Abstract
One of the primary outputs of the nucleus accumbens is directed to the mediodorsal thalamic nucleus (MD) via its projections to the ventral pallidum (VP), with the core andshell regions of the accumbens projecting to the lateral and medial aspects of the VP, respectively. In this study, the multisynaptic organization of nucleus accumbens projections was assessed using intracerebral injections of an attenuated strain of pseudorabies virus, a neurotropic α herpesvirus that replicates in synaptically linked neurons. Injection of pseudorabies virus into different regions of the MD or reticular thalamic nucleus (RTN) produced retrograde transynaptic infections that revealed multisynaptic interactions between these areas and the basal forebrain. Immunohistochemical localization of viral antigen at short postinoculation intervals confirmed that the medial MD (m-MD) receives direct projections from the medial VP, rostral RTN, and other regions previously shown to project to this region of the thalamus. At longer survival intervals, injections confined to the m-MD resulted in transynaptic infection of neurons in the accumbens shell but not in the core. Injections that also included the central segment of the MD produced retrograde infection of neurons in the lateral VP and the polymorph (pallidal) region of the olfactory tubercle (OT) and transynaptic infection of a small number of neurons in the rostral accumbens core. Injections in the lateral MD resulted in retrograde infection in the globus pallidus (GP) and in transynaptic infection in the caudate-putamen. Viral injections into the rostroventral pole of the RTN infected neurons in the medial and lateral VP and at longer postinoculation intervals, led to transynaptic infection of scattered neurons in the shell and core. Injection of virus into the intermediate RTN resulted in infection of medial VP neurons and second-order infection of neurons in the accumbens shell. Injections in the caudal RTN or the lateral MD resulted in direct retrograde labeling of cells within the GP and transynaptic infection of neurons in the caudate-putamen. These results indicate that the main output of VP neurons receiving inputs from the shell of the accumbens is heavily directed to the m-MD, whereas a small number of core neurons appear to influence the central MD via the lateral VP. Further segregation in the flow of information to the MD is apparent in the organization of VP and GP projections to subdivisions of the RTN that give rise to MD afferents. Collectively, these data provide a morphological basis for the control of the thalamocortical system by ventral striatal regions, in which parallel connections to the RTN may exert control over activity states of cortical regions.
- transneuronal tracing
- reticular thalamic nucleus
- ventral pallidum
- nucleus accumbens
- mediodorsal thalamic nucleus
- prefrontal cortex
- globus pallidus
- pseudorabies virus
The nucleus accumbens, which is the ventral extension of the striatum, has been implicated in a number of psychiatric diseases such as schizophrenia (Snyder, 1973; Matthysse, 1981; Csernansky et al., 1991; Gray et al., 1991; Grace, 1992) and Tourette’s syndrome (Comings, 1987; Braun et al., 1993). This structure is believed to subsume an integrative role in higher cortical functions, given its position as an interface between limbic and motor systems (Mogenson et al., 1980). The multisynaptic circuitry linking the striatum [i.e., the nucleus accumbens and caudate–putamen (CPu)] and basal forebrain with cortical areas is organized in the form of several parallel loops (Alexander and Crutcher, 1990; Berendse and Groenewegen, 1990; Groenewegen et al., 1990). The nucleus accumbens receives glutamatergic projections from the prefrontal cortex (PFC) (Beckstead, 1979; Fuller et al., 1987), hippocampus (DeFrance and Yoshihara, 1975; Kelley and Domesick, 1982; DeFrance et al., 1985), and amygdala (Swanson and Cowan, 1975; Groenewegen et al., 1980; McDonald, 1991) that converge on single accumbens neurons (O’Donnell and Grace, 1995b). In turn, the accumbens sends its primary output to the ventral pallidum (VP) (Heimer and Wilson, 1975; Mogenson et al., 1983), which inhibits thalamocortical activity by way of its projections to the mediodorsal thalamic nucleus (MD) (Young et al., 1984; Haber et al., 1985; Lavı́n and Grace, 1994).
Two major subdivisions of the nucleus accumbens have been defined according to distinct anatomical connections (Heimer et al., 1991; Brog et al., 1993; Zahm and Heimer, 1993). The portion of the nucleus accumbens surrounding the anterior commissure, known as thecore, has been reported to receive its primary cortical input from the prelimbic (PL) PFC (Sesack et al., 1989; Berendse et al., 1992; Brog et al., 1993; Montaron et al., 1996) and dorsal subiculum (Groenewegen et al., 1991; Brog et al., 1993) and projects to the dorsolateral aspect of the VP (Zahm and Heimer, 1990; Heimer et al., 1991). On the other hand, the medial-ventral aspect of the accumbens, called the shell, receives input primarily from the infralimbic (IL) PFC (Berendse et al., 1992; Brog et al., 1993) and the ventral subiculum (Kelley and Domesick, 1982; Yang and Mogenson, 1984; Sesack and Pickel, 1990; Aylward and Totterdell, 1993; Brog et al., 1993) and sends projections to the ventromedial part of the VP (Zahm and Heimer, 1990; Heimer et al., 1991). In addition to differences in their connectivity, the core and shell regions of the nucleus accumbens differ in neurochemical markers (Záborszky et al., 1985; Meredith et al., 1989, 1996; Deutch and Cameron, 1992;Jongen-Rêlo et al., 1994a,b), cell morphology (Meredith et al., 1992, 1993; O’Donnell and Grace, 1993b), physiological properties (Pennartz et al., 1992; O’Donnell and Grace, 1993a,b; Onn and Grace, 1995), and responses to pharmacological and behavioral manipulations (Deutch et al., 1992; Kalivas and Duffy, 1995;O’Donnell and Grace, 1995a).
The present study was designed to determine whether the pathways originating in the core and shell regions of the accumbens remain segregated within the VP and in the efferent projections of this area to the thalamocortical system. Although the primary thalamic target of the VP is the MD (Young et al., 1984; Haber et al., 1985; Heimer et al., 1991; Groenewegen et al., 1993), a projection from the VP to the reticular thalamic nucleus (RTN) has also been reported in the rat (Cornwall et al., 1990; Groenewegen et al., 1993). Furthermore, electrical stimulation of the lateral VP induces occasional monosynaptic responses in the rat RTN (Lavı́n and Grace, 1994), suggesting that a subset of VP neurons may project to the RTN. Nonetheless, the multisynaptic organization of the accumbens-VP-thalamic connectivity has been difficult to establish with conventional tract tracing or electrophysiological approaches, because these methods only define one order of synaptic contact. Therefore, resolution of the organization of connections between the nucleus accumbens and thalamus requires a tracer that will cross synapses and label second-order synaptically linked neurons. This was achieved by using a neurotropic swine α herpesvirus (pseudorabies virus, PRV) that has proven to be an effective tracer of multisynaptic pathways in a variety of systems (for review, see Card and Enquist, 1994; Loewy, 1995; Ugolini, 1995; Enquist and Card, 1996). The experimental approach used in this study is based on the demonstrated ability of this family of neurotropic viruses to replicate within synaptically linked populations of neurons after intracerebral injection (Zemanick et al., 1991; Middleton and Strick, 1994). Our data demonstrate a segregation of multisynaptic projections through the VP that arise in either the core or shell of the accumbens and terminate in either the MD or reticular thalamic nuclei.
