ventral tegmental area astrocytes orchestrate avoidance and approach behaviorNat Commun 10https://doi.org/10.1038/s41467-019-09131-y
- The glutamatergic component of the mesocortical pathway emanating from different subregions of the ventral midbrainCereb Cortex 22:327–336https://doi.org/10.1093/cercor/bhr107
- Morphine-induced activation of A10 dopamine neurons in the ratBrain Res https://doi.org/10.1016/0006-8993(83)90913-7
- Ventral tegmental area glutamate neurons: electrophysiological properties and projectionsJ Neurosci 32:15076–15085https://doi.org/10.1523/JNEUROSCI.3128-12.2012
- The diversity of GABAergic neurons and neural communication elementsNat Rev Neurosci 20:563–572https://doi.org/10.1038/s41583-019-0195-4
- Neural mechanisms of freezing and passive aversive behaviorsJ Comp Neurol 493:111–114https://doi.org/10.1002/cne.20734
- The rostromedial tegmental (RMTg) “brake” on dopamine and behavior: A decade of progress but also much unfinished workNeuropharmacology 198https://doi.org/10.1016/j.neuropharm.2021.108763
- The mesopontine rostromedial tegmental nucleus: A structure targeted by the lateral habenula that projects to the ventral tegmental area of Tsai and substantia nigra compactaJ Comp Neurol 513:566–596https://doi.org/10.1002/cne.21891
- Opioids excite dopamine neurons by hyperpolarization of local interneuronsJ Neurosci 12:483–488https://doi.org/10.1523/JNEUROSCI.12-02-00483.1992
- Behavioral and neurochemical effects of neurotesin microinjection into the VTA of the ratNeuroscience 8:495–505
- Persistent Adaptations in Afferents to Ventral Tegmental Dopamine Neurons after Opiate WithdrawalJ Neurosci 35:10290–10303https://doi.org/10.1523/JNEUROSCI.0715-15.2015
- gamma-Aminobutyric acid cells with cocaine-induced DeltaFosB in the ventral tegmental area innervate mesolimbic neuronsBiol Psychiatry 67:88–92https://doi.org/10.1016/j.biopsych.2009.08.001
- Physiological, morphological, and histochemical characterization of three classes of interneurons in rat neostriatumJ Neurosci 13:4908–4923https://doi.org/10.1523/JNEUROSCI.13-11-04908.1993
- Parvalbumin, somatostatin and cholecystokinin as chemical markers for specific GABAergic interneuron types in the rat frontal cortexJ Neurocytol 31:277–287https://doi.org/10.1023/a:1024126110356
- Particular subpopulations of midbrain and hypothalamic dopamine neurons express vesicular glutamate transporter 2 in the rat brainJ Comp Neurol 498:581–592https://doi.org/10.1002/cne.21054
- Dopamine Prediction Errors in Reward Learning and Addiction: From Theory to Neural CircuitryNeuron 88:247–263https://doi.org/10.1016/j.neuron.2015.08.037
- Diversity of transgenic mouse models for selective targeting of midbrain dopamine neuronsNeuron 85:429–438https://doi.org/10.1016/j.neuron.2014.12.036
- Projections from the brain to the spinal cord in the mouseBrain Struct Funct 215:159–186https://doi.org/10.1007/s00429-010-0281-x
- Development and Functional Diversification of Cortical InterneuronsNeuron 100:294–313https://doi.org/10.1016/j.neuron.2018.10.009
- The Emergence of a Circuit Model for AddictionAnnu Rev Neurosci 39:257–276https://doi.org/10.1146/annurev-neuro-070815-013920
- Drug-evoked synaptic plasticity in addiction: from molecular changes to circuit remodelingNeuron 69:650–663https://doi.org/10.1016/j.neuron.2011.01.017
- Spatial Distribution of Neurons Expressing Single, Double, and Triple Molecular Characteristics of Glutamatergic, Dopaminergic, or GABAergic Neurons in the Mouse Ventral Tegmental AreaJ Mol Neurosci 73:345–362https://doi.org/10.1007/s12031-023-02121-2
- Interneuron Diversity series: Hippocampal interneuron classifications--making things as simple as possible, not simplerTrends Neurosci 26:564–571https://doi.org/10.1016/j.tins.2003.08.002
- Interneurons of the neocortical inhibitory systemNat Rev Neurosci 5:793–807https://doi.org/10.1038/nrn1519
- Separate GABA afferents to dopamine neurons mediate acute action of opioids, development of tolerance, and expression of withdrawalNeuron 82:1346–1356https://doi.org/10.1016/j.neuron.2014.04.030
