Neuronal Premotor Networks Involved in Eyelid Responses: Retrograde Transneuronal Tracing with Rabies Virus from the Orbicularis Oculi Muscle in the Rat

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The Journal of Neuroscience, October 15, 2002, 22(20):8808-8818

Neuronal Premotor Networks Involved in Eyelid Responses: Retrograde Transneuronal Tracing with Rabies Virus from the Orbicularis Oculi Muscle in the Rat
Sara Morcuende¹, José-Maria Delgado-García¹, and Gabriella Ugolini²
¹ Laboratorio Andaluz de Biología, Universidad Pablo de Olavide, 41013 Sevilla, Spain, and ² Laboratoire de Virologie Moléculaire et Structurale, Centre National de la Recherche Scientifique, 91198 Gif-sur-Yvette, France

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Retrograde transneuronal tracing with rabies virus from the right orbicularis oculi muscle was used to identify neural networksunderlying spontaneous, reflex, and learned blinks. The kineticsof viral transfer was studied at sequential 12 hr intervals between3 and 5 d after inoculation. Rabies virus immunolabeling was combinedwith the immunohistochemical detection of choline acetyltransferaseexpression in brainstem motoneurons or Fluoro-Ruby injectionsin the rubrospinal tract. Virus uptake involved exclusively orbicularisoculi motoneurons in the dorsolateral division of the facial nucleus.At 3-3.5 d, transneuronal transfer involved premotor interneuronsof trigeminal, auditory, and vestibular reflex pathways (in medullaryand pontine reticular formation, trigeminal nuclei, periolivaryand ventral cochlear nuclei, and medial vestibular nuclei), motorpathways (dorsolateral quadrant of contralateral red nucleus andpararubral area), deep cerebellar nuclei (lateral portion of interpositusnucleus and dorsolateral hump ipsilaterally), limbic relays (parabrachialand Kölliker-Fuse nuclei), and oculomotor structures involvedin eye-eyelid coordination (oculomotor nucleus, supraoculomotorarea, and interstitial nucleus of Cajal). At 4 d, higher orderneurons were revealed in trigeminal, auditory, vestibular, anddeep cerebellar nuclei (medial, interpositus, and lateral), oculomotorand visual-related structures (Darkschewitsch, nucleus of theposterior commissure, deep layers of superior colliculus, andpretectal area), lateral hypothalamus, and cerebral cortex (particularlyin parietal areas). At 4.5 and 5 d the labeling of higher orderneurons occurred in hypothalamus, cerebral cortex, and blink-relatedareas of cerebellar cortex. These results provide a comprehensivepicture of the premotor networks mediating reflex, voluntary,and limbic-related eyelid responses and highlight potential sitesof motor learning in eyelid classicalconditioning.

Key words: cerebellum; eyelid responses; parietal cortex; rabies virus; rats; red nucleus; reflex blinks; reticular formation

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The kinematics and frequency domain properties of eyelid responses have been reported in a quantitative manner for spontaneous,reflex, passive, and learned movements in rabbits, cats, and humans(McCormick et al., 1982; Gormezano et al., 1983; Woody, 1986;Evinger et al., 1991; Welsh, 1992; Thompson and Krupa, 1994; Domingoet al., 1997; Gruart et al., 2000a). The activity of selectedneural structures has been related convincingly to different aspectsof reflex and learned eyelid responses. Thus, the properties oforbicularis oculi motoneurons involved in eyelid closing havebeen described previously (Trigo et al., 1999), and a relationshipbetween neural firing responses and eyelid movements has beenreported for several brain sites, e.g., red nucleus, cerebellarcortex and nuclei, motor cortex, and hippocampus (Berger et al.,1983; McCormick and Thompson, 1984; Berthier and Moore, 1986,1990; Aou et al., 1992; Keifer, 1993; Gruart et al., 2000b; Múneraet al., 2001). A map of the sites involved in the generation ofclassically conditioned eyelid responses has been proposed (Kimand Thompson, 1997) on the basis of lesion or inactivation ofgiven neuralstructures.

Nevertheless, despite some really valuable attempts (Courville, 1966; Takeuchi et al., 1979; Hinrichsen and Watson, 1983;Travers and Norgren, 1983; Fanardjian and Manvelyan, 1984, 1987a,b;Takada et al., 1984; Holstege et al., 1986a,b; Isokawa-Akessonand Komisaruk, 1987; Fort et al., 1989), available informationregarding the organization of the eyelid premotor system is limited.Eyelid movements are specialized motor responses, related notonly to corneal protection but also to emotional expression, visualperception, and eye movements and are susceptible to motor learning.Given the diversity of sensory sources able to activate eyelidmuscles and the variety of behavioral displays in which they areinvolved, the underlying neuronal network should be rather complex.A comprehensive map of such networks could not be obtained withconventional tracers (Mesulam, 1982; Kuypers and Huisman, 1984;Köbbert et al., 2000) but now can be accomplished with retrogradetransneuronal tracers that are able to reveal neuronal networksin their entirety. The most effective transneuronal tracers areviruses because of their ability to function as self-amplifyingmarkers (Ugolini et al., 1989; Kuypers and Ugolini, 1990; Ugolini,1995a,b). Rabies virus is the most valuable, particularly forstudying motor networks, because after its injection into musclesor nerves it is taken up exclusively by motoneurons, without uptakeby sensory or sympathetic neurons (Ugolini, 1995b; Tang et al.,1999; Kelly and Strick, 2000; Graf et al., 2002). Rabies viruspropagates exclusively by retrograde transneuronal transfer. Transferis time-dependent, enabling a sequential visualization of seriallyconnected neurons across an unlimited number of synapses. Rabies-infectedneurons remain viable and intact (Ugolini, 1995b; Tang et al.,1999; Graf et al., 2002).

We have exploited this powerful method to study the neural networks controlling the orbicularis oculi muscle. Our resultsprovide a comprehensive map of such networks, showing the involvementof different sensory modalities (trigeminal, vestibular, auditory,and visual) in the genesis and control of eyelid responses andthe participation of specific portions of sensorimotor cortex,red nucleus, reticular formation, and cortical and nuclear cerebellarareas.

Some results already have been published in abstract form (Ugolini et al., 1999).

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Viral tracer. The virus used in this study was the challenge virus standard (CVS), fixed strain 11 of rabies virus (Ugolini,1995b). Concentrated virus [titer 1-1.5 × 10¹⁰ plaque-forming units (pfu)/ml] was prepared by pelleting thesupernatant of baby hamster kidney-21 (BHK-21) cells infectedfor 72 hr through a cushion of 25% glycerol. The virus stock waskept frozen at $-$ 70°C until a few minutes beforeuse.

Animals, virus injection, and perfusion procedures. Experiments were performed in 55 albino Wistar rats (Iffa Credo, Les Oncins,France), weighing 250-300 gm. Animal care and experimental proceduresconformed with French Government, European Union Directive (86/609/EU),and National Institutes of Health guidelines. Surgery was performedaseptically under general anesthesia (Avertin 1.3-1.5 ml/100 gm,i.p., plus supplementary doses as required to maintain areflexia).The right orbicularis oculi muscle was exposed after a sagittalincision of the scalp. Using a glass micropipette connected toa pressure pump, we placed two injections of rabies virus (3-4.5µl each) into the preseptal and pretarsal portions of the muscle,respectively, to map premotor innervation of both muscle components.The pipette was inserted in the muscle under microscopic guidanceand kept in place for 5 min after each injection. Any eventualleakage of the inoculum was removed with cotton swabs. The woundswere sutured with sterile surgical silk. Rats were caged individuallyand examined daily. They were perfused for histological examinationat sequential 12 hr intervals from 3 to 5 d after injection (3d, n = 11 rats; 3.5 d, n = 16 rats; 4 d, n = 14 rats; 4.5 d, n= 4 rats; 5 d, n = 10 rats). None of the rats exhibited neurologicalsymptoms or behavioral changes at these times, which correspondto the asymptomatic period of rabies (Ugolini, 1995b; Tang etal., 1999). At the chosen time points the rats were anesthetizeddeeply (Avertin, 2.5 ml/100 gm of body weight) and perfused transcardiallywith 500 ml of PBS, followed by 500 ml of 4% paraformaldehydein 0.1 M phosphate buffer and 500 ml of 15% sucrose in 0.1 M phosphatebuffer (perfusates, pH 7.4). The brains were dissected out andtransferred to a 15% sucrose solution in which they were keptovernight at 4°C for cryoprotection before histologicalprocessing.

