Physiology and Plasticity of Morphologically Identified Cells in the Mormyrid Electrosensory Lobe

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Volume 17, Number 16, Issue of August 15, 1997 pp. 6409-6423
Copyright ©1997 Society for Neuroscience

Physiology and Plasticity of Morphologically Identified Cells in the Mormyrid Electrosensory Lobe

Curtis C. Bell¹, Angel Caputi², and Kirsty Grant³
¹ R. S. Dow Neurological Sciences Institute, Legacy Good Samaritan Hospital and Medical Center, Portland, Oregon 97209, ² Division de Neuroanatomia Comparada, Instituto de Investigaciones Biologicas Clemente Estable, Montevideo, 11600 Uruguay, and ³ Institut Alfred Fessard, Centre National de la Recherche Scientifique, 91190 Gif sur Yvette, France

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

The electrosensory lobe (ELL) of mormyrid electric fish is the first stage in the central processing of sensory input fromelectroreceptors. The responses of cells in ELL to electrosensoryinput are strongly affected by corollary discharge signals associatedwith the motor command that drives the electric organ discharge(EOD). This study used intracellular recording and staining todescribe the physiology of three major cell types in the mormyridELL: the medium ganglion cell, the large ganglion cell, and thelarge fusiform cell. The medium ganglion cell is a Purkinje-likeinterneuron, whereas the large ganglion and large fusiform cellsare efferent neurons that convey electrosensory information tohigher stages of the system.
Clear differences were observed among the three cell types. Medium ganglion cells showed two types of spikes, a small narrowspike and a large broad spike that were probably of axonal anddendro-somatic origin, respectively, whereas the large ganglionand large fusiform cells showed only large narrow spikes. Mostof the medium ganglion cells and all of the large ganglion cellswere inhibited by electrosensory stimuli in the center of theirreceptive fields, whereas the large fusiform cells were excitedby such stimuli.
Responses to the EOD corollary discharge were different in the three cell types, and these responses underwent plastic changesafter a few minutes of pairing with an electrosensory stimulus.Plastic changes were also observed in medium and large ganglioncells after the corollary discharge was paired with depolarizing,intracellular current pulses.
Key words: mormyrid; electric fish; electrosensory; cerebellum; plasticity; corollary discharge; efference copy

INTRODUCTION

Primary afferent input from electroreceptors, from hair cells of the mechanical lateral line system, and from hair cells ofthe eighth nerve end organs terminates within cerebellum-likestructures in fish. These structures integrate peripheral inputwith descending input from central sources. The central inputsconvey various types of information, such as corollary dischargesignals associated with motor commands, proprioceptive signalsindicating body positions, and recurrent feedback signals fromhigher central stages to which the cerebellum-like structuresproject (Montgomery et al., 1995).

The central or "descending" inputs exert various effects, including the gating of (re)afferent (von Holst and Mittelstaedt,1950) sensory input by corollary discharge signals associatedwith motor commands (Bell, 1989), and gain control by feedbackfrom higher stages of the same sensory system (Bastian, 1986).Some of the descending effects are plastic and depend on previousassociations with peripheral sensory input (Bell, 1981; Montgomeryand Bodznick, 1994; Bastian, 1995). A few minutes of associationbetween peripheral and central inputs results in the central inputeliciting a negative image of the previously paired sensory input.Thus, the central input acts as a predictor of expected sensoryinput. Addition of the negative image of predicted input to theactual input removes predictable features, allowing unpredictablefeatures to stand out more clearly.

This study focuses on the cerebellum-like electrosensory lobe (ELL) of mormyrid electric fish where the primary afferent fibersfrom electroreceptors terminate and more specifically in the regionsof ELL that receive input from mormyromast electroreceptors (Fig.1). These electroreceptors are responsible for active electrolocation,in which the fish senses external objects by their effect on thepattern of transcutaneous current flow generated by the fish'sown electric organ discharge (EOD). Afferents from mormyromastelectroreceptors project to the medial and dorsolateral zonesof ELL (see Fig. 1, MZ and DLZ) (Bell et al., 1989).
Fig. 1. Schematic diagram of a frontal section through ELL. The ELL is divided into medial (MZ), dorsolateral (DLZ), and ventrolateral(VLZ) zones. Much of ELL is covered by the eminentia granularisposterior (EGp), which contains the granule cells that give riseto the parallel fibers of ELL molecular layer.
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Corollary discharge signals associated with the motor command that elicits the EOD are prominent in the mormyrid ELL (Zipserand Bennett, 1976; Bell and Grant, 1992). Thus, the ELL is stronglyaffected at each EOD by EOD-evoked afferent input and by corollarysignals associated with the EOD motor command. Some corollarydischarge effects are fixed, but others are plastic and dependon the sensory input that has followed the EOD in the recent past(Bell, 1982; Bell and Grant, 1992).

Previous studies of the mormyromast ELL used extracellular recordings of field potentials and single cell activity to characterizethe responses to electrosensory stimuli and to the electric organcorollary discharge (Bell and Grant, 1992; Bell et al., 1992).The present study extends the previous work with intracellularrecording and staining to further characterize the cells and toidentify them morphologically. Three major cell types were examined:medium ganglion cells, large ganglion cells, and large fusiformcells (Grant et al., 1996; Meek et al., 1996). The large ganglionand large fusiform cells are glutamatergic efferent cells, whereasthe medium ganglion cells are GABAergic Purkinje-like interneuronsthat probably terminate on the efferent cells and on other mediumganglion cells (Fig. 2).
Fig. 2. Cell and fiber types of ELL discussed in the text (adapted from Meek, 1993). Primary afferent input terminates in the granularlayer (mormyromast afferent). Sensory information is then relayedto different types of interneurons, including two types of mediumganglion cells (MG₁ and MG₂) and efferent projection neurons (LGand LF). The apical dendritic trees of MG, LG, and LF neuronsextend through the molecular layer where they are contacted byparallel fibers from EGp. Small stellate cells in the molecularlayer are also contacted by the parallel fibers. Parallel fibersconvey corollary discharge signals, descending electrosensoryinformation from the preeminential nucleus (preem.), and informationfrom other sensory modalities. The preeminential nucleus alsoprojects directly to the inner molecular layer (preem. afferent).Corollary discharge input from the juxtalobar nucleus terminatesin the granular, plexiform, and ganglion layers. Output neuronsof ELL project to the mesencephalon via the lateral lemniscusand give off collaterals to the preeminential nucleus.
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MATERIALS AND METHODS
General. A total of 31 mormyrid fish of the species Gnathonemus petersii were used in these experiments. The fish ranged from12 to 15 cm in length. Surgery to expose the brain was performedunder anesthesia, and curare was given after the surgery. TheEOD motor command that would elicit an EOD in the noncurarizedfish continues to be emitted spontaneously under curare at ratesof 2-4/sec but without the normally consequent EOD. Responsesof cells in the ELL to this motor command alone are consideredcorollary discharge responses. The curare made it possible toexamine the corollary discharge responses in isolation from thenormally consequent EOD and to maintain the electrosensory inputunder experimental control.

