Abstract
Rabbit eyeblink conditioning is a well characterized model of associative learning. To identify specific neurons that are part of the eyeblink premotor pathway, a retrograde transsynaptic tracer (pseudorabies virus) was injected into the orbicularis oculi muscle. Four time points (3, 4, 4.5, and 5 d) were selected to identify sequential segments of the pathway and a map of labeled structures was generated. At 3 d, labeled first-order motor neurons were found in dorsolateral facial nucleus ipsilaterally. At 4 d, second-order premotor neurons were found in reticular nuclei, and sensory trigeminal, auditory, vestibular, and motor structures, including contralateral red nucleus. At 4.5 d, labeled third-order premotor neurons were found in the pons, midbrain, and cerebellum, including dorsolateral anterior interpositus nucleus and rostral fastigial nucleus. At 5 d, labeling revealed higher-order premotor structures. Labeled fourth-order Purkinje cells were found in ipsilateral cerebellar cortex in cerebellar lobule HVI and in lobule I. The former has been implicated in eyeblink conditioning and the latter in vestibular control. Labeled neurons in anterior interpositus were studied, using neurotransmitter immunoreactivity to classify individual cell types and delineate their interconnectivity. Labeled third-order premotor neurons were immunoreactive for glutamate and corresponded to large excitatory projection neurons. Labeled fourth-order premotor interneurons were immunoreactive for GABA (30%), glycine (18%), or both GABA and glycine (52%) and form a functional network within anterior interpositus involved in modulation of motor commands. These results identify a complete eyeblink premotor pathway, deep cerebellar interconnectivity, and specific neurons responsible for the generation of eyeblink responses.
Introduction
Delay eyeblink conditioning is a well characterized model of associative learning but the locus of learning is still a matter of debate. Possible sites of plasticity have been found in the anterior interpositus nucleus (AIN) of the deep cerebellar nuclei (DCN) (McCormick et al., 1982; Marek et al., 1984; Nowak and Gormezano, 1990; Thompson and Steinmetz, 2009; Freeman and Steinmetz, 2011), lobule HVI of the cerebellar cortex (Yeo et al., 1985; Gould and Steinmetz, 1996; Schreurs et al., 1998; Jirenhed et al., 2007; Kellett et al., 2010), and anterior lobule (Perrett and Mauk, 1995; Green and Steinmetz, 2005). Identification of a complete cerebellar premotor pathway of the eyeblink response can be of great value in elucidating the specific components involved in the generation and modulation of eyeblink conditioning.
DCN is the final filter that integrates all the information processed in the cerebellum and generates its sole output. However, unlike the cerebellar cortex, the circuitry of the DCN is poorly understood. There are at least six types of neurons in the DCN, including large glutamatergic projection neurons, two types of inhibitory projection neurons, and at least two types of interneurons. The only excitatory output of the DCN is generated by large glutamatergic neurons that project to different extra-cerebellar sites and comprise ∼50% of the total DCN neuronal population (Batini et al., 1992; Teune et al., 2000). The first type of inhibitory projection neuron is a small GABAergic neuron that projects to the inferior olive and forms the nucleo-olivary feedback loop (Tolbert et al., 1976; de Zeeuw et al., 1989). The second type is a large glycinergic neuron (recently discovered in the fastigial nucleus) that projects to vestibular and reticular sites (Bagnall et al., 2009). Recent electrophysiological studies in transgenic mice expressing GAD-eGFP or GlyT2-eGFP were able to distinguish at least two types of interneurons: a GABAergic or mixed GABA/glycinergic interneuron and a non-GABAergic (possibly glutamatergic) interneuron (Uusisaari and Knöpfel, 2010, 2011). However, the role of these interneurons is unknown and their interactions have not been studied.
Retrograde transsynaptic viral tracers are a powerful tool for identifying neuronal networks. Attenuated pseudorabies virus Bartha (PRV) (Bartha, 1961) reveals that hierarchical chains of functionally connected neurons and multisynaptic pathways can be identified by following the extent and time course of the PRV infection (Daniels et al., 1999; Billig et al., 2000; Kerman et al., 2006; Van Daele and Cassell, 2009). In the present study, the premotor pathway of the rabbit orbicularis oculi muscle (OOM) responsible for the eyeblink was traced retrogradely using PRV. Neurons in the AIN involved in the pathway were characterized based on their neurotransmitter content. Of particular importance, three different types of inhibitory interneurons that are part of the OOM premotor pathway were revealed to form a possible functional network within the AIN for the modulation of motor commands.
Materials and Methods
Animals
Twenty-four adult male New Zealand rabbits (Oryctolagus cuniculus), between 3 and 4 months of age, weighing ∼2.5 kg, were supplied by Harlan. Four rabbits were assigned to each of four different time points for PRV anatomical tracing (3 d, 4 d, 4.5 d, and 5 d) and four rabbits were assigned to each of two time points for neurotransmitter immunohistochemistry (4.5 d and 5 d). Rabbits were housed in individual cages, given ad libitum access to food and water, and maintained on a 12 h light/dark cycle, all in accordance with the National Institute of Health guidelines. All procedures were approved by the West Virginia University Animal Care and Use Committee.
PRV injections
An attenuated PRV expressing an enhanced green fluorescent protein (PRV-152) was used as a retrograde transsynaptic tracer (Smith et al., 2000). The PRV was a kind gift from L. W. Enquist (Princeton University, Princeton, NJ). PRV enters the neuron terminals by fusion. Once inside, the virus caspids interact with the neuron's dynein, a cellular microtubule-associated motor protein, and it travels retrogradely to the nucleus where it replicates. After replication, it moves to the dendrites where it infects synaptically connected cells (Curanović et al., 2009; Curanovic and Enquist, 2009). PRV does not label sensory pathways, and even though it can be taken up by sensory neurons, its exclusively retrograde properties confine the virus to the sensory neuron soma and it does not spread any further (Smith et al., 2000; Mettenleiter, 2002; Mettenleiter et al., 2006). The same batch of PRV was used for all injections at a concentration of 2.3 × 108 plaque-forming units per milliliter (PFU/ml). After arrival, PRV was aliquoted and stored at −80°C. Before PRV injections, rabbits were anesthetized with 20 mg/kg Ketamine and 4 mg/kg Xylazine. Their right eyelid was shaved and cleaned with isopropyl alcohol. After thawing, PRV was sonicated for 2 min. A glass, 10 μl Hamilton syringe with a 31-gauge needle was rinsed three times in 95% ethanol, sterile dH2O, sterile saline, and PRV. Fifteen microliters of PRV divided into 5 injections of 3 μl each were injected into the right OOM. Each injection was transverse to the muscle fibers and delivered at a constant rate through the orbital, preseptal, and pretarsal portions of the OOM to ensure adequate viral distribution. After injection, the syringe was left in place for 10 min to achieve complete viral absorption and to prevent any leakage. A basic diagram of the PRV procedures is depicted in Figure 1.
