Abstract
Although essential for understanding the mechanisms underlying sensorimotor integration and motor control of behaviors, very little is known about the degree to which different behaviors share neural elements of the sensorimotor command chain by which they are controlled. Here, we provide, to our knowledge, the first direct physiological evidence that various modulatory premotor inputs to a vertebrate central pattern generator, the pacemaker nucleus in gymnotiform electric fish, carrying distinctly different behavioral information, can remain segregated from their various sites of origin in the diencephalon to the synaptic termination sites on different target neurons in the medullary pacemaker nucleus. During pharmacological activation of each of the premotor inputs originating from the three prepacemaker nuclei so far identified, we determinedin vivo the changes in input resistance in the neuronal elements of the pacemaker nucleus, i.e., relay cells and pacemaker cells. We found that each input yields significantly different effects on these cells; the inputs from the two diencephalic prepacemaker nuclei, PPnC and PPnG, which resulted in increased oscillator activity, caused significantly lower input resistances in relay and pacemaker cells, respectively, exhibiting drastically different time courses. The input from the sublemniscal prepacemaker nucleus, which resulted in reduced oscillator activity, however, caused a significant increase in input resistance only in relay cells. Considering that the sensory pathways processing stimuli yielding these behaviors are separated as well, this study indicates that sensorimotor control of different behaviors can occur in strictly segregated channels from the sensory input of the brain all through to the synaptic input level of the final premotor command nucleus.
- premotor control
- parallel pathways
- input resistance
- Eigenmannia
- pacemaker nucleus
- jamming avoidance response
- communication behavior
The wide range of behaviors seen in most animals often requires different activation patterns of the same motor output, i.e, the contraction of leg muscles during walking and swimming. An important question is, therefore, how much of the neural circuitry is uniquely used for the control of one particular behavior and how much of it is shared to control different motor functions. In rhythmic behaviors, switching between different motor patterns often involves changes in the modulatory input to the rhythm- producing central pattern generator (Harris-Warrick and Marder, 1991; Arshavsky et al., 1993; Katz, 1995; Marder and Calabrese, 1996). Relatively little, however, is known about whether multiple descending inputs to a single pattern-generating network act strictly independently or whether they also interact with one another (Metzner, 1993; Brodfuehrer and Burns, 1995; Heiligenberg et al., 1996; Blitz and Nusbaum, 1997).
The pacemaker nucleus of weakly electric gymnotiform fish represents such a neuronal network in which separate modulatory inputs generate distinct behavioral motor patterns by altering the discharge rate of its neuronal components (see Fig. 1) (Heiligenberg, 1991; Metzner and Viete, 1996a,b; Moortgat et al., 1998). For orientation and communication purposes, these fish produce electric signals by discharging an electric organ situated in the tail region. Each electric organ discharge (EOD) is triggered by a medullary pacemaker nucleus that is composed of two types of neurons, pacemaker and relay cells. Relay cells project to spinal motoneurons that innervate the electrocytes of the electric organ. Pacemaker cells are connected with each other and with relay cells via mixed chemical and electrical synapses (Bennett, 1971; Elekes and Szabo, 1982, 1985).
In the electric knife fish Eigenmannia, three afferent synaptic inputs to the pacemaker nucleus are known so far (see Fig. 1). All inputs and intrinsic connections are excitatory (Kennedy and Heiligenberg, 1994) and presumably use Glu as their natural transmitter. One input generates chirp-like communicatory signals. It arises from the ventrolateral portion of a diencephalic prepacemaker nucleus (PPnC) and is mediated by non-NMDA-type receptors (Kawasaki et al., 1988; Dye et al., 1989; Metzner, 1993; Juranek and Metzner, 1997). The second input is part of a pathway that generates increases in EOD frequency that occur during a particular behavior related to orientation and prey detection, the jamming avoidance response (JAR) (Bullock et al., 1972). It originates from the dorsal portion of the diencephalic nucleus electrosensorius (Keller and Heiligenberg, 1989; Keller et al., 1990), sending excitatory connections to the medial portion of the diencephalic prepacemaker (PPnG), which projects to the pacemaker nucleus possibly via both NMDA and non-NMDA-type receptors (Metzner, 1993; Spiro et al., 1994; Juranek and Metzner, 1997). The third pathway controls frequency decreases during the JAR and originates in the ventral nucleus electrosensorius (nE↓) (Keller and Heiligenberg, 1989; Keller et al., 1990). It provides GABAergic input to the mesencephalic sublemniscal prepacemaker nucleus (SPPn). The SPPn is tonically active and also controls the EOD frequency, even in the absence of jamming signals. Its projection to the pacemaker nucleus is mediated by NMDA-type receptors (Metzner, 1993; Spiro et al., 1994; Juranek and Metzner, 1997).