Cells in ELL were recorded intracellularly with sharp microelectrodes containing biocytin. Responses to electrosensory stimuliwere examined by delivering brief current pulses through bipolarstimulating electrodes held close to the skin within the receptivefield of the cells. Responses to the corollary discharge signalswere examined as well as the effect of the corollary dischargeinput on electrosensory responses. The latter were tested by deliveringelectrosensory stimuli at various delays in relation to the EODmotor command. Corollary discharge plasticity was tested by deliveringelectrosensory stimuli or intracellular current pulses at fixeddelays with respect to the motor command and maintaining suchpairing for 1-5 min. Corollary discharge responses after the pairingwere compared with responses obtained before the pairing. Antidromicstimulating electrodes were placed in the lateral lemniscus atthe level of the mesencephalon in some experiments to determinewhether recorded cells were efferent cells. (Efferent axons fromELL reach the mesencephalon by way of the lateral lemniscus.)Intracellular current was passed into the cells to inject biocytinand stain them after their physiological characterization.

The specific methods used in this study are described only briefly here. More detailed information may be found in a previouspublication (Bell et al., 1992).

Surgery. Fish were anesthetized with tricaine methanesulfonate (MS-222; 1:25,000) and held against a wax block with the dorsalpart of the head out of the water. A plastic rod was cementedto the anterior part of the skull to hold the head firm. The bonewas removed from the caudal part of the skull on one side andthe underlying valvula cerebelli was reflected forward to exposethe eminentia granularis posterior (EGp). The EGp is a large massof granule cells that covers most of the lateral and dorsal surfacesof ELL (Fig. 1) and is the source of molecular layer parallelfibers. After surgery, the fish were given curare (0.1 mg, i.m.),and fresh aerated water was passed over the gills for respiration(50 ml/min).

Recording. The EOD motor command is initiated in the brainstem and is conveyed down the spinal cord to the motoneurons inthe tail that innervate the electric organ. The synchronized volleyin these motoneurons that would evoke an EOD in the noncurarizedfish was recorded with a Ag-AgCl disk placed against the skinover the electric organ in the tail (see Fig. 4A, bottom trace).This volley is known as the "command signal". The amplitude ofthe command signal was between 100 and 200 µV. The command signalwas amplified and fed to a trigger unit that generated a squarewave that was then used to trigger the oscilloscope and computer,as well as the stimulator, when electrosensory stimuli were deliveredat fixed delays after the command signal. The timing of all command-relatedevents is stated with respect to the first large negative peakof the command signal (see time 0 of the command signal, indicatedby an upward arrowhead labeled T0 in the bottom trace of Fig.4A). The EOD occurs 4.5 msec after this negative peak in the noncurarizedfish.
Fig. 4. Medium ganglion cell: intracellular recordings. A, Corollary discharge responses. Top traces, Superimposed intracellular recordingsof corollary discharge responses consisting of a compound EPSPgiving rise to a fixed latency small spike (s), followed by aburst of less strictly timed small spikes. A large broad spike(b) with an inflection on the rising phase (arrowhead) is evokedon one sweep. A medium broad spike (mb) with an amplitude correspondingto that of the inflection on the broad spike also occurs on onesweep. Raster display, Firing pattern of successive corollarydischarge responses. Each line of the raster is triggered by theelectric organ command signal. Each point in the raster showsthe occurrence of a spike. Most spikes are small narrow spikes,but some medium and large broad spikes are also included in theraster. Bottom trace, Electric organ command signal. T0, Time0, temporal reference point used in describing results. The recordedamplitude of the command signal varied between 100 and 200 µVin different fish. The exact amplitude of this signal is not indicatedin this or subsequent figures. B, Responses to depolarizing intracellularcurrent pulse. Pulse of 0.3 nA evokes small, medium, and broadspikes.
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Intracellular recordings were obtained with microelectrodes filled with potassium methyl sulfate (2 M) and biocytin (2%).Electrodes were 140-200 M $Omega$ . Biocytin was injected into recordedcells by passing depolarizing intracellular current pulses at3 Hz with a duty cycle of 50% and an amplitude of 1-2 nA for 2-15min.

Field potential recordings were made with low-resistance pipettes (2 M NaCl; 3-10 M $Omega$ ) to determine the best entry points forsubsequent penetrations with high-resistance pipettes. Field potentialrecording was also used to position the antidromic stimulatingelectrode in the lateral lemniscus. Antidromic stimulation evokesa characteristic negative wave in the cell layers of ELL (ourunpublished observations). The stimulus electrode was placed ata point where this negative wave was evoked with minimal stimulusintensity.

Stimulation. Electrosensory stimuli were delivered to local areas of the skin surface through a pair of chlorided silver balls.The silver balls were 0.5 mm in diameter, and the poles were 0.5cm apart. The axis of the dipole was held roughly perpendicularto the skin during stimulation, with the closest electrode being1-4 mm from the skin surface. Stimulus duration was 0.1 msec andintensities were 2-20 µA. The electrode closest to the skin wasnegative. Antidromic stimulation was performed with gold-platedtungsten electrodes (negative current pulses, 0.1 msec in durationand 10-50 µA in intensity).

Histology. At the end of the experiment, fish were deeply anesthetized with a concentrated solution of MS-222 (1:10,000) andperfused through the heart with saline followed by a fixativeconsisting of 4% paraformaldehyde in 0.1 M PBS. The brain wasremoved and post-fixed for 1-2 d. Vibratome sections were cutand reacted with the ABC reagents from Vector Laboratories (Burlingame,CA) and a modified Hanker-Yates procedure (Hanker et al., 1977;Bell et al., 1981). Sections were mounted on slides and counterstainedwith Richardson's stain.