Schematic diagram of the OOM premotor pathway labeled with PRV. A shows the location of 5 PRV injections (green dashed lines) in OOM that include the orbital, preseptal, and pretarsal muscles. B shows the retrograde transsynaptic spread of PRV through the OOM premotor pathway. Directional and sequential spread of PRV through first-order (1°) motor neurons in the facial nucleus (7N), second-order (2°) premotor neurons in the red nucleus (RN) and other areas, and third-order (3°) premotor neurons in the AIN of the cerebellum and other areas.
Tissue processing
The 16 rabbits used for the delineation of the OOM premotor pathway were injected with Euthasol (sodium pentobarbital, 390 mg/ml) and exsanguinated with 1.0 cc Euthasol (sodium pentobarbital, 390 mg/ml) at 3 (n = 4), 4 (n = 4), 4 1/2 (n = 4), or 5 (n = 4) d after PRV-injections. They were perfused transcardially with 1.5 l of 0.9% saline (pH 7.4 at room temperature) followed by 1 l of 4% formaldehyde. For anti-PRV immunohistochemistry, brains were collected and placed in fixative for 4 h and transferred to 30% sucrose for cryoprotection until they sank and 50 μm sections were cut on a freezing microtome.
Eight rabbits were used for characterization of AIN neurons based on their neurotransmitter immunoreactivity. Animals were injected with Euthasol (sodium pentobarbital, 390 mg/ml) and exsanguinated with 1.0 cc Euthasol (sodium pentobarbital, 390 mg/ml) at 4.5 (n = 4) or 5 (n = 4) d after PRV-injections. They were perfused transcardially with 1.5 l of 0.9% saline (pH 7.4 at room temperature) followed by 1 l of 2.5% glutaraldehyde and 1.5% formaldehyde. Brains were placed in fixative for 6 h, transferred to 30% sucrose for cryoprotection until they sank, and 25 μm sections were cut. All sections were marked on the contralateral side of injection to distinguish laterality.
Anti-PRV immunohistochemistry
Free-floating sections were washed in 0.5 m Tris and placed in 3% H2O2 for 30 min to quench endogenous peroxidases. Antigen retrieval was accomplished by incubating the sections in citrate buffer, pH 3.0, for 30 min at 37°C. After washing, the sections were blocked for 1 h in 3% normal rabbit serum and incubated in a goat anti-PRV primary antibody overnight at 4°C (polyclonal gb-320 developed by R. Miselis, Philadelphia, PA, 1:10,000). The PRV primary antibody has been described extensively (Chen et al., 1999; Aston-Jones and Card, 2000; Aston-Jones et al., 2004; James et al., 2008). After washing, the sections were placed in a secondary antibody (biotinylated rabbit anti-goat 1:200) for 1 h. The sections were then washed and placed in ABC (Vector Kit, Vector Labs) for 1 h, washed once more, and stained with DAB (Vector Kit, Vector Labs) for 2–4 min until color developed.
The location of each PRV-labeled neuron was plotted on sequential coronal sections of the rabbit brain but a specific structure was only considered to be labeled and reported here if more than one neuron was labeled in that structure in each of the four rabbits used for a given time point.
Fluorescence neurotransmitter immunoreactivity
The 25 μm free floating sections were treated with 0.5% sodium borohydride in 0.1 m PBS, pH. 7.2, for 30 min to quench autofluorescence produced by glutaraldehyde, and followed by repeated washes. Sections containing the DCN were incubated with primary antibodies for 72 h and with secondary antibodies for 48 h at 4°C in a buffer solution containing 0.1 m PBS, pH 7.2, 3% normal goat serum, and 0.1% sodium azide (preservative). After specificity tests, an optimal immunolabeling protocol was developed. First, sections were incubated in a polyclonal goat anti-PRV (gb-320 1:10,000) followed by its secondary antibody (donkey anti-goat Alexa 488, Invitrogen; 1:500). Second, sections were incubated in a mixture of monoclonal mouse anti-l-glutamate conjugated to glutaraldehyde and bovine serum albumin (anti-Glu-G-BSA; Millipore MAB5304, 1:1000), polyclonal guinea pig anti-GABA conjugated to glutaraldehyde and keyhole limpet hemocyanin (anti-GABA-G-KLH; Millipore AB175, 1:1000), and polyclonal rabbit anti-glycine conjugated to glutaraldehyde and BSA (anti-Gly-G-BSA; Millipore AB139, 1:1000). After primary antisera incubation, sections were washed several times over 24 h with 0.1 m PBS and 0.1% sodium azide. Sections were then incubated with secondary antibodies (goat anti-rabbit Alexa 405, goat anti-mouse Alexa 546, and goat anti-guinea pig Alexa 633; Invitrogen, 1:400). The sections were then washed and mounted on gelatin-covered mounting slides and coverslipped using Fluoromount-G mounting media (SouthernBiotech) and #1.5 coverslips (Fisher Scientific).
Antibody characterization
Monoclonal mouse anti-glutamate antiserum (Millipore, MAB5304) has been previously characterized in several studies (Chagnaud et al., 1989; Roche et al., 2003; Wu et al., 2005). Specificity testing by competition experiments using ELISA performed by the manufacturer showed no cross-reactivity with aspartate-G-BSA, GABA-G-BSA, or Gly-G-BSA.
Polyclonal guinea pig anti-GABA antiserum (Millipore, AB175) has been used to identify GABAergic neurons by light and electron microscopy (manufacturer's technical information) and tested in dot blots showing specificity for its conjugated antigen, and immunoreactivity can be removed by preabsorption with its antigen (Chalazonitis et al., 2008). In addition, anti-GABA-G-KLH has been extensively characterized in different preparations and species (McDonald and Pearson, 1989; Roettger et al., 1989; Dmitrieva et al., 2001; Rubio and Juiz, 2004; Stanić et al., 2010).
The polyclonal rabbit anti-glycine antiserum (Millipore, AB139) has been used in different tissue preparations and species (Avendaño et al., 2005; Fredrich et al., 2009; Kuo et al., 2009; Downie et al., 2010). Specificity testing by competition experiments using ELISA performed by the manufacturer showed no cross-reactivity with GABA-G-BSA, Glu-G-BSA, taurine-G-BSA, or aspartate-G-BSA. The specificity of this antiserum was also tested by Western blotting in sea lamprey brain homogenates and showed high specificity for Gly-G-BSA (Villar-Cerviño et al., 2006).