Here, we provide direct physiological evidence indicating that the segregation of these separate, behaviorally distinct premotor pathways extends even to the level of their synaptic targets in the pacemaker nucleus. Inputs yielding behaviors that involve increases in oscillatory firing rate, such as chirping and EOD accelerations during the JAR, affect different target cells, relay and pacemaker cells, respectively. In contrast, the inputs mediating chirping and EOD decelerations during the JAR, respectively, both affect relay cells, but yield opposite physiological effects, consistent with the involvement of different receptor subtypes.
MATERIALS AND METHODS
Nineteen Eigenmannia (12–15 cm body length) were used for this study. The animals were obtained from a tropical fish wholesaler (Bailey’s, San Diego, CA). The surgical techniques follow earlier studies (Dye et al., 1989; Kawasaki and Heiligenberg, 1989;Metzner, 1993; Juranek and Metzner, 1997). They are in accordance with National Institutes of Health guidelines for experiments involving vertebrate animals and were approved by the local Animal Care Committee. Briefly, fish were immobilized by injecting a 2% flaxedil solution (gallamine triethiodide; 2–4 μl, i.m.; Sigma, St. Louis, MO) and gently suspended in the center of an aquarium (resistivity, 9–12 kΩ cm; 26–28°C) by a pair of foam-lined forceps. Although Flaxedil strongly attenuated the EODs of Eigenmannia, residual signals (50 μV to 1 mV), locked to the spinal command cells, could still be monitored with a suction electrode fitted over the tip of the tail. Only the dorsal surface of the fish’s head was exposed above the water surface. The fish was respirated with a stream of aquarium water (3–4 drops/sec) via a glass tube inserted inside its mouth. After application of 2% lidocaine (Western Medical Supplies, Arcadia, CA), a small hole (<1 mm in diameter) was made in the occipital bone. The medullary pacemaker nucleus was then located ∼2500–3000 μm below the cerebellar surface (see below). An additional hole was made by removing parts of the parietal bone unilaterally to allow for penetration of the diencephalic prepacemaker nuclei (PPnC and PPnG) and the nE↓, ∼1500–2100 μm below the tectal surface. To stabilize the fish, a small plexiglass rod held by a micromanipulator was glued to a small area of the remaining contralateral parietal bone.
We selectively elicited the characteristic EOD frequency modulations occurring during chirping behavior and the JAR while we recorded intracellular changes of membrane potential in the two cell types of the pacemaker nucleus. By means of two separate microdrives (Burleigh Inchworm, Fishers, NY, and Narishige, Tokyo, Japan), one microelectrode was placed in the pacemaker nucleus for intracellular recordings and another electrode (tampered tip with 5–10 μm diameter) was advanced into one of the premotor nuclei, PPnC, PPnG, or nE↓, to pharmacologically activate its neurons (iontophoretic injection of 0.1ml-Glu, pH 8, ∼100 nA negative DC). InEigenmannia, it is quite difficult to localize and sufficiently inhibit the sublemniscal prepacemaker to generate a consistent drop in EOD frequency. Therefore, we used stimulation of the nE↓ (see Fig. 1) with l-Glu. The nE↓ provides GABAergic input to the SPPn, and thus its stimulation causes a decrease in EOD frequency (Keller et al., 1990; Metzner, 1993; Juranek and Metzner, 1997).
