Acquisition of Eyeblink Conditioning Is Critically Dependent on Normal Function in Cerebellar Cortical Lobule HVI

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The Journal of Neuroscience, August 1, 2001, 21(15):5715-5722

Acquisition of Eyeblink Conditioning Is Critically Dependent on Normal Function in Cerebellar Cortical Lobule HVI
Philip J. E. Attwell, Shbana Rahman, and Christopher H. Yeo
Department of Anatomy and Developmental Biology, University College London, London WC1E 6BT, United Kingdom

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Classical conditioning of the nictitating membrane response (NMR)/eyeblink response of rabbits is a simple form of cerebellar-dependent,associative motor learning. Reversible inactivations of the cerebellarnuclei and inferior olive have implicated the olivo-cortico-nuclearloop in the acquisition of nictitating membrane conditioning,but the role of the cerebellar cortex in acquisition has not beentested directly. Here we have used local infusions of the water-soluble,disodium salt of 6-cyano-7-nitroquinoxaline-2,3-dione reversiblyto block cerebellar cortical AMPA/kainate receptors in lobuleHVI during acquisition training. After the drug effects dissipated,there was no evidence that acquisition had taken place; the subjectsbehaved as if naive. Further training without inactivation thenallowed normal acquisition, and further inactivations during performanceof conditioned responses abolished these established responses.There was a strong correlation between the inactivation effectson acquisition and subsequent inactivation effects on performance,indicating that the same eyeblink-control cortical microzonesare engaged in learning and expressing this behavior. The corticalcomponent of the olivo-cortico-nuclear loop is essential for acquisitionof classically conditioned nictitating membrane response learning,and eyeblink control areas in HVI are critical. Our findings areconsistent with models of cerebellar learning that assign essentialplasticity to the cortex or to a distribution between levels inolivo-cortico-nuclearmodules.

Key words: classical conditioning; acquisition; nictitating membrane; cerebellar cortex; AMPA receptors; reversible inactivation

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The cerebellum is implicated in the acquisition and performance of motor skills, but whether motor memories are stored withinits circuitry has not been resolved. Classical conditioning ofthe eyeblink and nictitating membrane response (NMR) has beenuseful for investigating motor learning mechanisms. NMR conditioningis known to be cerebellar dependent because lesions of discrete,eyeblink control regions of the cerebellar cortex, cerebellarnuclei, or inferior olive all impair performance of previouslyconditioned NMRs (for review, see Kim and Thompson, 1997; Yeoand Hesslow, 1998).

To analyze acquisition and storage processes for NMR conditioning, recent studies have used reversible inactivations of neuralfunction during acquisition training. Localized infusions of theGABA_A agonist muscimol during NMR conditioning trials, with subsequenttesting after the drug effects have dissipated, revealed thatnormal activity in the cerebellar nuclei is critical for acquisition(Krupa et al., 1993; Hardiman et al., 1996; Yeo et al., 1997)and extinction (Hardiman et al., 1996; Ramnani and Yeo, 1996).Together with evidence that inactivations of cerebellar outputin the superior cerebellar peduncle do not prevent acquisition(Krupa and Thompson, 1995), these findings provide strong supportfor the suggestion that essential plasticity for NMR conditioningis within thecerebellum.

Several theories suggest that a major component of motor learning is within the cerebellar cortex (Marr, 1969; Albus, 1971;Gilbert, 1974, 1975; Ito, 1982, 1998), and we have shown thatthere is convergence of information essential for NMR conditioningin cerebellar cortical lobule HVI (Yeo et al., 1985b), which containsthe major eyeblink control regions (Hesslow, 1994a,b). However,if NMR conditioning is mainly mediated by cortical plasticity,why should inactivation of the cerebellar nuclei completely preventit? We previously suggested one possibility (Ramnani and Yeo,1996; Yeo et al., 1997). In addition to its effects on the excitatoryoutput neurons of the cerebellar nuclei, muscimol will also deeplyinhibit the inhibitory neurons that provide regulatory feedbackto the inferior olive (Andersson et al., 1988). So, nuclear muscimoltreatments would disturb the olivo-cortico-nuclear loop and couldimpair acquisition wholly, or partially, by disturbance of corticalexcitability mediated by changed climbing fiber input (Fig. 1),consistent with the finding that direct inactivation of the inferiorolive also prevents acquisition of NMR conditioning (Welsh andHarvey, 1998).