RESULTS

Medium ganglion cells
Five cells of this type were identified morphologically by biocytin labeling after being studied physiologically (Fig. 3,left column). These cells have a relatively small soma in thesuperficial part of the ganglion layer, a dense apical dendriticarbor extending throughout the molecular layer, and a single primarybasilar dendrite extending from the base of the cell (for a morecomplete description of the morphology of these cells, see Meeket al., 1996). Golgi studies show two types of medium ganglioncells with basal dendrites in different layers, but these dendriteswere not sufficiently well stained in our material to distinguishbetween these two types. Axonal arbors could be observed in onlytwo of the stained cells and were restricted to the ganglion andplexiform layers in the near neighborhood of the soma. An additional23 cells with similar physiological properties were recorded butnot identified morphologically. The physiological similarity isbased on the types of spikes recorded intracellularly, the corollarydischarge responses of the cells, and the effects of electrosensorystimuli. Recorded membrane potentials of the 33 cells of thistype ranged from $-$ 70 to $-$ 50 mV (mean, $-$ 60.1 mV; SEM, 1.0 mV).
Fig. 3. Reconstructions of intracellularly recorded, biocytin-labeled neurons. Left column, Two medium ganglion cells; middle column,large ganglion cells; right column, large fusiform cells. mo,Molecular layer; ga, ganglion layer; pl, plexiform layer; gr,granular layer; *, axon. Scale bars, 50 µm.
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Two types of spikes were consistently observed in these neurons: a large broad spike, 25-60 mV in amplitude (mean, 49.8 mV;SEM, 1.7mV; n = 28) and 10-20 msec in duration (mean, 12.2 msec;SEM, 0.4 msec; n = 28) with a small after hyperpolarization; anda small, narrow spike, 1-10 mV in amplitude (mean, 5.8 mV; SEM,0.4 mV; n = 27) and 1-2 msec in duration (mean, 1.5 msec; SEM,0.1 msec; n = 28) (labeled b and s, respectively, in Fig. 4).Both types of spikes could be evoked by the corollary discharge-drivenEPSP that was characteristic of these cells (Fig. 4A; see below)or by intracellular current pulses (Fig. 4B). The small narrowspike had a lower threshold than the large broad spike, and thelarge broad spike usually occurred on top of a small narrow spike(as in Fig. 4A,B). In addition, the large broad spike usuallyhad an inflection on its rising phase (arrowheads in Fig. 4A,B)that became more pronounced when two broad spikes were evokedin quick succession by two intracellular current pulses (not shown).The inflection reflected the presence of a third type of spike,a medium broad spike, which occasionally occurred in isolationfrom the large broad spike (mb in Fig. 4A,B). A small inflectionoften occurred on the rising phase of the medium broad spike,reflecting the occurrence of a small narrow spike (Fig. 4B, doublearrowhead). The medium broad spike was 8-20 mV in amplitude and4-6 msec in duration. Rather broad spikes of 4-8 msec in durationwere commonly recorded extracellularly in the molecular layeras the electrode passed through this layer to the deeper celllayers where the intracellular recordings were made. These extracellularspikes had a timing in relation to the corollary discharge thatwas similar to that of medium ganglion cell broad spikes and couldtherefore reflect the propagation of broad spikes into the apicaldendrites of these cells. Antidromic activation by stimulationof the lateral lemniscus in the mesencephalon was tested in 5of the 28 cells of this type. No spikes were evoked, a resultthat is consistent with the identification of these cells as mediumganglion cells, i.e., interneurons.
Corollary discharge responses of medium ganglion cells The electric organ corollary discharge (or "corollary discharge") evoked a compound EPSP in these cells with an onset latencyof 10-12 msec, an amplitude of 3-8 mV, and a duration of ~40 msec(Fig. 4A). The EPSP consisted of two phases: a brief initial phasewith a highly consistent latency and amplitude followed by a longerlasting phase with a more variable amplitude. The initial phaseusually elicited a single small spike with a relatively fixedlatency, whereas the later phase elicited a brief burst of smallspikes with more variable latencies (see raster display of Fig.4A). Some of these cells showed a brief hyperpolarizing IPSP betweenthe two phases of the EPSP, and some showed a brief hyperpolarizingIPSP just before the corollary discharge EPSP (see Fig. 6, arrows).
Fig. 6. Medium ganglion cell: corollary discharge plasticity after pairing with an intracellular current pulse. Each column showsa different pairing of the corollary discharge with an intracellularlyevoked broad spike. The top row (C before) shows superimposedtraces of the corollary discharge response before pairing. Themiddle row (C + intra) shows superimposed traces during the 2min of pairing (at a lower gain). The bottom row (C after) showssuperimposed traces after the pairing. Arrows point to IPSPs thatprecede the EPSPs in some traces. Left column, Broad spike beforethe corollary discharge EPSP during pairing. Middle column, Broadspike at the time of the corollary discharge during pairing. Rightcolumn, Broad spike after the corollary discharge EPSP duringpairing. Note that the corollary discharge EPSP is enhanced duringpairings in which the broad spike is evoked before or after theEPSP during pairing but is depressed when the broad spike is evokedat the time of the EPSP during pairing. In the right column, thepairing-induced increase in the peak of the EPSP is less obviousthan the general increase in size and duration of the EPSP. Notethe hyperpolarization late in the after-pairing sweeps of theright column, presumably attributable to previous pairing withthe broad spike at this delay. The vertical calibration bar atthe right of the middle row is for the middle row only. The verticalcalibration bar at the right of the bottom row is for both thetop and bottom rows.
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Electrosensory responses of medium ganglion cells Most of these medium ganglion cells showed an IPSP in response to local electrosensory stimulation at the skin surface (Fig.5A, bottom trace). Twenty-one of the twenty-five cells that respondedto electrosensory stimulation showed only an IPSP, one cell showedan IPSP at threshold and a longer latency EPSP at higher intensities,and three cells showed only an EPSP. The IPSPs had minimal latenciesof 4-7 msec and were relatively small in amplitude (1-3 mV) whenevoked in isolation from the corollary discharge (Fig. 5A, bottomtrace) in comparison to the electrosensory IPSPs in large ganglioncells (see below). IPSPs could be evoked by near-threshold stimuliwithin small skin regions of a few square millimeters in area.Stimulation outside this inhibitory receptive field did not haveclear effects in these cells, in contrast to the opponent-surroundeffects of such stimulation that were observed in the large ganglionand large fusiform cells (see below).
Fig. 5. Medium ganglion cell: interactions between corollary discharge and electrosensory responses. A, Corollary discharge enhancementof inhibition by electrosensory stimulus. C, Postsynaptic responseto corollary discharge alone; C+ ES, response to corollary dischargeplus electrosensory stimulus given at 4 msec delay; (C+ ES) $-$ C, computed response to ES when locked to corollary discharge,calculated by subtracting the top trace from the second trace(C+ ES); ES independent, response to ES given independently ofcorollary discharge. The IPSP is quite shallow and has a latencyof ~10 msec. B, Corollary discharge plasticity after pairing withelectrosensory stimulus. Same cell as that shown in A. C before,Response to corollary discharge before pairing; C + ES, responseto corollary discharge during pairing. C after, Response to corollarydischarge after 4 min of pairing. Note the increase in EPSP size.All traces in A and B are averages of 10 responses. $bullet$ indicateselectrosensory stimulus in this and subsequent figures.
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The effect of the electrosensory IPSP was enhanced when the electrosensory stimulus was linked to the electric organ corollarydischarge by giving the stimulus at the time of the EOD, i.e.,3-5 msec after the command signal when reafferent input wouldnormally occur in the discharging fish. This enhancement of theinhibitory effect is illustrated in Figure 5A, which shows theeffect of the motor command (C), the effect of the motor commandplus an electrosensory stimulus at the time of the EOD (C+ ES),and the computed subtractive effect of the electrosensory stimulus[ES paired (C+ ES) $-$ C]. Note that the computed subtractive effectof the electrosensory stimulus when given at the time of the EODis much larger than the IPSP evoked by the same electrosensorystimulus given at a long delay of 200 msec after the command signal(ES independent). Some of the observed enhancement could be attributableto simple shunting of the excitatory current responsible for theEPSP by the electrosensory IPSP, but some of the enhancement couldalso be attributable to excitatory convergence of corollary dischargeand primary afferent inputs onto interneurons that are responsiblefor the electrosensory inhibition of medium ganglion cells. Thelatter mechanism is clearly the best explanation for the facilitationof electrosensory responses that are observed in large ganglioncells and large fusiform cells, as described below.

The predominantly inhibitory effect of electrosensory stimuli in these cells, the characteristic corollary discharge responseof a relatively fixed spike at 11-15 msec latency followed bya more variable burst lasting 20-40 msec, and the absence of spontaneousspike activity between corollary discharge-evoked bursts makeit possible to categorize these cells as I₂ cells, one of thethree I-cell classes described in a previous extracellular studyof ELL (Bell and Grant, 1992). Thus, the I₂ cells of the previousstudy appear to be medium ganglion cells, i.e., GABAergic interneuronswith axons that terminate locally on other medium ganglion cellsand on efferent neurons.
Plasticity of corollary discharge responses in medium ganglion cells The EPSP evoked by the corollary discharge alone was enhanced after pairing with an inhibitory electrosensory stimuli in fiveof the seven medium ganglion cells tested (Fig. 5B). The maximalenhancement occurred after 2-4 min of pairing, and the enhancementdecayed with a similar time course after the end of the pairing.Similar enhancement of corollary discharge responses of I₂ cellsafter pairing with an inhibitory sensory stimulus was observedin the previous extracellular study.