Before intracellular recordings from pacemaker and relay cells could be performed, the exact location of the unpaired pacemaker nucleus had to be determined by using a glass capillary filled with 3 mNaCl for recordings of its field potential. After localization of the pacemaker nucleus, the NaCl-filled capillary was removed, and a glass micropipette filled with 2% neurobiotin (Vector Laboratories, Burlingame, CA) in 3 m KCl (borosilicate glass pulled on a Sutter P-87; 30–50 MΩ) was advanced to the same location for intracellular recordings. Penetrations of pacemaker and relay cells were achieved by applying brief overcompensation of capacitance neutralization and/or slight mechanical tapping of the head stage of the microdrive. Once the membrane potential of each penetrated cell had stabilized and a steady baseline membrane potential was recorded, cells were characterized physiologically as either pacemaker or relay cells based on action potential wave forms; action potentials in pacemaker cells exhibited gradually depolarizing potentials between spikes that are lacking in relay cells (Bennett et al., 1967; Juranek and Metzner, 1997). After data collection from each cell, a positively biased sinusoidal current (∼2.0 nA for 5–10 min) was used to inject neurobiotin into the cell. Subsequent histological verification allowed us to unequivocally classify the cells as relay cells or pacemaker cells.
A high-impedance amplifier with active bridge circuitry (Intra 767; World Precision Instruments, New Haven, CT) was used to record the membrane potential of penetrated cells and to inject 0.5-msec-long hyperpolarizing constant current pulses ranging from −2 nA to −6.5 nA. The fish’s EOD was used to trigger the intracellular current pulses and to deliver them at a constant phase between each recorded spike during synaptically elicited frequency changes. The resolution of our input resistance measurements was 30 kΩ (0.2 mV). Intracellular signals and the fish’s EODs were stored on video tape using a recording adapter (Vetter 3000A; sample rate, 40 and 20 kHz, respectively).
At the conclusion of each experiment, fish were killed in 3-aminobenzoic acid ethylester (MS-222; Sigma, St. Louis, MO) and transcardially perfused with 0.9% saline, followed by 4% paraformaldehyde in 0.1 m phosphate buffer, pH 7.4 (30 min). Subsequently, brains were removed and stored overnight in the fixative solution. The hindbrain was then coronally sectioned on a vibratome at 50 μm intervals and collected in 0.02 mPBS, pH 7.3. After a standard Vectastain ABC (Vector Laboratories) and DAB (Sigma) reaction (Heiligenberg et al., 1996;Metzner and Juranek, 1997a), the tissue was mounted onto subbed slides and allowed to dry before it was counterstained with neutral red and coverslipped with Permount (Fisher Scientific, Fair Lawn, NJ). Light-microscopical inspection allowed us to identify neurobiotin-filled cells. This provided histological verification of the physiological classification of cell types made during the actual experiment. Furthermore, the site of electrode impalement during intracellular recordings was indicated in our neurobiotin-filled cells by a slight rupture in the cell membrane. We only included recordings obtained from somata in our data sample.
For off-line data analysis, both EODs and intracellular recordings were analog-to-digital converted using a commercial data analysis system (sample rate, 40 kHz/channel; Datawave, Denver, CO). Spike rates were determined by zero-crossing analysis. Changes in input resistance were calculated by measuring the amplitude of downward voltage deflections produced by constant current pulses and dividing by the amount of current injected. Data obtained during PPnG and nE↓ stimulation are presented as mean ± SEM of 10 consecutive measurements. Data obtained during chirping elicited during PPnC stimulation were not averaged and are presented in their raw format, because the rapid changes during chirps occur over the course of only a few EOD cycles and each chirp usually covers a different EOD frequency change. All changes in input resistance were normalized to the average input resistance of each cell before pharmacological manipulation of the various descending synaptic inputs. Changes in input resistance were plotted as a function of frequency changes using linear regression techniques (SigmaPlot; Jandel Scientific, San Rafael, CA). All but one (effect of nE↓ stimulation on pacemaker cells) data set were normally distributed and varied equally with respect to the regression line. An analysis of covariance revealed that regression slopes for a given cell type were not significantly different (p > 0.25) for a common stimulation site. Therefore, data from each cell type were separately pooled, and a new regression line was calculated according to the method of least squares for each of these pooled data sets. Quantitative comparisons between cell types was done by comparing the slopes of each regression line and noting differences at the 0.001 level of significance.
