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The Journal of Neuroscience, March 1, 2002, 22(5):1985-1993
Highly Dissimilar Behaviors Mediated by a Multifunctional Network in the Marine Mollusk Tritonia diomedea
Ion R. Popescu and William N. Frost Department of Cell Biology and Anatomy, Finch University of Health Sciences, The Chicago Medical School, North Chicago, Illinois 60064
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
Several motor networks have now been found to be multifunctional, in which one group of neurons participates in the generation of multiple behavioral motor programs. Not surprisingly, the behaviors involved are frequently closely related, often using the same or similar muscle groups. Here we describe an interneuronal network in the marine mollusk Tritonia diomedea that is involved in producing two highly dissimilar behaviors, rhythmic, muscle-based escape swimming and nonrhythmic, cilia-mediated crawling. Several observations support this conclusion. First, the dorsal swim interneurons (DSIs) of the swim central pattern generator (CPG) directly excite Pedal neuron 21 (Pd21) and Pd5, the only identified cilia-activating efferent neurons in Tritonia. Second, stimulation of a single DSI elicits beating of the foot cilia in semi-intact preparations and crawling in intact animal treadmill preparations. Third, the DSIs fire at an elevated rate for nearly 1 hr after a swim motor program, which correlates reasonably well with the period freely behaving animals were found to crawl after they swam. Fourth, silencing the tonically active DSIs after a swim motor program substantially reduces or eliminates ongoing cilia neuron firing, indicating that the DSIs are major contributors to the synaptic input driving these cells. Finally, all of the other swim CPG neurons also connect to the cilia neurons, most monosynaptically. Taken together, these observations indicate that the Tritonia swim CPG network participates in producing both escape swimming and crawling. Given the extreme differences between these behaviors
-rhythmic versus tonic, muscular versus ciliary, and brief versus prolonged
Key words: Tritonia; multifunctional network; central pattern generator; cilia; locomotion; mollusk; CPG; evolution; multifunctional neuron
INTRODUCTION
An emerging principle of motor control is that some neural networks mediate multiple behaviors (Getting, 1989
; Pearson, 1993
The existence of such networks prompts a number of questions. How are the different motor programs of such networks selectively activated? Can multifunctional networks incorporate modulation specific to one behavior, as might occur in learning, without altering the other behaviors mediated by the same network? Just how dissimilar can behaviors be and still be mediated by a single neuronal network? Are multifunctional networks relatively rare, or are they a widespread feature of most nervous systems? Such questions can most effectively be addressed in preparations allowing detailed electrophysiological dissection of the individual components of multifunctional networks.
The escape swim network of the marine mollusk Tritonia diomedea has previously been suggested to be multifunctional for swimming and reflexive withdrawal (Getting and Dekin, 1985b
Although no role for the swim network in crawling had been suggested before this study, certain previous findings led us to suspect such a role. First, this laboratory and others had noted that one particular group of central pattern generator (CPG) neurons, the dorsal swim interneurons (DSIs), fire tonically at an elevated rate for several minutes after swim motor programs elicited in isolated brain preparations (Lennard et al., 1980
MATERIALS AND METHODS
Behavior. The duration of postswim crawling was measured in an 88 × 57 cm test arena created within a 120 gallon, 10°C recirculating artificial seawater aquarium. A plastic mesh (grid dimensions, 1.5 × 2.0 mm) fixed to the arena floor provided a background against which crawling could be visually assessed. During each observation period, animals were scored as crawling if the tip of the tail was observed to progress at least 1 grid unit along the substrate during a 15 sec period. Any animal whose foot was not in contact with the substrate during the observation period was not scored for that session rather than scored as not crawling. This was because such animals are often observed to have a steady stream of debris particles moving along the upturned foot, indicating that they are in "crawling mode."