Controls and specificity tests
In the present study, additional neurotransmitter antisera specificity tests were performed. First, omission controls in which the primary antibodies were replaced with incubating buffer eliminated immunoreactivity. Second, preabsorption of the primary antibodies with the immunizing peptide (purchased from Invitrogen or Vector Labs) also eliminated immunoreactivity. Third, preabsorption of each primary antibody with the other two conjugated peptides did not reduce immunoreactivity (e.g., 5 μl of anti-GABA-G-BSA preabsorbed with 1 μl of glycine-G-BSA and 1 μl of glutamate-G-BSA did not reduce immunoreactivity for GABA; the same was true for the other two conjugated antibodies). In addition, identical immunoreactivity was seen in experiments where the three preabsorbed primary antibodies were used sequentially compared with experiments where primary antibodies were used simultaneously. All control tests were performed on the cerebellar cortex where the neurotransmitter profile of cells has been well characterized and where granule cells are exclusively glutamatergic, stellate and basket cells are GABAergic, globular cells are glycinergic, and Golgi cells are both GABAergic and glycinergic (Ottersen et al., 1988; Simat et al., 2007).
Image acquisition
Light microscopy.
Images were acquired using an upright Olympus AX70 light microscope with a motorized stage and with 4× (NA 0.15) or 10× (NA 0.4) objectives. Some pictures of different brain structures were acquired using the virtual slice module to produce high resolution images (West Virginia University, Microscopic Imaging Facility).
Confocal microscopy.
Neurotransmitter immunofluorescent reactivity of the DCN of rabbits previously injected with PRV (4.5 and 5 d) was visualized using a confocal laser scanning microscope (Zeiss LSM 710; Carl Zeiss International). Images were acquired using 405, 488, 514, and 633 nm lasers, sequential multichannel line scan, averaged twice, pinhole aperture of 1 AU, 1024 × 1024 resolution, and the filters were set manually to detect the spectral peak of each fluorophore. All coronal sections (25 μm) of the DCN were visualized first using a 10× objective (NA 0.4) to locate all PRV-labeled neurons. Only PRV-labeled neurons with a visible nucleus were included in this study to standardize data acquisition and to avoid over counting. Classification of DCN cell neurotransmitter immunoreactivity was performed using a 63× oil-immersion objective (NA 1.4). Images were exported to Adobe Photoshop 8.0 and only minor adjustments of brightness and contrast were made.
Results
The directional and temporal pattern of PRV retrograde spread through synaptically connected circuits can be used to identify specific pathways. In the present study, four different time points were used to identify each step in the rabbit OOM premotor pathway. Based on pilot data, four time points were selected to best represent the progression of PRV labeling through each step in the pathway (3 d, n = 4; 4 d, n = 4; 4.5 d, n = 4; and 5 d, n = 4).
Mapping the OOM premotor pathway
Three days after PRV injections in the OOM, first-order motor neurons labeled with PRV were seen in the ipsilateral facial nucleus (Fig. 2A). Labeled neurons were located in the dorsolateral and dorsal portions of the intermediate and lateral subdivisions of the nucleus, forming a cap-like distribution in agreement with the location of motor neurons innervating the OOM found in previous studies (Radpour, 1977; Komiyama et al., 1984; Klein et al., 1990; VanderWerf et al., 1998; Horta-Júnior et al., 2004; McNeal et al., 2008). Importantly, the same region of the nucleus was labeled in all rabbits. Exclusive PRV uptake by OOM motor neurons was corroborated by examination of motor and preautonomic structures known to innervate other ocular muscles and glands. The abducens nucleus that innervates extraocular muscles was not labeled with PRV at any of the time points examined (Fig. 2B). In addition, the superior lacrimal and salivatory nucleus, which contains preganglionic autonomic efferents to the eyelid glands and smooth muscle, was also not labeled with PRV in any of the subjects used in this study at any of the time points (Fig. 2B). The facial nucleus and other structures labeled with PRV at 3, 4, 4.5, and 5 d are shown in Table 1.
Examples of PRV-labeled neurons in the rabbit brain 3 and 4 d after injection. A, PRV-labeled first-order motor neurons are located in the dorsolateral facial nucleus ipsilaterally 3 d after PRV injection into the right OOM. DL, Dorsolateral; L, lateral; Int, intermediate; M, medial; VM, ventromedial subnuclei. B–F, PRV-labeled neurons 4 d after PRV injection. B shows PRV-labeled neurons in the medial vestibular nucleus (MVe) ipsilaterally and absence of PRV labeling in the superior salivatory nucleus (SSN) and abducens nucleus (6N). C shows PRV labeling in the ventral spinal trigeminal nucleus, oral part (Sp5O) ipsilaterally. D, Discrete PRV labeling in the rostral dorsal cochlear nucleus (DC) ipsilaterally. E shows PRV-labeled neurons in the parabrachial nucleus (PB) and Kölliker-fuse nucleus (KF) ipsilaterally. F shows PRV-labeled neurons in the dorsolateral red nucleus (RN) contralaterally. Scale bars: 1 mm.
Labeled areas after PRV injection into the right OOM
Four days after PRV injection, premotor structures were labeled. A group composite of PRV-labeled neurons was plotted in a map of coronal sections (Fig. 3) to best represent the distribution of labeled neurons at this time. PRV-labeled neurons were found in the dorsal, intermediate, and ventral medullary reticular nucleus predominately ipsilaterally but some were seen on the contralateral side. In addition, labeled neurons were found in the magnocellular, gigantocellular, lateral paragigantocellular, parvicellular, and lateral reticular nucleus mostly ipsilaterally. Vestibular second-order labeled neurons at this time were seen only in the ventral part of the medial vestibular nucleus ipsilaterally (Fig. 2B). In addition, labeled neurons were found in the medial and ventral portions of the caudal, interpolar, and oral spinal trigeminal nucleus and in the ventral part of the principal sensory trigeminal nucleus exclusively on the ipsilateral side, in agreement with the location of spinal and principal sensory trigeminal neurons that have been shown to make monosynaptic connections to the facial motor nucleus and generate reflex eyeblink responses (Hinrichsen and Watson, 1983; Yokota et al., 1991; van Ham and Yeo, 1996a, 1996b; Henriquez and Evinger, 2007). Figure 2C depicts a characteristic neuron located in the ventral spinal trigeminal nucleus (oral part). Second-order auditory areas including the nucleus of the trapezoid body, periolivary nuclei, and dorsal cochlear nucleus were labeled ipsilaterally at this time. Labeling of the trapezoid body was confined to the dorsolateral region. A few labeled neurons were seen in the medial and lateral periolivary nuclei. The rostral portion of the dorsal cochlear nucleus was also labeled with PRV on the ipsilateral side at this time (Fig. 2D). A discrete group of labeled neurons were found in the Kölliker-fuse nucleus and the ventral part of the medial parabrachial nucleus on the ipsilateral side (Fig. 2E). The Kölliker-fuse and the parabrachial nucleus are involved in the modulation of breathing and may play a role in synchronizing OOM activity and respiration (Chamberlin and Saper, 1994; Bonis et al., 2010; Song et al., 2012). Finally at this time point, labeled neurons were seen in the dorsolateral red nucleus on the contralateral side (Fig. 2F). These neurons were located in the caudal portion of the magnocellular red nucleus, a region that has been shown to innervate the OOM portion of the facial nucleus and generates blink responses when stimulated (Takada et al., 1984; Daniel et al., 1987; Chapman et al., 1988; Holstege and Tan, 1988). In addition, a small number of labeled neurons were found in the adjacent contralateral pararubral nucleus.