Parts of these data were presented at the 1995 Society for Neuroscience meeting (O’Donnell et al., 1995).
MATERIALS AND METHODS
Animal handling and preparation. Adult male Sprague Dawley rats (200–420 gm at time of virus injection) were used in these experiments. They were housed in pairs with food and water availablead libitum, and under a 12:12 hr light/dark cycle (light on at 6:00 A.M.). Animal handling and experimental protocols were in accordance with the NIH Guide for the Care and Use of Laboratory Animals and were approved by the University of Pittsburgh Animal Care and Use Committee. Injections of PRV were administered to anesthetized animals in a Biosafety Level 2 containment facility in accordance with regulations stipulated in Health and Human Services Publication No. 88–8395 entitled “Biosafety in Microbiological and Biomedical Laboratories”. Animals were inoculated, housed, and killed in this facility.
Virus. An attenuated strain of PRV (Bartha strain) was used in this study. The virus, initially developed as a swine vaccine in 1961 (Bartha, 1961), exhibits reduced virulence compared with wild-type strains and replicates efficiently in rodent CNS (Enquist, 1994; Card and Enquist, 1995). It has been used extensively for characterizing multisynaptic circuits associated with the visual system (Card et al., 1991, 1992; Moore et al., 1995) and autonomic nervous system (Strack et al., 1989; Card et al., 1990, 1993; Strack and Loewy, 1990; Jansen et al., 1992, 1995; Nadelhaft et al., 1992; Standish et al., 1995; Vizzard et al., 1995). More recently, intracerebral injection of this strain of virus has been shown to produce retrograde transneuronal patterns of infection (Enquist et al., 1993; Leak et al., 1995). The virus used in the present study was grown in PK 15 cells to a titer of 1.4 × 109 plaque forming units (pfu) per milliliter. Procedures for growing and harvesting the virus have been published elsewhere (Enquist and Card, 1996). Aliquots of virus were stored at −80°C before use and thawed immediately before injection. Unused portions of each aliquot were inactivated with Chlorox and discarded.
Antibodies. A rabbit polyclonal antiserum (Rb134) generated against acetone-inactivated virus was used to localize infected neurons. The serum recognizes numerous virion proteins and produces robust immunohistochemical staining of the somata and dendrites of PRV-infected neurons (Card and Enquist, 1994). Rb134 was used at a dilution of 1:10,000. In some cases, PRV was co-injected with the β fragment of cholera toxin (CT), a conventional tracer that identifies one order of synaptic contact. A goat polyclonal antiserum (List Biochemicals, Campbell, CA) was used at a 1:20,000 dilution to localize CT in tissue from these animals.
Calbindin immunolocalization provided a precise definition of the boundaries of the core and shell regions of the nucleus accumbens. This calcium-binding protein is densely concentrated in the accumbens core and absent in the shell (Zahm and Heimer, 1993), and it has been shown to be the most accurate marker for core–shell boundaries (Jongen-Rêlo et al., 1994b). Calbindin was localized using a rabbit polyclonal antiserum at a final dilution of 1:20,000. The extent of the electrolytic lesion in two animals lesioned in the VP and globus pallidus (GP) (see following section) was assessed by means of immunohistochemical localization of glial fibrillar acidic protein, an intermediate filament protein found within astrocytes, with a mouse monoclonal antibody (Chemicon, Temecula, CA) used at a dilution of 1:10,000.
Injection procedures. Animals were anesthetized with ketamine and xylazine (60 mg/kg ketamine, 7 mg/kg xylazine, i.p.) before being placed in a stereotaxic apparatus (Kopf, Tujunga, CA). Virus was injected through a 1 μl Hamilton syringe lowered into target areas through a hole drilled in the skull. The stereotaxic coordinates used, obtained from a rat brain stereotaxic atlas (Paxinos and Watson, 1986), were as follows. For the medial segment of the MD (m-MD; 10 rats) coordinates were anteroposterior (AP): −3.2, mediolateral (ML): 0.5, dorsoventral (DV): −5.9; for the central segment of the MD (c-MD; 5 rats), AP: −3.2, ML: 0.7, DV: −5.8; and for the lateral segment of the MD (l-MD; 6 rats), AP: −3.3, ML: 1.0, DV: −5.7. Injections in the RTN were grouped in the following three rostrocaudal locations. The rostral pole of the RTN (AP: −1.3 to −1.5, ML: 1.6, DV: −6.3; 2 rats); the intermediate RTN (AP: −1.5 to −2.0, ML: 2.0, DV: −6; 2 rats); and the caudal RTN (AP: −2.0 to −3.3, ML: 3.8, DV: −5.6; 4 rats). A total of 100–200 nl of the PRV-Bartha (1–2 × 105 pfu) was injected at a rate of 10 nl/min, and the syringe was left in place for an additional 5 min to reduce reflux of the viral inoculum up the cannula tract. A subset of animals were injected with a mixture of PRV and the β subunit of CT. The CT was diluted to 0.25% with isotonic saline, whereupon 10 μl was mixed with 10 μl of PRV and 200 nl (2 × 105pfu) of the mixture was injected intracerebrally at 10 nl/min. The concentration of virus injected in all experiments produces an infection in 100% of animals after intravitreal inoculation (Card et al., 1995).
Two animals received an electrolytic lesion in the VP or the GP before receiving the PRV injection into the MD. The lesions were performed under deep anesthesia using a coated insect pin and a current generator (Grass, Quincy, MA). Monopolar current (4 mA for 20 sec) was passed though the electrode, placed in the rostral VP region (AP: 0.2, ML: 0.8, DV: −8.3). After recovery, the animals were returned to their home cage. One week later, PRV was injected into the m-MD, and the animals were killed for immunohistochemical detection of viral infection in the neuraxis at 60 and 62 hr postinoculation.