Isolated brain preparation. For most electrophysiology experiments, the brain, consisting of the fused cerebral-pleural ganglia and the pedal ganglia (with the pedal-pedal commissure cut), was dissected from the animal and pinned dorsal side-up in a Sylgard-lined recording chamber perfused with normal saline at 4-6°C. Normal saline consisted of (in mM): 420 NaCl, 10 KCl, 10 CaCl2, 50 MgCl2, 10 HEPES, pH 7.6, and 11 D-glucose. All procedures used stainless steel minuten pins (0.1 and 0.2 mm thickness) to stabilize the nervous system for recording. After dissecting away the connective tissue sheath covering the cerebral-pleural ganglia, a polyethylene suction electrode was attached to left or right pedal nerve 3 (PdN3; for nomenclature, see Willows et al., 1973
Intracellular recordings were made with 15-40 M
electrodes filled with 3 M KCl or 3 M K-acetate. Neurons were identified on the basis of their location, size, color, synaptic connections with other identified neurons, and activity during the swim motor program, as described previously (for Pd5 and Pd21, see Willows et al., 1973
Synaptic connections were considered direct if presynaptic action potentials produced one-for-one, constant-latency postsynaptic potentials in the postsynaptic neuron that persisted in a high divalent cation solution. This solution consisted of (in mM): 285 NaCl, 10 KCl, 25 CaCl2, 125 MgCl2, 10 HEPES, pH 7.6, and 11 D-glucose and has been shown to be effective at reducing the recruitment of polysynaptic pathways in Tritonia (Katz and Frost, 1995b
Dorsal semi-intact preparation. Animals were anesthetized by injecting 60 ml of a solution composed of half 350 mM MgCl2 and half artificial seawater (Instant Ocean; Aquarium Systems). A recording chamber was used in which the animal could be positioned dorsal side-up, with the brain exposed and stabilized on the Sylgard surface of a 1-cm-diameter post rising from the chamber floor. A thin cylindrical sleeve, containing slits to allow the nerves passage, was raised around the brain; the slits were closed with Vaseline; and the brain and body chambers were perfused separately with saline. The brain chamber was initially perfused at 2°C, during which the thin sheath enclosing the ganglia was removed to expose the neurons for intracellular recording. Once the neurons were exposed, both brain and body chambers were perfused at 11°C for the duration of the experiment.
Ventral semi-intact preparation. This preparation, used for measuring the rate of charcoal particle transport on one side of the foot while driving a contralateral DSI, is identical in methods to the dorsal semi-intact preparation, with the following exceptions. After the anesthesia, the animal was placed ventral side-up in a dissection tray filled with 50% MgC12 and 50% artificial seawater originally at 4°C but allowed to reach room temperature over the course of the dissection (~l hr). A midline incision was made in the foot to expose pedal nerve 3, which courses intimate to the viscera. The buccal mass was rotated forward until pedal nerve 3 was exposed rostrally all the way to the brain. The esophagus was cut, and the viscera and buccal mass were removed after the nerve was dissected free from the viscera. Next, an ~4 cm midline incision was made in the dorsal body wall under the brain. After the cerebral nerves were cut, the brain was pinned dorsal side-up on the Sylgard-covered surface of the post rising from the chamber floor through the dorsal incision.
After resting the preparation overnight at 4°C, a suspension of charcoal particles (M. Grumbacher Inc., New York, NY) in saline was sprinkled over several square centimeters of foot contralateral to an impaled DSI, about midway to the tail. This area was projected onto a video monitor via a microscope-mounted camera, and particle movement was assessed with the help of a calibrated grid placed over the screen of the monitor. DSI was driven to fire action potentials at 0.5, 1, or 2 Hz by applying discrete current pulses at these rates through the intracellular electrode. DSI activity and accompanying video of charcoal particle movement were recorded together on videotape with a Vetter 402 data recorder (A. R. Vetter Inc., Rebersburg, PA).
Intact animal treadmill preparation. This preparation (for additional details, see Popescu and Willows, 1999
Data analysis. Results are reported as means ± SE. Statistical procedures included repeated measures ANOVAs followed by Newman-Keuls post hoc tests and repeated measures t tests with Bonferroni-adjusted p values (two-tailed). ANOVA analyses were conducted with the Statistica software package (Statsoft).
RESULTS
A network diagram depicting the multifunctional Tritonia network is shown in Figure 1A. This figure represents the previously known and newly reported synaptic connections and illustrates the involvement of the network in both escape swimming and crawling.