Distribution of PRV-labeled neurons in the brain 4 d after PRV injection in the right OOM. A composite of the location of PRV-labeled neurons found across four animals plotted in sequential sections to best represent the pattern of PRV labeling. Sections are arranged caudorostrally (A–K). The arrow indicates the side of PRV injection. Each dot represents one PRV-labeled neuron. 3N, Oculomotor nucleus; 4N, trochlear nucleus; 5N, motor trigeminal nucleus; 7N, motor facial nucleus; 12N, hypoglossal nucleus; AIN, anterior interpositus; CG, central gray; Cn, cuneiform nucleus; DC, dorsal cochlear; Dk, nucleus of Darkschewitsch; LL, lateral lemniscus; dMe, deep mesencephalic nucleus; DN, dentate nucleus; PAG, periaqueductal gray; DpG, deep layer of the superior colliculus; FN, fastigial nucleus; Gi, gigantocellular reticular nucleus; Gr, gracile nucleus; IC, inferior colliculus; InC, interstitial nucleus of Cajal; InG, intermediate gray layer of the superior colliculus; InW, intermediate white layer of the superior colliculus; KF, Kölliker-fuse nucleus; LRt, lateral reticular nucleus; MdD, dorsal medullary reticular nucleus; MdV, ventral medullary reticular nucleus; MG, medial geniculate nucleus; MVe, medial vestibular nucleus; Op, optic nerve layer of the superior colliculus; PaR, pararubral nucleus; PB, parabrachial nucleus; Pn, pontine nucleus; PnO, pontine reticular nucleus, oral; PO, periolivary nucleus; Pr5, principal sensory trigeminal nucleus; RN, red nucleus; RRF, retrorubral field; SN, substantial nigra; Sol, solitary nucleus; Sp5C, spinal trigeminal nucleus, caudal; Sp5I, spinal trigeminal nucleus, interpolar; Sp5O, spinal trigeminal nucleus, oral; SpVe, spinal vestibular nucleus; SuG, superficial gray layer of the superior colliculus; tth, trigeminothalamic tract; Tz, nucleus of the trapezoid body; VC, ventral cochlear nucleus. Scale bar, 5 mm.
Examples of PRV-labeled premotor neurons 4.5 d after PRV injection and a group composite are depicted in Figures 4 and 5, respectively. An increase in labeling was seen at this time and higher-order structures that comprise third-order neurons were revealed. Labeled neurons in the medullary and reticular nuclei became more numerous bilaterally. The nucleus of the trapezoid body and the medial and lateral periolivary nuclei showed an increase in labeling that remained mostly ipsilateral. In addition, PRV-labeled neurons were seen in the medial ventral periolivary nucleus. The spinal and principal sensory trigeminal nucleus showed an increase in labeling, and a few labeled neurons were seen on the contralateral side. A few labeled neurons were found in the ipsilateral motor trigeminal nucleus. The dorsal cochlear nucleus was labeled bilaterally and also some labeled neurons were seen in the ventral cochlear nucleus ipsilaterally. The parabrachial and Kölliker-fuse nucleus showed a small increase in labeling and only a few neurons were seen on the contralateral side. Labeling in the medial vestibular nucleus became more dense and bilateral. In addition, PRV-labeled neurons were found in the superior and lateral vestibular nuclei bilaterally. PRV-labeled neurons became more numerous in the contralateral red nucleus and the pararubral nucleus, and a few labeled cells were seen on the ipsilateral side of these nuclei at this time (Fig. 4A). Also, PRV-labeled neurons were found in the interstitial nucleus of Cajal (Fig. 4A) and the nucleus of Darkschewitsch bilaterally, with ipsilateral predominance. Labeled neurons were also found in the oculomotor nucleus, supraoculomotor nucleus (Fig. 4A) bilaterally, and periaqueductal gray (Fig. 4B) mostly ipsilaterally. Some PRV-labeled neurons were also seen in the lateral lemniscus, mainly ipsilaterally (Fig. 4B). More importantly, the first labeled neurons in the DCN were seen at this time in the dorsolateral AIN and rostral fastigial nucleus ipsilaterally (Fig. 4C,D). It should be noted that the PRV-labeled neurons found in the AIN 4.5 d after PRV injection were located in a region that has been extensively implicated in eyeblink conditioning. In addition, electrical stimulation of dorsolateral AIN neurons can generate blink responses (Lavond et al., 1984; Steinmetz et al., 1992; Thompson and Steinmetz, 2009). The fastigial nucleus projects primarily to vestibular and reticular nuclei and its rostral part is involved in vestibulospinal control, including regulation of muscle tone (Gardner and Fuchs, 1975; Büttner et al., 1991; Siebold et al., 1997).
A–D, Examples of PRV-labeled premotor neurons 4.5 d after injection. A shows PRV-labeled neurons in the dorsolateral red nucleus (RN) and pararubral nucleus contralaterally. The oculomotor nucleus (3N), interstitial nucleus of Cajal (InC), and supraoculomotor periaqueductal gray are labeled bilaterally. B shows PRV-labeled neurons in the lateral lemniscus (LL) and periaqueductal gray (PAG) ipsilaterally. C shows a few PRV-labeled neurons in the dorsolateral AIN ipsilaterally. D shows PRV-labeled neurons in the rostral fastigial nucleus (FN) ipsilaterally. Scale bars: 1 mm.