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Figure 1. Olivo-cortico-nuclear loops: lesions and inactivations. A, A model of the cerebellum as a mediator of eyeblink conditioning. CS- and US-related information converges within the cerebellar cortex and within the cerebellar nuclei through mossy fiber and climbing fiber inputs, respectively (for review, see Yeo and Hesslow, 1998). Excitatory neurons and synapses are shown in white; inhibitory neurons and synapses are shown in black. AIP, Anterior interpositus nucleus; Ba, basket cell; cf, climbing fiber; DAO, dorsal accessory olive; Go, Golgi cell; Grc, granule cell; HVI, cortical lobule HVI; NV, trigeminal nucleus; Pc, Purkinje cell; pf, parallel fibers; RN, red nucleus; St, stellate cell. B-E, Simplified views of the circuitry shown in A, with cortical interneurons, multiple mossy fiber inputs, and some brainstem circuits omitted for clarity. Each panel shows how information transmission and excitabilities within the olivo-cortico-nuclear loop may change after a different intervention. Excitability increases ( $up-arrow$ ) and decreases ( $down-arrow$ ) are indicated. B, After a cortical lesion, loss of Purkinje cell inhibition leads to increased excitabilities in the cerebellar nuclei and their efferent targets, consistent with enhanced unconditioned reflex eyeblinks (Yeo and Hardiman, 1992; Gruart and Yeo, 1995). In previously conditioned subjects, this lesion abolishes conditioned NM responses (Yeo et al., 1985a; Yeo and Hardiman, 1992) but can unmask short-latency, CS-driven eyelid responses (Perrett et al., 1993), consistent with the suggestion that conditioning induces plasticity within the cerebellar nuclei. C, Blockade of GABA_A receptors in the cerebellar nuclei (indicated by barred synapses) by local picrotoxin infusions disinhibits excitatory output neurons and the inhibitory nucleo-olivary projection. Increased inhibition in the inferior olive has effects similar to cutting or reversibly cooling climbing fiber inputs to the cortex (Colin et al., 1980; Montarolo et al., 1982) to produce a loss of complex spikes but a significant increase in Purkinje cell, simple spike frequencies. This blockade can also unmask short-latency, CS-driven eyelid responses (Garcia and Mauk, 1998). D, Muscimol infusions in the cerebellar nuclei (active at synapses marked with an asterisk) agonize GABA_A receptors and strongly depress nuclear excitabilities. Nucleo-olivary inhibition is depressed so olivary excitability will be increased. Increased climbing fiber activity increases complex spike activity with a corollary reduction in simple spike activity (Andersson and Hesslow 1987); this dual excitability change is indicated by $up-arrow$ and $down-arrow$ . Nuclear muscimol infusions prevent acquisition and extinction of NMR conditioning (Krupa et al., 1993; Hardiman et al., 1996; Ramnani and Yeo, 1996; Yeo et al., 1997). The disruption of acquisition can relate to loss of normal function at any level in the olivo-cortico-nuclear loop. E, CNQX infusions in the cerebellar cortex block ionotropic, non-NMDA receptor-mediated transmission. The main targets (shown as barred synapses) are parallel fiber inputs to Purkinje cells (and cortical interneurons; data not shown), climbing fiber inputs to Purkinje cells, and mossy fiber to granule cell synapses. The block of parallel fiber synapses would reduce simple spike activity in Purkinje cells but may not abolish spontaneous activity. Cerebellar nuclear neurons would be partially disinhibited. Cortical CNQX infusions block performance of established NM conditioned responses (Attwell et al., 1999). In the present study, CNQX infusions reveal no short-latency, CS-driven responses but they do prevent acquisition in naive subjects.

Reversible inactivation of critical cortical regions directly could test whether acquisition is dependent on normal corticalactivity. If acquisition were to be normal, cerebellar cortexcould be critically involved in neither acquisition nor informationstorage for NMR conditioning. In contrast, impairment of acquisitionwould implicate the cortex in the acquisition process and wouldalso be consistent with information storage in the cortex, eitheras a principal component of the memory (Yeo et al., 1985a,b; Yeoand Hesslow, 1998) or as part of a distribution between the cortexand nuclei (Raymond et al., 1996; Ohyama and Mauk, 2001). Here,we test for these possibilities using localized infusions of thenon-NMDA ionotropic glutamate receptor antagonist 6-cyano-7-nitroquinoxaline-2,3-dione(CNQX) reversibly to block cerebellar cortical AMPA/kainate receptorfunction during acquisitiontraining.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Surgery
Nineteen male Dutch belted Rabbits (1.8-2.5 kg) were implanted with a guide cannula directed toward the right cerebellar lobuleHVI. Subjects were anesthetized using a fentanyl-fluanisone mixture(0.1-5.0 mg/kg, i.m.) with benzodiazepam (0.5 mg/kg, i.v.). Mannitol(20% w/v, 30 ml over 30 min, i.v) was given to facilitate exposureof the cerebellum. Then, anesthesia was by fluothane (1-2%) inoxygen/nitrous oxide (2:1). A cranial opening exposed cerebellarcortex and a 26 gauge (ga), 11 mm stainless steel guide cannulawas implanted into the right HVI and fixed with acrylic cement.A 33 ga dummy cannula fitted into the guide kept the implant sealed.Postoperative analgesia (buprenorphine, 100 µg · kg¹ · d¹, i.m.) and antibiotic cover (chloramphenicol, 30 mg · kg¹ · d¹, i.m.) were given for 3 d. Subjects were kept on a 12 hr day/nightcycle with ad libitum access to food andwater.
Seven to 13 d after cannula guide implantation, a nylon monofilament suture loop was placed in the right nictitating membrane(NM) under local anesthesia (proxymetacaine hydrochloride, 0.5%w/v).