Corollary discharge plasticity was also observed after pairing with depolarizing intracellular current pulses, strongly suggestingthat plastic change can take place at synapses between fibersthat convey corollary discharge signals and the recorded cells,at least after pairing with depolarizing pulses. Two to four minutesof pairing the corollary discharge-evoked EPSP with a depolarizingintracellular current pulse that evoked a broad spike coincidentwith the EPSP resulted in depression of the corollary discharge-evokedEPSP (Fig. 6, middle column). This effect was observed in sevenof the nine medium ganglion cells in which it was tested. Pairingsat other delays in which the intracellular current pulse evokeda broad spike either just before the EPSP (Fig. 6, left column)or just after the EPSP (Fig. 6, right column) resulted in theEPSP becoming larger after the pairing. Such increases with pairingat delays other than coincidence were observed in four cells.Delivering the broad spike at random times with respect to thecorollary discharge did not result in any plastic change. Pairingswith hyperpolarizing current pulses, which might be expected tosimulate the pairings with inhibitory sensory stimuli, were noteffective (see Discussion). Some of the cells in this study wereincluded in a previous study of plasticity in cells with broadspikes, i.e., cells that are now known to be medium ganglion cells,in the ampullary and mormyromast regions of ELL (Bell et al.,1993). The previous study was concerned with corollary dischargeplasticity after pairing with intracellular current pulses andcontains additional information about these experiments.

Large ganglion cells
Six cells of this type were identified morphologically after being studied physiologically (Fig. 3, middle column). Theseare efferent cells with a relatively large soma in the deeperpart of the ganglion layer, a relatively small number of apicaldendrites (in comparison to medium ganglion cells) extending throughoutthe molecular layer, and several short primary basilar dendritesextending from the bottom of the soma into the plexiform layerbut no further. Unbranched axons projecting into the deep fiberlayer were observed in three of the cells (for a more completedescription of these cells, see Grant et al., 1996). An additional19 cells with similar physiological properties were studied physiologicallybut were not morphologically identified. Recorded membrane potentialsof the 25 cells of this type ranged from $-$ 72 to $-$ 55 mV (mean, $-$ 62.2 mV; SEM, 1.0 mV).

In contrast to the medium ganglion cells, these large ganglion cells showed only a single type of spike, a large narrow spikethat was 20-55 mV in amplitude (mean, 35.7; SEM, 2.2 mV; n = 25)and 1-2 msec in duration (mean, 1.3 msec; SEM, 0.1 msec; n = 25)with a pronounced after-hyperpolarization (Figs. 7D, 8B). Thesecells often showed spontaneous spike activity that was not tightlylocked to the command signal, again in contrast to the mediumganglion cells. The spikes could also be evoked antidromicallyfrom the mesencephalon in two of the six cells tested, showingthat they are efferent projection neurons.
Fig. 7. Large ganglion cells: corollary discharge and electrosensory responses. A, Cell with minimal corollary discharge response.Top trace, Response at resting membrane potential of $-$ 62 mV. Middletrace, Response with cell hyperpolarized to $-$ 69 mV. Note synapticpotential. Bottom trace, Command signal. B, Cell with pronouncedcorollary discharge response. Top trace, Response at resting membranepotential of $-$ 59 mV, showing IPSP-EPSP-IPSP sequence. Second fromtop trace, Response with cell hyperpolarized to $-$ 65 mV. Thirdfrom top trace, Response with cell hyperpolarized to $-$ 80 mV. Notethe inversion of the IPSPs. Bottom trace, Command signal. C, Corollarydischarge enhancement of inhibitory response to electrosensorystimulus. Top trace, Cell with minimal corollary discharge response.Electrosensory stimulus given at a long delay after the commanddoes not evoke a visible response. Middle trace, The same electrosensorystimulus evokes a large IPSP when given at a short delay. Bottomtrace, Command signal. D, Responses to electrosensory stimuliin center and periphery of receptive field with enhancement bycorollary discharge (superimposed traces). Left traces, Electrosensorystimulus in center of receptive field evokes an IPSP. Right traces,Electrosensory stimulus in periphery evokes an EPSP. Top row,Stimulus given independent of command. Bottom row, Stimulus givenat short delay after command. Note that both IPSPs and EPSPs areenhanced when stimulus is locked to command. E, Drawing of thehead of a fish showing location of points on the skin where electrosensorystimuli cause excitation and inhibition for a cell like that shownin D ( $-$ , inhibition; +, excitation).
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Fig. 8. Large ganglion cell: plasticity of the corollary discharge response after pairing with an electrosensory stimulus. A, Rasterdisplay showing spike responses. C before, Corollary dischargeresponse before pairing. C + ES (initial), Responses to corollarydischarge plus stimulus at start of stimulation. The verticalblack line indicates the delay and presence of the stimulus. C+ ES (late), Responses to corollary discharge plus stimulus atthe end of 2 min of pairing. C after, Corollary discharge responseafter pairing. Note the newly developed burst. B, Superimposedintracellular records from same cell and epochs as in A. Notereduction in electrosensory IPSP after pairing.
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Corollary discharge responses of large ganglion cells The corollary discharge had variable effects in cells of this type. The most common response (11/27 cells) was a complex oflow amplitude "ripples" in which the excitatory and inhibitoryeffects of the corollary discharge appeared to be almost balancedso that the response was essentially flat at the resting membranepotential (Fig. 7A,C, top traces). Injection of hyperpolarizingcurrent into these cells revealed the synaptic response to thecorollary discharge more clearly by increasing the size of EPSPsand reducing the size of IPSPs (Fig. 7A, middle trace), showingthat the flatness of the response at resting membrane potentialwas attributable to a balance of EPSPs and IPSPs. The next mostcommon corollary discharge response (8/27 cells) was an IPSP-EPSP-IPSPsequence in which the first IPSP occurred at a latency of ~7 msecafter the command and the second IPSP at a latency of ~12 msec(Fig. 7B). This sequence of synaptic potentials was sometimesfollowed by a final long-lasting EPSP (Fig. 9A). The corollarydischarge-driven IPSPs of these cells could be inverted easilyby passing hyperpolarizing current (Fig. 7B), suggesting thatthe inhibitory synaptic terminals are close to the presumed somaticrecording site. Six of the 27 cells showed only an IPSP that beganat 7 msec in some cells and at 12 msec in other cells. Finally,2 of the 27 cells showed only a low amplitude EPSP.
Fig. 9. Large ganglion cells: corollary discharge plasticity after pairing with electrosensory stimuli and intracellular current pulses.A, Plasticity after pairing with an electrosensory stimulus. Tracesshow corollary discharge responses before pairing (C before),during pairing with an electrosensory stimulus (C + ES), and afterpairing (C after). Note that the late components are stronglyaffected by the pairing but the early components are not. Intracellularrecordings are the averages of 10 sweeps. B, Plasticity afterpairing with an intracellular current pulse. A different cellfrom that shown in A. a, Pairing with intracellular current pulsewith onset at 15 msec after the command. Traces show corollarydischarge responses before pairing (C before), during pairingwith intracellular current pulse that evokes a burst of four spikes[C + intra (15 ms)], and after pairing for 3 min (C after). Notedepression of corollary discharge-evoked EPSP. b, Pairing withintracellular current pulse with onset at 40 msec after the command.Traces show corollary discharge responses before pairing (C before),during pairing with intracellular current pulse [C + intra (40ms)], and after pairing for 3 min (C after). The first trace showsthat the corollary discharge response has not fully recovered26 min after the pairing in a. Note that the effect of this secondpairing is delayed with respect to the effects of the first pairing,and that a long-lasting hyperpolarization developed in the responseto the corollary discharge that was roughly centered on the timeof the previously paired burst of spikes. c, Corollary dischargeresponse 14 min after previous pairing. The response has almostrecovered to the level observed before the second pairing in b.
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Electrosensory responses of large ganglion cells The lowest threshold response to electrosensory stimulation in all of these cells was an IPSP (Fig. 7D, left traces). All-or-noneIPSPs could sometimes be evoked by low-intensity stimulation,reflecting the excitation of a single primary afferent or interneuron.As stimulus intensity was increased, the latency of the IPSP decreased,and the amplitude and duration increased. Minimum latencies werebetween 3 and 7 msec, the amplitudes could be as large as 15 mV,and durations were generally >100 msec. The electrosensory-evokedIPSPs of these large ganglion cells were thus much more prominentthan those observed in medium ganglion cells. Near-threshold stimulationevoked pure IPSPs within skin regions of a few square millimeters.Higher-intensity stimulation sometimes evoked EPSPs after theinitial IPSPs. Such EPSPs were probably attributable to activationof receptors outside the inhibitory center of the receptive field,because pure EPSPs could be evoked by stimulating 0.5-1.5 cm eitherrostrally or caudally to the inhibitory center (Fig. 7D,E). Stimuliof the same intensity could evoke an IPSP at the center and anEPSP in the periphery. Opponent excitatory effects outside thecentral inhibitory region of the receptive field were clearlymore prominent in the large ganglion cells than in the mediumganglion cells. Much higher currents were required to invert theelectrosensory-evoked IPSPs than were required to invert the corollarydischarge-evoked IPSPs in the same neurons, suggesting that thesynapses responsible for the electrosensory IPSPs may be locatedat a greater electrotonic distance or are mediated by a differenttype of receptor.