In five rats the rabies virus injections as above were combined in the same surgical session with ipsilateral spinal injectionsof the retrograde fluorescent tracer Fluoro-Ruby to identify rubrospinalneurons in the same experiment. For this purpose a hemi-laminectomywas performed to expose the right side of the C3-C5 spinal segments,and two injections (3 µl each) of Fluoro-Ruby 10% were made intothe white and gray matter, centered on the dorsolateral funiculusin which the rubrospinal tract is located. These rats were killedfor analysis 5 dlater.

Histology. Brains were cut on a cryostat in coronal sections (50 µm) that were collected free-floating in four parallel series.In two alternative series the rabies immunolabeling was detectedby using the peroxidase-antiperoxidase method (Ugolini, 1995b).One series was counterstained with cresyl violet. Sections fromthe remaining series were used for dual-color immunofluorescencedetection of rabies virus and choline acetyltransferase, for doublefluorescence detection of rabies virus and Fluoro-Ruby, or asa positive control in the various immunohistochemicalreactions.

For immunoperoxidase staining the free-floating sections were incubated at room temperature in 0.3% H₂O₂ in PBS for 1 hr,followed by 0.2% swine normal serum in PBS for 1 hr, and thenwere incubated overnight at 4°C with rabbit polyclonal antibodiesraised against rabies virus nucleocapsid (dilution, 40 µg/ml;Sanofi Pasteur, Paris, France). Subsequently, the sections wereincubated at room temperature for 2 hr in swine anti-rabbit IgG(Dako, Trappes, France) diluted 1:200, followed by 2 hr in rabbitimmunoperoxidase complex (Dako) diluted 1:200. Several washeswith PBS were performed between steps. Peroxidase activity wasrevealed by incubation (2-10 min) in a metal-enhanced diaminobenzidinesubstrate kit (Pierce, Rockford, IL). Staining specificity waschecked by incubating each series together with positive controls(i.e., sections from brains having shown rabies immunolabelingin previous reactions) and negative controls (sections from noninfectedbrains). Sections were mounted on gelatin-coated slides, air-dried,and coverslipped with Entellan (Merck, Whitehouse Station,NJ).

One series of sections from rats killed at 4 d was treated by using a dual-color immunofluorescence protocol for simultaneousdetection of rabies virus and choline acetyltransferase, usedhere as a marker for motoneurons. Free-floating sections wereincubated in 0.4% Triton X-100 for 30 min and in 3% donkey serum(Chemicon, Temecula, CA) for 1 hr, followed by incubation (20hr) at 4°C in a mixture of mouse monoclonal antibodies recognizingthe rabies P-protein (Laboratoire de Génétique des Virus, Gif-sur-Yvette,France) diluted 1:100 and goat anti-choline acetyltransferase(Chemicon AB144P) diluted 1:100. After being rinsed in PBS, thesections were incubated for 2 hr at room temperature in a mixtureof fluorescein isothiocyanate (FITC)-conjugated donkey anti-mouseIgG (1:100; Jackson ImmunoResearch, West Grove, PA), and indocarbocyanine(Cy3)-conjugated donkey anti-goat IgG (1:100; Chemicon). Primaryand secondary antibodies were diluted in PBS containing 3% donkeynormal serum and 2% bovine serum albumin. Staining specificitywas checked by omitting the primary or secondary antibody andby using positive and negative controls. After several washesin PBS the sections were mounted on slides and coverslipped withVectashield (Vector Laboratories, Burlingame,CA).

In the experiments involving rabies immunolabeling in combination with retrograde labeling of rubrospinal neurons by meansof the red fluorescent tracer Fluoro-Ruby, the sections were treatedfor immunofluorescent (FITC, green) visualization of the rabiesantigen as describedabove.

Analysis. Fluorescent preparations were observed with a Leitz epifluorescence microscope. Selected images were captured byusing a digital camera (Leitz DC-250, Wetzlar, Germany) and theIM-1000 Image Manager (Leica, Nussloch,Germany).

Rabies-immunolabeled neurons in the brain were plotted by using an analog x-y plotter connected by potentiometers to the microscopestage or the computer-assisted Neurolucida system (MicroBrightField,Colchester, VT). The location of labeled neurons was illustratedin various drawings. In all drawings the retrogradely labeledorbicularis oculi motoneurons are indicated by asterisks. Eachdot represents one rabies transneuronally labeled neuron. Thenomenclature is according to Paxinos and Watson (1986).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Kinetics of infection of orbicularis oculi motoneurons (first-order neurons)

After rabies virus injection into the right orbicularis oculi muscle, rabies-immunolabeled motoneurons were found exclusivelywithin the dorsolateral subdivision of the ipsilateral facialnucleus (Fig. 1A), where orbicularis oculi motoneurons are knownto be located (Martin and Lodge, 1977; Faulkner et al., 1997).Primary sensory neurons in Gasser's ganglion, which also innervatethe orbicularis oculi muscle, were not labeled, confirming thelack of peripheral uptake of rabies virus by sensory neurons (Tanget al., 1999; Kelly and Strick, 2000; Graf et al., 2002). At noneof the time points that were explored (3-5 d after inoculation)were labeled motoneurons found in other subdivisions of the facialnucleus (Fig. 1A), showing that no spurious diffusion of the virustracer occurred either from the orbicularis oculi muscle to neighboringfacial muscles or within the facial nucleus itself.

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Figure 1. Shown are photomicrographs of rabies-immunolabeled brainstem neurons at 3 d (A), 3.5 d (B, D, F), and 4 d (C, E) after rabies virus injection into the right orbicularis oculi muscle. A, Labeled orbicularis oculi motoneurons in the dorsolateral (dl) division of the facial nucleus. Note the absence of labeling in the other divisions. B, Labeled neurons in the ipsilateral medullary reticular formation. C, Labeled neurons in the ipsilateral spinal trigeminal nucleus, pars oralis (SPVo). D, Labeled neurons in the ipsilateral ventral cochlear nucleus (VCN). E, Labeled neurons in the ipsilateral medial vestibular nucleus (MV) and in the nucleus reticularis paragigantocellularis dorsalis (RPgcd). F, Labeled neurons in the dorsolateral quadrant of the contralateral red nucleus (R) and overlying pararubral area. Scale bars: A, 100 µm; B-F, 500 µm. i, l, m, vm, Intermediate, lateral, medial, and ventromedial divisions of the facial nucleus; III, oculomotor nucleus; DV, descending vestibular nucleus; RCf, nucleus reticularis cuneiformis; RD, nucleus reticularis dorsalis; RV, nucleus reticularis ventralis, SPVc, spinal trigeminal nucleus, pars caudalis.

Rabies-immunolabeled orbicularis oculi motoneurons showed normal size, morphology, and Nissl staining as well as normal levelsof expression of the choline acetyltransferase marker. Glial cellswere not infected. As illustrated in Figure 1A, the number ofpositive motoneurons quantified at 3 d after inoculation was low(12 ± 4 SD; n = 8 animals) and did not show any significant increaseat later time points (13 ± 3; counted from n = 10 animals at 5d). The low number of retrogradely labeled motoneurons is probablyattributable to the fact that the tracer injections had involvedonly a few motor endplates because of their restricted, nonintermingleddistribution in the orbicularis oculi muscle. Notably, the findingthat labeled orbicularis oculi motoneurons did not become morenumerous with time indicates that rabies virus uptake remainedrestricted to the injection sites, i.e., the virus tracer didnot diffuse even within the muscleitself.

Retrograde transneuronal labeling of eyelid premotor networks

The kinetics of retrograde transneuronal transfer of rabies virus was studied at sequential 12 hr intervals from 3 to 5 dafter injection. Transneuronal transfer was time-dependent. Theresults obtained at successive time points were highly reproducible,showing a progressive increase in the number of labeled neuralsites and in the number of rabies-immunolabeled neurons. As observedin other rodent models (Ugolini, 1995b; Tang et al., 1999), 3d after injection was sufficient for the onset of transneuronallabeling of second-order neurons, i.e., neurons projecting monosynapticallyonto orbicularis oculi motoneurons. At this time point, however,transneuronal labeling occurred only in some cases and involvedonly a subset of the total population of second-order neurons,presumably those that are connected more heavily with orbicularisoculi motoneurons and that synapse proximally on the motoneuronssoma-dendritic trees (Ugolini, 1995b; Graf et al., 2002). Thus,only a few labeled neurons were found in specific portions ofthe brainstem reticular formation (nuclei reticularis ventralis,dorsalis, magnocellularis, and cuneiformis) and auditory (periolivary)structures (see below) and at the ventral border of the spinaltrigeminal nucleus in somecases.