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Figure 1. The multifunctional Tritonia network. A, Diagram of synaptic connections, showing the afferent neurons (S), pre-CPG interneurons (Tr1, DRI), swim CPG neurons (DSI, C2, VSI-A, VSI-B), swim flexion neurons (DFN-A, DFN-B, VFN), and the locomotion cilia neurons (Pd21, Pd5; (Willows et al.; 1973
DSI stimulation elicits crawling in an intact animal treadmill preparation
Previous work noted that after a swim motor program, the DSI neurons of the swim CPG fire tonically at an elevated rate for an undetermined period (Fig. 1B; Lennard et al., 1980
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Figure 2. DSI activity elicits crawling. This experiment used an intact animal treadmill electrophysiology preparation, in which ciliary locomotion caused a drum positioned beneath the animal's foot to rotate. Sufficient depolarizing current was injected into a single DSI to elicit several seconds of firing (bottom trace). This produced a period of crawling that outlasted the DSI train by tens of seconds (top trace). With the treadmill apparatus, crawling, which is steady and nonrhythmic, is transduced into an oscillating voltage signal. The distance between two consecutive peaks represents 2 mm of locomotion. The maximum rate of treadmill turning corresponded to 1 mm/sec of locomotion.
The DSIs excite cilia-activating neurons with direct excitatory synaptic connections
Pd21 and Pd5 are presumptive motor neurons that, when driven with intracellular stimulation, excite the locomotor cilia on the animal's foot (Audesirk, 1978a
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Figure 3. The DSIs directly excite the Pd21 and Pd5 cilia neurons. A, A DSI train evoked by intracellular stimulation produced excitation of the contralateral Pd21 in normal saline. B, Same result for Pd5. In this case, the duration of DSI stimulation is indicated by a bar. C, DSI produced constant latency, one-for-one EPSPs in Pd21 in high divalent cation saline. D, Same result for Pd5. R, Right; L, left.
DSI firing correlates with both crawling and cilia neuron activity
The treadmill experiment showed that directly activating a single DSI elicits crawling. We also tested the hypothesis that postswim DSI firing (Fig. 1B) mediates crawling by comparing the duration of crawling, DSI firing, and cilia neuron firing. If the DSIs drive crawling, their firing should correspond to both cilia neuron firing and crawling behavior.
Behavior
Although it has been noted previously that Tritonia crawl after they swim (Audesirk, 1978b
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Figure 4. DSI firing correlates with crawling and cilia neuron activity. A, Duration of postswim crawling in freely behaving animals. Twenty animals were transferred to a test arena, and their crawling was assessed once every 5 min for 6 hr. Each point represents the mean of the six determinations of how many were crawling during the corresponding 30 min period. The transfer itself stimulated crawling, which declined over the first 3 hr. At that point, all animals were made to swim (time 0). For statistical analysis, each of the six postswim means was compared with the final pretest mean. The swim was followed by significantly enhanced crawling lasting 90 min. The dotted boxes in this and the subsequent graphs represent the duration of the significant effect. At 5 min after the swim, all animals that had their foot in contact with the substrate were crawling (13 of 13 animals). B, Duration of enhanced DSI firing after a swim motor program in the isolated brain. The motor program was elicited at time 0. DSI firing was significantly enhanced for 55 min (14 cells, 10 preparations). C, Duration of enhanced Pd21 firing. Pd21 firing was significantly enhanced for 75 min (8 cells, 7 preparations). D, Duration of enhanced Pd5 firing. Pd5 firing was significantly enhanced for 35 min (7 cells, 4 preparations). E, Example of DSI and Pd21 firing before and after a nerve stimulus-elicited swim motor program. Arrows in E and F indicate the time of the nerve stimulus. The individual cycles of the motor program cannot be clearly seen in the DSI trace at this time base but are visible as voltage oscillations in Pd21. F, Example of DSI and Pd5 firing before and after a nerve stimulus-elicited swim motor program. The statistics for B-D were only applied to the cells (numbers listed in Results) that were recorded for the full period shown on the graphs.