As with the medium ganglion cells, the IPSPs of large ganglion cells were enhanced when the electrosensory stimulus was givennear the time of the EOD. The enhancement was seen in 11 of the12 cells tested. In most cases, the peak amplitude, the initialslope, and the time to peak of the IPSP all increased. For mostof the tested cells, the peak amplitude of the tested IPSP wastwo to eight times greater when the IPSP was given at the timeof the EOD. In two cells, a weak stimulus had no visible effectwhen given at a long delay but evoked a large IPSP when givenat the time of the EOD (Fig. 7C). On the other hand, when stimulusintensity was high and the IPSP was close to the maximum, stimulationat the time of the EOD did not affect the amplitude but did increasethe slope and reduce the time to peak of the IPSP (Fig. 7D, lefttraces). The EPSPs evoked by electrosensory stimuli in the peripheryof the receptive field were also facilitated by the corollarydischarge (Fig. 7D, right traces).

Enhancement such as that shown in Figure 7C cannot be explained by interaction or summation within the recorded large ganglioncell, because there is almost no effect of the corollary dischargealone (top trace). The enhancement implies the presence of aninterneuron that is responsible for the inhibition and is excitedby both the corollary discharge and the primary afferent fibers.

The strong inhibitory effect of electrosensory stimuli, the complex and rather modest effect of the corollary discharge onspikes (Fig. 8A, top), and the occurrence of spontaneous activityunrelated to the corollary discharge (Fig. 8) made it possibleto categorize these cells as I₃ cells, another one of the threecategories of I-cells identified in the previous extracellularstudy of ELL (Bell and Grant, 1992). Thus the I₃ cells of theprevious study appear to be large ganglion cells.
Plasticity of corollary discharge responses in large ganglion cells The large ganglion cells of the present study, like the I₃ cells of the previous study, showed clear corollary discharge plasticityafter pairing with electrosensory stimuli. Such plasticity wasobserved in all 15 of the 15 cells tested. An example is illustratedin Figure 8, which shows the spike responses of a cell in rasterform on the left and the intracellular recordings from the samecell on the right. The corollary discharge effect was first examinedduring an initial period without sensory input (C before). Anelectrosensory stimulus (indicated by a vertical black line) wasthen applied for 3 min just after the command signal (C + ES)and then stopped abruptly. The enhanced response to the corollarydischarge alone after turning off the stimulus can be seen inboth the raster display and the superimposed intracellular recordings(compare C after with C before). The effective reduction in electrosensoryinhibition after 3 min of pairing, attributable to the increasein corollary discharge excitation, can also be seen in the intracellularrecordings [compare C + ES (initial) with C + ES (late)]. A secondexample is shown in Figure 9A with averaged intracellular recordings.In this case, a later component of the corollary discharge response,an EPSP with an onset at ~16 msec, is greatly enhanced after 2min of pairing with an IPSP evoked by electrosensory stimulation.Note that the early components of the corollary discharge-evokedresponse are not much affected by the pairing (see Discussion).As in the previous extracellular study, the plastic changes reacheda maximum after 2-4 min of pairing with an electrosensory stimulusand took a similar amount of time to return to baseline afterthe end of pairing.

Plasticity of the corollary discharge response of these cells was also observed after pairing with depolarizing intracellularcurrent pulses that evoked a brief train of spikes, indicatingthat plastic change can take place at synapses between fibersthat convey corollary discharge signals and large ganglion cells,at least after pairing with depolarizing current pulses. The effectwas observed in six of the nine cells tested. The effect was temporallyspecific and depended on the precise timing relation between theEOD motor command and the intracellular current pulse, as wasalso observed in previous studies of ELL cells using extracellularrecording and pairing with electrosensory stimuli (Bell, 1982;Bell and Grant, 1992). This temporal specificity is illustratedby the cell shown in Figure 9B. The top set of three traces showsthe effect of pairing with an intracellular depolarizing currentpulse given at a delay of 15 msec after the command signal. Thispairing led to a marked reduction in the corollary discharge-evokedEPSP that began at ~20 msec after the command signal. The secondset of three traces shows the effect of pairing with the sameintracellular current pulse given at a delay of 40 msec afterthe command signal. This pairing led to a reduction of only thelater phases of the EPSP and the development of a long-lastinghyperpolarizing response that was roughly centered on the timeof the previously paired intracellular current pulse. In thisand other cells, the return to the pre-pairing corollary dischargeresponse after pairing with intracellular current pulses tookmuch longer than the return after pairing with electrosensorystimuli (see Discussion). Complete recovery did not seem to bepresent in this cell even at 26 min after the first pairing or14 min after the second pairing. No attempt was made to assesswhether postsynaptic spikes were required for these plastic changesor whether depolarization alone was sufficient. As with mediumganglion cells, pairing with hyperpolarizing pulses did not giveconsistent results (see Discussion).

Large fusiform cells
Five cells of this type were morphologically identified after physiological recording. These are efferent cells with a largefusiform soma at the boundary between the plexiform and granularlayer or in the superficial granular layer, apical dendrites arisingfrom one or two primary dendrites and extending throughout themolecular layer, and several primary basilar dendrites arisingfrom the bottom half of the cell and extending into the granularlayer (for a more complete description of these cells, see Maler,1973; Grant et al., 1996). Axons descending to the deep fiberlayer could be traced in two of these cells, showing that theywere efferent projection neurons. An additional 10 cells withsimilar physiological properties were recorded but not identifiedmorphologically. Recorded membrane potentials of the 15 cellsof this type ranged from $-$ 75 mV to $-$ 55 mV.