Tissue processing. After postinoculation periods ranging from 36 to 72 hr, the animals were deeply anesthetized with an overdose of ketamine and xylazine and perfused transcardially with a buffered aldehyde fixative (McLean and Nakane, 1974). The brains were removed, post-fixed for 1 hr at 4°C, and cryoprotected in 20% sucrose in 0.1m phosphate buffer for a minimum of 12 hr before they were cut using a freezing microtome. The entire brain was sectioned serially in the coronal plane at 35 μm per section and collected sequentially in six bins of buffer. One bin of tissue was processed immediately for immunohistochemical localization of viral antigen using the avidin–biotin modification of the immunoperoxidase procedures (Hsu et al., 1981) and Vectastain Elite reagents (Vector Laboratories, Burlingame. CA). The details of this procedure, as it is applied in our laboratory, have been published (Card and Enquist, 1994). The remaining bins of tissue were transferred to a cryopreservant (Watson et al., 1986) and stored at −20°C to preserve antigenicity. Some of this tissue was subsequently processed with Rb134 to provide more frequent series of sections for analysis of viral transport. Other bins of tissue were processed for localization of CT immunoreactivity to define first-order connections or for immunohistochemical localization of calbindin to define core–shell boundaries.
RESULTS
PRV was injected intracerebrally in 52 rats. Twenty-nine of these animals contained injection sites that included one or more of the subdivisions of the MD or the RTN. Twelve animals contained injections that missed the MD or RTN. These cases were used as controls for the specificity of the results obtained from injection of virus into either the MD or the RTN. In two cases, electrolytic lesions of the VP or GP preceded injection of virus into the m-MD. Eleven cases were discarded because of poor placement of the injection (n = 7) or failure to detect viral immunoreactivity at short postinoculation intervals (n = 4; 36–44 hr survival). Temporal analysis of the extent of viral replication and transport indicated that postinoculation survival intervals of 36–50 hr were the most effective time span for characterizing the multisynaptic connections between the MD, RTN, and nucleus accumbens. At longer survival intervals, the more extensive transynaptic passage of virus made it more difficult to ascertain the routes of viral transport.
Diffusion of PRV from the injection site
Controlled injection of PRV resulted in very little diffusion of virus from the site of injection, as demonstrated by the restricted distribution of infected cells at injection sites, even at the longest postinoculation intervals (Fig.1A,C,E; see also Figs. 3A, 5A, 6A,7A). Analysis of viral immunoreactivity at the injection sites in closely spaced sections revealed that infected neurons were confined to the immediate vicinity of the injection cannula. The effective area of viral injection, as defined by the distribution of neurons displaying viral immunoreactivity, ranged between 100 and 500 μm in diameter surrounding the tip of the cannula. Injection of equivalent volumes of PRV produced smaller injection sites in the m-MD compared with the l-MD (compare Figs. 3A and 5A), and the injections in any region of the RTN produced the largest injection sites (see Figs. 6A, 7A). Co-injection of the β subunit of CT with the viral inoculum resulted in more extensive diffusion of CT from the injection site. An example of the differing extents of diffusion of CT and PRV from the same injection is shown in Figure 1. In this case, which is representative of all of those incorporating the co-injection paradigm (n = 10), PRV immunoreactive neurons were confined to a single segment of the MD (Fig.1A,C,E), whereas CT immunoreactivity extended into other subdivisions of the MD as well as into adjacent thalamic nuclei (Fig.1B,D,F).
Temporal analysis and specificity of transynaptic passage of PRV
Intracerebral injection of PRV produced patterns of neuronal infection consistent with retrograde transneuronal passage of virus from the site of injection, as shown by temporal analysis of viral replication and transport and the co-extensive distribution of PRV- and CT-labeled neurons at sites of first-order projection. We analyzed the distribution of viral infection at various postinoculation intervals as an initial means of determining first- and second-order infections and used the co-injection of a classical tracer (the β fragment of CT) to define further the pattern of first-order infection at longer postinoculation intervals. The absence of anterograde viral transport from the site of injection was established by comparing the patterns of infection with the known connectivity of these regions, as shown in previous investigations using conventional tracers. Using this approach, we were unable to demonstrate any evidence of anterograde transport of virus, either from the site of injection or through a multisynaptic circuit. A good example of this can be found in the patterns of infection resulting from injections in the MD, which failed to produce an anterograde transneuronal infection of layers II or III of PFC regions but did produce a retrograde infection of projection neurons in deeper cortical layers (Fig. 2). Furthermore, injections of virus that involved the m-MD resulted in infection of neurons located in the rostral pole of the RTN, which is known to project to the m-MD. Injections into the same region of the RTN failed to induce infection of neurons in the m-MD, which should be expected if the virus were anterogradely transported.
The temporal aspects of viral replication allowed us to distinguish first- and second-order infection in neurons. Continued replication of virus in neurons that projected directly to the injection sites (first-order neurons) eventually produced pathological changes in the neurons and, at the longest postinoculation intervals, such neurons were associated with immunoreactive glia (Fig.3E,F). In contrast, neurons in synaptic contact with the initially infected neurons (second-order neurons) exhibited fewer pathological changes (Fig. 3E,G), because the virus had undergone replication in these neurons for a shorter period of time. Thus, temporal order can be inferred by the degree of pathological changes in the infected neurons and the association of infected glia. The significance of the glial response in maintaining specific transynaptic passage of PRV has been published (Card et al., 1993;Rinaman et al., 1993) and is considered in greater detail in Discussion.
Transport of virus from the MD
m-MD (n = 8)
PRV was confined to the m-MD in two animals that survived 49 hr. The injection site in one case (94-H38; Fig.3A,B) covered the m-MD throughout most of its rostrocaudal extent, whereas in the other animal (94-H39), the injection site was limited to the caudal third of the m-MD. Although the survival times were similar in both animals, the extent of infection was less in the case in which the injection was restricted to the caudal m-MD. Large numbers of infected neurons were observed in the VP in both animals, particularly in the ventral and medial aspects of its rostral extent, at the region bordering the nucleus of the diagonal band of Broca (NDBB) (Fig.3E,F). Infected neurons were also found in the rostral and intermediate regions of the RTN, but not in its caudal region. All these cells showed signs of advanced viral infection and were associated with infected glia, suggesting that they gave rise to a first-order, direct projection to the m-MD. Labeling in the striatal regions involved only the accumbens shell, predominantly in its caudal aspect (Fig. 3E,G), as defined by the distribution of calbindin immunoreactivity (Fig.3D). A clear temporal organization was observed in the infection of these neurons compared with neurons in the medial VP. Infection of medial VP neurons always preceded infection of shell neurons (compare Fig. 3, C and E). Similarly, when both populations were infected, neurons in the medial VP always showed signs of more advanced viral replication (Fig.3E–G). No infected neurons were present in the CPu and accumbens core of these cases.
Injection in the m-MD also revealed a first-order infection of the RTN. In cases in which the injection site was confined to the m-MD, we observed a large number of infected neurons in the rostral and intermediate RTN and no infected neurons at caudal levels of the RTN (compare Fig. 4, A and B). Furthermore, infected neurons in rostral and intermediate regions of the RTN were confined to the ventral third of the nucleus (Fig.4B).