Neuronal correlates
DSIs. A minimum of 3 hr after any previous swim motor program, the DSI spontaneous firing rate was recorded before and after a swim motor program elicited by a brief stimulus applied to PdN3 (10 Hz, 2 sec, 5 msec pulses). An ANOVA revealed a significant effect of nerve shock on DSI firing rate (F(8,80) = 47.5; p < 0.001). The DSI firing rate increased from 5 ± 2 spikes per minute just before to a peak rate of 111 ± 10 spikes per minute (1.9 Hz) during the first 30 sec after the swim motor program, after which it progressively declined back to baseline. Post hoc testing indicated that DSI firing was significantly higher for 55 min after the motor program (Fig. 4B,E,F; p < 0.05; 11 cells, eight preparations). Postswim elevated DSI firing was also observed after salt-elicited swims in intact animal electrophysiology preparations, but the duration of the effect was not determined in those experiments (four preparations). Cilia neurons. The spontaneous firing rates of Pd21 and Pd5 also underwent a long-lasting increase after the swim motor program. An ANOVA revealed a significant effect of nerve shock on Pd21 firing rate (F(6,24) = 18.5; p < 0.001). Post hoc testing indicated that the firing rate of Pd21 was significantly increased for 75 min (Fig. 4C,E; p < 0.05; five cells, four preparations). An ANOVA also demonstrated a significant effect of nerve shock on Pd5 firing rate (F(6,36) = 9.96; p < 0.001). Post hoc testing indicated that Pd5 firing was significantly increased for 35 min (Fig. 4D,F; p < 0.05; seven cells, four preparations).Low rates of DSI stimulation activate the foot cilia
To test whether the recorded rates of post-swim motor program DSI activity were sufficient to activate the locomotory cilia, we used a semi-intact preparation in which individual DSIs could be driven intracellularly while monitoring the movement of charcoal particles applied to the contralateral foot. In all instances, cilia that had been stationary before DSI stimulation (particles moving at <0.5 mm/min) became active (particles moving at >2.25 mm/min) when single DSIs were driven at 2 Hz (five trials in three preparations), 1 Hz (five trials in two preparations), and 0.5 Hz (four trials in two preparations). The average latency to movement onset was on the order of minutes and depended on the stimulation rate: 0.5 Hz = 5.0 min; 1 Hz = 2.6 min; and 2 Hz = 1.0 min. In all cases, charcoal particle transport continued for tens of seconds after the cessation of DSI stimulation.
Tonic DSI firing actively maintains the elevated cilia neuron firing after the swim motor program
The above observations support the hypothesis that after a swim, elevated DSI firing acts to increase the tonic firing rate in the cilia neurons, resulting in enhanced crawling. To more directly test this idea, we next examined the effect of transiently removing this postswim DSI input to the cilia neurons.
In isolated brain preparations, a Pd21 and two or three of its three contralateral DSIs were simultaneously impaled with intracellular electrodes. After a rest period, a nerve stimulus was delivered to PdN3 to elicit the swim motor program, resulting in the usual elevated tonic firing in both neuron types. During this period of enhanced firing, a hyperpolarizing current was simultaneously injected into all impaled DSIs to suppress their firing for several seconds. This was found to reduce or eliminate the tonic firing in the Pd21 neurons (Fig. 5A; three Pd21 cells, two preparations). In the one instance in which it was tested, suppressing the firing of all three ipsilateral DSIs also eliminated the enhanced post-swim motor program firing in the contralateral Pd5 (Fig. 5B). The DSIs are not electrically coupled to either Pd21 or Pd5; thus the effect of suppressing DSI firing on the cilia neuron firing rate is not attributable to the spread of the hyperpolarizing current. These results are consistent with a role for the DSIs in actively maintaining the post-swim motor program elevated cilia neuron firing rate.