RESULTS
The pacemaker nucleus in gymnotiform fish is composed of two morphologically distinct cell types: pacemaker cells and relay cells. In Eigenmannia, pacemaker cells are coupled both with each other and with relay cells via electrotonic and chemical synapses (Fig.1) (Elekes and Szabo, 1982). The mixed chemical and electrotonic coupling between cells in the pacemaker nucleus poses a technical challenge for the identification of cellular effects occurring in response to changes in the activity of its synaptic inputs in vivo. Even exceptionally large hyperpolarizing currents injected intracellularly (Dye, 1991) were ineffective in halting oscillatory changes in membrane potential. Intracellular application of a voltage-gated sodium channel blocker QX-314 is also only partially effective and reduces the spike amplitudes of pacemaker and relay cells only by up to 50% (our unpublished observations). Therefore, measuring changes in input resistance appears to be the only direct means of quantifying postsynaptic effects of the inputs to the pacemaker nucleus in vivo.
Whereas the diameter of relay cells varies between 65 and 70 μm, pacemaker cells are approximately half that size, with diameters ranging between 30 and 35 μm. Correspondingly, the input resistance of pacemaker cells was significantly different from that of relay cells (Mann–Whitney U test; p < 0.001). The smaller pacemaker cell type had an average input resistance of 3.7 ± 0.30 MΩ (n = 10), whereas the larger relay cell type showed an average input resistance of 2.7 ± 0.11 MΩ (n = 8). This overall range of input resistance in pacemaker and relay cells is consistent with earlier reports in other gymnotiform fish (Bennett et al., 1967; Spiro, 1997).
To assess whether voltage-gated conductance changes could have masked the effects caused by the synaptic input to pacemaker and relay cells, we determined the change in membrane voltage as a function of the amount of injected current (Fig.2A,B). A highly significant linear relationship (r2 = 0.99; p < 0.001) was observed for changes in membrane potential caused by DC current injections. Hence, the input resistance, extracted from the slope of the regression lines, was independent of the amount of current injected and corresponded well to the average values given above [2.97 MΩ for a relay cell (Fig. 2A) and 3.75 MΩ for a pacemaker cell (Fig. 2B)]. In addition, in both cell types, the height of the hyperpolarizing current pulses were unaffected by shifts in the membrane potential (Fig.2C,D) over a behaviorally relevant frequency range (Fig. 2E,F). Therefore, the changes in input resistance that we observed during activation of the three synaptic inputs to the pacemaker nucleus were not attributable to activation of voltage-gated ion channels intrinsic to pacemaker and relay cells but were, instead, only attributable to modulatory effects of the synaptic inputs.
We also tested whether input resistances of pacemaker cells and relay cells were correlated with different EOD resting frequencies in different fish ranging from 380 to 500 Hz. No significant correlation between EOD resting frequency and input resistance in either of the two cell types was found (Spearman’s rank test; p> 0.10).
In the following, we present physiological evidence for the assumption that the synaptic input from each of the three prepacemaker nuclei affects pacemaker and relay cells in a distinctly different manner. We measured the changes in input resistance in pacemaker cells and in relay cells during pharmacological activation or inhibition of the three premotor pathways terminating on these two cell types of the pacemaker nucleus (Fig. 1). Because it is difficult to localize and sufficiently inhibit the SPPn to generate a consistent drop in EOD frequency, we stimulated the nE↓ with l-Glu instead. The nE↓ provides GABAergic input to the SPPn, and thus its stimulation causes a decrease in EOD frequency comparable with that caused by direct inhibition of the SPPn with GABA (Keller et al., 1990; Metzner, 1993; Juranek and Metzner, 1997).
We collected data from 12 pacemaker cell somata and 12 relay cell somata in 19 animals. During recordings from a particular cell type, each premotor input was repeatedly activated, or in the case of the nE↓–SPPn, inhibited 2–15 times.