Distribution of PRV-labeled neurons in the brain 4.5 d after PRV injection in the right OOM. A composite of the location of PRV-labeled neurons found across four animals plotted in sequential sections to best represent the pattern of PRV labeling. Sections are arranged caudorostrally (A–L). The arrow indicates the side of PRV injection. Each dot represents one PRV-labeled neuron. See Figure 3 for abbreviations. Scale bar, 5 mm.
Five days after PRV injection, an increase in PRV-labeled neurons was seen throughout. In addition to previously labeled regions, labeled neurons were found in the cuneate (Fig. 6A), and gracile nucleus bilaterally. Labeled neurons were seen in the superficial gray and optic nerve layer of the contralateral superior colliculus (Fig. 6B) (McCormick et al., 1983; Halverson et al., 2009). An increase in labeling was seen in the pararubral nucleus, the deep mesencephalic nucleus, and periaqueductal gray bilaterally (Fig. 6C). A few labeled neurons were seen in the substantia nigra, mainly ipsilaterally. At this time, an increase in labeling was seen in the DCN. Labeled neurons were found in specific regions of the fastigial, interpositus, and dentate nuclei bilaterally with ipsilateral predominance.
A–F, Examples of PRV-labeled premotor neurons 5 d after injection. A shows PRV-labeled neurons in the Cu (cuneate nucleus) ipsilaterally. B shows PRV-labeled neurons in the superior colliculus (SC) contralaterally. C shows PRV labeling in the red nucleus (RN) and pararubral nucleus (PaR) mainly contralaterally and deep mesencephalic nucleus (DMe) bilaterally. D shows PRV-labeled neurons in HVI longitudinal zone C-3 ipsilaterally; note AIN PRV-labeled neurons in the same section. E shows a group of PRV-labeled Purkinje cells in HVI zone C-3 ipsilaterally. F shows PRV-labeled cerebellar lobule I (L1) longitudinal zone A ipsilaterally, note PRV-labeling in the rostral fastigial nucleus (FN), lateral and medial vestibular nucleus (MVe) ipsilaterally. Scale bars: A–D, F, 1 mm; E, 200 μm.
Only two discrete regions in the ipsilateral cerebellar cortex showed PRV-labeled Purkinje cells at this time. The first region corresponds to lobule HVI in the longitudinal zone C3 (Fig. 6D,F). Interestingly, HVI has been extensively implicated in delay eyeblink conditioning (Yeo et al., 1985; Schreurs et al., 1991; Gould and Steinmetz, 1996; Schreurs et al., 1997; Schreurs et al., 1998; Jirenhed et al., 2007; Kellett et al., 2010). Purkinje cells in HVI can generate a blink response and can be activated by periocular stimulation (Berthier and Moore, 1986; Hesslow, 1994). In addition, these Purkinje cells receive inputs from climbing fibers that also send collaterals to the AIN (Yeo et al., 1985; Pijpers et al., 2005; Sugihara and Shinoda, 2007).
The location of PRV-labeled Purkinje cells was determined by careful analysis of their location using three different rabbit brain atlases (McBride and Klemm, 1968; Girgis and Shih-Chang, 1981; Shek et al., 1986) and publications by Ramnani and Yeo (1996), Kellet et al. (2010), and Vogel et al. (2009). PRV-labeled Purkinje cells were located in a small region of HVI. This region corresponds to the dorsolateral posterior portion of HVI, adjacent to the ventromedial region of the paramedian lobule. Labeled Purkinje cells were found in the same coronal plane as the anterior interpositus nucleus and located −3.0 through −4.0 mm relative to lambda based on the coordinates used by Yeo and colleagues (Kellett et al., 2010; Ramnani and Yeo, 1996), and 0.0 mm through 1.0 mm anterior to lambda based on the coordinates used by Vogel et al. (2009). Based on their direct connection to the AIN and their topographical and anatomical location, labeled Purkinje cells were located in longitudinal zone C3. Further comparison with the Sanchez et al. (2002) study of the parasagittal compartmentalization of the rabbit cerebellar cortex revealed by the expression of zebrin II +/− stripes shows that PRV-labeled Purkinje cells were located between zebrin II +/− stripes p4+ and p5+ of HVI, and most probably in p4−. The pattern of expression of zebrin II +/− stripes is highly reproducible between individuals and conserved across species (Brochu et al., 1990; Sanchez et al., 2002; Sillitoe et al., 2005). Purkinje cells located in zebrin II +/− stripe p4− have been shown to project to AIN in mice and rats (Sugihara and Shinoda, 2007; Sugihara and Quy, 2007; Sugihara, 2011), and in the rabbit it may correspond to p4b− (Sanchez et al., 2002). However, in the present study, the location of PRV-labeled Purkinje cells within a specific zebrin II +/− stripe can only be inferred.
The second region of Purkinje cell labeling corresponds to the rostral part of lobule I in longitudinal zone A (Fig. 6E). Purkinje cells located in lobule I longitudinal zone A have been shown to project to the fastigial nucleus (Armstrong and Schild, 1978). Labeled Purkinje cells in lobule I may be part of a cortico-nucleo-vestibular pathway involved in controlling the tone and position of the eyelid with respect to the eyeball and may serve as a muscle position and motion detector to modulate the coordination of different muscles during eyelid movements (Shaikh et al., 2005; Brooks and Cullen, 2009). The distribution of labeled Purkinje cells seems to delineate two distinct cerebellar OOM premotor pathways. The first involves HVI, AIN, red nucleus, and facial nucleus, whereas the second may involve lobule I, fastigial nucleus, vestibular nucleus, and facial nucleus. Together, these data show a comprehensive map of the premotor pathway of the OOM and important structures involved in the eyeblink response.
PRV rate of spread
We found that PRV consistently traced the same pathway in a time-dependent manner across all subjects. PRV axonal transport and the replication cycle seem to be dependent on viral titer, neuronal activity, strength of functional synapses, and species. Axonal transport has been estimated to occur at rates of 8–12 mm/h in vivo (Tomishima et al., 2001) and on average, the virus's complete replication cycle in the nervous system is ∼6–16 h to the point of egress (Whealy et al., 1988; Ugolini, 2011). It has been suggested that postsynaptic neurons that innervate the soma and make numerous synapses onto an infected cell may become infected sooner than those making distal and fewer contacts (Song et al., 2005). Likewise, neuronal activity seems to influence the rate of PRV labeling and this is supported by our data. Neurons in the red nucleus that project to the facial nucleus are phasically active (Gibson et al., 1985), whereas DCN neurons are tonically active. PRV labeled the red nucleus (second-order neurons) in 24 h and DCN (third-order neurons) in 12 h, even though PRV had to travel the same distance. In addition, PRV labeled fourth-order Purkinje cells (that are also tonically active) in 12 h, suggesting that the time-dependent spread of PRV correlates with neuronal activity rather than distance traveled, and it could be of particular importance for delineating functionally relevant pathways.
