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The Journal of Neuroscience, May 15, 1998, 18(10):3977-3989
Compartmentalization of Information Processing in an Aplysia Feeding Circuit Interneuron through Membrane Properties and Synaptic Interactions
Ray Perrins and Klaudiusz R. Weiss Department of Physiology and Biophysics, Mount Sinai School of Medicine, Mount Sinai Medical Center, New York, New York 10029-6574
ABSTRACT
Top
Abstract
Introduction
We describe a pair of cerebral-to-buccal interneurons, CBI-5/6, which have outputs and inputs in two ganglia. The soma in the cerebral ganglion received synaptic inputs during buccal motor programs (BMPs) and after mechanical stimulation of the lips. During BMPs the soma received antidromic spikes generated in processes in the buccal ganglion. The soma was driven into a plateau potential by each of these inputs, during which it fired orthodromically at 0-5 Hz. The soma had outputs in the cerebral ganglion consisting of electrical coupling to the adjacent CBI-5/6 and to a cerebral-to-pedal neuron (CPN1). The buccal terminals of CBI-5/6 received inputs that generated rhythmic barrages (up to 25 Hz) of antidromic spikes during BMPs. The buccal terminals had chemical and electrical outputs to motor and premotor elements of feeding circuitry. This combination of synaptic interactions and endogenous properties mean that CBI-5/6 can process information in a number of ways. During the barrage of antidromic spikes, high-frequency firing will produce strong inputs to buccal followers and on their arrival at the soma will transfer excitation electrotonically to CPN1. Subthreshold input to the soma will be transferred electrotonically to cerebral followers but will not be relayed to postsynaptic buccal neurons. Plateau potentials after the antidromic spikes or local cerebral inputs will locally excite CPN1 via electrical coupling but will have little influence on buccal events because of the low orthodromic firing rate. Thus, CBI-5/6 may transmit information locally within the cerebral ganglion or more extensively in both buccal and cerebral ganglia simultaneously.
Key words: plateau potential; feeding; mollusk; motor program; central pattern generator; Aplysia
INTRODUCTION
The traditional view of information flow through a neuron comprises input to the soma and dendrites summating to produce all-or-none action potentials that then travel down the axon and result in output through transmitter release at distal terminals. Recently, however, it has become apparent that in several systems the processing of information by neurons is not necessarily strictly limited to a single "input-output" pathway. Distinct anatomical parts of a neuron may differentially integrate and relay information using different mechanisms. Such compartmentalization is important in neuronal circuits because it theoretically allows information flow in different parts of a neuron to be dissociated under some conditions but enables the neuron to act as a single unit under other conditions. In both the stomatogastric nervous system (Hartline and Graubard, 1992
) and Aplysia neurons B31/32 (Hurwitz et al., 1994
In the stomatogastric system there are also examples of neurons with axons or terminals that receive inputs different from those received at the soma. For example, transmission of spikes generated in the soma of motoneuron OD1 (in the esophageal ganglion) can be rhythmically blocked in the commissural ganglion (Nagy et al., 1981
Extending these concepts, we report here that in Aplysia californica interganglionic neurons CBI-5/6 can process information separately in two ganglia. In CBI-5/6 the segregation is more complete than for OD1 and MCN1, because output from the soma of CBI-5/6 in the cerebral ganglion can be controlled independently of output from the terminals in the buccal ganglion. The soma and terminals can also act as a single unit under other circumstance. Because different ganglia often subserve specialized functions, this type of organization may be advantageous for controlling distinct but related components of a behavior. An important feature of the functional separation within CBI-5/6 is the demonstration of how plateau potentials in the soma of a neuron can be almost completely dissociated from spiking in the axon.
In this paper we present evidence that the CBI-5/6 are part of the consumatory feeding circuit of Aplysia. We then describe a number of specific characteristics of these neurons (including the ability to generate plateau potentials, to initiate action potentials in two ganglia, and to use both chemical and electrical transmission) that combine to create a functional separation of anatomically distinct parts of CBI-5/6, endowing them with the ability to segregate their inputs and outputs, both spatially and temporally.