Conditioning apparatus and stimuli
Rabbits were trained using techniques similar to those first developed by Gormezano et al. (1962) and described in detailby Yeo and Hardiman (1992). Subjects were placed in a restrainingstock and movement of the NM was recorded using an isotonic transducer(Gormezano and Gibbs, 1988) linked to the membrane by the monofilamentloop.
Each subject was placed in a ventilated, sound-attenuating chamber facing a centrally mounted loudspeaker. The conditionedstimulus (CS) was a 1 kHz sine wave tone of 410 msec durationand an intensity of 87 dBA. Background noise produced by ventilationfans was 57 dBA. The unconditioned stimulus (US) was peri-orbitalelectrical stimulation. Each US was a 60 msec train of three biphasiccurrent pulses (2 mA). The interstimulus interval between theCS and US onsets on paired trials was 350 msec. The intertrialinterval was randomly selected between 25 and 35 sec. Each sessionconsisted of 50 trials, and so the mean session duration was 25min.

Nictitating membrane response recording
Output from the NM transducer was fed to a 12-bit analog-to-digital convertor (CED 1401). Baseline and within-trial NM excursionswere recorded to produce conditioned response (CR) frequency andlatencymeasures.
CR frequency. A CR was defined as an NMR within the CS-US interval with amplitude $>=$ 0.5 mm and with onset latency >35 msecfrom CS onset (Hardiman and Yeo 1992). CR frequency (% CR) wascalculated for each block of nine paired trials throughout theconditioning sessions and for each completesession.
CR onset latencies. The onset latency of every CR (defined as above) was measured as the first displacement of 0.05 mm beyondbaseline after CS onset. These latencies were measured on allCS-US paired and CS alone, unpairedtrials.

Drug infusions
When cortical infusions were given (see below), the dummy cannula was removed, and a sterile, 33 ga infusion cannula was insertedthrough the guide to project 1.7 mm below the guide tip. Eachsubject then received an infusion of CNQX (disodium salt, Tocris;3 mM, 2 µl in PBS, pH 7.4) or vehicle (PBS, 2 µl) over 2 min intothe right cerebellarcortex.

Experimental design
A previous study (Attwell et al., 1999) and pilot experiments revealed that intracortical CNQX infusions can block cerebellarfunction and performance of all previously acquired CRs for 35min. Therefore, in the present study all behavioral sessions wereset at 25 min (containing 50 trials) so that they were withinthe expected duration of the drugeffects.
Habituation phase. After placement of a suture in the nictitating membrane (see above), all subjects received a single adaptationsession. They were placed in the restraining stock within theconditioning chamber, and the NM transducer was fitted. Each subjectrested quietly in the conditioning chamber for 25 min, which isequivalent to the duration of one conditioning session, and nostimuli were presented. Subjects were randomly assigned to oneof two groups: a CNQX-treated group or a vehicle-treatedgroup.
Experimental phase 1: acquisition training with cortical infusions. Subjects received four daily sessions of acquisition trainingthat began 5 min after the completion of either CNQX or vehicleinfusions in the right cerebellar cortex. Each session consistedof 50 trials and lasted 25 min. In 45 trials the CS and US werepaired, and in 5 trials the CS was presented alone with no US.The CS-alone was presented on every 10th trial. Effective inactivationwould produce low levels of conditioned responses in the CNQX-treatedgroups during thisphase.
Experimental phase 2A: acquisition training with no infusions. Three days after the end of Phase 1, subjects received fourdaily sessions of acquisition training. Each session consistedof 50 trials (45 paired trials and 5 unpaired CS trials) and lasted25 min. All protocols were as in phase 1 except that no CNQX orvehicle infusions were given. If CNQX treatment had impaired acquisitionin phase 1, then the absence of CRs at the beginning of phase2A would be evidence for the impaired acquisition in phase 1.The development of conditioning in phase 2 would be evidence thatthe cannulation and drug infusions had produced no permanent damageto criticalstructures.
Experimental phase 2B: acquisition training with no infusions (continued). Three days after the end of phase 2A, all CNQX-treatedsubjects received a further four daily sessions of acquisitiontraining with all protocols as in phase 2A. If drug infusionshad completely prevented acquisition in phase 1, then CR frequenciesfor CNQX-treated subjects in phase 2B would be similar to thosefor vehicle-treated subjects in phase2A.
Experimental phase 3: performance testing for efficacy of cortical infusions. To test whether the CNQX infusions in phase1 had been in appropriate locations and sufficient to fully inactivatethe critical control regions, in phase 3 we tested their efficacyin blocking the performance of conditioned responses establishedpreviously in phases 2A and 2B. The phase 3 session began with20 trials (18 paired CS-US trials and 2 unpaired CS trials). CNQX(same dose and concentration as in phase 1) was then infused.After 2 min, the session continued with 50 trials (45 paired CS-USand 5 unpaired CS) as in the conditioning sessions of phase 1.In most cases, a further block of 50 trials was given immediatelyto establish stable asymptotic levels. In this way, the effectsof CNQX infusion were assessed for a time period equivalent to,or beyond, a full training session in phase1.