Distribution of premotor neurons in the DCN
To further characterize the distribution of DCN premotor neurons, the location of PRV-labeled cells 4.5 and 5 d after injection was plotted in a map of coronal sections. The first PRV-labeled neurons seen in the DCN at 4.5 d were consistent with third-order premotor neurons and were found in the dorsolateral AIN and rostral fastigial nucleus exclusively on the ipsilateral side at this time (Fig. 7A). These two distinct areas may hold particular importance in the cerebellar premotor pathway of the OOM. An increase in PRV labeling was seen bilaterally in the DCN 5 d after injection (Fig. 7B). At this time, groups of large and small PRV-labeled neurons were seen in all three nuclei consistent with third and fourth-order neurons. The distributions of these neurons could be of importance in elucidating the somatotopic organization of the OOM in all three nuclei.
Distribution of PRV-labeled premotor neurons in the DCN 4.5 and 5 d after PRV injection. Sections are arranged rostrocaudally (a–e). Note each dot represents a group of 2–5 PRV-labeled neurons of a typical subject. A shows the distribution of PRV-labeled neurons in the rostral fastigial nucleus (FN) and dorsolateral AIN that are found exclusively on the ipsilateral side 4.5 d after PRV-injection. B shows the distribution of PRV-labeled neurons in the FN, AIN, posterior interpositus nucleus (PIN), and dentate nucleus (DN) that are found bilaterally with ipsilateral predominance 5 d after PRV injection. Scale bar, 5 mm.
Neurotransmitter immunoreactivity in the AIN
The large and small PRV-labeled neurons seen in the ipsilateral AIN 5 d after injection (Fig. 7B) were presumably third-order glutamatergic projection neurons and fourth-order interneurons. To further investigate this local network, we used glutamate, GABA, and glycine immunoreactivity to label these neurons. All sections containing the ipsilateral DCN were immunolabeled, and as a control, the cerebellar cortex was examined in each section to confirm the specificity of neurotransmitter immunoreactivity. Figure 8 shows glutamate-, GABA-, and glycine-immunoreactive neurons in the cerebellar cortex. Granule cells and their numerous axon terminals extending through the molecular layer were immunoreactive for glutamate. Purkinje cells, small basket and stellate cells in the molecular layer, and Golgi cells in the granule cell layer were immunoreactive for GABA. Neurons immunoreactive for glycine include Lugaro cells in the Purkinje cell layer and Golgi cells in the granule cell layer. Colocalization of GABA and glycine immunoreactivity can be seen in some Golgi and Lugaro cells in the granule cell layer, known to be GABA/glycinergic neurons (Crook et al., 2006; Simat et al., 2007).
Glutamate, GABA, and glycine immunoreactivity in the cerebellar cortex. Glutamate-immunoreactive granule cells and their numerous axon terminals extending through the molecular layer are seen in the top left panel. GABA-immunoreactive neurons including Purkinje cells, basket, and stellate cells in the molecular layer, and Golgi cells in the granule cell layer are shown in the top right panel. Glycine-immunoreactive neurons in the cerebellar cortex including Lugaro cells in the Purkinje cell layer, and Golgi cells in the granule cell layer are shown in the bottom left panel. A merged image of glutamate-, GABA-, and glycine-immunoreactive neurons is shown in the bottom right panel. Colocalization of GABA and glycine-immunoreactive neurons can be seen in some Golgi and Lugaro cells. Glu, Glutamate; Gly, glycine. Scale bar, 200 μm.
Glutamate-, GABA-, and glycine-immunoreactive neurons in the DCN including the AIN, dentate nucleus, and granule cell layer of the cerebellar cortex are shown in Figure 9. Large neurons in the DCN and small granule cells in the cerebellar cortex are glutamate immunoreactive. Small neurons and numerous terminals in the DCN are GABA immunoreactive. In addition, several Golgi cells in the granule cell layer in the same section are also GABA immunoreactive. Glycine-immunoreactive neurons are small and evenly distributed in the DCN. In addition, glutamate was found to colocalize with most GABA-immunoreactive neurons to various degrees. Because glutamate is a precursor of GABA, it is present in GABAergic cells as a function of their metabolic state (Ottersen and Storm-Mathisen, 1984; Sultan et al., 2002). Also, glutamate labeling was never found in purely glycine-immunoreactive neurons. However, GABA/glycine-immunoreactive neurons showed glutamate labeling to various degrees. Consequently, glutamate-immunoreactive neurons were classified as glutamatergic only when they did not colocalize with other neurotransmitters. An example of a 4.5 d PRV-labeled neuron immunoreactive for glutamate is shown in Figure 10. PRV-labeled neurons immunoreactive for glutamate were large (29 μm; range 21–27 μm), and an average of 20 neurons (range 13–27) were found in the AIN 4.5 dafter injection.
Glutamate, GABA, and glycine immunoreactivity in the DCN and cerebellar cortex. A section that contains the dorsolateral AIN, dorsal dentate nucleus (DN), and the granule cell layer of the cerebellar cortex is shown. Glutamate-immunoreactive neurons are shown in the top left panel. Note large glutamate-immunoreactive neurons in the DCN and numerous granule cells in the cerebellar cortex. GABA-immunoreactive neurons are shown in the top right panel. Note smaller GABA-immunoreactive neurons and numerous terminals in the DCN and several Golgi cells in the granule cell layer. Glycine-immunoreactive neurons are shown in the bottom left panel. Note small distinctive glycine-immunoreactive neurons evenly distributed in the DCN. A merged image of glutamate, GABA, and glycine-immunoreactive neurons is shown in the bottom right panel. Glu, Glutamate; Gly, glycine. Scale bar, 400 μm.
Glutamate immunoreactive PRV-labeled neuron in the AIN 4.5 d after injection into the OOM. Glutamate immunoreactivity is shown in the top left panel. Note a large glutamate-immunoreactive neuron at the bottom of the panel indicated by the asterisk. GABA-immunoreactivity is shown in the top middle panel. Four GABA-immunoreactive interneurons are visible and note the presence of glutamate immunoreactivity in their cell bodies. Numerous GABA-immunoreactive terminals are evident apposed to different neuronal processes and glutamate-immunoreactive somas. Glycine-immunoreactivity is shown in the top right panel. Note a small interneuron that is exclusively glycine-immunoreactive. A few glycine-immunoreactive terminals apposing dendrites and somas of glutamate-immunoreactive and GABA-immunoreactive neurons are shown. A PRV-labeled neuron is shown in the bottom left panel. A merged image of glutamate-, GABA-, and glycine immunoreactivity and PRV is shown in the bottom right panel. Note that the PRV-labeled neuron colocalizes with a large glutamate-immunoreactive neuron. A small interneuron immunoreactive for both GABA and glycine is also shown. Glu, Glutamate; Gly, glycine. Scale bar, 40 μm.