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Figure 5. Tonic DSI firing actively maintains the elevated cilia neuron firing that follows the swim motor program. A, After a swim motor program (data not shown), the DSIs and cilia neurons fire at an elevated tonic rate. Hyperpolarizing two of the three contralateral DSIs during this period acted to eliminate the tonic firing in Pd21. B, In a similar experiment, hyperpolarizing all three contralateral DSIs repeatedly reduced or eliminated the elevated tonic firing in Pd5. R, Right; L, left.
Prolonged DSI firing also occurs in response to stimuli too weak to trigger the swim motor program
Although Tritonia crawl after they swim, they also crawl in other contexts, such as in response to water flow (Willows, 1978
We found that nerve stimuli below the threshold for eliciting the swim motor program produced prolonged enhanced DSI firing in the isolated brain preparation. An ANOVA revealed a significant effect of weak nerve shock on DSI firing rate (F(11,44) = 28.5; p < 0.001). Post hoc testing indicated that the DSI firing rate was significantly higher for at least 10 min (Fig. 6; p < 0.05; five cells, three preparations). Longer recordings were not made, so the duration of this effect is not known. This result is consistent with the hypothesis that the multifunctional swim network mediates crawling in contexts other than swimming (see Discussion).
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Figure 6. Stimuli subthreshold for producing the swim nonetheless cause long-lasting DSI firing. A weak nerve stimulus administered to PdN3 at the arrow (10 Hz, 2 sec) elevated the rate of spontaneous DSI firing for at least 10 min.
All members of the swim CPG make direct or indirect connections to the cilia neurons
Previous studies reported that CPG neuron C2 makes direct, mixed excitatory and inhibitory synaptic connections to both Pd21 and Pd5 (Snow, 1982
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Figure 7. CPG neuron VSI-A monosynaptically inhibits the cilia neurons. A, VSI-A action potentials elicited unitary, one-for-one IPSPs in the contralateral Pd5 in high divalent cation saline. The third current pulse caused two action potentials and two corresponding IPSPs in Pd5. B, In high divalent cation saline, a train of VSI-A spikes elicited one-for-one, summating IPSPs in the contralateral Pd21. C, The inhibitory VSI-A connection to Pd21 was sufficient to inhibit P21 firing in normal saline. VSI-A was driven via the intracellular electrode to fire two trains of action potentials. The slight depolarization of Pd21 during the inhibition was attributable to a reversal of the IPSP, which had initially been hyperpolarizing when Pd21 was penetrated. R, Right; L, left.
Stimulating CPG neuron VSI-B also reduced the elevated post-swim motor program firing of Pd21 (Fig. 8A). However, when tested in high divalent cation saline, this connection was clearly not one-for-one (Fig. 8B; four preparations), indicating that it is polysynaptic, involving the recruitment of an as yet unidentified inhibitory interneuron. We also tested for, but did not observe, a connection between VSI-B and the contralateral Pd5 (two preparations). In summary, every member of the swim CPG network was found to make either direct (DSI, C2, and VSI-A) or indirect (VSI-B) connections with one or both of the cilia neurons Pd21 and Pd5 (Fig. 1A), indicating that the previously described swim network is wired appropriately to mediate both swimming and the excitatory and inhibitory control of crawling.
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Figure 8. CPG neuron VSI-B polysynaptically inhibits Pd21. A, Driving VSI-B caused a decrease in the firing rate of the contralateral Pd21. B, In high divalent cation saline, a train of VSI-B spikes recruited IPSPs into Pd21 in a non-one-for-one manner, indicating that this inhibitory connection is indirect. L, Left; R, right.
What are the functions of the non-DSI connections from the swim CPG to the cilia neurons? These neurons either undergo no apparent long-lasting change in spontaneous firing rate after swimming (VSI-A) or are silent when not swimming (C2 and VSI-B; Fig. 1B). A possible function for the inhibitory connections (VSI-A and VSI-B) might be to mediate touch-induced inhibition of crawling. A previous report (Audesirk, 1978b
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Figure 9. Response of DSI and VSI-B to tactile skin stimulation. Poking the skin with a glass probe (arrow) elicited action potentials in VSI-B and inhibition in DSI.