Changes in input resistance during PPnC stimulation
PPnC stimulation elicited brief accelerations in spike rate in both pacemaker cells and relay cells that lasted between 5 and 20 msec. The resulting modulations in spike rate varied between 30 and 160 Hz (n = 31 chirps in four relay cell somata;n = 36 chirps in four pacemaker cell somata). Figure3 exemplifies that, during similar frequency changes of ∼60 Hz, the amplitude of the brief negative deflections in membrane voltage caused by hyperpolarizing current pulses was consistently reduced more profoundly in relay cells than in pacemaker cells. When quantified, the same recordings shown in Figure 3reveal a 34% decrease in the input resistance of the relay cell (Fig.4A), whereas that of a pacemaker cell decreased only by 9% (Fig. 4B). These decreases in input resistance also showed different time courses in pacemaker and relay cells (Mann–Whitney U test;p < 0.001). In all relay cells tested, input resistances were reduced over an average duration of 13.02 msec (SD ± 2.65 msec; range, 8.29–20.14 msec), whereas the average duration of decreased input resistances in pacemaker cells was only 9.88 msec (SD ± 2.24 msec; range, 5.02–15.58 msec).
In summary (Fig. 4C), a linear regression analysis revealed for relay cells a significantly greater change in input resistance than in pacemaker cells (p < 0.001). In all relay cells analyzed, the input resistance decreased by 14.0 kΩ/Hz (r2 = 0.50), whereas in our entire sample of pacemaker cells, the input resistance decreased by merely 3.5 kΩ/Hz (r2 = 0.47). This decrease in input resistance observed in relay cells during PPnC stimulation is indicative of a large conductance increase characterized by a brief time course lasting between 8 and 20 msec.
Occasionally, brief interruptions of the ongoing spike rate did occur in relay cells, particularly after a dramatic acceleration in instantaneous spike frequency (EOD frequency followed that of the relay cell spikes) (Fig. 5). In all four relay cells analyzed, a skipped spike during an interruption was preceded by a “shoulder” on the repolarizing flank of the previous action potential. This shoulder consistently appeared at membrane potentials that were 10–25 mV depolarized relative to baseline (mean, 17.7 mV; SD = 3.9 mV; n = 54). After the skipped spike, instantaneous spike frequency was dramatically reduced yet recovered to the resting frequency in the next cycle. This phenomenon was never observed in pacemaker cell recordings. Furthermore, such shoulders never occurred during the rising phase of relay cell spikes.
Changes in input resistance during PPnG stimulation
Pharmacological stimulation of the PPnG with [scap]l-Glu elicited gradual frequency accelerations varying between 5 and 30 Hz. We recorded from four pacemaker cell somata during seven stimulations of the PPnG and from four relay cell somata during eight PPnG stimulations. In contrast to PPnC stimulations, we observed a greater decrease in input resistance in pacemaker cells than in relay cells (Fig.6A,B). In addition, the time courses of the decrease in input resistance were much slower during PPnG stimulation and reflected the slower and longer lasting frequency acceleration extending over a period of several seconds compared with the brief acceleration observed during stimulation of the PPnC, which lasted for only a few milliseconds. This difference is likely to be based on the involvement of different Glu receptor subtypes (NMDA and AMPA, respectively) and will be addressed in the Discussion.
Figure 6C summarizes the changes in input resistance with changing frequency for our entire data pool. Input resistance in pacemaker cells decreased by 27.1 kΩ/Hz (r2 = 0.67), whereas in relay cells the input resistance was reduced by only 8.6 kΩ/Hz (r2 = 0.66). The regression coefficients for the two regression lines were significantly different (p < 0.001).
Changes in input resistance during SPPn inhibition
Gradual frequency decelerations varying between 3 and 5 Hz and similar to those obtained by inhibiting the SPPn with GABA (Metzner, 1993) were elicited by stimulation of the nE↓ with l-Glu (see Materials and Methods, experimental procedures; Fig. 1 ). We tested the effects of nine stimulations of the nE↓ in four relay cell somata and of eight nE↓ stimulations in four pacemaker cell somata. In contrast to decreases in input resistance observed during frequency accelerations attributable to either PPnC or PPnG stimulation, indirect SPPn inhibition resulted in increases in input resistance, whereas the spike (and EOD) frequency gradually decelerated. When quantified, during a 4 Hz frequency shift, the input resistance of a relay cell increased by 8% (Fig.7A), whereas in the pacemaker cell, it increased by 5% (Fig. 7B).