Next, characterization of PRV-labeled neurons 5 d after injection revealed an average of 34 (range 25–43) glutamate-immunoreactive neurons and an average of 66 (range 54–78) interneurons immunoreactive for GABA and/or glycine. The interneurons were immunoreactive for GABA (30%), glycine (18%), or for both GABA and glycine (52%). The average soma diameter for PRV-labeled interneurons immunoreactive for GABA was 16 μm (range 12–20 μm), for glycine 15 μm (range 11–19 μm), and for GABA/glycine 17 μm (range 12–22 μm). An example of a PRV-labeled interneuron 5 d after injection is shown in Figure 11. In this case, a PRV-labeled interneuron is immunoreactive for both GABA and glycine. We were able to follow the PRV-labeled axon of this neuron and found its terminal apposed to an adjacent interneuron that was also GABA/glycine-immunoreactive. Interestingly, the terminal of the PRV-labeled interneuron was glycine immunoreactive only, suggesting that mixed GABA/glycinergic interneurons in the DCN can selectively release either neurotransmitter from their terminals. Differential neurotransmitter release from mix GABA/glycinergic neurons has been previously hypothesized (Dumoulin et al., 2001; Dugué et al., 2005; Dufour et al., 2010; Benarroch, 2011).
GABA and glycine immunoreactive interneuron labeled with PRV. GABA immunoreactivity is shown in the top left panel. Note two GABA-immunoreactive interneurons and numerous GABA-immunoreactive terminals. Glycine immunoreactivity is shown in the top right panel. Note two Glycine-immunoreactive interneurons and a few and densely packed Glycine-immunoreactive terminals. PRV-labeled fourth-order interneuron and its PRV-labeled terminal are shown in the bottom left panel. A merged image of GABA immunoreactivity, glycine immunoreactivity, and PRV is shown in the bottom right panel. Note that the PRV-labeled interneuron is immunoreactive for both GABA and glycine and its PRV-labeled terminal is immunoreactive solely for glycine. Glu, Glutamate; Gly, glycine. Scale bar 20 μm.
Discussion
The present study shows the premotor pathway of the rabbit OOM using PRV as a retrograde transneuronal tracer. Relevant structures involved in the generation or modulation of the rabbit eyeblink response were identified and provide anatomical validation of a direct premotor network that involves the dorsolateral AIN of the DCN and HVI of the cerebellar cortex, which have been implicated in eyeblink conditioning. Of particular importance, classification of fourth-order premotor interneurons based on their neurotransmitter immunoreactivity revealed three different types of inhibitory interneurons that are part of the OOM premotor pathway and form a functional network within the AIN for the modulation of motor commands.
Premotor pathway of the rabbit OOM
At 3 d after PRV injection, first-order motor neurons were found ipsilaterally in the dorsolateral facial nucleus. At 4 d, the dorsolateral magnocellular red nucleus was labeled contralaterally. At 4.5 d, third-order premotor neurons were found in dorsolateral AIN and the rostral fastigial nucleus ipsilaterally. At 5 d, the fastigial, interpositus, and dentate nucleus were labeled bilaterally with ipsilateral predominance. A number of fourth-order Purkinje cells were found in two cerebellar cortex locations, HVI zone C3 and lobule I zone A, and two distinct pathways were discerned. The first involves HVI, AIN, red nucleus, and facial nucleus, and the second may involve lobule I, fastigial nucleus, vestibular nucleus, and facial nucleus. In addition, second- and third-order premotor neurons were found in reticular nuclei and sensory trigeminal, auditory, vestibular, and motor structures. These may constitute secondary pathways and are no doubt involved in the modulation of eyelid movements by other response systems (e.g., startle, orientation, attention). These higher-order pathways have been reviewed extensively by Morcuende et al. (2002).
Cerebellar cortex
There is an ongoing controversy about which lobules in cerebellar cortex control conditioned eyeblinks. Rabbit lesion, infusion, and recording studies have implicated HVI in eyeblink conditioning (Berthier and Moore, 1986; Gould and Steinmetz, 1996; Attwell et al., 2001). More recent studies suggest anterior lobules HIV and HV are also involved in conditioning (Garcia et al., 1999; Green and Steinmetz, 2005; Kalmbach et al., 2010). However, the functional organization of cerebellar cortex is consistent with longitudinal zones that span multiple lobules, and regions controlling the rabbit eyelid may not be confined to a single lobule. In fact, there are multiple eyelid microzones in cerebellar cortex that receive climbing fiber inputs during periocular stimulation, exhibit eyeblink-related activity patterns, and project to the AIN. An additional rabbit eyelid microzone has been identified in the ventral portion of HVI (Mostofi et al., 2010). It is conceivable that different eyeblink microzones encode different types of information including time, position, intensity, and duration, and that together these microzones convey information to their target nuclear cells that then elicit a motor command.
To date, it is not clear how Purkinje cell activity controls eyelid movement. On the one hand, a pause in inhibitory, tonically active Purkinje cells allows target nuclear cells to produce the necessary activation required to generate a motor command. On the other hand, a burst of Purkinje cell activity may produce inhibition of target nuclear cells that is followed by rebound depolarization that results in a motor command (Pugh and Raman, 2006; Alviña et al., 2008; Molineux et al., 2008). Recordings from eyeblink microzones show that some Purkinje cells increase their firing rate while others decrease their firing during performance of a conditioned eyeblink response.
The microcircuit of the AIN
Information processed in the cerebellum is integrated in the DCN where motor commands are generated and executed. Despite their importance, little is known about the components that constitute this local network and their interconnections. Potential interactions among interneurons in the DCN and their role in learning are largely unknown. The AIN has been implicated in eyeblink conditioning, and synaptic changes responsible for a conditioned response are hypothesized to occur in this nucleus. Lesion and inactivation studies show that the AIN is critical for conditioned responses (Lavond et al., 1984; Steinmetz et al., 1992; Krupa and Thompson, 1997). Single unit recordings in AIN show some neurons increase their firing rate during conditioned responses in a pattern that precedes and predicts the response (McCormick and Thompson, 1984). In vitro studies in the interpositus show large neurons can undergo different types of synaptic plasticity, including LTP and LTD (Pugh and Raman, 2006). Recently, the electrophysiological properties of DCN interneurons have been studied in transgenic mice expressing GAD-eGFP or GlyT2-eGFP (Uusisaari and Knöpfel, 2011). However, little is known about the synaptic connections and interactions among the different neuronal types.