Several injections that included the m-MD also extended into neighboring regions. Two animals received PRV injections that involved the paraventricular nucleus of the thalamus (PVT) (94-H40 and 94-H41). These animals were killed at 39 and 51 hr after injection and, as in the MD injected cases, they contained first-order infected neurons in the medial VP and rostral RTN and second-order neurons in the shell region of the accumbens. Two additional animals with an injection site that involved the m-MD, PVT, and habenula (cases 94-H22 and 95-H6) exhibited a similar pattern of infection, as seen in other animals in which the injection involved the m-MD along with either the lateral habenula (94-H13) or the anteromedial thalamic nucleus (95-H148). All these cases also exhibited infected neurons consistent with projections to these other thalamic nuclei. For example, cases involving the PVT contained large numbers of infected neurons in the hypothalamic suprachiasmatic nuclei, consistently with the recently demonstrated projection between these nuclei (Moga et al., 1995). In contrast, cases in which the injection was confined to the m-MD did not exhibit infected neurons in the suprachiasmatic nucleus.
C-MD (n = 5)
Five animals received viral injections in regions that included the c-MD and were killed 39 to 52 hr after the viral injection. However, none of the injection sites were actually restricted to this relatively small subdivision. The injection sites covered most of the c-MD and part of l-MD in two animals (95-H149 and 96-H6) (Fig.5A) and most of c-MD and part of m-MD in the other three cases (95-H7, 94-H21, and 96-H5). All of these animals showed advanced infection of a large number of neurons in the polymorph region of the OT (Fig. 5D) as well as in the lateral, subcommissural region of the caudal VP (Fig.5E,F). In cases including the l-MD in the injection site (Fig. 5A), first-order projection cells were also detected in the GP (Fig. 5C), and in cases in which the injection also involved the m-MD, cells with advanced infection were detected in the medial, rostral VP. Infection in striatal regions varied according to the extent of the injection site in these cases. We never observed infection of accumbens shell neurons when the injection was restricted to the c-MD and l-MD (Fig.5D). When injections involved the c-MD along with either the lateral or medial segments, we observed a limited number of infected core neurons that were found almost exclusively at rostral levels in the core (Fig. 5G). In contrast, when the viral injection was confined to the l-MD, we never observed infected neurons in either of the accumbens regions (see below). A few scattered infected cells at an early stage of infection at the septal border of the shell region of the accumbens, as well as some infected cells in the core region of the accumbens, were found in the cases in which the injection included the m-MD and the c-MD. A few infected cells in the core and the CPu were observed in the cases in which injections covered both the c-MD and l-MD.
Cells in the RTN were also infected after injections that included the c-MD (Fig. 5B). The distribution of infected RTN neurons was different depending on the involvement of the m-MD or l-MD in the injection site. The animals in which PRV was injected in the m-MD and c-MD showed infected neurons in the rostral pole of the RTN, similar to those with an injection selectively placed within the m-MD. On the other hand, injections in the l-MD and c-MD resulted in infection of neurons in more caudal parts of the RTN (Fig. 5B), similar to that observed after injections restricted to the l-MD (see below). Thus, these patterns appear to be the result of transynaptic passage after m-MD and l-MD PRV rather than after c-MD PRV.
L-MD (n = 5)
Five animals received injections within the l-MD that largely excluded the c-MD. Four animals were examined after survival periods of 44 to 50 hr. In one of these cases (94-H18), the injection site encompassed the caudal half of the l-MD, whereas the other two animals (94-H12 and 95-H150) received the PRV injection in the l-MD and the lateral habenula. Infected neurons at an advanced stage were detected in the GP, but no infected cells were seen in the VP. In addition, neurons at an early stage of infection were detected in the CPu but not in the accumbens. In these cases, cells in advanced stages of infection were also seen in the caudal aspects of the RTN.
Two animals were killed after relatively long survival periods (∼68 hr) that yielded a widespread infection that was extensive across most of the structures studied. The injection site in one of these animals (94-H7) was centered in the caudal third of the l-MD and extended into the lateral habenula in the other (94-H9). Both animals exhibited infected neurons in the VP at different stages of infection. Several neurons showing signs of advanced infection could be observed in the GP as well. Few scattered infected cells could be observed in both the core and the shell regions of the nucleus accumbens in one case (94-H7), and only in the shell in the other (94-H9). The sparse number of infected neurons in the nucleus accumbens contrasted to the heavy labeling throughout most other structures in these cases.
Control experiments (n = 8)
In two cases, PRV injections were made into the m-MD in rats that had received an electrolytic lesion of the medial VP or the GP. The injection sites in these cases were restricted to the m-MD. These animals were killed after long incubation periods of 60 and 62 hr. In one case with a GP lesion that spared most of the VP (95-H63), neurons at an advanced stage of infection were observed in the medial VP, and neurons earlier in the course of infection were detected in the accumbens shell. In the case with an extensive lesion of the VP (95-H64), PRV injection in the m-MD failed to label neurons in the shell.
Three animals received viral injections in regions adjacent to, but avoiding entirely, the m-MD. In one of the cases, the injection included the medial habenula and the overlying dentate gyrus of the hippocampus (94-H17), and no infected neurons could be detected in striatal or pallidal regions. In another animal (95-H11), PRV was injected in the dentate gyrus of the hippocampus, and no viral immunoreactivity was observed in any basal ganglia or thalamic region. A third case received the PRV injection into the lateral septum with spread of virions into the lateral ventricle (95-H78), but no viral infection could be detected in the basal ganglia.
Two additional animals received PRV injections in structures close to, but not in, the l-MD. In one case (95-H8), PRV was injected into the ventricle. No labeling was found in the basal ganglia in this animal. In another animal (94-H47), PRV was injected in the laterodorsal thalamic nucleus, which is located laterally to the MD. In this case, infected neurons were observed in the septum and NDBB but not in the basal ganglia.
The injection site in another animal encompassed all three segments of the MD (case 95-H9), and the pattern of viral infection was similar to that of the cases of injection in each segment combined. Thus, heavily infected neurons were observed in the medial and lateral VP as well as in the GP, and second-order neurons were detected in the shell and core regions of the accumbens as well as in the CPu.
Transport of virus from the RTN
The injection sites that included the RTN were distributed along most of the rostrocaudal axis of this thalamic nucleus. To analyze the results without losing any potential topographic information, the cases were sorted according to the location of the center of injection along the rostrocaudal axis.