- Ventral tegmental area glutamate neurons establish a mu-opioid receptor gated circuit to mesolimbic dopamine neurons and regulate opioid-seeking behaviorNeuropsychopharmacology 48:1889–1900https://doi.org/10.1038/s41386-023-01637-w
- The medial habenula and interpeduncular nucleus circuitry is critical in addiction, anxiety, and mood regulationJ Neurochem 142:130–143https://doi.org/10.1111/jnc.14008
- Ventral tegmental area GABA, glutamate, and glutamate-GABA neurons are heterogeneous in their electrophysiological and pharmacological propertiesEur J Neurosci https://doi.org/10.1111/ejn.15156
- Ventral tegmental area: cellular heterogeneity, connectivity and behaviourNat Rev Neurosci 18:73–85https://doi.org/10.1038/nrn.2016.165
- Heterogeneous somatostatin-expressing neuron population in mouse ventral tegmental areaElife 9https://doi.org/10.7554/eLife.59328
- Is there a common molecular pathway for addiction?Nat Neurosci 8:1445–1449https://doi.org/10.1038/nn1578
- Decoding neural circuits that control compulsive sucrose seekingCell 160:528–541https://doi.org/10.1016/j.cell.2015.01.003
- Inhibition of non-dopamine cells in the ventral tegmental area by benzodiazepines: relationship to A10 dopamine cell activityEur J Pharmacol 142:343–354https://doi.org/10.1016/0014-2999(87)90072-0
- Ventral tegmental (A10) system: neurobiology. 1. Anatomy and connectivityBrain Res 434:117–165https://doi.org/10.1016/0165-0173(87)90011-7
- Immunocytochemical studies of GABAergic neurons in rat basal ganglia and their relations to other neuronal systemsNeurosci Lett 47:233–238https://doi.org/10.1016/0304-3940(84)90519-6
- Topographical organization of GABAergic neurons within the ventral tegmental area of the ratSynapse 61:87–95https://doi.org/10.1002/syn.20345
- Ultrastructural analysis of local collaterals of rat ventral tegmental area neurons: GABA phenotype and synapses onto dopamine and GABA cellsSynapse 63:895–906https://doi.org/10.1002/syn.20668
- Inhibitory Plasticity of Mesocorticolimbic Circuits in Addiction and Mental IllnessTrends Neurosci 41:898–910https://doi.org/10.1016/j.tins.2018.07.014
- A Paranigral VTA Nociceptin Circuit that Constrains Motivation for RewardCell 178:653–671https://doi.org/10.1016/j.cell.2019.06.034
- nNOS-Expressing Neurons in the Ventral Tegmental Area and Substantia Nigra Pars CompactaeNeuro 5https://doi.org/10.1523/ENEURO.0381-18.2018
- Transcriptional profiling aligned with in situ expression image analysis reveals mosaically expressed molecular markers for GABA neuron sub-groups in the ventral tegmental areaEur J Neurosci 50:3732–3749https://doi.org/10.1111/ejn.14534
- Hippocampal GABAergic Inhibitory InterneuronsPhysiol Rev 97:1619–1747https://doi.org/10.1152/physrev.00007.2017
- DeltaFosB accumulates in a GABAergic cell population in the posterior tail of the ventral tegmental area after psychostimulant treatmentEur J Neurosci 21:2817–2824https://doi.org/10.1111/j.1460-9568.2005.04110.x
- Petilla terminology: nomenclature of features of GABAergic interneurons of the cerebral cortexNat Rev Neurosci 9:557–568https://doi.org/10.1038/nrn2402
- An atlas of transcriptionally defined cell populations in the rat ventral tegmental areaCell Rep 39https://doi.org/10.1016/j.celrep.2022.110616
- Classification of Midbrain Dopamine Neurons Using Single-Cell Gene Expression Profiling ApproachesTrends Neurosci 43:155–169https://doi.org/10.1016/j.tins.2020.01.004
- Dissecting the diversity of midbrain dopamine neuronsTrends Neurosci 36:336–342https://doi.org/10.1016/j.tins.2013.03.003
- Distinct Signaling by Ventral Tegmental Area Glutamate, GABA, and Combinatorial Glutamate-GABA Neurons in Motivated BehaviorCell Rep 32https://doi.org/10.1016/j.celrep.2020.108094
- Aversion or Salience Signaling by Ventral Tegmental Area Glutamate NeuronsiScience 2:51–62https://doi.org/10.1016/j.isci.2018.03.008
- Role of glutamatergic projections from ventral tegmental area to lateral habenula in aversive conditioningJ Neurosci 34:13906–13910https://doi.org/10.1523/JNEUROSCI.2029-14.2014