During indirect inhibition of the SPPn, therefore, the input resistances in relay cells changed in a manner different from those observed in pacemaker cells (Fig. 7C). In relay cells, the input resistance increased by 42.8 kΩ/Hz (r2 = 0.72). In pacemaker cells, on the other hand, the change in input resistance was not linearly related to the decreases in spike (and EOD; data not shown) frequency (r2 = 0.07). Using nonlinear regression techniques, we tried to quantitatively describe the changes observed in pacemaker cells during EOD decelerations. However, the highly variable nature of these data points did not lend them to this form of analysis. Hence, we concluded that the responses of pacemaker cells were qualitatively different from the responses of relay cells, and only in relay cells, spike frequency (and EOD frequency) was clearly related with a change in input resistance. The increases in input resistance we observed in relay cells during SPPn inhibition is the first direct physiological evidence for EOD decelerations being mediated by a reduced level of tonic excitatory input.
In conclusion, as summarized in Figure 8, two forms of EOD frequency accelerations, rapid and gradual, are mediated by selective termination of glutamatergic inputs onto different cell types, relay cells and pacemaker cells, respectively. Quantitative differences in changes in input resistance between cell types for a given premotor input, e.g., from PPnC, is indicative of selective synapse formation; the greatest changes are expected to be observed in the target cell type. In contrast, EOD decelerations are attributable to “turning off” a tonic glutamatergic input to relay cells. Thus, opposing gradual frequency changes, decelerations and accelerations are independently controlled at the level of a single cell type, i.e., relay cells, by decreasing a tonic conductance and transiently increasing a conductance, respectively.
DISCUSSION
The three synaptic inputs to the pacemaker nucleus in gymnotiform electric fish are not only behaviorally strictly segregated (Kawasaki et al., 1988; Dye et al., 1989; Metzner, 1993; recent review: Metzner and Viete, 1996a,b) but, as we have shown here, also involve qualitatively and quantitatively different cell responses, as well as different target cells. This enables us to finally adopt a model circuit diagram (Fig. 1) that has been proposed previously (Metzner, 1993; Juranek and Metzner, 1997) but in which the innervation pattern of the cellular components of the pacemaker nucleus was only based on indirect evidence from pharmacological and preliminary physiological and histological experiments. This model (Fig. 1) accounts for the emergence of three different behavioral patterns from a single oscillatory network consisting of only two different cell types and the single neurotransmitter Glu. The observed small changes in input resistance seen also in “coupled cells”, i.e., those cell types that do not represent primary targets for projections from the three premotor nuclei, cannot be explained by a presence of voltage-gated channels (Fig. 2). Although we cannot completely rule out marginal input from the three premotor structures to coupled cells, the effect could be attributable to the presence of intrinsic chemical synapses between pacemaker and relay cells (Bennett, 1971; Elekes and Szabo, 1982, 1985) (Fig. 1). It could also be attributable to voltage-dependent changes in the conductance of the gap junctions between pacemaker and relay cells (for review, see Bennett et al., 1990; Bennett, 1997).
We are not aware of any other vertebrate system in which different premotor pathways mediating different behavioral patterns remain segregated to the level of the synaptic input to their target cells in the premotor command nucleus. In two of the best studied systems, the central pattern generators in the spinal cord of lampreys controlling various modes of swimming behavior (Grillner et al., 1995; Grillner, 1997; Viana Di Prisco et al., 1997) and that in the mammalian brainstem controlling different forms of breathing (Feldman and Smith, 1989;Ramirez and Richter, 1996), separation of synaptic modulation of network properties from synaptic modulation of cellular properties is a difficult task, owing to the complex interactions between the cellular elements composing the central pattern generators. InXenopus larvae, two distinct motor patterns, swimming and struggling, are driven by a common premotor pathway (Soffe, 1993). They can be controlled by the level of excitation within the spinal motor circuitry and need not involve the activity of a specific external neuromodulator (Soffe, 1996). In invertebrates, on the other hand, modulation of premotor control circuits appears to be far more distributed, and no clear behavior-specific segregation at the level of individual target cells has been described (Harris-Warrick and Marder, 1991; Marder and Calabrese, 1996).