Rostral RTN (n = 2)
Two animals received PRV injections in the rostral pole of the RTN and were killed 48 and 50 hr after the injection. The injection site included the ventral aspect of the rostral RTN in one case (94-H45; Fig. 6A), in the same region of the RTN that showed infection after m-MD injections. In this case, neurons at a comparatively advanced stage of infection were observed in the medial/rostral VP (Fig. 6F) as well as in the lateral and caudal aspects of the VP (Fig. 6B). Also, scattered neurons very early in their infection were observed in both the accumbens core and shell (Fig.6F,G). The other animal (case 95-H143) received the PRV injection into the ventral and dorsal aspects of the RTN rostral pole. In this case, first-order projection neurons were observed in the lateral and caudal VP as well as in the GP. Neurons at an early stage of infection were detected in the accumbens core and CPu. No infected cells were found in the accumbens shell in any of these cases. In the animal injected in the ventral aspect of the rostral RTN, neurons advanced in infection were detected in the c-MD but not in the m-MD. In the other, more extensively injected, case, heavily infected neurons were detected in the c-MD and l-MD (Fig.6C–E).
Intermediate RTN (n = 2)
Two cases were injected in the intermediate region of the RTN. In one of them (95-H145), neurons advanced in infection were observed in the medial and rostral VP and in the m-MD. The distribution of first-order projection neurons was matched by CT immunoreactivity in this animal (see Fig. 10). Neurons at an early stage of infection were detected in the accumbens shell. In the other case (95-H75), which received the PRV injection at a more dorsal location within the intermediate RTN, no viral infection could be found in any pallidal or striatal region.
Caudal RTN (n = 4)
Four animals received the PRV injection at caudal locations within the RTN. Two of these animals received the injections at 2.0–2.5 mm caudal to bregma. In one of them (case 94-H46), the injection site was tightly confined to the RTN (Fig.7A,B), and no detectable infection was observed in the accumbens or VP. The other case with a similar injection site (95-H12) extending medially into the VPL thalamic nucleus did not result in viral infection in the accumbens or VP. However, both cases exhibited a large number of neurons advanced in infection within the GP (Fig.7D,E) and some infected neurons in the l-MD (Fig. 7C). Cells in early stages of infection were detected in the CPu (Fig. 7F). In two other animals, the injection site was placed at even more caudal locations within the RTN; i.e., 3.0 or 3.3 mm caudal to bregma. In these cases (95-H76 and 95-H146), no infected cells were labeled in any region within the basal ganglia.
Control injections for the RTN (n = 7)
A group of animals received PRV injection in the vicinity of the RTN rostral pole but without including the RTN. Three cases involved the bed nucleus of the stria terminalis (BNST) rostral to the RTN (cases 94-H44, 94-H49, and 94-H51). In these cases, neurons at an advanced stage of infection were detected in the medial and rostral VP, and neurons with early infections were seen in the accumbens shell, but not in the core, which is a different pattern from that of rostral RTN injections. In two additional animals (cases 94-H48 and 95-H14), the injection sites were restricted to the internal capsule with a little involvement of the GP in one, just lateral to where the rostral RTN injections were placed. Although widespread infection was seen throughout most of the neocortex in those cases in which tissue damage was present at the injection sites, no infected neurons were detected in the accumbens or VP. In the case in which the GP was included in the injection site, however, heavily infected cells were detected in the CPu.
Two animals received PRV injection in regions adjacent to the caudal RTN. One of them received the viral injection in the lateral geniculate nucleus and dentate gyrus of the hippocampus (case 95-H13). In this animal, neurons advanced in infection were observed in the dorsomedial hypothalamus but not in the basal ganglia. Another animal (case 95-H77) received the injection in the internal capsule, in a site located laterally to that of the caudal RTN injection cases. In this animal, no evidence of infected neurons was observed in the basal ganglia, although extensive labeling was detected in most cortical regions.
Other circuits labeled after MD and RTN injections
The cortical regions retrogradely infected after PRV injections in the MD also differ according to the segment injected. Thus, injections in the m-MD resulted in viral infection in the infralimbic, medial orbital, and agranular insular cortices. In the cases in which the injection sites included the c-MD, neurons advanced in infection were detected in orbital and PL cortices. In addition, selective injections in the l-MD resulted in first-order infected neurons in the piriform and cingulate cortices. Injections in the rostral RTN resulted in infected neurons in cingulate and PL cortices, whereas injections in the caudal RTN labeled the cingulate cortex.
In addition to structures in the basal ganglia, basal forebrain, and cortex, a number of other brain regions exhibited viral immunoreactivity after PRV injections in the different divisions of the MD or RTN. These were different for each of the regions studied, and they were consistent with previously reported data using conventional tract tracing techniques. The brain regions in which we observed neurons with advanced infection (first order) and neurons with early stages of infection (second order) are listed in Tables 1 and 2. Briefly, injections in the m-MD resulted in viral infection in NDBB, VTA, and laterodorsal tegmental nucleus (LDTg) (Fig. 8). In the cases in which the injections sites extended into the PVT, cells at an advanced stage of infection were also found in the suprachiasmatic nucleus and dorsomedial hypothalamus. In the cases in which the injection sites included the c-MD, neurons advanced in infection were detected in the lateral septum, OT, NDBB, and LDTg (Fig. 9). In the cases injected in the l-MD, infected neurons were seen in lateral septum, NDBB, raphe magnus, substantia nigra pars reticulata, and LDTg (Fig. 10).
Injections in the rostral RTN resulted in infected neurons at a relatively advanced stage in the medial nucleus of the amygdala, SI, NDBB, septum, VPL and VPM thalamic nuclei, pedunculopontine nucleus, LDTg, and contralateral RTN (Fig. 11). Injections in the intermediate RTN labeled the m-MD and LDTg (Fig.12). Also, injections in the caudal RTN resulted in advanced neuronal infection in the medial nucleus of the amygdala, SI, BNST, VPL-VPM thalamic nuclei, and SNc (Fig. 13).
DISCUSSION
An important issue in correlating the anatomy of the limbic system with psychiatric disorders lies in the specificity of connections among key components of these systems. Although studies using sequential labeling of retrogradely transported compounds have been powerful in assessing such connections, the existence of several multisynaptic pathways presents unique constraints that render such an approach problematic. For this reason, we used PRV for tracing transynaptic projections from the core and shell regions of the nucleus accumbens to the VP and thalamus. The affinity of the virus for axon terminals and astrocytes (Vahlne et al., 1978, 1980; Marchand and Schwab, 1986) permits discrete injections of subfields in the thalamic target nuclei; only the VP cells projecting to the injection site will become infected by retrograde transport of virus, and furthermore, only accumbens neurons that specifically synapse with the retrogradely infected VP cells will exhibit transynaptic and second-order infection. In this way, we can determine with confidence the specificity of accumbens output projections to the VP and thalamus.