Histology
In the final stage of the experiment, infusion cannulas were reinserted, and ³H-CNQX in PBS (3 mM, containing 1 µCi/µl, 2 µl over 2 min) wasinfused. This dose corresponds to that in phases 1 and 3. ³H-CNQX was infused in all subjects, including those from the PBScontrol group, so that the equivalence of cannula position andfluid delivery could be compared in the control and experimentalsubjects. Each subject was then given heparin sodium (500 U/kg,i.v.) and an overdose of pentobarbitone sodium (90 mg/kg, i.v.)17 min after the end of the CNQX infusion. This time was chosenwith reference to previous time course data (Attwell et al., 1999),and it corresponds to a time point in the middle of a trainingsession. Each subject was perfused transcardially with 0.9% saline(1 liter) followed by 4% formaldehyde solution (2 liters). Thebrain was removed, embedded in gelatin, and cryoprotected in 20%sucrose solution, and then serial, 50 µm frozen transverse sectionswerecut.

Autoradiography and image analysis
Every sixth brain section was opposed to tritium-sensitive film (Hyperfilm, Amersham) for autoradiography together with tritiumstandards (Microscales, Amersham) for 6 weeks at 4°C. After filmdevelopment, the sections were stained with cresyl violet. Theautoradiograph of every brain section was imaged with a monochromecharge-coupled device camera and analyzed using standard densitometrytechniques (M5+, Imaging Research Inc.,); the resultant imageswere calibrated, and their densities were color coded with referenceto the tritium standards as picomoles of CNQX per milligram oftissueequivalent.
The stained sections were realigned to allow registration of the histology and autoradiography. An image of each Nissl-stainedsection was captured and processed to reveal the brain edges andgranule cell layer boundaries. Composites of the color-coded densitometryand the brain contours were thenmade.
The Nissl-stained sections were examined for signs of cannula-induced damage in critical cerebellar regions. In particular,the more ventral regions of lobule HVI and the cerebellar nucleiwere studied. Subjects with damage to these regions were excludedfrom thestudy.

Data analysis
Where CR frequency and latency data passed tests for normality and homogeneity of variance, they were analyzed using a two-way,repeated measures ANOVA followed, where appropriate, by Newman-Keulsmultiple comparisons test on the individual means. Data that failednormality or homogeneity of variance tests were analyzed usingthe Wilcoxon rank-sum test on main group effects over eachphase.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Assessment of infusion sites, infusion efficacies, and cannulation-related damage

To effectively test cerebellar cortical function in NMR conditioning, the cannulation and infusions in each subject neededto satisfy three criteria. First, the CNQX infusions needed tobe restricted to the cerebellar cortex. This criterion was testedby analysis of the ³H-CNQX autoradiography. Second, the CNQX infusions needed to havebeen effective in blocking function in the critical cerebellarcortical regions. This criterion was tested in phase 3. Only ifCNQX fully blocked expression of conditioned responses for atleast some part of the period after infusion was the subject includedin the effective HVI-CNQX group. Finally, the cannulation shouldnot have produced permanent damage sufficient to invalidate assessmentof cortical function. To enable this control, the Nissl-stainedsections were critically examined, and subjects with extensive,cannulation-related cortical damage in HVI or adjacent regionswere excluded from furtheranalysis.

The study began with 19 cannulated subjects. Ten were allocated to the CNQX group, and 9 were allocated to the PBS controlgroup. At the end of the experiment, two subjects (one from theCNQX group and one from the PBS group) were found to have substantialcannulation-related damage in the cerebellar cortex. These twosubjects were rejected from the study, and their data are notanalyzedfurther.