At 3.5 d, transneuronally labeled neurons at these locations became more numerous, and additional sites became labeled (Fig.2). On the basis of the correspondence with the results of tracingstudies (Courville, 1966; Takeuchi et al., 1979; Hinrichsen andWatson, 1983; Travers and Norgren, 1983; Takada et al., 1984;Holstege et al., 1986a,b; Isokawa-Akesson and Komisaruk, 1987;Fort et al., 1989), neuronal labeling at this time point stillinvolved second-order neurons (Ugolini, 1995b). Notably, onlya few labeled neurons were seen within the medial border of theipsilateral spinal trigeminal nucleus, pars spinalis, interpolaris,and oralis (Fig. 2). Most of the labeled neurons were locatedipsilaterally in specific portions of the caudal medullary lateralreticular formation (labeled already at 3 d), i.e., in the nucleusreticularis dorsalis and in the ventral part of the caudalmostportion of the nucleus reticularis parvocellularis as well asin the adjoining nucleus reticularis ventralis (Figs. 1B, 2B-D).Contralaterally, labeling in the reticular formation at theselevels was sparse and located mainly ventrally in the nucleusreticularis ventralis and parvocellularis (Fig. 2B-D). More rostralportions of the medullary lateral reticular formation showed verylittle labeling. In the medullary medial reticular formation thelabeling involved primarily the nucleus reticularis magnocellularisbilaterally, mainly ipsilaterally (Fig. 2E-G). A few labeled neuronsalso were found in the nucleus reticularis gigantocellularis,in the medial part of the nucleus reticularis paragigantocellularisdorsalis, and in the adjoining medial longitudinal fasciculus.More rostrally, some labeled neurons were seen in the nucleusreticularis pontis caudalis and oralis, particularly in the ventralreticular area neighboring the superior olivary complex. Notably,a dense accumulation of labeled neurons was found, mainly ipsilaterally,in auditory structures in which labeling already had been observed12 hr previously, particularly in the caudal periolivary nuclei,in the nucleus of the trapezoid body and the ventral periolivarynucleus, and, to a lesser degree, in the rostral periolivary nucleus(Fig. 2H-J). Labeling also occurred bilaterally in the caudalpart of the ventral cochlear nucleus (Figs. 1D, 2F). A dense accumulationof labeled neurons was seen in the nucleus of Kölliker-Fuse andventral parabrachial nuclei ipsilaterally (Fig. 2J). Sparse labelingwas found in the nucleus of the solitary tract in only two (of16) cases. A few labeled neurons were seen in the medial vestibularnucleus at rostral levels (Fig. 2). Notably, dense labeling atthis time point appeared in specific portions of the deep cerebellarnuclei, i.e., in the caudolateral part of the anterior interpositusnucleus and dorsolateral hump ipsilaterally (Fig. 2G). In themesencephalon a dense accumulation of labeled neurons was seenin the dorsolateral quadrant of the contralateral red nucleusand in the dorsally adjoining pararubral area (Ruigrok and Cella,1995), which is part of the nucleus reticularis cuneiformis (Figs.1F, 2K,L), suggesting strong synaptic links with orbicularis oculimotoneurons. Sparse labeling occurred in the interstitial nucleusof Cajal (Fig. 2L). Some labeled neurons also were found consistentlywithin the ipsilateral oculomotor nucleus and in the dorsallyadjoining supraoculomotor area (Fig. 2K). The neurons labeledwithin the oculomotor nucleus appeared to be smaller than motoneurons.They were identified clearly as oculomotor internuclear neuronsand not motoneurons because they were not cholinergic, as shownby the results of dual-color immunofluorescence for simultaneousvisualization of rabies and choline acetyltransferase antigens(see below).

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Figure 2. Brainstem distribution of rabies-immunolabeled neurons at 3.5 d after rabies virus injection into the right orbicularis oculi muscle. A-L, Labeled sections are arranged caudorostrally. The arrows indicate the side that is ipsilateral to the injection. Asterisks in F, G, Retrogradely labeled orbicularis oculi motoneurons in the dorsolateral division of the facial (VII) nucleus. Each dot represents one labeled neuron. Scale bar, 2 mm. CG, Central gray; CPO, caudal periolivary nucleus; D, nucleus of Darkschewitsch; DCN, dorsal cochlear nucleus; Dlh, dorsolateral hump; DH, dorsal horn; DV, descending vestibular nucleus; I, interpositus nucleus; INC, interstitial nucleus of Cajal; IO, inferior olive; KF, Kölliker-Fuse nucleus; L, lateral (dentate) nucleus; LV, lateral vestibular nucleus; M, medial (fastigial) nucleus; MV, medial vestibular nucleus; NST, nucleus of the solitary tract; PB, parabrachial nucleus; PT, pyramidal tract; PV, principal trigeminal nucleus; R, red nucleus; RCf, nucleus reticularis cuneiformis; RD, nucleus reticularis dorsalis; RGc, nucleus reticularis gigantocellularis; RMc, nucleus reticularis magnocellularis; RPc, nucleus reticularis parvocellularis; RPgcd, nucleus reticularis paragigantocellularis dorsalis; RPO, rostral periolivary region; RPoC, nucleus reticularis pontis caudalis; RPoO, nucleus reticularis pontis oralis; RSc, nucleus reticularis subceruleus; RV, nucleus reticularis ventralis; sai, stratum album intermedialis; SC, superior colliculus; sgi, stratum griseum intermedialis; sgs, stratum griseum superficialis; SNr, substantia nigra pars reticulata; so, stratum opticum; SO, superior olive; sp, strata profunda; SPO, superior paraolivary nucleus; SPVc, SPVi, SPVo, spinal trigeminal nuclei, pars caudalis, interpolaris, and oralis; tz, trapezoid body; VCN, ventral cochlear nucleus; VPO, ventral periolivary nucleus; III, oculomotor nucleus; XII, hypoglossal nucleus.

A great increase in the distribution and number of labeled neurons occurred at 4 d after inoculation. This additional 12 hrinterval is consistent with an additional synaptic step of transfer(Ugolini, 1995b; Tang et al., 1999; Graf et al., 2002). Correspondingly,transneuronal labeling obtained at this time point clearly involvedhigher order (presumably third-order) neurons connected polysynapticallyto orbicularis oculimotoneurons.

The distribution of labeling in the medulla, pons, and mesencephalon at 4 d is illustrated in Figures 3-5. At medullary levelsone of the characteristic features of this time point was theappearance of extensive labeling ipsilaterally in the principaland spinal trigeminal nuclei and in the dorsal horn of the firstcervical segments (Figs. 1C, 3B, 4). Labeling was particularlydense and widely distributed in deep layers of the dorsal horn(Figs. 3B, 4A) and in the adjoining caudalmost portion of thespinal trigeminal nucleus, pars caudalis (Fig. 4B). At more rostrallevels of the ipsilateral spinal trigeminal nucleus (pars caudalis,interpolaris, and oralis) and in the principal trigeminal nucleus,labeled neurons were seen only in the ventral part of these nuclei(Figs. 1C, 4C-I). Only sparse labeling was found in the contralateralspinal trigeminal nuclei and dorsal horn (Fig. 4).

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Figure 3. Rabies-immunolabeled neurons at 4 d after rabies virus injection into the right orbicularis oculi muscle. A, Transneuronally labeled neurons in nucleus reticularis magnocellularis (RMc). B, Labeled neurons in the ipsilateral dorsal horn (DH) and intermediate zone of the upper cervical cord. C, Labeled neurons in the contralateral dorsal nucleus of the lateral lemniscus (DLL) and inferior colliculus (IC). D, Labeled neurons in the dorsolateral quadrant of the contralateral red nucleus (R) and overlying pararubral area at 4 d (see also 3.5 d) (Fig. 1F). E, Labeled neurons in the nucleus of Darkschewitsch (D) and nucleus of the posterior commissure (NCP). Scale bars, 500 µm. III, Oculomotor nucleus; LL, lateral lemniscus.

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Figure 4. Distribution of rabies-immunolabeled neurons in the medulla and pons at 4 d after rabies virus injection into the right orbicularis oculi muscle. A-J, Labeled sections are arranged caudorostrally. Arrows indicate the side that is ipsilateral to the injected muscle. Asterisks in G, Retrogradely labeled orbicularis oculi motoneurons in the dorsolateral division of the facial (VII) nucleus. Each dot represents one labeled neuron. Scale bar, 2 mm. For abbreviations see the legend of Figure 2.