Specificity of viral labeling
Controlled intracerebral injection of PRV into the MD or RTN produced highly restricted cell labeling at the site of injection that was confined to the subdivisions of the MD or RTN in many cases. This technique has been used previously to assess the central neural connections labeled after injections of virus into peripheral structures (for review, see Card and Enquist, 1994; Loewy, 1995; Mettenliter, 1995; Enquist and Card, 1996). However, because this study used intracerebral injections, one issue that should be carefully addressed is the potential of the virus to diffuse away from the injection site and infect neighboring cells, an event that may confound interpretation. We were able to control for such a possibility by using animals in which the injections were made into structures surrounding, but not including, the MD and RTN. The remarkable differences in labeling between MD/RTN injections and these controls argue strongly against the possibility that the results may be confounded by the diffusion of virus into the area surrounding the injection site. Thus, structures such as the VP or NDBB that were consistently labeled after MD/RTN injections were not infected after injections in the septum, BNST, internal capsule, or habenula. The results clearly show that injections confined to the medial, c-MD, or l-MD infect restricted sets of afferent sources, suggesting that there is little, if any, spread of virus onto the neighboring MD segments. Therefore, PRV-Bartha can be used effectively as a specific transynaptic tracer in the CNS.
The direction of viral transport was an important consideration in interpreting our findings. Zemanick and colleagues (1991) have reported differential transport of two strains of HSV from the primate motor cortex after intracerebral injection, with one strain passing only in an anterograde transynaptic direction and the other exclusively in a retrograde transynaptic direction. In preliminary studies (Enquist et al., 1993), we also observed differential transport of two strains of PRV injected into the rat PFC. Wild-type virus was transported in both directions (anterograde and retrograde) from the injection site, whereas the attenuated PRV-Bartha strain only moved in a retrograde transynaptic manner. The results of the present study support the unidirectional retrograde passage of PRV-Bartha after intracerebral injection and demonstrate the utility of this virus for defining multisynaptic circuitry. The mechanisms that lead to the restricted transport of PRV-Bartha compared with wild-type virus remain to be established, but may be related to the deletions of envelope glycoprotein genes known to characterize this strain (Enquist, 1994).
A potential source of concern relates to whether viral uptake by fibers of passage may have confounded our results. As mentioned above, the virus has a high affinity for axon terminals and astrocytes. Thus, if substantial tissue damage is avoided at the injection site, virions are not likely to enter intact fibers of passage. Our cases involving internal capsule injections show widespread cortical infection. However, these were designed to test whether the spread of virus beyond the injection site could account for any of our results; and furthermore were provided by exceedingly large injections coupled with long survival times. Thus, the presence of tissue damage in the internal capsule in cases with long incubation periods did indeed result in viral uptake and cortical infection, but nonetheless did not result in infection in the VP. Furthermore, none of the cases involving MD- or RTN-selective injections that were included in the results exhibited signs of tissue damage in the injection sites.
First- and second-order projection neurons
The morphology of infected neurons allowed us to identify first- and second-order projection neurons. First-order neurons are infected by preferential uptake of virions at axon terminals at the site of intracerebral injection. Indeed, previous in vitro studies (Vahlne et al., 1978, 1980; Marchand and Schwab, 1986) demonstrated that PRV and HSV have a higher affinity for axon terminals than perikarya. After uptake, virions are transported by retrograde mechanisms to the soma of the cells of origin of those afferent fibers (Card et al., 1990, 1993; Strack and Loewy, 1990). This results in infection of those cells, with an eventual transynaptic infection of second-order projection neurons (Card et al., 1995). In time, first-order infected neurons often become associated with PRV-immunoreactive astrocytes. Nevertheless, the patterns of infected neurons observed in this and in other studies using PRV-Bartha were consistent with transynaptic passage of virus rather than lytic spread through the extracellular space. Systematic temporal analysis has shown that replication and transynaptic passage of PRV-Bartha occurs before the development of any pathological changes in infected neurons or the appearance of viral antigen in astrocytes (Rinaman et al., 1993). Furthermore, the appearance of viral antigen in astrocytes late in the course of infection appears to reflect a protective response of the CNS aimed at isolating the infected neurons. Most importantly, it has been shown that astrocytes harbor a replication defect that prevents them from producing infectious progeny (Card et al., 1993). Consequently, the appearance of immunoreactive astrocytes in relation to infected neurons provides a means of determining which populations of neurons have been replicating virus for the longest period of time and, thereby, to assess the rank order of viral transport through a multisynaptic pathway.
The reliability of the labeling observed with these viral injections is remarkable. We compared our findings with the large body of literature using conventional retrograde and anterograde tracers in these regions. With a few exceptions, our findings involving direct, first-order projections are consistent with those reported previously (Mogenson, 1987; Ray and Price, 1992). It is worth noting, however, that some regions reported as projecting to the MD were not labeled in this study. A region repeatedly proposed to project to the m-MD is the basolateral nucleus of the amygdala (BLA) (Krettek and Price, 1974,1977; Siegel et al., 1977; Kuroda and Price, 1991; McDonald, 1992; Ray and Price, 1992). The absence of labeling in the BLA after m-MD injections in this study may be the result of amygdaloid neurons being refractory to viral infection. Indeed, refractoriness of certain cell groups to PRV infection has been demonstrated previously (Card et al., 1991; Standish et al., 1995). An alternative explanation for our negative finding may be related to a recently identified characteristic of viral uptake by afferents. It has been shown recently that viral concentration and the density of innervation influences the onset of viral replication (Park et al., 1996). Because BLA projections reported previously do not appear to be numerous, it is possible that they did not accumulate sufficient virus to initiate a productive infection. We were also unable to detect labeled infected neurons in the PL PFC after PRV injections in the m-MD. Injection of the anterograde tracer PHA-L in the PL cortex has shown labeling in the m-MD (Sesack et al., 1989;Groenewegen et al., 1990; Hurley et al., 1991; Ray and Price, 1992), and similar findings were obtained with WGA-HRP (Kuroda and Price, 1991). Others have found anterograde labeling of axons in the l-MD (but not m-MD) after tracer injection in the PL PFC (Beckstead, 1979), but we also failed to detect infected neurons in the PL PFC after l-MD injections. Although it is possible that PL-MD projections may indeed be refractory to viral infection in our experimental conditions, we have observed infected neurons in the PL after injections that included the c-MD. Furthermore, these injections resulted in labeling of CT immunoreactive neurons in the PL. Therefore, it is possible that the c-MD, but not m-MD or l-MD, receives input from the PL PFC.