Preliminary evidence from light-microscopical studies, so far lacking direct physiological confirmation, indicates that the segregation of behavior-specific inputs onto different cell types might be a general feature in pacemaker nuclei of various gymnotiform fish. AlthoughSternopygus, for instance, does not perform a JAR (Bullock, 1969) or produce chirps (Hopkins, 1974a), it can interrupt its EOD for several seconds via NMDA receptor-mediated input originating from the SPPn and presumably terminating on relay cells. In addition,Sternopygus can gradually raise its EOD frequency via NMDA receptor-mediated input originating from the diencephalic prepacemaker nucleus, which seems to project to pacemaker cells (Keller et al., 1991). Other possible examples for this segregation of synaptic input from different behavior-specific premotor pathways are found inApteronotus (Heiligenberg et al., 1996) andHypopomus (Kennedy and Heiligenberg, 1994; Spiro, 1997).
Maintaining segregation of premotor inputs to not only different target cells, but also to different receptor subtypes (Fig. 1), bears the potential of increasing the behavioral repertoire even more; the channel kinetics of AMPA-type receptors make them particularly well suited for brief and rapid accelerations, such as those occurring in most chirps, whereas NMDA-type receptors are better suited for long, gradual frequency increases. (Of course, this does not exclude the possibility that the slower, gradual EOD frequency changes observed during PPnG stimulation could also be caused by activity changes of PPnG cells occurring with a slow time constant.) Segregation of these receptors onto different cell types in the pacemaker nucleus would ensure reproducibility of each form of frequency modulation. Brief changes would be encoded more reliably by the output cell type, relay cells, because any internal noise would be least detrimental to the generation of distinct, abrupt changes in firing rate at this peripheral level. On the other hand, stable sustained changes are more noise tolerant and can be introduced into the pacemaker network more “upstream” by the rhythm-generating cell type, pacemaker cells.
If separate excitatory inputs that carry different information streams, such as those generating chirps and those mediating EOD deceleration during the JAR, terminate onto the same cells within a premotor command nucleus, in our example onto relay cells (Fig. 1), they often involve different receptor subtypes. Similarly, in the oscine song system, inputs from two neostriatal nuclei, the lateral magnocellular nucleus of the neostriatum (lMAN) and high vocal center (HVc), believed to carry auditory feedback and temporal patterning, respectively, terminate on neurons of the vocal premotor command nucleus, the robust nucleus of the archistriatum (Doupe and Konishi, 1991). However, the lMAN input is mediated by NMDA receptors, whereas the HVc input is mediated by AMPA receptors (Mooney, 1992; Mooney and Konishi, 1991). In the spinal locomotor circuit in lamprey, computer simulations have revealed that the relative contribution of NMDA and non-NMDA receptor-mediated inputs plays a significant role in modifying the frequency of rhythmic bursting in spinal motoneurons (Grillner et al., 1995). Thus, different swim rates can be attributed to differential weighting of NMDA–AMPA receptor-mediated inputs. When glutamatergic inputs from reticulospinal cells is weighted in favor of NMDA receptors, slow rates of rhythmic bursting emerge from the network. In contrast, higher rates of rhythmic bursting can be generated by weighing the glutamatergic inputs in favor of AMPA receptors. The cellular basis for this differential weighing of NMDA–AMPA receptor activation has, however, not yet been identified.
In the present study, the large conductance increases in relay cells lasting 8–20 msec during PPnC stimulation share remarkable similarity with measurements of purely AMPA receptor-mediated currents in rat retinal ganglion cells (Taschenberger et al., 1995). Because the time course of input resistance changes is expected to parallel the time course of postsynaptic currents, our results provide additional physiological evidence suggesting the involvement of AMPA receptor-mediated currents in relay cells underlying chirp-like communication behavior. Whether receptor desensitization and/or receptor deactivation shapes the time course of conductance changes in our system will be addressed in future studies. Arguably, the consistency of the behavior is dependent on rapid termination of postsynaptic currents. Prolonged depolarization of relay cells for >20 msec would be expected to additionally recruit NMDA receptors if Glu had not been sufficiently cleared from the synaptic cleft. This would, of course, shape the magnitude and time course of frequency modulations. An entirely different behavior could thus be sculpted at the subcellular level. Long EOD interruptions, which often occur during courtship (Hopkins, 1974b; Hagedorn and Heiligenberg, 1985), are characteristically three to five times longer in duration (≥70 msec) than the short chirps investigated in the present study, which naturally occur during agonistic encounters (Hopkins, 1974b). It is thus tempting to speculate that the longer chirps inEigenmannia could be attributed to a combined role for AMPA and NMDA receptors. Interestingly, long chirps can be elicited inApteronotus, a related gymnotiform (Alves-Gomez et al., 1995), by electrical stimulation of cells in the SPPn. In contrast toEigenmannia, this form of stimulation “turns on” an otherwise quiescent glutamatergic input to relay cells, which appears to be mediated by NMDA receptors (Heiligenberg et al., 1996). The behavioral result is a long chirp that resembles those produced by males during courtship.