Of the remaining nine CNQX group subjects, six were found to show a complete suppression of CRs in phase 3. In five of these,autoradiography of ³H-CNQX binding revealed that the infusions were confined to corticallobule HVI. In one of these six, there was CNQX binding in thecortex but also in the cerebellar nuclei, so this subject wasrejected. The five effective cortically confined infusions variedslightly in their spread in the rostral-caudal dimension, butin all cases, there was clear evidence of CNQX binding in themedial aspect of rostral HVI (Fig. 2, HVI-CNQX 1-5). This locationis consistent with the region identified in our earlier analysisof cortical regions engaged in CR performance (Attwell et al.,1999). There was no evidence of any CNQX binding in the cerebellarnuclei in these five subjects, so they form the HVI-CNQX group(Fig. 2). The three remaining subjects showed incomplete impairmentsof CR frequency during phase 3 of the experiment, suggesting thatcritical regions of the cerebellar cortex had not been infused,and autoradiography confirmed that CNQX binding was distributeddifferently in these subjects. In all cases the binding was moremedial than that in the HVI-CNQX group subjects, and it includedlobules IV and V of the anterior lobe. In one case (Fig. 2, CTX-CNQX1), there was some binding in medial HVI, but it was at more caudallevels than in the HVI group, and so it appears to be mostly outsidethe previously identified critical region in HVI. Similarly, subjectCTX-2 had some CNQX binding in medial HVI, but less than, forexample, subject HVI-3 in the HVI-CNQX group. There was no evidenceof CNQX binding in the cerebellar nuclei in these subjects, whichform the CTX-CNQX subgroup.

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Figure 2. Cannula tip positions and ³H-CNQX distributions after localized infusions into cerebellar cortex. In column 1, cannula tip locations are shown for all subjects on a series of six, standard transverse sections at levels from 0.5 mm anterior to 3.0 mm posterior to skull lambda. White rings indicate locations for the vehicle-infused subjects in the HVI-control group. Colored rings indicate locations for subjects in the HVI-CNQX and CTX-CNQX groups and are identified against each of these subjects in the autoradiography column headings. The cerebellar nuclei are shown with pink boundaries. Columns 2-6 and 7-9 show a series of actual transverse sections for all CNQX-infused subjects at levels corresponding to the standards. Subjects HVI-CNQX 1-5 are ranked by CNQX effects on behavior; HVI-CNQX 1 is most affected. Lobule and granule cell boundaries are shown in white. The density of ³H-CNQX binding is color-coded. Densitometry calibration: picomoles of CNQX per milligram tissue equivalent.

Of the remaining eight PBS control group subjects, autoradiography (data not shown) revealed that in three subjects, the cannulatips and the majority of ³H-CNQX binding were in the inferior colliculus. These three subjectswere excluded from the study. All of the final residual five PBScontrols had cannula tip placements centered in HVI, and controlCNQX binding was confined mainly to this lobule. These five subjectsform the HVI-controlgroup.

Cerebellar cortical CNQX infusions impaired acquisition

Subjects in the HVI-control group acquired CRs normally, reaching a stable level of learning (at least eight CRs in the ninepaired presentations per block) in 166 ± 22.5 trials (mean ± 1SEM). Comparison of CR frequencies in the HVI-CNQX and the HVI-controlgroup revealed significant overall main group differences duringphase 1 (Wilcoxon rank-sum, W = 484.0; n₁ = 20, n₂ = 20; p < 0.05).HVI-control subjects reached 63.2 ± 18.9% CR (mean ± SEM) by session4, whereas the HVI-CNQX-treated subjects showed no responses (0%)throughout this phase (Fig. 3). The complete absence of CRs throughphase 1 in the HVI-CNQX subjects is consistent with the completeperformance block that the drug can produce (Attwell et al., 1999),but at this stage it does not reveal whether acquisition was prevented.The test for whether there was acquisition during cortical inactivationin phase 1 is performance during session 5, at the start of phase2A, when there was no inactivation. During this session, the controlgroup produced 94.6 ± 4.2% CR (mean ± 1 SEM), whereas the HVI-CNQXsubjects only achieved 0.9 ± 2.0% CR (mean ± 1 SEM), indicatinga substantial impairment of acquisition in phase 1. For the entirephase 2A, main group comparisons reveal a highly significant differencebetween HVI-CNQX and HVI-control groups (Wilcoxon rank-sum, W= 535.5; n₁ = 20, n₂ = 20; p < 0.05); therefore, the corticalinactivation had produced a highly significant impairment of acquisition.This impairment was severe, because acquisition by HVI-controlsubjects during phase 1 did not differ significantly from thatof HVI-CNQX subjects during phase 2A (RM ANOVA, F = 1.09; p >0.05). Thus, the HVI-CNQX subjects had acquired little or no CS-USassociation during the inactivation in phase 1, and they startedacquisition in phase 2A, as if naive. That they then acquiredat a rate similar to naive control animals indicates that theyrecovered fully from the inactivation and that any general impairmentsattributable to cannulation were similar in the two groups.