Our results show three types of interneurons that are directly connected to large glutamatergic projection neurons and possibly involved in modulating their output. The DCN is a complex structure and different components and interactions contribute to the integration of a final cerebellar output. Here, we show a local network within AIN consisting of a glutamatergic projection neuron and three types of inhibitory interneurons that are part of the OOM premotor pathway. PRV-labeled fourth-order interneurons were immunoreactive for GABA, glycine, or both GABA and glycine. Interconnectivity was found in a PRV-labeled mixed GABA/glycinergic interneuron in which we were able to follow the axon. The terminal of this interneuron was labeled with PRV and apposed the soma of another GABA/glycinergic-immunoreactive interneuron that was not labeled with PRV, suggesting these two interneurons contact different glutamatergic neurons. GABA and glycine are frequently coexpressed in the same cell and coreleased from the same terminals (Ottersen et al., 1988; Dumoulin et al., 2001; Dugué et al., 2005). Mixed GABA/glycinergic neurons are thought to modulate the ratio of neurotransmitter release as these neurotransmitters have different effects on their postsynaptic targets (Benarroch, 2011). Interestingly, the synaptic terminal of the PRV-labeled mixed GABA/glycinergic interneuron was immunoreactive solely for glycine, suggesting differential neurotransmitter release. Glycine has been implicated in different types of synaptic plasticity, including LTP (Martina et al., 2004), and is required for the activation of NMDA receptors (Johnson and Ascher, 1987), suggesting another possible mechanism of plasticity in AIN.
Based on the observed interconnectivity of interneurons described above and current knowledge of AIN organization, a schematic diagram of possible interactions is depicted in Figure 12. The figure shows Purkinje cell inhibitory inputs as well as excitatory mossy fiber and climbing fiber collateral inputs arriving at large glutamatergic projection neurons. Also depicted are Purkinje cell inhibitory inputs and presumed mossy fiber and climbing fiber collateral projections to interneurons that provide their only excitatory input. Finally, the figure proposes inhibitory connections between interneurons. These connections allow one to speculate about the consequences of interactions among and between interneurons and projection neurons. For example, although mossy fiber and climbing fiber collaterals activate a PRV-positive glutamatergic projection neuron, they also activate inhibitory interneurons that, in turn, inhibit adjacent PRV-negative projection neurons creating an inhibitory surround. In addition, the inhibitory interneuron contacted by these mossy fiber and climbing fiber collaterals also synapses onto a second interneuron, which, in turn, disinhibits the PRV-positive projection neuron. As a result of releasing inhibition, sensory inputs could increase excitation of the PRV-positive projection neuron while indirectly inhibiting adjacent PRV-negative projection neurons. These interactions are modulated by Purkinje cell inhibition. One consequence of this combination of excitation and inhibition of projection neurons could be coordination of the OOM and levator palpebrae, allowing closure of the eyelids (Sánchez-Campusano et al., 2012). In the case of eyeblink conditioning, increased Purkinje cells inhibition of the inhibitory interneurons apposing a projection neuron would increase the likelihood of that cell firing and producing a conditioned response.
Organization of the AIN circuit. A schematic representation of different neuronal populations and their connections in the AIN. The premotor pathway of the OOM is shown with black arrows that delineate the direction of PRV labeling. Two representative glutamatergic (GLU) projection neurons are shown. A PRV-labeled third-order GLU neuron projecting to the red nucleus (RN) is depicted with a black arrow. Three types of PRV-labeled fourth-order interneurons are shown to make a direct connection onto the PRV-labeled GLU neuron. Possible connections among different AIN neurons are represented with excitatory (+) and inhibitory (−) terminals (colored triangles). Excitatory input reaches the AIN by mossy fiber (MF) and climbing fiber (CF) collaterals that make connections on GLU neurons and possibly (dashed lines) on different interneurons. Inhibitory input to AIN neurons is provided by Purkinje cells (PC) and local interneurons. 7N, Facial nucleus; GrC, granule cell layer; IO, inferior olive; PF, parallel fibers.
Comparison with other transsynaptic studies of the OOM
A study in mouse using PRV (Sun, 2012) and another in rat using rabies virus (Morcuende et al., 2002) also delineated the eyeblink premotor pathway. Despite some similarities, there are significant differences between our results and those of Sun (2012). Although motor neurons were found in ipsilateral facial nucleus after PRV injection, labeling was also found in ventral and dorsal red nucleus bilaterally, rather than our contralateral labeling in dorsolateral red nucleus that agrees with previous research (Takada et al., 1984; Holstege and Tan, 1988). This suggests Sun (2012) may have identified pathways not directly connected to the facial nucleus because averaging across different time points combined different synaptic steps. This is true for the cerebellum as well because of extensive bilateral labeling of all three deep nuclei as well as bilateral labeling throughout the cerebellar cortex. Thus, a direct premotor pathway from cerebellum to the facial nucleus may have been present in PRV-injected mice, but it was obscured by more indirect pathways.
An earlier study of the rat OOM premotor pathway was performed using rabies (Morcuende et al., 2002) and corresponds well with the rabbit OOM premotor pathway identified using PRV, at least to the level of third-order premotor neurons. Morcuende et al. (2002) found rabies-labeled neurons in caudolateral AIN and dorsolateral hump of DCN, whereas in the rabbit, third-order neurons were located in dorsolateral AIN and the rostral fastigial nucleus. In addition, they found fourth-order labeled Purkinje cells in the vermis and paravermis zones C1–C3, whereas in the rabbit, fourth-order Purkinje cells were found exclusively in HVI zone C3 and Lobule I zone A. These differences may reflect anatomical or functional differences between species or variations in viral kinetics.
Footnotes
This research was supported in part by NIH Grant NS061103, a WVU Bridge Grant, and funds from Blanchette Rockefeller Neurosciences Institute. PRV strains were provided by L.W. Enquist supported by NIH P40 OD010996. We thank Carrie Smith-Bell and Roger Bell for technical assistance.
The authors declare no competing financial interests.
- Correspondence should be addressed to either of the following: Jimena Gonzalez-Joekes, Blanchette Rockefeller Neurosciences Institute, 8 Medical Center Drive, West Virginia University, Morgantown, WV 26506, jgonzalez{at}hsc.wvu.edu; or Bernard G. Schreurs, Blanchette Rockefeller Neurosciences Institute, 8 Medical Center Drive, West Virginia University, Morgantown, WV 26506, bschreurs{at}hsc.wvu.edu