A considerable increase in the number and distribution of labeled neurons occurred also in the medullary and pontine reticularformation, where labeling became much more bilateral but stillshowed a clear dominance ipsilaterally in the portions of thenuclei reticularis dorsalis, ventralis, and parvocellularis thatalready had shown labeling at previous time points (Fig. 4). Theincrease in areal distribution of reticular neurons was particularlynoticeable in the intermediate zone of the upper cervical segments,in the nucleus reticularis gigantocellularis, reticularis pontiscaudalis and oralis, and reticularis cuneiformis (Fig. 4). Rabiesimmunolabeling provided a complete visualization of neuronal morphology,including distal dendrites (Fig. 3A).

Another feature of the 4 d time point was the dense labeling bilaterally in the medial, descending, and superior vestibularnuclei, particularly in the medial vestibular nucleus (Figs. 1E,4F-I). Labeling of the parabrachial nuclei became more pronouncedand bilateral, and some labeling occurred consistently in thenucleus of the solitary tract (Fig. 4C,D).

Besides a moderate increase in the number of labeled neurons in the auditory structures labeled at previous time points, additionallabeling appeared bilaterally in the dorsal cochlear nucleus (Fig.4H), in external layers of the inferior colliculus, and in thearea ventral to it corresponding to the dorsal nucleus of thelateral lemniscus (Figs. 3C, 5A,B). Sparse labeling occurred alsoin more ventral portions of the nucleus of the lateral lemniscus.

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Figure 5. Distribution of rabies-immunolabeled neurons in the mesencephalon and caudal diencephalon at 4 d after rabies virus injection into the right orbicularis oculi muscle. A-G, Labeled sections are arranged caudorostrally. Arrows indicate the side that is ipsilateral to the injected muscle. Each dot represents one labeled neuron. Scale bar, 2 mm. For abbreviations see the legend of Figure 2. APT, Anterior pretectal nucleus; CM, central medial nucleus; CP, cerebral peduncle; Hab, habenula; IC, inferior colliculus, LH, lateral hypothalamus; LL, lateral lemniscus, MGB, medial geniculate body; MN, mamillary nuclei; NCP, nucleus of the posterior commissure; PN, pontine nuclei; PO, posterior thalamic nucleus; PR, prerubral field; RR, retrorubral nucleus; Rt, reticular thalamic nucleus; VPM, ventral posteromedial thalamic nucleus; VTA, ventral tegmental area; ZI, zona incerta.

In the contralateral red nucleus the labeled neurons increased in number but remained restricted to the dorsolateral quadrantof the red nucleus and the adjoining pararubral area (Figs. 3D,5C,D). The contralateral prerubral and retrorubral areas alsowere labeled densely (Fig. 5).

At 4 d, labeling also appeared in intermediate and deep layers of the superior colliculus, mainly contralaterally (Fig. 5C-E).Several mesencephalic oculomotor-related structures were labeled,such as the nucleus of Darkschewitsch, the interstitial nucleusof Cajal, and the nucleus of the posterior commissure (Fig. 3E),mainly ipsilaterally, the supraoculomotor area, and some internuclearinterneurons located inside the oculomotor complex (Fig. 5C-F).Besides the supraoculomotor area, labeling involved more dorsalportions of the central gray and the dorsal raphe nucleus (Fig.5B-D). Some labeling also was seen in the pretectal nuclei (Fig.5F). Because the pretectal area receives afferences from the retina(Holstege et al., 1986a,b), this pathway is potentially involvedin flash-evoked blinks (Evinger et al., 1991; Gruart et al., 1995).Some labeling also was found bilaterally in the substantia nigra,lateral hypothalamus, and zona incerta (Fig. 5E-G).

In the deep cerebellar nuclei (Figs. 4H, 6A, 7), dense labeling occurred in the dorsolateral hump and in the lateral partof the anterior interpositus nucleus and posterior interpositusnucleus, except its caudalmost portion (Figs. 4H, 6A, 7B-E). Labelingwas bilateral with a clear ipsilateral dominance (contralaterallabeling involving mainly the dorsolateral hump) (Fig. 7C). Bilaterallabeling with a clear ipsilateral dominance appeared also in themedial (fastigial) nucleus and in the lateral (dentate) nucleus(Figs. 4H, 6A, 7B-E).

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Figure 6. Rabies-immunolabeled neurons in the cerebellar cortex and nuclei. A, Transneuronally labeled neurons in the medial (M, fastigial) nucleus, interpositus (I) nucleus, and dorsolateral hump (Dlh) at 4 d after the injection of rabies virus into the ipsilateral orbicularis oculi muscle. B, Transneuronal labeling of higher order neurons in the cerebellar vermis at 5 d after injection. Note the zonal distribution of labeled Purkinje cells. C, Coronal section through the paravermis, illustrating another area in which rabies-immunolabeled Purkinje cells were observed at 5 d after rabies virus injection in the ipsilateral orbicularis oculi muscle. Scale bars: A, B, 500 µm; C, 150 µm.

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Figure 7. Distribution of rabies-immunolabeled neurons in the deep cerebellar nuclei at 4 d after rabies virus injection into the right orbicularis oculi muscle (arrow indicates ipsilateral side). Sections in A-F are arranged from caudal to rostral. The dashed line denotes the midline. Each dot represents one labeled neuron. Note transneuronally labeled neurons bilaterally, with clear ipsilateral dominance, in medial (M, fastigial) nucleus, dorsolateral hump (Dlh), lateral part of posterior interpositus (PI) and anterior interpositus (AI), and lateral (L, dentate) nuclei. Scale bar, 2 mm.

Another distinctive feature of the 4 d time point was the appearance of labeling in the cerebral cortex (Figs. 8C, 9), whichis a clear reflection of polysynaptic links with orbicularis oculimotoneurons. Labeling involved exclusively pyramidal neurons inlayer V (see example in Fig. 8A). Most of the labeled neuronswere located in parietal cortex areas 1 and 2 (Pa1 and Pa2; Paxinosand Watson, 1986) bilaterally, with a clear contralateral dominance(Fig. 9). A few labeled neurons also were located in frontal (F1,F2) and occipital (Oc2L) cortices contralaterally. In four (of14) animals some labeled pyramidal cells also were found in theperirhinal and temporal (Te1) cortices (data not shown).

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Figure 8. Photomicrographs illustrating transneuronally labeled pyramidal cells in the contralateral parietal cortex at 4-5 d after rabies virus injection into the right orbicularis oculi muscle. A, Coronal section of the parietal cortex, area 1 (Pa1) at 4 d. B, Parietal cortex, area 1, at 5 d. Note the increase in the number of rabies-immunolabeled pyramidal cells. C, High-power photomicrograph of parietal cortex at 4.5 d. Note Golgi-like labeling of a pyramidal cell in layer V. Scale bars: A, B, 500 µm; C, 100 µm.

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Figure 9. Distribution of rabies-immunolabeled neurons in the cerebral cortex at 4 d after rabies virus injection into the right orbicularis oculi muscle. A-J, Labeled sections are arranged from caudal to rostral. Arrows indicate the ipsilateral side. Each dot represents one labeled neuron. Scale bar, 2 mm. At 4 d the labeled neurons were concentrated in parietal cortex, areas 1 and 2 (Pa1 and Pa2) bilaterally, with a clear contralateral dominance. APT, Anterior pretectal area; CG, central gray; D, nucleus of Darkschewitsch; Ent, entorhinal cortex; F1, frontal cortex, area 1; F2, frontal cortex, area 2; HL, hindlimb area of parietal cortex; INC, interstitial nucleus of Cajal; Oc2L, occipital cortex area 2, lateral; PrC, precommissural nucleus; Prh, perirhinal cortex; R, red nucleus; SNr, substantia nigra, pars reticulata; Te1, temporal cortex, area 1; Te3, temporal cortex, area 3; VPM, ventral posteromedial thalamic nucleus.

Data collected at 4.5 and 5 d were characterized by an increase in the number of labeled interneurons in trigeminal, vestibular,auditory, and oculomotor-related structures as well as in thereticular formation plus labeling at some additional sites, forexample some neurons within the lateral vestibular nucleus. Evenat these time points the specificity of transfer was illustratedby the lack of invasion of brainstem sites that clearly are unrelatedto eyelid motoneurons, such as other brainstem motor nuclei (hypoglossus,abducens, ambiguous, etc.).