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Figure 3. Effects of cerebellar cortical CNQX on acquisition of NMR conditioning. Daily, mean session % CR (±SEM) for control, CTX-CNQX, and HVI-CNQX groups. Subjects in control and CTX-CNQX groups developed CRs during phase 1 and reached asymptotic CR frequencies in phase 2A. Subjects in the HVI-CNQX group showed no CRs in phase 1 and reached asymptotic CR frequencies in phase 2B.

The three subjects in the CTX-CNQX group showed clear evidence of acquisition during phase 1 and through phase 2A (Fig. 3)consistent with testing in phase 3, which revealed that theircortical infusions did not fully block CR performance. Thus subjectswith incomplete inactivation of the critical, eyeblink/NM controlregions of lobule HVI were able to acquire conditioned responsesrelativelynormally.

Acquisition impairments correlate with efficacy of cortical AMPA/kainate receptor inactivations

After the acquisition phases of the experiment, all subjects reached asymptotic performance, and then, during a training sessionin phase 3, the effects of cortical CNQX on performance of existingCRs was assessed. Within and across the HVI-CNQX and CTX-CNQXgroup subjects there were differences in the severity of performanceimpairments (as measured in phase 3) and acquisition impairments(as measured in phase 2A). Previously, we have proposed that theseverity of CR performance impairments reflects the completenessof the inactivation of the cortical eyeblink control areas (Attwellet al., 1999). Here we find that there is a strong correlationbetween the degree of performance block (as measured by the numberof 10-trial blocks with 0% CR in phase 3) and the rate of acquisition(as measured by the number of trials until responses reached 90%on paired trials within a block in phase 2A) (Spearmans rank correlationcoefficient = 0.851; p < 0.05) (Fig. 4). This finding supportsthe suggestion that the same cortical regions involved in theperformance of conditioned responses are those that actively engagein the acquisition process.

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Figure 4. Correlation of CNQX effects on acquisition and subsequent performance. Acquisition and performance measures for subjects CTX-CNQX 1-3 (each subject numbered in a square symbol) and HVI-CNQX 1-5 (each subject numbered in a circle symbol) groups. Subject identifiers correspond to those in Figure 2. y-axis: CNQX effects on acquisition (expressed as number of trials in phases 1, 2A, and 2B needed to reach a criterion of 90% CR within a 10-trial block). x-axis: CNQX effects on performance (expressed as total number of 10-trial blocks in which CR frequency was 0%, during the phase 3 performance testing session).

CNQX infusions in lobule HVI abolish CRs or extend their latencies

Recent studies have revealed short-latency, CS-driven eyelid responses in conditioned rabbits after anterior lobe lesionsor blockade of GABAergic inhibition on the cerebellar nuclei bynuclear infusions of picrotoxin (Garcia and Mauk, 1998). Here,we report the onset latencies of all CRs during the whole of phase3 performance testing (Fig. 5). The main effect of CNQX infusionsin HVI was to abolish CRs, so CR frequencies are significantlyreduced, but as the drug effects dissipated, CRs gradually returnedand their onset latencies were seen to be mildly extended in theHVI-CNQX group. Subjects in the CTX-CNQX group had infusions inanterior lobe regions adjacent to HVI, and these were largelyineffective in abolishing CRs. However, these subjects also showedextensions of CR onset latency that may relate to weak spreadof the CNQX into HVI eyeblink control areas. There is no evidence,in either group, for CNQX-related reductions of CR onset latencies.

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Figure 5. Distribution of CR onset latencies during administration of, and recovery from, cortical CNQX infusions. A, Frequency histogram (25 msec bin widths) of CR onset latencies for all subjects in the HVI-CNQX group before and after CNQX infusions. % CRs are derived from 20 preinfusion trials (all subjects) and 50 (1 subject) or 100 (4 subjects) post-infusion trials. There is an overall reduction of CR frequency but little effect on the distribution of CR onset latencies. B, Frequency histogram (25 msec bin widths) of CR onset latencies for all subjects in the HVI-CTX group before (20 trials) and after (100 trials) CNQX infusions. There is a mild extension of some CR onset latencies to between 250 and 350 msec and no evidence of CR onset latency reductions.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In an earlier study, we identified a region of the cerebellar cortex critical for the expression of conditioned NM/eyelidresponses. Blockade of cerebellar cortical AMPA/kainate receptorsusing CNQX infusions into a specific region of lobule HVI completelybut reversibly blocked the production of previously establishedconditioned responses (Attwell et al., 1999). Now we have shownthat in naïve subjects a similar blockade of glutamatergic transmissionin this same cortical region prevents the acquisition of conditioning.So, normal function in the cerebellar cortical lobule HVI eyeblinkcontrol regions is essential for acquisition of eyeblink/NM classicalconditioning. What are the implications of these findings forour understanding of where and how this motor learning isstored?