Only large narrow spikes were observed in these cells. The spikes were 40-60 mV in amplitude (mean, 42.2 mV; SEM, 3.8 mV;n = 15) and 1-2 msec in duration (mean, 1.3 msec; SEM, 0.1 msec;n = 15) and had a pronounced after-hyperpolarization (Figs. 10C,D).These spikes could be evoked antidromically from the mesencephalonin five of the eight cells tested, confirming again that theywere efferent projection neurons.
Fig. 10. Large fusiform cells: corollary discharge and electrosensory responses. A, B, Corollary discharge-evoked IPSPs. Records fromtwo different neurons. Each is shown at resting potential andat a hyperpolarized potential. Note that the IPSPs are invertedby hyperpolarization. C, Small depolarizations preceding electrosensory-evokedspike. Depolarizations indicated by arrowheads in inset (see Results).D, Responses to electrosensory stimuli in center and peripheryof receptive field and interaction with corollary discharge (superimposedtraces). Same neuron as in B. Left column, Stimuli to center ofreceptive field. Stimuli given independently of the command evokesmall, slowly rising EPSPs, with a spike occurring on one of theEPSPs (top traces). The same stimuli given 5 msec after the commandevoke short-latency, sharply rising EPSPs, with a burst of threeor four spikes on each of the EPSPs (bottom traces). Right column,Stimuli to periphery of receptive field. Stimuli given independentlyof the command evoke small IPSPs (top traces). Same stimuli given5 msec after the command evoke EPSPs and spikes. E, Drawing ofthe head of a fish showing location of points on the skin whereelectrosensory stimuli alone cause excitation and inhibition fora cell like that shown in D ( $-$ , inhibition; +, excitation).
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Corollary discharge responses of large fusiform cells The predominant effect of the corollary discharge in all of these cells was an IPSP. In most cases (10/17 cells) the IPSPhad two phases, an initial phase beginning at ~7 msec latencyand a second phase beginning at ~12 msec (Fig. 10A). In the remainingcells (7/17 cells) the IPSP had a single phase that began at ~12msec (Fig. 10B). The IPSP at 12 msec was sometimes preceded orfollowed by small EPSPs. The IPSPs could be readily inverted byintracellular injection of hyperpolarizing current (Fig. 10A,B).
Electrosensory responses of large fusiform cells The lowest threshold effect of local electrosensory stimulation in all of these cells was an EPSP. Increasing stimulus intensitylead to a decrease in latency and an increase in amplitude thatresulted in a brief burst of spikes. The decrease in latency wassimilar to that seen in primary mormyromast afferents with increasingintensity. The minimum latency of the EPSP ranged from 3 to 4msec in different cells. In seven cells the minimum latency EPSPsthat evoked spikes were preceded by one or two small deflections(Fig. 10C). The minimal latencies of the small deflections (1.5-2.5msec) were the same as those observed in a previous study foraction potentials in intracellular recordings from primary mormyromastafferents in ELL (Bell, 1990) and presumably reflect the arrivalof spikes in mormyromast afferents. The small deflections werenot field potentials, because they were not observed when theelectrode was outside the cell but still within a few micrometersof the intracellular recording site. The deflections thus suggesta small amount of direct electrical coupling between primary afferentsand large fusiform cells through electrical synapses or some othertype of ephaptic interaction. Large fusiform cells have theirbasilar dendrites in the granular layer where the primary afferentsterminate; however, the fact that the EPSPs giving rise to thespikes occurred at least 1.5 msec after the first small deflectionindicates that such direct electrical coupling is not of primaryimportance in the activation of these cells by afferent input.Such a delay is also rather long for a single synaptic delay ata chemical synapse and suggests the possibility of an interneuronbetween primary afferents and large fusiform cells, a conclusionthat is strongly supported by the facilitatory effect of the corollarydischarge on electrosensory responses (see below).

Electrosensory stimulation rostral or caudal to the central excitatory receptive field of these cells often (9/17 cells) evokeda small IPSP (Fig. 10D, top traces on right). Thus, the center-surroundorganization of receptive fields for both large fusiform and largeganglion cells was more prominent than that for the medium ganglioncells.

The excitatory effect of an electrosensory stimulus to the center of the receptive field was markedly enhanced when the stimuluswas given just after the command signal at the time of the EOD(Fig. 10D, left traces). The traces of Figure 10A were recordedfrom the same cell as that shown in Figure 10D and show that theeffect of the command alone for this cell was an IPSP. Thus thestrongly facilitatory effect of the motor command was not attributableto a simple summation of a corollary discharge EPSP and the peripherallyevoked EPSP in the recorded large fusiform cell. Instead, thestrong facilitatory effect of the command in this cell, and inother cells like it, indicates the presence of an interneuronbetween the afferent input and the large fusiform cell, an interneuronthat is excited by both primary afferent and corollary dischargeinput.

The inhibitory effect of stimulating outside the excitatory center was not enhanced by giving the stimulus just after thecommand signal at the time of the EOD in any of the cells in whichthis was tested. Instead, such coupling inverted the sign of thestimulus effect, converting it to a weak excitation (Fig. 10D,right traces). Presumably, such stimuli in the periphery of thereceptive field caused a mixture of excitation and inhibition,and the facilitatory effect of the motor command on the excitatorycomponent was larger than any facilitatory effect on the inhibitorycomponent.

The strong excitatory effect of a local electrosensory stimulus delivered to the most sensitive point on the skin surfaceindicates that the large fusiform cell is an E-cell. Similar cellswith a small corollary discharge-driven inhibition and strongexcitation within a well localized skin region were also recordedin the previous extracellular study (Bell and Grant, 1992).
Plasticity of corollary discharge responses in large fusiform cells Corollary discharge responses of large fusiform cells, like those of many E-cells in the previous study, showed clear plasticchanges after pairing with an electrosensory stimulus. The plasticitywas observed in all seven of the seven tested cells. An exampleis illustrated in Figure 11. The small corollary discharge-evokedIPSP present before pairing was greatly enhanced after 2-5 minof pairing with an excitatory electrosensory stimulus (Fig. 11).Corollary discharge plasticity after pairing with intracellularcurrent pulses was not tested in any of the large ganglion cells.
Fig. 11. Large fusiform cell: corollary discharge plasticity after pairing with an electrosensory stimulus. C before, Corollary dischargeevokes only a small IPSP before pairing. C + ES, Electrosensorystimulus evokes a burst of spikes when paired with the corollarydischarge. C after, Corollary discharge evokes a much large IPSPafter 2 min of pairing with an electrosensory stimulus.
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Additional observations
Morphological studies have shown that there are several other types of cells in ELL in addition to medium ganglion cells,large ganglion cells, and large fusiform cells (Meek et al., 1996),and other elements were recorded with physiological propertiesquite different from any of these cells. These included cellswith regular bursts in response to the corollary discharge, primaryafferent fibers from mormyromast electroreceptors, and glial cells.