A noticeable increase in the number of labeled structures occurred at diencephalic levels. In the hypothalamus the labelingappeared in the anterior hypothalamus and the dorsomedial hypothalamicnuclei, besides the lateral hypothalamic area, already labeledat 4 d. The ventral posteromedial and the posterior thalamic nucleishowed some labeling bilaterally, presumably via their connectionsto the labeled cortical areas. Labeling in the cerebral cortexbecame more extensive. As illustrated in Figure 8, B and C, thenumber of labeled cells in the parietal cortex showed a greatincrease (>300%) compared with that obtained at 4 d (Fig. 8B),and the labeling of individual pyramidal neurons in layer V becameGolgi-like (Fig. 8C, compare with B). Both parietal areas Pa1and Pa2 (Paxinos and Watson, 1986) were heavily labeled bilaterally,still with a contralateral dominance. Labeling also occurred consistentlyin some portions of temporal (Te1 and Te3) and Oc2L cortices contralaterallyand in frontal (F1 and F2 areas) and perirhinal cortices bilaterally,whereas no labeling was found in entorhinal cortex orhippocampus.

In the cerebellum (Fig. 6B,C) the labeling appeared in vermal and paravermal (c₁-c₃ areas) Purkinje cells (for references,see Gruart et al., 1997). The labeled Purkinje cells showed aclear zonal organization, being arranged in narrow rostrocaudalbands (Fig. 6B,C).

Identification of oculomotor internuclear neurons projecting to orbicularis oculi motoneurons

Some rabies-immunolabeled neurons were found in the oculomotor nucleus, mainly ipsilaterally, in all cases from 3.5 d onward(monosynaptic time point). Their number and distribution did notincrease substantially with time. To clarify whether they wereinterneurons or motoneurons, we treated sections through the oculomotornuclei with a dual-color immunofluorescence protocol for simultaneousvisualization of rabies and choline acetyltransferase. Sectionsthrough the facial nucleus, containing rabies-immunolabeled orbicularisoculi motoneurons, were reacted together as positive controls.Choline acetyltransferase is an excellent motoneuron marker, andwe have shown previously that rabies-infected motoneurons areable to express choline acetyltransferase antigen at normal levels(Tang et al., 1999; Graf et al., 2002). The results showed unequivocallythat rabies-immunolabeled neurons in the oculomotor nucleus areinterneurons (and not motoneurons), because they are not cholinergic(Fig. 10). The possibility of false negative results for colocalizationof rabies and choline acetyltransferase antigen in motoneuronsclearly can be ruled out in view of the positive expression ofthe choline acetyltransferase antigen in rabies-infected orbicularisoculi motoneurons in the same experiments.

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Figure 10. Dual-color immunofluorescence for choline acetyltransferase (a motoneuron marker; A, C) and rabies virus (B, D) in the oculomotor nucleus at 4 d after the injection of rabies virus into the right orbicularis oculi muscle. A, C, Motoneurons in the oculomotor nucleus, identified by their expression of choline acetyltransferase (Cy3; red). B, D, Rabies-immunolabeled neurons (FITC; green) in the ipsilateral oculomotor nucleus in the same sections. They are identified here as interneurons and not motoneurons, because they are not positive for choline acetyltransferase (arrows in C point to the empty spaces corresponding to the rabies-immunolabeled neurons shown in D). Scale bars: A, B, 500 µm; C, D, 100 µm.

Specificity of rubral projection to orbicularis oculi motoneurons

Until now, it was unknown whether the rubral projections to the facial nucleus are mediated by separate rubral populationor are axon collaterals of rubrospinal-projecting neurons (Mizunoand Nakamura, 1971). To clarify this issue, retrograde transneuronallabeling with rabies virus of the rubral neurons innervating orbicularisoculi motoneurons was combined in the same experiments with conventional(single-step) retrograde labeling of rubrospinal neurons by usingFluoro-Ruby. As expected, the injections of Fluoro-Ruby into therubrospinal tract at upper cervical levels resulted in comprehensivelabeling of rubrospinal neurons, as shown by their widespreaddistribution in all spinal-projecting portions of the red nucleus,including its lateral horn (Fig. 11A,C) (Huisman et al., 1981;Strominger et al., 1987; Ugolini, 1992; Tang et al., 1999). Incontrast, the transneuronally labeled rubrofacial neurons occupiedexclusively the dorsolateral quadrant of the red nucleus and thedorsally adjoining pararubral area (Fig. 11B,D). Our results (Fig.11) show that rubrofacial neurons innervating orbicularis oculimotoneurons monosynaptically and disynaptically are clearly aseparate population from the rubrospinal-projecting ones. Despitethe topographical overlap between the two populations in the dorsolateralquadrant, we found only a very small percentage (2%) of double-labeledneurons projecting with axon collaterals to both targets (Fig.11C,D, arrows). This has negligible functional significance, ifany, considering also that the projections from the red nucleusto functionally different targets generally are more collateralizedin the rat than in other mammals (cat and monkey) (Huisman etal., 1981, 1982).

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Figure 11. Rubrospinal neurons, labeled retrogradely after injections of Fluoro-Ruby into the right rubrospinal tract in the upper cervical spinal segments (A, C), and orbicularis oculi-related rubrobulbar neurons in the same section, labeled by retrograde transneuronal transfer of rabies virus from the right orbicularis oculi muscle (B, D). The photomicrographs illustrate the contralateral (left) magnocellular red nucleus at 5 d. A, Rubrospinal neurons (Fluoro-Ruby; red). Note their widespread distribution in all spinal-projecting portions of the red nucleus, including its lateral horn (left). B, Orbicularis oculi-related rubrofacial neurons (rabies immunolabeling, FITC; green). Note their exclusive location in the dorsolateral quadrant of the red nucleus. Note well that the orange spots are tissue autofluorescence, inevitably shining through the fluorescence filters. C, D, High-power view of the dorsolateral quadrant of the red nucleus from A and B. Despite their extensive overlap, rubrospinal and rubrofacial neurons are two separate populations. Arrows in C and D point to rare examples of double-labeled neurons (projecting with axon collaterals to orbicularis oculi motoneurons and to the spinal cord). Scale bars: A, B, 500 µm; C, D, 100 µm.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

General remarks

Neuronal networks involved in the generation and control of spontaneous, reflex, and learned eyelid responses were revealedhere by transneuronal transfer of rabies virus from the orbicularisoculi muscle. Because of its highly specific propagation by retrogradetransneuronal transfer across an unlimited number of synapses(Ugolini, 1995b; Tang et al., 1999; Kelly and Strick, 2000; Grafet al., 2002), the rabies virus tracer represents a formidablestep forward compared with previous attempts to map such networkswith conventional tracers (Takeuchi et al., 1979; Hinrichsen andWatson, 1983; Holstege et al., 1984, 1986a,b; Takada et al., 1984;Fort et al., 1989; Travers, 1995), which could help to locateputative sources of monosynaptic input to orbicularis oculi motoneurons,but not higher order relays. Virus uptake involved exclusivelyorbicularis oculi motoneurons in the dorsolateral facial nucleusdivision (Martin and Lodge, 1977; Faulkner et al., 1997). Infectedmotoneurons remained viable and did not become more numerous ormore widely distributed with time, showing that rabies virus didnot diffuse either within the muscle or within the facial nucleus.Transneuronal transfer was time-dependent. The observation thatall known sources of monosynaptic input to orbicularis oculi motoneuronswere labeled at 3.5 d confirms that the efficacy of transfer ofrabies virus is not dependent on transmitter types (Ugolini, 1995b;Graf et al., 2002). However, second-order neurons that synapseproximally on the motoneurons soma-dendritic tree may be visualizedearlier than neurons establishing more distal or weaker synapticcontacts (Ugolini, 1995b; Graf et al., 2002).

The results highlight the reflex pathways by which sensory inputs of trigeminal, auditory, vestibular, and visual originscan evoke eyelid responses and the participation of reticular,rubral, cerebellar, and cortical neurons to eyelid control. Potentialsites of interactions between networks controlling eye and eyelidmovements also are revealed here. Based on our results and aspointed out previously (Holstege et al., 1986a,b; Bracha and Bloedel,1996), multiple pathways (with coinciding nodal points for differentsensory modalities) are available in the eyelid premotor systemas putative memory storage sites for classical conditioning ofeyelid responses, a widely used model for associative motor learning(Gormezano et al., 1983; Woody, 1986; Thompson and Krupa, 1994).