Organization of connections between the accumbens and MD
Injections of virus into subdivisions of the MD and RTN revealed distinct patterns of infection, suggesting the presence of parallel circuits between the basal forebrain and thalamus. First, multisynaptic projections arising in the accumbens shell relay via the medial VP and terminate selectively within the m-MD. The retrograde infection of neurons in the ventromedial part of the rostral VP after PRV injection in the m-MD is consistent with what has been reported by several groups using conventional tracers (Young et al., 1984; Haber et al., 1985; Mogenson et al., 1987; Groenewegen et al., 1990, 1993; Kuroda and Price, 1991; Ray and Price, 1992), as is the heavy labeling observed in the NDBB (Young et al., 1984; Woolf and Butcher, 1986; Hallanger et al., 1987; Mogenson et al., 1987;Groenewegen, 1988; Ray and Price, 1990, 1992) and rostral RTN (Siegel et al., 1977; Gerfen et al., 1982; Price and Slotnick, 1983; Young et al., 1984; Woolf and Butcher, 1986; Groenewegen, 1988; Kuroda and Price, 1991; Ray and Price, 1992). Moreover, the only striatal region infected after m-MD injections was the accumbens shell in the cases with more advanced infection. The following findings in this study strongly support the conclusion that the VP serves as a relay station for shell projections to the m-MD: (1) m-MD injections resulted in more advanced signs of infection in VP neurons than in the shell; (2) labeling in the shell was consistently detected in the cases with more advanced signs of infection, whereas it was minimal or absent in animals killed earlier in the course of the infection; and (3) infected cells could not be observed in the shell after m-MD viral injections in the VP-lesioned animal. Thus, the most likely route of infection in the shell is via the medial VP; this is consistent with reports of accumbens shell neurons projecting to the ventromedial aspect of the VP (Zahm and Heimer, 1990; Záborszky and Cullinan, 1992; Napier et al., 1995). In addition, a shell medial VP/m-MD-axis has recently been proposed in a study combining conventional tracers in the VP and MD (Zahm et al., 1996).
A second circuit involves projections from the accumbens core to the lateral VP and the pallidal region of the OT, then to the c-MD and rostral RTN. Injections that included the c-MD resulted in first-order infection of neurons in the polymorph (pallidal) region of the OT and in the caudal and lateral subcommissural region of the VP and in second-order infection of neurons in the core and striatal OT. It should be noted that in all these cases, the injections also extended into the neighboring m-MD or l-MD, and the pallidal and striatal infection patterns were a combination of those typical of m-MD and l-MD injections with the lateral VP and accumbens core. This projection arising from the core should be taken with caution, because in all cases, the number of cells infected in the core was very sparse. It is possible that the primary thalamic target of core-originated projections was missed in this study. Indeed, it has been proposed that neurons in the laterodorsal VP receiving input from the core project to the caudal and ventral parts of the m-MD (Groenewegen et al., 1990). We consistently found second-order infected cells in the accumbens core in every case in which the c-MD was included in the injection site. This argues for a core-lateral VP-c-MD pathway. However, it has been demonstrated recently that the accumbens-VP projections to the MD arise disproportionately from the shell compared with those originating in the core (Zahm et al., 1996). Thus, it is possible that the primary core output is directed to regions other than the MD. Indeed, a subset of core neurons has been reported to preferentially project to the substantia nigra pars reticulata (Montaron et al., 1996).
A third circuit shown by our data involves projections from the CPu to the GP to the l-MD. Injections in the l-MD resulted in a pattern of retrograde labeling consistent with that reported previously (Haber et al., 1985; Groenewegen, 1988; Ray and Price, 1992). First-order projection neurons were observed in the GP, and second-order neurons were detected in the CPu. With the exception of the two cases with survival times well beyond the others, first-order projection cells were not observed in the VP. This is consistent with classical tracer studies showing that the l-MD does not receive input from the VP (Ray and Price, 1992; Groenewegen et al., 1993).
Organization of connections between accumbens and RTN
Different regions within the RTN were also targets of striatal and accumbal projections via the GP and VP. Injections into the ventral part of the rostral RTN resulted in an extensive infection of VP neurons and in second-order infection in the nucleus accumbens core and shell. In the animals injected in more dorsal and caudal regions of the rostral RTN, infected cells were detected in the VP, and second-order neurons were observed in the accumbens shell and not in the core. This suggests that the shell, in addition to its projection to the m-MD via the VP, may also target a discrete region within the RTN, whereas the core, in addition to targeting the c-MD via the VP, also projects to a different RTN region. The absence of this pattern of infection in cases in which the injection was close to, but did not involve, the RTN supports this conclusion.
PRV injections into the caudal RTN resulted in infection of cells in the GP that had the characteristic labeling pattern of first-order projection cells. In addition, second-order projection neurons were labeled in the CPu but were absent in the accumbens. These findings are consistent with results from injections of anterograde tracers in the GP that yielded labeling of terminals in the caudal RTN (Gandia et al., 1993; Philipson et al., 1993) and suggest that the so-called “indirect pathway” of striatal circuits may have a target in the RTN, as proposed by Parent and colleagues in monkeys (Hazrati and Parent, 1991; Parent and Hazrati, 1995). This pathway includes projections from the CPu to the GP (or GPe in primates), which in turn projects to the entopeduncular nucleus (GPi in primates), providing an input to thalamocortical projections that are distinct from the “direct pathway.” In this case, a GP-RTN projection may serve as a means to further control the flow of information in the basal ganglia circuits that may be particularly relevant to the integration of limbic, motor, and sensory systems. Indeed, the RTN injection that resulted in GP labeling also labeled first-order projection cells in the ventral anterior-VL thalamic nuclei. Because RTN-ventral thalamic connections are known to be reciprocal (Cornwall et al., 1990), it is possible that GP input to the caudal RTN may be conveyed to the ventrolateral nucleus of the thalamus. This thalamic region is also a target of projections originating in the CPu via the “direct pathway” (Alexander and Crutcher, 1990).
Parallel circuits involving the MD and RTN
The results presented here reveal a substantial degree of segregation in the projections from the accumbens core and shell regions to the thalamus. Indeed, while efferents from the shell region of the accumbens, via its projections to the medial VP, contact the m-MD and rostral-intermediate regions of the RTN, the projections from the core region, via the lateral VP, affect primarily the c-MD and rostral pole of the RTN. In addition, CPu efferents target the l-MD and a caudal region of the RTN via the GP. These parallel circuits revealed by the transynaptic passage of this neurotropic virus are a confirmation of what has been proposed by the analysis of separate conventional tracer studies (Groenewegen et al., 1990, 1993; Zahm et al., 1996), with the shell-medial VP/m-MD-axis being the strongest in our dataset (Fig. 14 ).
As suggested by in vivo intracellular recordings in the RTN (Lavı́n and Grace, 1994), we have provided additional anatomical evidence for parallel VP-RTN projections. Furthermore, the RTN and MD regions studied appear to project to each other. Discrete RTN regions receiving inputs from discrete MD areas in turn send projection to restricted areas within the MD that are not necessarily the same as those projecting to these RTN regions. Nonetheless, the shell, core, and CPu-originated circuits remain segregated within both the MD and RTN. These findings are consistent with previous studies using anterograde tracers injected in the rostral pole of the RTN that labeled terminals within the c-MD (Philipson et al., 1993), as well as with the ability of HRP injections in the MD to retrogradely label cells in the rostral pole of the RTN (Tai et al., 1995).