Three cells were recorded intracellularly with a very regular burst of three to seven action potentials in response to thecorollary discharge (Fig. 12), with the first spike occurring ata latency of 7 to 9 msec (several milliseconds earlier than thefirst spike of the medium ganglion cells). Electrosensory stimuligiven at the time of the EOD inhibited the spikes of this burstin a graded fashion. The spikes of these cells were only a fewmillivolts in amplitude and lacked an after-hyperpolarization,suggesting that they might be axonal spikes arising at some distancefrom the presumed somatic recording site. The properties of thesecells were the same as those of the I₁ cells recorded in the previousextracellular study. None of these cells were identified morphologically.
Fig. 12. I₁-type cell: corollary discharge and electrosensory responses. A, Corollary discharge responses of I₁ cell shown with rasterdisplay of spikes and superimposed intracellular traces. B, Corollarydischarge enhancement of electrosensory IPSP in I₁ cell. Top traces,Electrosensory stimuli at a delay of 70 msec after the commandevoke small IPSPs. Bottom traces, The same stimuli at a delayof 3 msec evoke much larger IPSPs that reduces the size of thecorollary discharge EPSP.
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Recordings from mormyromast afferent fibers were also obtained. These recordings show a highly stereotyped corollary discharge-drivenEPSP with a latency of 6 to 8 msec after the command signal, asdescribed in a previous study of these afferents (Bell, 1990).The EPSP is probably attributable to synaptic input to granulecells that is observed in the afferent fiber via the electricalsynapses between afferent fibers and granule cells (Bell et al.,1989). The EPSP is not affected by prolonged pairing with an electrosensorystimulus that excites the afferent, i.e., it does not show plasticity.An example of the corollary discharge EPSP in a mormyromast afferentis shown in Figure 13 [trace marked granule cell (primary afferent)].
Fig. 13. Summary figure showing the timing of corollary responses in ELL: intracellularly recorded cells and extracellularly recordedfield potentials. E - LF, Corollary discharge responses of twolarge fusiform cells (E-cells). I₃ - LG, Corollary discharge responsesof two large ganglion cells (I₃ cells). I₂ - MG, Corollary dischargeresponses of a medium ganglion cell (I₂ cell). I₁ - ?, Corollarydischarge response of I₁ cell with unknown morphology. granulecell (primary afferent), Corollary discharge response recordedinside primary afferent that is attributable to synaptic inputto granule cells. field potentials, Corollary discharge responsesshown with extracellularly recorded field potentials in ganglion(ga) and granule (gr) layers. Arrow points to small deflectionsignaling arrival of juxtalobar input at ELL. Shaded bars showdivision of responses into shorter and longer latency events.The gains for the first five sets of traces, which are intracellularrecordings, are given by the 5 mV vertical scale bar. The gainsfor the two bottom traces, which are extracellularly recordedfield potentials, are given by the 1 mV vertical scale bar.
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Presumptive glial cells were also recorded. These cells had large stable membrane potentials of $-$ 85 to $-$ 90 mV, and no actionpotentials could be evoked by intracellularly injected currents.The voltage responses to electrosensory stimuli and to the corollarydischarge were similar but not identical to the extracellularlyrecorded field potentials just outside the cell. Initial componentsof both responses were the same, but later positive-going componentsbeginning at ~7 msec delay were two to three times larger in theintracellular recordings than in the extracellular recordings.The larger positivities probably reflect the accumulation of potassiumin the extracellular space outside the glial cells at the longerdelays. Such accumulation could be attributable to action potentialsor to the opening of potassium channels during inhibition.

Stimulation of the lateral lemniscus at the level of the mesencephalon evoked synaptic responses in some cells in additionto the previously described antidromically driven action potentials.Such responses were recorded in seven different cells and includedEPSPs, IPSPs, and EPSP-IPSP sequences. The synaptic responsesare probably not attributable to local recurrent collaterals ofefferent cells because no such collaterals have been observedanatomically (Grant et al., 1996). Axons of efferent cells dogive off extensive collaterals to the nucleus preeminentialis,however, and the cells of preeminentialis send axons to the deepmolecular layer of ELL (Bell et al., 1981), forming a feedbackloop. The synaptic potentials evoked by stimulation of the laterallemniscus are most likely attributable to antidromic activationof the axon collaterals to nucleus preeminentialis followed byactivation of preeminentialis cells that project to ELL.

DISCUSSION

General
This study has described the physiological properties of three different types of neurons of the mormyrid ELL: the mediumganglion cell, the large ganglion cell, and the large fusiformcell. These three types of neurons are the major cells with apicaldendrites that extend throughout the molecular layer and basilardendrites that extend into the deeper cell layers. As such, theyare of central importance for the integration of parallel fibersignals, with primary afferent signals to the deeper layers.

The efferent neurons, the large ganglion, and large fusiform cells are of particular interest because they convey the resultsof ELL integration to the next higher levels of the electrosensorysystem. The large ganglion cell is inhibited by electrosensorystimuli in the center of its receptive field, whereas the largefusiform cell is excited by such stimuli. Two types of efferentneurons with such opposite properties are also found in the gymnotidELL (Saunders and Bastian, 1984) and in the retina. Local decreasesin stimulus strength convey as much information as local increasesin each of these different systems, and this appears to be reflectedin separate efferent cells for the two directions of stimuluschange.

This study showed a rather remarkable difference in the intrinsic physiology of medium ganglion cells on the one hand andthe two types of efferent cells on the other. The medium ganglioncells consistently showed two types of spikes, a small narrowspike and a large broad spike, whereas the large ganglion andfusiform cells showed only a single type of large narrow spike.The same clear difference in spike types has been obtained ina recent in vitro study of the mormyrid ELL (C. Bell, V. Han,Y. Sugawara, L. Gomez Sena, and K. Grant, unpublished observations).

The cellular origins of the two types of spikes in the medium ganglion cells have not been established, but the large broadspikes probably originate from the somas or dendrites, and thesmall narrow spikes probably originate in the axon or initialsegment but do not invade the soma and are conducted only passivelyto the recording site. The intracellular recordings of this studywere most likely taken from the soma or dendrites rather thanthe axons, because the axons of medium ganglion cells are only0.5 µM in diameter (Meek et al., 1996). Thus, the relative sizesof the two types of spikes suggest that the large broad spikesoriginate electrotonically close to the soma, whereas the smallnarrow spikes originate at some electrotonic distance. The lowerthreshold of the small narrow spikes to intracellular currentinjection suggests an axonal origin for these spikes, becauseaxon spikes are known to have a lower threshold than somatic ordendritic spikes in other central cells (Stuart and Häusser,1994; Stuart and Sakmann, 1994).

Circuitry of ELL
The present results imply certain features of ELL circuitry. One such feature is the presence of interneurons between primaryafferent input and the types of neurons examined here. This isobviously true for the medium and large ganglion cells that areinhibited by electrosensory stimuli, because primary afferentfibers are excitatory (Bell, 1990) and an inhibitory interneuronis required to mediate such inhibition. The need for an interneuronbetween primary afferents and large fusiform cells, based on strongfacilitation by the corollary discharge, was unexpected. Primaryafferents terminate in the granular layer where the somas andbasilar dendrites of large fusiform cells are located, and theefferent E-cell in the gymnotid ELL appears to be directly excitedby primary afferents (Maler et al., 1981; Saunders and Bastian,1984). The conclusion regarding the lack of primary afferent synapseson large fusiform cells is supported, however, by an anatomicalstudy of the mormyrid ELL (Grant et al., 1996). Electrosensoryresponses of all three neurons were strongly enhanced by the corollarydischarge, indicating that the interneurons that mediate theseresponses must be excited by the corollary discharge, and suchexcitation has been demonstrated for granule cells on which primaryafferents terminate with electrical synapses (Bell, 1990).

Golgi studies show two different types of medium ganglion cells (Meek et al., 1996), one with basilar dendrites restrictedto the plexiform layer like the large ganglion cell and anotherwith basilar dendrites in the granular layer like the large fusiformcell (Fig. 2, MG₁ and MG₂, respectively). These comparisons suggestthat the MG₁ cells might be I-cells and the MG₂ cells might beE-cells, although our study does not confirm this. A large majorityof the MG cells in this study had a predominantly inhibitory responseto electrosensory stimulation. A few MG cells were mainly excitedby electrosensory stimuli, but it is not known whether this wasbecause such cells represent a separate class of cells or becauseof a failure to locate the inhibitory center of the receptivefields of these cells.