Sensory modalities to orbicularis oculi motoneurons

Projections to orbicularis oculi motoneurons from the ipsilateral trigeminal nuclei (Erzurumlu and Killackey, 1979; Holstegeet al., 1986a, 1988; Pellegrini et al., 1995; Van Ham and Yeo,1996) mediate the R1 component of the blink reflex (Hiraoka andShimamura, 1977). Such projections, visualized here at 3-3.5 d,were not substantial. Extensive neuronal labeling in the ipsilateralprincipal and spinal trigeminal nuclei and upper cervical dorsalhorn appeared later (4 d), compatible with additional synapticsteps. The labeled sites receive trigeminal afferents of cornealand periocular origin (Panneton and Burton, 1981; Pellegrini etal., 1995). Polysynaptic trigeminal afferents to orbicularis oculimotoneurons mediate the R2 blink reflex component via reticularformation and dorsal horn synaptic relays (Hiraoka and Shimamura,1977; Pellegrini et al., 1995).

Auditory pathways were already labeled heavily at monosynaptic time points, an unexpected result according to the paucityof tone-evoked reflex blinks in rabbits and cats (Gruart et al.,1995, 2000a). A likely explanation is that the rat presents anoticeable startle response. Our results indicate that the underlyingconnections are derived from the nucleus of the trapezoid body;the caudal, ventral, and rostral periolivary nuclei and neighboringportions of the nucleus reticularis pontis caudalis and oralis(López et al., 1999; Sinex et al., 2001); and the caudal partof the ventral cochlear nuclei bilaterally, mainly ipsilaterally.Higher order neurons are located in the dorsal cochlear nucleus,lateral lemniscus nuclei, and inferiorcolliculus.

Monosynaptic and disynaptic excitatory and inhibitory potentials have been evoked in facial motoneurons by stimulation ofthe medial and superior vestibular nuclei (Shaw and Baker, 1983).Our results reveal a few monosynaptic and numerous polysynapticvestibular afferents (from the medial, superior, and descendingvestibular nuclei) to orbicularis oculi motoneurons. Such pathwaysmay be involved in eye-eyelid coordination, for example to preventblinking during vestibulo-ocular reflexperformance.

Visual information involved in light-evoked blinks reaches orbicularis oculi motoneurons via the olivary pretectal nucleusand related mesencephalic structures (Itoh et al., 1983), as confirmedhere. Although both orbicularis oculi and accessory abducens motoneuronsreceive such visual input in the cat (Holstege et al., 1986a,b),only orbicularis oculi motoneurons are able to fire to flashlightpresentation in alert behaving animals. Visual afferents to accessoryabducens motoneurons are an example of "silent" pathways (Delgado-Garcíaet al., 1988; Delgado-García, 1998).

Reticular formation and limbic brainstem afferents

Our results show that specific areas of the medullary, pontine, and mesencephalic reticular formations project onto orbicularisoculi motoneurons. Particularly, ipsilateral projections havesubstantial monosynaptic (and polysynaptic) components. From ourresults, these reticular areas are connected more heavily withorbicularis oculi motoneurons than are the trigeminal nuclei.Reticular neurons in such areas that project to the orbicularisoculi division are activated by ipsilateral supraorbital nervestimulation (Inagaki et al., 1989). Bilateral reticular projectionsto orbicularis oculi motoneurons explain the bilateral blinks(R2 component; Kugelberg, 1952) evoked by unilateral electricalstimulation of the supraorbital nerve (Pellegrini et al., 1995).They also may explain why eyelid classically conditioned responsespresent a (weaker) component contralateral to the side of theunconditioned stimulus presentation (Gruart et al., 1995).

The different reticular nuclei probably are involved in the generation and/or integration of commands of different origin(motor cortex, basal ganglia, limbic system). Based on in vitroeffects of acetylcholine on facial motoneurons (Magariños-Asconeet al., 1999), it may be proposed, for instance, that cholinergicneurons in the dorsal medullary reticular formation, near thehypoglossal nucleus, are involved in the generation of orbicularisoculi motoneuron tonic firing, which is characteristic of R2 responses,eyelid-friendly displays, and classically conditioned responses(Holstege et al., 1986a,b; Fort et al., 1989; Travers, 1995; Trigoet al., 1999).

Some of the identified pathways, such as those derived from the parabrachial and Kölliker-Fuse nuclei, may be involved inthe genesis of premotor signals related to the expression of internalemotional states, because limbic structures project to these nucleithrough the central amygdala and hypothalamus. Such pathways arenot affected by lesions of the pyramidal fibers, explaining thepossibility of emotional expression in the absence of voluntaryeyelid responses (Holstege et al., 1986a,b).

Eye muscles-eyelid premotor relationships

As shown here, structures belonging to eye movement networks (oculomotor internuclear neurons, supraoculomotor area, interstitialnucleus of Cajal, nucleus of Darkschewitsch, superior colliculus)also innervate monosynaptically or polysynaptically the orbicularisoculi motoneurons. This common network is likely to be involvedin coordination of eyelid and eye movements during blink (Bouret al., 2000), intentional saccades, and fast phases of the vestibulo-ocularand optokinetic reflexes, mostly for eye movements in the verticalplane. No labeling occurred in the prepositus hypoglossi nucleus,which is involved in horizontal eye movements. Projections tofacial motoneurons from these structures were reported in tracingstudies (Takeuchi et al., 1979; Hinrichsen and Watson, 1983; Takadaet al., 1984; Holstege et al., 1986a; Isokawa-Akesson and Komisaruk,1987; Fort et al., 1989) and electrophysiological experiments(Fanardjian and Manvelyan, 1987b; Vidal et al., 1988; May et al.,1990).

Red nucleus and cerebellum

Our results indicate that eyelid-related rubrofacial neurons are clustered in the dorsolateral quadrant of the contralateralred nucleus and pararubral area. As shown here, eyelid-relatedrubrofacial pathways are clearly independent (i.e., not a collateralbranch) of the rubrospinal tract. This was unknown previously(Courville, 1966; Mizuno and Nakamura, 1971; Yu et al., 1972).

Monosynaptic and polysynaptic projections to orbicularis oculi motoneurons also are derived from the lateral part of the anteriorand posterior interpositus nuclei, mainly ipsilaterally. Notably,interpositus neurons at these locations project to the red nucleusand to the labeled oculomotor-related nuclei (interstitial nucleusof Cajal, nucleus of Darkschewitsch, oculomotor interneurons,superior colliculus) (Fanardjian and Manvelyan, 1984; Gonzalo-Ruizand Leichnetz, 1987). This double-projecting system probably isinvolved in regulating and/or reinforcing eyelid responses byexciting the rubrofacial pathway and disfacilitating the (antagonist)eyelid levator palpebrae muscle (Gruart et al., 2000b). Moreover,the interpositus nuclei project to the medullary reticular formationand other labeled brainstem structures (Mehler, 1983; Rubertoneet al., 1990; Voogd, 1995). Evidence of polysynaptic connectionsto orbicularis oculi motoneurons from the medial and lateral cerebellarnuclei also was obtained. Labeling of cerebellar nuclei is inkeeping with the involvement of motor cortex, red nucleus, andreticular formation in eyelid motor control. At later time pointsconsistent with additional steps of transfer, labeling appeared,with a zonal distribution, in vermal and paravermal (c₁-c₃ zones)Purkinje cells. Notably, the c₁-c₃ zones have been related totrigeminally evoked eyelid blinks (Gruart et al., 1997).

Higher order forebrain structures

Cerebral cortical areas and hypothalamic and thalamic nuclei were labeled starting from 4 d, consistent with polysynapticconnections with orbicularis oculi motoneurons. Correspondingly,cortical afferents to facial motoneurons in the cat are not monosynapticbut reach them through the trigeminal nuclei and/or the nearbyreticular formation (Fanardjian and Manvelyan, 1987a). Labelingwas restricted to corticofugal pyramidal cells in layer V. Parietalcortex labeling was bilateral, with a contralateral dominance.Bilateral cortical projections to the orbicularis oculi divisionof the facial nucleus exist in other mammals, including humans(Morecraft et al., 2001). In a study of the early gene c-fos expressionduring classical conditioning of eyelid responses, wide areasof parietal cortex were labeled (Gruart et al., 2000c). However,labeling was restricted to nonpyramidal cells located mainly inlayers 2 and 3. Apparently, layer V pyramidal cells, which asshown here represent the highest level of eyelid motor control,are not involved in this plasticresponse.

  FOOTNOTES

Received Feb. 26, 2002; revised July 8, 2002; accepted July 22, 2002.

This work was supported by European Union Grant BIO4-CT98-0546. We are grateful to Dr. A. Gruart for her comments and suggestionsand to R. Churchill for help in the editing of this manuscript.S.M. was a visiting doctoral fellow at G.U.'s laboratory (fellowshipsupported by the Spanish Ministerio de Educación y Ciencia programFP-96).