- Activation of VTA GABA neurons disrupts reward seeking by altering temporal processingBehav Brain Res 410https://doi.org/10.1016/j.bbr.2021.113292
- Gene expression and neurochemical characterization of the rostromedial tegmental nucleus (RMTg) in rats and miceBrain Struct Funct 224:219–238https://doi.org/10.1007/s00429-018-1761-7
- Anatomic resolution of neurotransmitter-specific projections to the VTA reveals diversity of GABAergic inputsNat Neurosci 23:968–980https://doi.org/10.1038/s41593-020-0657-z
- Circuit coordination of opposing neuropeptide and neurotransmitter signalsNature 619:332–337https://doi.org/10.1038/s41586-023-06246-7
- Periaqueductal Gray and Rostromedial Tegmental Inhibitory Afferents to VTA Have Distinct Synaptic Plasticity and Opiate SensitivityNeuron 106:624–636https://doi.org/10.1016/j.neuron.2020.02.029
- A unique population of ventral tegmental area neurons inhibits the lateral habenula to promote rewardNeuron 80:1039–1053https://doi.org/10.1016/j.neuron.2013.08.023
- Electrophysiological characterization of GABAergic neurons in the ventral tegmental areaJ Neurosci 18:8003–8015https://doi.org/10.1523/JNEUROSCI.18-19-08003.1998
- GABA neurons of the VTA drive conditioned place aversionNeuron 73:1173–1183https://doi.org/10.1016/j.neuron.2012.02.015
- GABAergic and glutamatergic efferents of the mouse ventral tegmental areaJ Comp Neurol 522:3308–3334https://doi.org/10.1002/cne.23603
- Heterogeneity and Diversity of Striatal GABAergic Interneurons: Update 2018Front Neuroanat 12https://doi.org/10.3389/fnana.2018.00091
- Heterogeneity and diversity of striatal GABAergic interneuronsFront Neuroanat 4https://doi.org/10.3389/fnana.2010.00150
- A Designer AAV Variant Permits Efficient Retrograde Access to Projection NeuronsNeuron 92:372–382https://doi.org/10.1016/j.neuron.2016.09.021
- The neurobiology of opiate motivationCold Spring Harb Perspect Med 2https://doi.org/10.1101/cshperspect.a012096
- Inhibitory Interactions Between Spiny Projection Neurons in the Rat StriatumJ Neurophysiol :1263–1269https://doi.org/10.1152/jn.2002.88.3.1263
- Activation of VTA GABA neurons disrupts reward consumptionNeuron 73:1184–1194https://doi.org/10.1016/j.neuron.2012.02.016
- Rewarding Effects of Optical Stimulation of Ventral Tegmental Area Glutamatergic NeuronsJ Neurosci 35:15948–15954https://doi.org/10.1523/JNEUROSCI.3428-15.2015
- Mesoaccumbal glutamate neurons drive reward via glutamate release but aversion via dopamine co-releaseNeuron 112:488–499https://doi.org/10.1016/j.neuron.2023.11.002
- Intravenous GABA agonist administration stimulates firing of A10 dopaminergic neuronsEur J Pharmacol 66:141–144https://doi.org/10.1016/0014-2999(80)90308-8
- Mesocorticolimbic glutamatergic pathwayJ Neurosci 31:8476–8490https://doi.org/10.1523/JNEUROSCI.1598-11.2011
- Effect of picrotoxin and nipecotic acid on inhibitory response of dopaminergic neurons in the ventral tegmental area to stimulation of the nucleus accumbensBrain Res 199:466–473https://doi.org/10.1016/0006-8993(80)90705-2
- Ventral tegmental area glutamate neurons co-release GABA and promote positive reinforcementNat Commun 7https://doi.org/10.1038/ncomms13697
- VTA Glutamate Neuron Activity Drives Positive Reinforcement Absent Dopamine Co-releaseNeuron 107:864–873https://doi.org/10.1016/j.neuron.2020.06.011
- Activity of a direct VTA to ventral pallidum GABA pathway encodes unconditioned reward value and sustains motivation for rewardSci Adv 8https://doi.org/10.1126/sciadv.abm5217
Article and author information
Author information
Version history
- Sent for peer review:
- Preprint posted:
- Reviewed Preprint version 1:
Copyright
© 2024, Oriol et al.
This article is distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use and redistribution provided that the original author and source are credited.
Metrics
- views
- 426
- downloads
- 12
- citations
- 0
Views, downloads and citations are aggregated across all versions of this paper published by eLife.