Especially during such longer chirps resulting in interruptions of the otherwise continuous spike train (and EOD), a shoulder-like phenomenon during prolonged spike duration was commonly observed in relay cell recordings (Fig. 5). This shares some essential features with well described modulations of intrinsic membrane properties found in other systems, such as the spinal locomotor network in lamprey and the mammalian respiratory network in the medulla (Feldman and Smith, 1989;Grillner et al., 1995; Ramirez and Richter, 1996). Recent pharmacological experiments in the isolated pacemaker nucleus ofApteronotus might help to explain this phenomenon. These studies have indicated a role for a nickel- and cadmium- sensitive Ca2+ current in maintaining the normal resting frequency of spike discharge (Smith and Zakon, 1997). Because voltage-gated Ca2+ channel blockers had no effect on the ongoing spike rate, the type of Ca2+ channel contributing to the resting oscillation frequency has yet to be more fully characterized (Smith and Zakon, 1997). As reported in other oscillatory systems (Grillner et al., 1995; Ramirez and Richter, 1996;Grillner, 1997), modulation of Ca2+-activated channels is an especially effective means to alter spike rates. It is tempting to speculate that the spike broadening we observed could be caused by an increased Ca2+ influx during membrane depolarization. It appears therefore that different cellular mechanisms might have contributed to the widening of the behavioral repertoire of weakly electric fish.
Results from recent lesion experiments in the electrosensory system of gymnotiform fish suggest that the sensory signals evoking chirp-like communication behavior and yielding a JAR are processed in segregated pathways as well (Metzner and Juranek, 1997b). The first order nucleus of the electrosensory system, the electrosensory lateral line lobe, consists of four segments, three of them receiving identical input from electroreceptors. Although the centromedial segment was both necessary and sufficient for the JAR, it did not affect the communicative response to external electric signals. Conversely, the lateral segment did not affect the JAR but was necessary and sufficient to evoke communication behavior. Combined with the findings described in the present study, this system illustrates that sensorimotor control of different behaviors can occur in strictly segregated channels from the sensory input of the brain all through to its motor output.
What is the reason for the distinctly distributed organization of the electrosensory and premotor systems in these fish? For the existence of multiple electrosensory maps, it is conceivable that duplication of existing brain maps could efficiently accommodate the increased information flow associated with a growth in the behavioral repertoire, as originally proposed for the sensory maps in mammalian cortex (Allman and Kaas, 1971; Kaas, 1982; see also Metzner and Juranek, 1997b). On the premotor side, accurate electrolocation requires an extremely low jitter in EOD discharges (Bullock, 1969; Heiligenberg, 1991; Moortgat et al., 1998). This demand for highly synchronous and regular discharge of the pacemaker nucleus probably was the leading selective pressure yielding the strict functional separation of its cellular components into pacemaking units, i.e., pacemaker cells, and output units, i.e., relay cells (Bennett et al., 1967). This rigid design of the premotor command nucleus may, in turn, have required its synaptic inputs to remain distinctly segregated to produce the different motor patterns.
Footnotes
This work was supported by academic research grants from University of California at Riverside and by the National Science Foundation. We thank C. Condon, S. Currie, K. Moortgat, G. Stanley, and S. Viete for their comments on this study. Y. T. Yan, D. Welsbie, Y. Song, and B. Andersen provided assistance with histological procedures and data analysis.
Correspondence should be addressed to Walter Metzner, Department of Biology, University of California at Riverside, Riverside, CA 92521-0427.