Correspondence should be addressed to Dr. Gabriella Ugolini, Laboratoire de Virologie Moléculaire et Structurale, Institutde Neurobiologie Alfred Fessard, Bâtiment 32, Centre Nationalde la Recherche Scientifique, 91198 Gif-sur-Yvette, France. E-mail:gabriella.ugolini{at}gv.cnrs-gif.fr.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Aou S, Woody CD, Birt D (1992) Changes in the activity of units of the cat motor cortex with rapid conditioning and extinction of a compound eye blink movement. J Neurosci 12:549-559[Abstract].
Berger TW, Rinaldi P, Weisz DJ, Thompson RF (1983) Single-unit analysis of different hippocampal cell types during classical conditioning of rabbit nictitating membrane response. J Neurophysiol 50:1197-1219[Abstract/Free Full Text].
Berthier NE, Moore JW (1986) Cerebellar Purkinje cell activity related to the classically conditioned nictitating membrane response. Exp Brain Res 63:341-350[Web of Science][Medline].
Berthier NE, Moore JW (1990) Activity of deep cerebellar nuclear cells during classical conditioning of nictitating membrane extension in rabbits. Exp Brain Res 83:44-54[Web of Science][Medline].
Bour LJ, Aramideh M, De Visser BW (2000) Neurophysiological aspects of eye and eyelid movements during blinking in humans. J Neurophysiol 83:166-176[Abstract/Free Full Text].
Bracha V, Bloedel JR (1996) The multiple-pathway model of circuits subserving the classical conditioning of withdrawal reflexes. In: The acquisition of motor behavior in vertebrates (Bloedel JR, Ebner TJ, Wise SP, eds), pp 175-204. Cambridge, MA: MIT.
Courville J (1966) Rubrobulbar fibres to the facial nucleus and the lateral reticular nucleus (nucleus of the lateral funiculus). An experimental study in the cat with silver impregnation methods. Brain Res 1:317-337[Medline].
Delgado-García JM (1998) Output-to-input approach to neural plasticity in vestibular pathways. Otolaryngol Head Neck Surg 119:221-230[Web of Science][Medline].
Delgado-García JM, del Pozo F, Spencer RF, Baker R (1988) Behavior of neurons in the abducens nucleus of the alert cat. III. Axotomized motoneurons. Neuroscience 24:143-160[Web of Science][Medline].
Domingo JA, Gruart A, Delgado-García JM (1997) Quantal organization of reflex and conditioned eyelid responses. J Neurophysiol 78:2518-2530[Abstract/Free Full Text].
Erzurumlu RS, Killackey HP (1979) Efferent connections of the brainstem trigeminal complex with the facial nucleus of the rat. J Comp Neurol 188:75-86[Web of Science][Medline].
Evinger C, Manning KA, Sibony PA (1991) Eyelid movements. Mechanisms and normal data. Invest Ophthalmol Vis Sci 32:387-400[Abstract/Free Full Text].
Fanardjian VV, Manvelyan LR (1984) Peculiarities of cerebellar excitation of facial nucleus motoneurons. Neurosci Lett 49:265-270[Web of Science][Medline].
Fanardjian VV, Manvelyan LR (1987a) Mechanisms regulating the activity of facial nucleus motoneurons. III. Synaptic influences from the cerebral cortex and subcortical structures. Neuroscience 20:835-843[Web of Science][Medline].
Fanardjian VV, Manvelyan LR (1987b) Mechanisms regulating the activity of facial nucleus motoneurons. IV. Influences from the brainstem structures. Neuroscience 20:845-853[Web of Science][Medline].
Faulkner B, Brown TH, Evinger C (1997) Identification and characterization of rat orbicularis oculi motoneurons using confocal laser scanning microscopy. Exp Brain Res 116:10-19[Medline].
Fort P, Sakai K, Luppi P-H, Salvert D, Jouvet M (1989) Monoaminergic, peptidergic, and cholinergic afferents to the cat facial nucleus as evidenced by a double immunostaining method with unconjugated cholera toxin as a retrograde tracer. J Comp Neurol 283:285-302[Medline].
Gonzalo-Ruiz A, Leichnetz GR (1987) Collateralization of cerebellar efferent projections to the paraoculomotor region, superior colliculus, and medial pontine reticular formation in the rat: a fluorescent double-labeling study. Exp Brain Res 68:365-378[Medline].
Gormezano I, Kehoe EJ, Marshall BS (1983) Twenty years of classical conditioning research with rabbits. Prog Psychobiol Physiol Psychol 10:197-275[Web of Science].
Graf W, Gerrits N, Yatim-Dhiba N, Ugolini G (2002) Mapping the oculomotor system: the power of transneuronal labeling with rabies virus. Eur J Neurosci 15:1557-1562[Web of Science][Medline].
Gruart A, Blázquez P, Delgado-García JM (1995) Kinematics of spontaneous, reflex, and conditioned eyelid movements in the alert cat. J Neurophysiol 74:226-248[Abstract/Free Full Text].
Gruart A, Pastor AM, Armengol JA, Delgado-García JM (1997) Involvement of cerebellar cortex and nuclei in the genesis and control of unconditioned and conditioned eyelid motor responses. Prog Brain Res 114:511-528[Web of Science][Medline].
Gruart A, Schreurs BG, Domínguez del Toro E, Delgado-García JM (2000a) Kinetic and frequency-domain properties of reflex and conditioned eyelid responses in the rabbit. J Neurophysiol 83:836-852[Abstract/Free Full Text].
Gruart A, Guillazo-Blanch G, Fernández-Mas R, Jiménez-Díaz L, Delgado-García JM (2000b) Cerebellar posterior interpositus nucleus as an enhancer of classically conditioned eyelid responses in alert cats. J Neurophysiol 84:2680-2690[Abstract/Free Full Text].
Gruart A, Morcuende S, Martínez S, Delgado-García JM (2000c) Involvement of cerebral cortical structures in the classical conditioning of eyelid responses in rabbits. Neuroscience 100:719-730[Web of Science][Medline].
Hinrichsen CFL, Watson CD (1983) Brain stem projections to the facial nucleus of the rat. Brain Behav Evol 22:153-163[Medline].
Hiraoka M, Shimamura M (1977) Neural mechanisms of the corneal blink reflex in cats. Brain Res 125:265-275[Web of Science][Medline].
Holstege G, Tan J, Van Ham J, Bos A (1984) Mesencephalic projections to the facial nucleus in the cat. An autoradiographical tracing study. Brain Res 311:7-22[Web of Science][Medline].
Holstege G, van Ham JJ, Tan J (1986a) Afferent projections to the orbicularis oculi motoneuronal cell group. An autoradiographical tracing study in the cat. Brain Res 374:306-320[Web of Science][Medline].
Holstege G, Tan J, van Ham JJ, Graveland GA (1986b) Anatomical observations on the afferent projections to the retractor bulbi motoneuronal cell group and other pathways possibly related to the blink reflex in the cat. Brain Res 374:321-334[Web of Science][Medline].
Holstege G, Tan J, Van Ham (1988) Anatomical observations on afferent projections of orbicularis oculi and retractor bulbi motoneuronal cell groups and other pathways possibly related to the blink reflex in the cat. In: Cellular mechanisms of conditioning and behavioral plasticity (Woody CD, Alkon DL, McGaugh JL, eds), pp 273-286. New York: Plenum.
Huisman AM, Kuypers HGJM, Verburgh CA (1981) Quantitative differences in collateralization of the descending spinal pathways from red nucleus and other brain stem cell groups in rat as demonstrated with the multiple fluorescent retrograde tracer technique. Brain Res 209:271-286[Web of Science][Medline].
Huisman AM, Kuypers HGJM, Verburgh CA (1982) Differences in collateralization of the descending pathways from red nucleus and other brain stem cell groups in cat and monkey. Prog Brain Res 57:186-217.
Inagaki M, Takeshita K, Nakao S, Shiraishi Y, Oikawa T (1989) An electrophysiologically defined trigemino-reticulo-facial pathway related to the blink reflex in the cat. Neurosci Lett 96:64-69[Medline].
Isokawa-Akesson M, Komisaruk BR (1987) Difference in projections to the lateral and medial facial nucleus: anatomically separate pathways for rhythmical vibrissae movements in rats. Brain Res 65:385-398.
Itoh K, Takada M, Yasui Y, Mizuno N (1983) A pretectofacial projection in the cat: a possible link in the visually triggered blink reflex pathways. Brain Res 275:332-335.