DISCUSSION
The multifunctional Tritonia network
Previous work suggested that the Tritonia escape swim network mediates two different behaviors. Weak-to-moderate stimuli were proposed to elicit withdrawal responses, whereas strongly aversive stimuli reconfigure the network into its swim pattern-generating mode (Getting and Dekin, 1985a
Multifunctional networks are frequently found to mediate closely related behaviors that use the same or similar muscle groups. The present example is a striking exception. In Tritonia, swimming is a brief, rhythmic behavior mediated by alternating ventral and dorsal whole-body muscular contractions. Postswim crawling, on the other hand, is two orders of magnitude longer lasting, nonrhythmic, and cilia-mediated. To our knowledge, this is the first direct demonstration of multifunctional network control over muscular and ciliary effector systems. Similar control has been proposed for swimming and ciliary crawling by the As1-4 neurons, homologs of the DSIs, in the marine mollusk Pleurobranchaea (Jing and Gillette, 2000
An additional difference between these two Tritonia behaviors concerns their degree of flexibility. Swimming is a stereotyped, nondirectional behavior that is relatively unaffected by sensory feedback once under way. Crawling, on the other hand, varies in speed and direction and is readily modified by sensory input, inhibited when the animal's oral veil comes into contact with food or tactile stimuli (Audesirk, 1978b
Many studies have described multifunctional networks that mediate motor programs underlying different, muscle-based behaviors (Getting, 1989
Taken together, the present results and previous studies support the view that the Tritonia swim CPG may be involved in the production of a highly diverse set of behaviors, including (1) reflexive withdrawal (Getting and Dekin, 1985a
Additional features
Although multifunctionality has the advantage of neural economy, it has inherent problems as a design strategy. How, for example, do the different functional subcircuits of anatomically superimposed networks operate without interfering with one another? In this Tritonia example, the two motor programs are coactive during the swim, when the DSIs excite the efferent neuron populations for both swimming and crawling. There is no behavioral conflict, however, because although the foot cilia are active during the swim (Audesirk, 1978b
In Tritonia, there is an obvious survival advantage to having a single network mediate withdrawal, swimming, and crawling. Although withdrawal and crawling can occur in the absence of swimming, strongly aversive stimuli elicit all three behaviors in a defined temporal sequence. Having a common network control these functionally related but disparate behaviors would ensure the efficient coordination of this complex, integrated escape response. It seems reasonable to suppose that the network originally evolved to mediate crawling (and withdrawal) to a wide range of stimulus intensities, with its rhythm-generating ability added later. This hypothesis is supported by the fact that DSI homologs are present in opisthobranch species that do not swim (Katz et al., 2001
The neural mechanisms by which this multifunctional network abruptly reconfigures into its swim mode are emerging (see below; Getting and Dekin, 1985a
Neuromodulation in the network
The role of the DSIs in network function is multifaceted. In addition to their conventional excitatory synaptic connections in the swim-crawling circuitry, these serotonergic interneurons produce a potent neuromodulatory enhancement of the excitability and synaptic connections of C2 (Katz et al., 1994
Our results also have relevance for another issue regarding multifunctional networks, the degree to which they can incorporate modulation specific to one behavior without modifying the other behaviors mediated by the same network. As discussed, the persistent enhancement of DSI firing affects both the crawling and swimming functions of the network (its effect on withdrawal has not yet been tested). However, such conjoint effects need not always occur. For example, because C2 and VSI-B are silent during postswim crawling, learning-related changes specific to these neurons could affect subsequent swims without affecting ongoing crawling. Tritonia, because of its well characterized swimming and crawling circuitry, is an attractive model system in which to explore issues concerning the organization and operation of multifunctional networks.
FOOTNOTES Received Aug. 6, 2001; revised Dec. 10, 2001; accepted Dec. 18, 2001.
This research was supported by National Institutes of Health Grant NS36500. We thank Lise Eliot for comments on this manuscript and Friday Harbor Laboratories for use of their facilities during the summer.
Correspondence should be addressed to William N. Frost, Department of Cell Biology and Anatomy, Finch University of Health Sciences, The Chicago Medical School, 3333 Green Bay Road, North Chicago, IL 60064. E-mail: wfrost{at}finchcms.edu.
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