Even though core and shell neurons project to different thalamic target areas, there are some interactions between these parallel circuits (Fig. 14). The MD itself is not likely to be a site for interactions between these parallel circuits, because dendritic trees of cells located in the different segments of the MD were found to be confined to each MD subdivision (Kuroda et al., 1992). Furthermore, there was no evidence for local connections between MD subdivisions in our analysis; i.e., injections of PRV in one segment did not lead to retrograde infection of MD neurons in other MD segments, nor did the analysis of CT transport provide evidence of such connection. However, the shell medial VP/m-MD-axis could be affected by core output by virtue of the core-receiving region of the RTN (rostral pole) projections to the m-MD. Furthermore, these circuits may also be interconnected at the level of thalamocortical projections. The m-MD is known to project to both PL and IL PFC, the former of which projects to the accumbens core. These results support the idea of these parallel circuits being “open interconnected” instead of segregated (Joel and Weiner, 1994), although the closed or open nature of the cortical components of these loops remains to be explored.
Functional implications
The MD regions targeted by the striatal regions have been demonstrated to be the origin of projections to cortical regions that in turn project back to the accumbens and striatum. Thus, the m-MD projects to the PL and IL PFC, the c-MD to the lateral orbital and ventral agranular insular cortex, and the l-MD to the anterior cingulate cortex (Leonard, 1972; Siegel et al., 1977; Sesack et al., 1989; Kuroda and Price, 1991; Ray and Price, 1992; Groenewegen and Berendse, 1994; Condé et al., 1995). The involvement of the RTN in these circuits may provide the bases for a control of MD-cortical activity. Indeed, it is known that the RTN controls thalamocortical activity by modulating the oscillatory activity of thalamic cells (Steriade et al., 1994). Because different regions within the RTN control discrete thalamic regions (Mitrofanis and Guillery, 1993), it is possible that the RTN areas identified in these experiments selectively control the MD-PFC activity. Thus, the RTN region that receives inputs from the striatopallidal system appears to control the activity of the thalamocortical regions that are targeted by the same component of the striatopallidal system. Such an arrangement bears a striking similitude to that of cortical inputs on RTN-thalamic nuclei interactions in that the pallidal regions send projections to mutually interconnected RTN/MD areas. In this way, the VP and GP exert a tight control over RTN-MD interactions similar to that of cortical input. However, pallidal input to the thalamus is known to be GABAergic (Young et al., 1984). Although highly speculative, it is possible that these pallidal regions are involved in rhythm generation within the thalamocortical system. This is particularly attractive, because most accumbens neurons and many VP neurons recorded in vivoexhibit a bistable pattern of activity, alternating between active and silent states at ∼1 Hz (O’Donnell and Grace, 1995b; Lavı́n and Grace, 1996), which is precisely the frequency at which many RTN units oscillate (Steriade et al., 1993a; Lavı́n and Grace, 1994). Although it may be possible that this 1 Hz RTN activity reflects basal ganglia input via the striatopallidal system, it is also possible that basal ganglia oscillatory activity is the result of RTN-dependent cortical activity.
The RTN is known to exert a control on the oscillatory activity of thalamocortical projections (Steriade et al., 1993a), including those that appear to be involved in wakefulness or selective attention (Steriade et al., 1993b). Therefore, the activity of accumbens-RTN projections may have an impact on functions such as general attentiveness or a broadening of attentional focus via its modulation of overall thalamocortical activity (Lavı́n and Grace, 1994). It has been suggested that the RTN comprises “topographic maps” representing different cortical areas (Mitrofanis and Guillery, 1993), and our data are consistent with this view. In this way, the RTN may be capable of selectively activating specific thalamocortical circuits to allow a focusing of attention toward a specific stimulus or cognitive state, with limbic inputs originating in the accumbens directing the orientation of such activation based on the affective associations generated by the stimulus. This takes place, as shown by Steriade et al. (1988), by RTN and thalamic relay cells switching their firing pattern in the waking process from rhythmic bursts to single spike activity. Although these changes have been discussed primarily with respect to the role of sensory inputs and attention, the results presented here, when combined with our previous electrophysiological data (Lavı́n and Grace, 1994), suggest a role for limbic regions in modulating such activity changes. In this way, striatopallidal activity may ultimately adjust the level of rhythmicity within the RTN-MD system by acting on RTN neuron dendrites, which have been proposed to “tune” RTN response to cortical inputs (Destexhe et al., 1996). Furthermore, the RTN has been proposed to synchronize the 40 Hz thalamocortical activity (Paré and Llinás, 1995). The connections reported here may represent the means by which the limbic striatum (i.e., the nucleus accumbens) has an influence on the activity of systems proposed to have a role in consciousness. A computational analogy for these interactions would be that setting a particular level of RTN activity (and therefore of control of thalamocortical function) is like loading the appropriate drivers for the activation of the cortical regions required at a given moment. Basal ganglia input, via GP and VP, may change the status of RTN drivers for PFC activation. In this way, our analysis by viral tracing techniques provides an anatomical basis for the proposed involvement of the nucleus accumbens in attentional mechanisms (Reading et al., 1991; Joseph et al., 1992;Lavı́n and Grace, 1994) and for the attentional disturbances that have been observed in schizophrenics (Goldberg et al., 1993). Indeed, a malfunction of the basal ganglia may eventually result in the loading of inappropriate RTN-MD drivers in the schizophrenic brain, resulting in improper cortical activation. Such a disturbance may also be reflected in the reported coincidence between slow-wave sleep deficit and negative symptoms in schizophrenia (Keshavan et al., 1995).
In summary, our data show that multisynaptic circuits from the CPu and accumbens core and shell to the MD and reticular thalamic nuclei via the VP are organized in a series of parallel loops that nonetheless exhibit some interactions. The accumbens shell is the primary source of transynaptic striatal input to the MD, whereas the sparse accumbens core transynaptic projections to the thalamus appear to be primarily directed to the RTN.
Footnotes
This work was supported by National Institutes of Health Grants MH53574 (J.P.C.), NINDS33506 (L.W.E.), and MH45156 and MH01055 (A.A.G.); and a National Alliance for Research on Schizophrenia and Depression Young Investigator Award (P.O.). We thank Ms. Jen-Shew Yen for her excellent technical assistance and Dr. Susan R. Sesack and Dr. Holly Moore for comments on this manuscript. We also thank Dr. Robert Y. Moore for generously providing the use of his BSL-2 facility.
Correspondence should be addressed to Dr. Patricio O’Donnell, Department of Neuroscience, 446 Crawford Hall, University of Pittsburgh, Pittsburgh, PA 15260.