Keifer J (1993) In vitro eye-blink reflex model: role of excitatory amino acids and labeling of network activity with sulforhodamine. Exp Brain Res 97:239-253[Web of Science][Medline].
Kelly RM, Strick PL (2000) Rabies as a transneuronal tracer of circuits in the central nervous system. J Neurosci Methods 103:63-71[Web of Science][Medline].
Kim JJ, Thompson RF (1997) Cerebellar circuits and synaptic mechanisms involved in classical eye blink conditioning. Trends Neurosci 20:177-181[Web of Science][Medline].
Köbbert C, Apps, Bechmann I, Lanciego JL, Mey J, Thanos S (2000) Current concepts in neuroanatomical tracing. Prog Neurobiol 62:327-351[Web of Science][Medline].
Kugelberg E (1952) Facial reflexes. Brain 75:385-396[Free Full Text].
Kuypers HGJM, Huisman AM (1984) Fluorescent neuronal tracers. Adv Cell Neurobiol 5:307-340.
Kuypers HGJM, Ugolini G (1990) Viruses as transneuronal tracers. Trends Neurosci 13:71-75[Web of Science][Medline].
López DE, Saldaña E, Nodal FR, Merchán MA, Warr WB (1999) Projections of cochlear root neurons, sentinels of the rat auditory pathway. J Comp Neurol 415:160-174[Medline].
Magariños-Ascone C, Núñez A, Delgado-García JM (1999) Different discharge properties of rat facial nucleus motoneurons. Neuroscience 94:879-886[Web of Science][Medline].
Martin MR, Lodge D (1977) Morphology of the facial nucleus on the rat. Brain Res 123:1-12[Medline].
May PJ, Vidal P-P, Baker R (1990) Synaptic organization of the tectal-facial pathways in cat. II. Synaptic potentials following midbrain tegmentum stimulation. J Neurophysiol 64:381-402[Abstract/Free Full Text].
McCormick DA, Thompson RF (1984) Cerebellum: essential involvement in the classically conditioned eyelid response. Science 223:296-299[Abstract/Free Full Text].
McCormick DA, Lavond DG, Thompson RF (1982) Concomitant classical conditioning of the rabbit nictitating membrane and eyelid responses: correlations and implications. Physiol Behav 28:769-775[Medline].
Mehler WR (1983) Observations on the connectivity of the parvocellular reticular formation with respect to a vomiting center. Brain Behav Evol 23:63-80[Web of Science][Medline].
Mesulam MM (1982) Principles of horseradish peroxidase neurohistochemistry and their applications for tracing neural pathways $---$ axonal transport, enzyme histochemistry and light microscopic analysis. In: Tracing neural connections with horseradish peroxidase (Mesulam MM, ed), pp 1-153. Chichester, UK: Wiley.
Mizuno N, Nakamura Y (1971) Rubral fibers to the facial nucleus in the rabbit. Brain Res 28:545-549[Web of Science][Medline].
Morecraft RJ, Louie JL, Herrick JL, Stilwell-Morecraft KS (2001) Cortical innervation of the facial nucleus in the nonhuman primate. A new interpretation of the effects of stroke and related subtotal brain trauma on the muscles of facial expression. Brain 124:176-208[Abstract/Free Full Text].
Múnera A, Gruart A, Muñoz MD, Fernández-Mas R, Delgado-García JM (2001) Hippocampal pyramidal cells activity encodes conditioned stimulus predictive value during classical conditioning in alert cats. J Neurophysiol 86:2571-2582[Abstract/Free Full Text].
Panneton WM, Burton H (1981) Corneal and periocular representation within the trigeminal sensory complex in the cat studied with transganglionic transport of horseradish peroxidase. J Comp Neurol 199:327-344[Medline].
Paxinos G, Watson C (1986) In: The rat brain in stereotaxic coordinates. New York: Academic.
Pellegrini JJ, Horn AK, Evinger C (1995) The trigeminally evoked blink reflex. I. Neuronal circuits. Exp Brain Res 107:166-180[Web of Science][Medline].
Rubertone JA, Haroian AJ, Vincent SL, Mehler WR (1990) The rat parvocellular reticular formation. I. Afferents from the cerebellar nuclei. Neurosci Lett 119:79-82[Medline].
Ruigrok TJH, Cella F (1995) Precerebellar nuclei and red nucleus. In: The rat nervous system (Paxinos G, ed), pp 277-308. San Diego: Academic.
Shaw MD, Baker R (1983) Direct projections from vestibular nuclei to facial nucleus in cats. J Neurophysiol 50:1265-1280[Abstract/Free Full Text].
Sinex DG, López DE, Warr WB (2001) Electrophysiological responses of cochlear root neurons. Hear Res 158:28-38[Medline].
Strominger RN, McGiffen JE, Strominger NL (1987) Morphometric and experimental studies of the red nucleus in the albino rat. Anat Rec 219:420-428[Medline].
Takada M, Itoh K, Yasui Y, Mitani A, Nomura S, Mizuno N (1984) Distribution of premotor neurons for orbicularis oculi motoneurons in the cat, with particular reference to possible pathways for blink reflex. Neurosci Lett 50:251-255[Web of Science][Medline].
Takeuchi Y, Nakano K, Uemura M, Matsuda K, Matsushima R, Mizuno N (1979) Mesencephalic and pontine afferent fiber system to the facial nucleus in the cat: a study using the horseradish peroxidase and silver impregnation techniques. Exp Neurol 66:330-342[Web of Science][Medline].
Tang Y, Rampin O, Giuliano F, Ugolini G (1999) Spinal and brain circuits to motoneurons of the bulbospongiosus muscle: retrograde transneuronal tracing with rabies virus. J Comp Neurol 414:167-192[Web of Science][Medline].
Thompson RF, Krupa DJ (1994) Organization of memory traces in the mammalian brain. Annu Rev Neurosci 17:519-549[Web of Science][Medline].
Travers JB (1995) Oromotor nuclei. In: The rat nervous system (Paxinos G, ed), pp 239-255. San Diego: Academic.
Travers JB, Norgren R (1983) Afferent projections to the oral motor nuclei in the rat. J Comp Neurol 220:280-298[Web of Science][Medline].
Trigo JA, Gruart A, Delgado-García JM (1999) Discharge profiles of abducens, accessory abducens, and orbicularis oculi motoneurons during reflex and conditioned blinks in alert cats. J Neurophysiol 81:1666-1684[Abstract/Free Full Text].
Ugolini G (1992) Transneuronal transfer of herpes simplex virus type 1 (HSV 1) from mixed limb nerves to the CNS. I. Sequence of transfer from sensory, motor and sympathetic nerve fibers to the spinal cord. J Comp Neurol 326:527-548[Web of Science][Medline].
Ugolini G (1995a) Transneuronal tracing with $alpha$ -herpes viruses: a review of the methodology. In: Viral vectors: gene therapy and neuroscience applications (Keplitt M, Loewy AD, eds), pp 293-317. New York: Academic.
Ugolini G (1995b) Specificity of rabies virus as a transneuronal tracer of motor networks: transfer from hypoglossal motoneurons to connected second-order and higher order central nervous system cell groups. J Comp Neurol 356:457-480[Web of Science][Medline].
Ugolini G, Kuypers HGJM, Strick PL (1989) Transneuronal transfer of herpes virus from peripheral nerves to cortex and brainstem. Science 243:89-91[Abstract/Free Full Text].
Ugolini G, Morcuende S, Delgado-García JM (1999) Brainstem and cerebellar centres mediating neural control of orbicularis oculi motoneurons: retrograde transneuronal tracing with rabies virus. Soc Neurosci Abstr 25:1403.
Van Ham JJ, Yeo CH (1996) Trigeminal inputs to eye blink motoneurons in the rabbit. Exp Neurol 142:244-257[Web of Science][Medline].
Vidal P-P, May PJ, Baker R (1988) Synaptic organization of the tectal-facial pathways in the cat. I. Synaptic potentials following collicular stimulation. J Neurophysiol 60:769-797[Abstract/Free Full Text].
Voogd J (1995) Cerebellum. In: The rat nervous system (Paxinos G, ed), pp 309-352. San Diego: Academic.
Welsh JP (1992) Changes in the motor pattern of learned and unlearned responses following cerebellar lesions: a kinematic analysis of the nictitating membrane reflex. Neuroscience 47:1-19[Web of Science][Medline].
Woody CD (1986) Understanding the cellular basis of memory and learning. Annu Rev Psychol 37:433-493[Web of Science][Medline].
Yu H, DeFrance JF, Iwata N, Kitai ST, Tanaka T (1972) Rubral inputs to the facial motoneurons in cat. Brain Res 42:220-224[Medline].

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