Because simple, delay eyeblink or NMR conditioning can be obtained in reduced, decerebrate preparations (Mauk and Thompson,1987; Hesslow, 1995), it is clear that cerebellar and brainstemcircuitry are sufficient to support its development and maintenance.Furthermore, inactivation of cerebellar output, in the superiorcerebellar peduncle, does not impair acquisition (Krupa and Thompson,1995), so we can be certain that memory storage for NMR conditioningis not further downstream, in the rubral, thalamic, or brainstemtargets of cerebellar output. Instead, essential plasticity foreyeblink/NMR conditioning must be within the cerebellum itself,or the precerebellar brainstem circuitry, or both. The early successof cerebellar nuclear inactivations, using the GABA_A agonist muscimol,in preventing acquisition (Krupa et al., 1993; Hardiman et al.,1996; Yeo et al., 1997) and extinction (Hardiman et al., 1996;Ramnani and Yeo, 1996) invited the suggestion that major plasticityfor NMR conditioning could be within the cerebellar nuclei, butit is not clear how the relatively simple circuitry and synapticorganization of the nuclei might account for all of the complexitiesof context recognition and response timing that are critical featuresof learned motor skills, even those as apparently simple as theconditionedeyeblink.

An alternative interpretation of cerebellar nuclear inactivation effects is that they destabilize the olivo-cortico-nuclearloop and thereby have more general effects on cerebellar functionby altering information processing at olivary, cortical, and nuclearlevels (Ramnani and Yeo, 1996; Yeo et al., 1997). Muscimol infusionswithin the cerebellar nuclei affect two populations of Purkinjecell target neurons. One set is excitatory to rubral and thalamictargets, and the other set is inhibitory on inferior olive neurons(Andersson et al., 1988). Disturbance of this inhibitory, nucleo-olivarypathway leads to distinct changes in olivo-cortical transmission(Andersson and Hesslow, 1987), with further consequences for corticaland nuclear excitability changes (Colin et al., 1980; Montaroloet al., 1982). So, impairments of acquisition during muscimol(Krupa et al., 1993; Hardiman et al., 1996; Yeo et al., 1997)or lidocaine (Nordholm et al., 1993) inactivations of the cerebellarnuclei do not directly confirm the locus of plasticity essentialfor conditioning. This plasticity may be at nuclear, olivary,or cortical levels or, indeed, distributed between them. Consistentwith this idea is the finding that inactivation of the inferiorolive also prevents acquisition of NMR conditioning (Welsh andHarvey, 1998) because olivary inactivation also profoundly changescortical and nuclear activities (Colin et al., 1980; Montaroloet al., 1982). Furthermore, inactivations of cerebellar output,in the superior cerebellar peduncle, that do not prevent conditioning(Krupa and Thompson, 1995) were probably sufficiently distal tospare the nucleo-olivary inhibitory fibers, which exit the mainbody of the peduncle proximally and travel ventrally to the oliveand so would not be expected to disturb olivary excitability throughthis directroute.

In the experiment reported here, inactivation of AMPA/kainate receptor-mediated transmission in the cerebellar cortex wasalso fully effective in preventing the acquisition of NMR conditioning,again consistent with the suggestion that normal function throughoutthe olivo-cortico-nuclear loop is necessary. If acquisition hadnot been affected by cortical disruption, then it would have beenclear that there is no essential plasticity for NMR conditioningwithin the cerebellar cortex; however, because acquisition wasprevented, we conclude that cortical, nuclear, and olivary plasticityare all candidate mechanisms in NMRconditioning.