Corollary discharge responses
The electric organ corollary discharge has various effects on ELL cells that extend from ~5 msec to ~100 msec after the EODmotor command. The corollary discharge responses of some elementssuch as the granule cells and I₁ cells are stereotyped EPSPs,whereas the responses of other elements are a variable mixtureof excitation and inhibition. Figure 13 shows the relative timingof intracellularly recorded responses from a number of differentelements, as well as extracellular field potentials recorded inthe ganglion and granular layers (the initial ramp-like positivityin the field potentials is attributable to volume conduction fromEGp and does not reflect the excitation of ELL cells). The figureshows that many of the EPSP and IPSP onsets cluster around twotime periods, 6-8 msec and 11-13 msec after the command, as indicatedby the vertical gray bars. Juxtalobar fibers discharge with asingle spike at ~5 msec after the command, and the events withinthe first time period are probably driven by fibers from thisnucleus, either directly or within a few synaptic delays (thearrival of this input at ELL is indicated by a small negativewave indicated by an arrow in the next to last trace of Fig. 13)(Bell and von der Emde, 1995). Events beginning within the secondtime period, and later, probably represent a combination of responsesto ELL cell activity initiated during the first period togetherwith corollary discharge inputs from other sources such as EGp(Bell et al., 1992) and nucleus preeminentialis (von der Emdeand Bell, 1996).

The corollary discharge responses of most large ganglion and large fusiform cells were quite small and largely inhibitoryin the absence of previous pairing with an electrosensory stimulus,in comparison with the strong excitatory responses of interneuronssuch as the medium ganglion cell, the morphologically unidentifiedI₁ cells, or granule cells (the last cell type revealed by recordingsfrom primary afferent fibers, as described above). In severalefferent cells, the absence of a strong corollary discharge responseat the resting membrane potential was shown to be attributableto a balance between excitatory and inhibitory synaptic inputsto the cell. Thus, the strong excitatory corollary discharge responsesin the initial stages of processing are not present at the outputstage. This suggests that strong excitatory corollary dischargeresponses found at subsequent stages of the electrosensory system,such as those in the preeminential nucleus (von der Emde and Bell,1996), are not caused by input from ELL but by an independentcorollary discharge input.

Plasticity
Some corollary discharge responses are plastic and some are not. Thus the corollary discharge-driven EPSPs of granule cellsare not modified at all by long periods of pairing with an electrosensorystimulus (Bell, 1990). Similarly the I₁ type of cell shows a highlystereotyped burst that is not modified after pairing with an electrosensorystimulus that silences the burst (Bell and Grant, 1992). Evenwithin a single cell, some components of the corollary responseare modified after pairing but other components are not. For example,the initial components of the corollary discharge responses oflarge ganglion cells are only minimally affected by pairing, whereasthe later components are markedly affected (compare C before andC after in Fig. 9A). Similarly, the initial EPSP and spike ofthe corollary discharge response of medium ganglion cells areonly minimally affected by pairing, whereas the later EPSP andspike burst are greatly affected, as was also noted in the previousextracellular study of I₂ cells (Bell and Grant, 1992). Thus,the earliest components, which are probably driven most stronglyby the juxtalobar nucleus, show little plasticity in comparisonwith the later components beginning at ~14 msec.

The later more plastic responses are probably driven predominantly by parallel fiber inputs from EGp and by direct inputsto the deep molecular layer from nucleus preeminentialis. Theexact timing of parallel fiber inputs has not been determined,but the timing of corollary discharge inputs to EGp is distributedover a wide temporal window from 0 to ~80 msec after the command.Similarly, all of the corollary discharge responses of cells innucleus preeminentialis have latencies longer than 10 msec (vonder Emde and Bell, 1996). Furthermore, recent findings supportthe conclusion that responses of ELL cells to these two inputsare plastic. Plasticity at parallel fiber synapses has been demonstratedin a recent in vitro study of the mormyrid ELL (Bell et al., 1997a,b),and evidence for such plasticity has been obtained in the gymnotidELL (J. Bastian, personal communication) and the elasmobranchdorsal octavolateral nucleus (Bodznick et al., 1996). Responsesof ELL cells to input from nucleus preeminentialis has also beenshown to be plastic in gymnotid fish (Bastian, 1996).

Corollary discharge plasticity was observed in medium ganglion and large ganglion cells after pairing with electrosensorystimuli that evoked hyperpolarizations (IPSPs), but with intracellularcurrent pulses plasticity was observed only after pairing withdepolarizing current pulses and not after pairing with hyperpolarizingcurrent pulses, unless those pulses evoked a rebound postsynapticspike. Depolarizations occur naturally in these cells after stimulationof the surround region of the receptive field or when the cellis disinhibited after reduction of electrosensory input to thecenter of the field, but the lack of effect of pairing with hyperpolarizingpulses that do not evoke rebound spikes is puzzling. In othercerebellum-like structures, plasticity of responses to descendinginput appears to occur after pairing with such pulses (Bastian,1996) (D. Bodznick, personal communication). Changes in the pairingprotocol might yield positive results with hyperpolarizing currentpulses, but it is also possible that cells in the mormyrid ELLshow plasticity only when a postsynaptic spike occurs. Reciprocallyinhibitory circuitry between E- and I-cells would still allowfor the observed effects of pairing with purely inhibitory electrosensorystimuli.

Propagation of a spike into the apical dendrites of the molecular layer may be important for synaptic plasticity. Plasticityin neocortical cells (Markram et al., 1997) and some types ofplasticity in the hippocampus (Magee and Johnston, 1997) dependon the coincidence of EPSPs with apical dendritic spikes duringpairing. A similar process may occur in the ELL of mormyrid fishand in the cerebellum-like structures of other fish. Propagatedspikes have been demonstrated in the molecular layer dendritesof ELL cells in gymnotid fish (Turner et al., 1994), and evidencefor such spikes has been obtained in in vitro studies of the mormyridELL (C. Bell, V. Han, Y. Sugawara, L. Gomez Sena, and K. Grant,unpublished observations). In vitro work in the mormyrid ELL hasalso shown that plasticity of the parallel fiber-evoked EPSP isdependent on the relative timing of EPSP and the postsynapticbroad spike, suggesting that the broad spike is necessary forthe plasticity. Evidence for the importance of the broad spikein the corollary discharge plasticity of cells showing such spikeswas also obtained in a previous in vivo study (Bell et al., 1993).Propagation of a spike into the apical dendrites would providea mechanism of communication between the basilar parts of thecells where sensory inputs terminate and the apical dendriteswhere the parallel fibers terminate, allowing sensory and parallelfiber inputs to interact.

In summary, this study has determined the corollary discharge responses, the electrosensory responses, and some of the intrinsiccellular properties of three important and morphologically distinctcell types in the mormyrid ELL. Functional aspects of the circuitryhave been established as well as some of the properties of corollarydischarge plasticity in the different cell types.

FOOTNOTES

Received Dec. 12, 1996; revised May 22, 1997; accepted May 28, 1997.

This study was supported by a grant from the National Science Foundation (C.C.B.), by a Fogarty International Fellowship fromNational Institutes of Health (A.C.), and by funds from the CentreNational de la Recherche Scientifique of France (K.G.). We thankDr. Charles Russell for a critical reading of this manuscript.

Correspondence should be addressed to Curtis Bell, R. S. Dow Neurological Sciences Institute, 1120 Northwest 20th Avenue,Portland, OR 97210.

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