Autoradiography confirmed that the region of cerebellar cortex critical for acquisition of NMR conditioning is within themedial part of rostral lobule HVI, a region that we identifiedpreviously as critical for performance of existing conditionedNM responses in lesion studies (Yeo et al., 1984, 1985a; Hardimanand Yeo, 1992; Yeo and Hardiman, 1992) and with reversible inactivations(Attwell et al., 1999). In cats and ferrets, eyeblink corticalmicrozones have been identified electrophysiologically withinthe C1 and C3 zones of lobule HVI (Hesslow, 1994a; Hesslow andIvarsson, 1994). Those locations are highly consistent with theseidentified here as essential for acquisition of NMR conditioningin rabbits. In the present experiment, we retested the CNQX effectson the performance of established CRs in phase 3, after assessingits effects on acquisition in phases 1, 2A, and 2B. We saw a strongcorrelation between the severity of acquisition and performanceimpairments produced by cortical inactivations in individual subjects,consistent with the view that this same cortical region is involvedin both the acquisition and performance of learned responses andwith the basic features of a cerebellar cortical conditioningmodel (Yeo and Hesslow, 1998). In this model, plasticity essentialfor NMR conditioning is assumed to develop at parallel fiber/Purkinjecell synapses within eyeblink control microzones. There is goodevidence to support the suggestion that mossy fiber-parallel fiberpathways signal the CS in conditioning (Hesslow et al., 1999),although evidence supporting the role of the climbing fibers supplyingUS-related information as a reinforcing input is less clear (forreview, see Yeo and Hesslow, 1998).

As in our earlier study of conditioned response performance, we have not systematically studied the possible engagement ofother cerebellar cortical regions beyond lobule HVI because inactivationswithin this region were clearly sufficient to produce major impairmentsof acquisition and performance. However, electrophysiologicalmapping has revealed additional eyeblink control regions in HVIIand paramedian lobes in cats, and one HVI eyeblink microzone mayhave an extension into lobule V (Hesslow, 1994b). We do not ruleout the possibility that these other cerebellar cortical regionsmay also contribute to the development of NMR conditioning, butwe have not explored them in any detail. It should be noted, however,that in two subjects (CTX-2 and CTX-3) there was clear bindingof CNQX in lateral parts of lobules V and IV of the anterior lobe.Neither of these subjects had significantly impaired acquisitionor performance of NMR conditioning, so our evidence suggests thatthese regions do not play an important role in NMRconditioning.

In other studies, anterior lobe lesions in previously conditioned rabbits abolished the long-latency, adaptively timed componentof the CS-elicited eyeblink response (NM responses were not studied)and replaced it with a short-latency, short-duration responsethat could not be extinguished (Perrett et al., 1993; Perrettand Mauk, 1995). In related studies, blockade of GABAergic Purkinjecell inputs to the cerebellar nuclei with nuclear infusions ofpicrotoxin produced similar short-latency CS-elicited responses,although now with a longer plateau phase extending through theCS period (Garcia and Mauk, 1998; Ohyama and Mauk, 2001). It hasbeen suggested that these studies reveal learning-related plasticitiesat the cerebellar nuclear and cerebellar cortical levels. At thenuclear level, CS-related mossy fiber collateral inputs may bepotentiated, whereas at the cortical level, the CS-US intervalis learned so as to provide an accurately timed inhibition onthe nuclei and thereby to produce a CR with appropriate topography(Medina and Mauk, 2000; Ohyama and Mauk, 2001).

Here, we see no evidence for short-latency, CS-driven NM responses after inactivation of lobule HVI or lobule IV/V. The maineffect of CNQX inactivation of lobule HVI was to abolish CRs,but as the effects dissipated, CR latencies were mildly extended(Fig. 5). However, it should be remembered that short-latencyresponses have been revealed by lesioning, or pharmacologicallyblocking, inhibition on the cerebellar nuclei. In contrast, weblocked AMPA receptor-mediated transmission within the cortexso that intrinsic properties of Purkinje cells would maintainsome inhibitory drive to the cerebellar nuclei. Our procedureswould produce less disinhibition on the cerebellar nuclei, sothe absence of short-latency, CS-driven responses does not ruleout the possibility of plasticity at the cerebellar nuclei. Thesuggestion that cortical and nuclear plasticities combine to mediateeyeblink/NMR conditioning remains an attractive one, because itexplains how the timed, inhibitory cerebellar cortical outputmight control increased excitability in the nuclei to generatea learnedmovement.

Our findings do differ sharply, however, from others described above in that the region of cerebellar cortex critical foracquisition and performance involves the eyeblink control regionsof lobule HVI and does not involve the anterior lobe. These locationsin lobule HVI are consistent with those in our earlier lesionand inactivation studies and with electrophysiological mapping(Yeo and Hesslow, 1998). Further studies will be needed to revealwhether there are memory consolidation processes within HVI andwhat aspects of this motor memory might beencoded.

  FOOTNOTES

Received March 6, 2001; revised May 9, 2001; accepted May 18, 2001.

This study was supported by Biotechnology and Biological Sciences Research Council Grant 31/S10225. We thank Magnus Ivarssonfor help with data and imageanalysis.
Correspondence should be addressed to Dr. Christopher H. Yeo, Department of Anatomy and Developmental Biology, UniversityCollege London, London WC1E 6BT, UK. E-mail: c.yeo{at}ucl.ac.uk.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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