MATERIALS AND METHODS
Experiments were performed on Aplysia californica weighing 100-300 gm. Animals were anesthetized by injection of isotonic MgCl2 (50% of body weight) into the body cavity. The cerebral ganglion was dissected out in isolation for some experiments and removed with the buccal ganglion attached for others (see Results for details). The ganglia were pinned onto a Sylgard-coated dish at room temperature in artificial seawater (ASW). Cerebral ganglia were pinned ventral surface up, and buccal ganglia were pinned rostral surface up. The connective tissue overlying the uppermost surface of each ganglia was surgically removed. The cerebral-to-pedal connective was rotated through 180° and repinned to allow access to the lateral area of the E-cluster. Simultaneous intracellular recordings were made from up to four neurons using single- or double-barreled microelectrodes filled with 2 M potassium acetate and beveled to a resistance ranging from 5 to 10 M
, depending on the size of the cell to be penetrated. In preparations in which the buccal ganglion was attached, buccal motor output was monitored using a polyethylene suction electrode placed over buccal nerve 2 (Morton and Chiel, 1993
To help identify previously described cells and to reveal the morphology of new ones, microelectrodes, beveled to a resistance of 10-15 M
To determine the response of CBI-5/6 to feeding-related stimuli, experiments were performed on preparations in which the cerebral ganglion was removed with the lips and anterior tentacles still attached by their peripheral nerves. The ganglion was pinned on an elevated Sylgard platform, ventral surface uppermost, and desheathed as described above. The head structures were pinned, ventral surface uppermost, to the bottom of the Sylgard-coated dish in such a way as to reveal the inner portions of the lips and perioral zone (Rosen et al., 1982
Salines, all at pH 7.6, were composed as follows: ASW (in mM): 460 NaCl, 10 KCl, 11 CaCl2, 55 MgCl2, and 5 NaHCO3; high-divalent saline (3× Mg2+ and 3× Ca2+): 460 NaCl, 10 KCl, 33 CaCl2, 165 MgCl2, and 5 NaHCO3; Ca2+-free saline: 460 NaCl, 10 KCl, 11 CaCl2, 66 MgCl2, 5 NaHCO3, and 1 EGTA; and Na+-free saline: 460 N-methyl-D-glucamine, 10 KCl, 11 CaCl2, 55 MgCl2, and 5 NaHCO3. In some experiments (see Results for details) 11 mM Co2+ was added to Ca2+-free saline. Experiments were performed at least six times, unless otherwise stated. Figures quoted are mean ± SEM.
RESULTS
Morphology and electrophysiological properties of CBI-5/6
CBI-5/6 are a pair of cerebral neurons that are indistinguishable in both morphology and physiology. Injections of 5(6)-carboxyfluorescein into the soma revealed CBI-5/6 as a pair of oval neurons ~25-40 µm in diameter adjacent to each other in the E-cluster (Jahan-Parwar and Fredman, 1979
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Figure 1. Morphological and electrical properties of CBI-5/6. A, Drawing of the right cerebral hemiganglion, showing the position of both right CBI-5/6 somata in the E-cluster and axons in the CBC. B, Higher-magnification drawing of the soma of a single CBI-5/6 filled by intracellular injection of 5(6)-carboxyfluorescein, illustrating the oval shape of the cell body and short dendrites. C, Drawing of the buccal processes of CBI-5/6, showing the axon arriving from the CBC, crossing the buccal commissure, and terminating in the contralateral hemiganglion. There were short processes in both buccal hemiganglia. D, Each ipsilateral CBI-5/6 was electrically coupled to the other. Negative current injected into either cell (solid bars) produced a smaller hyperpolarization in the other. E, A brief depolarizing current pulse (bottom trace) into one CBI-5/6 (middle trace) resulted in depolarization and firing in both ipsilateral CBI-5/6s, followed by a plateau potential in both cells. During the plateau potential, the membrane potential remained constant and both cells fired at low frequency (~2.5 Hz). The plateau in both cells was terminated by a hyperpolarizing current pulse in one CBI-5/6. ULAB, Upper labial nerve; AT, anterior tentacular nerve; LLAB, lower labial nerve; CBC, cerebral-to-buccal connective; CPC, cerebral-to-pedal connective; CPlC, cerebral-to-pleural connective; bn, buccal nerve.
CBI-5/6 had quite distinct electrophysiological properties from neighboring E-cluster neurons. The mean resting potential was
57.3 ± 4.1 mV (n = 13). The two ipsilateral CBI-5/6s were electrically coupled to each other so that either positive or negative current injected into one cell resulted in a smaller membrane potential change of the same polarity, but reduced magnitude, in the other (Fig. 1D). Coupling ratios (membrane potential change in the postsynaptic cell divided by membrane potential change in the other) were 0.15:0.25. CBI-5/6 also possessed the ability to generate plateau potentials (Fig. 1E). CBI-5/6 could be driven into a plateau potential after various stimuli. Most simply, a brief depolarizing current pulse injected into CBI-5/6 could lead to a sustained depolarization that was usually accompanied by the firing of action potentials. These were true plateau potentials, rather than long afterdepolarizations, according to the criteria of Hartline and Graubard (1992)
The generation of a plateau potential (current threshold for plateau potentials was 0.82 ± 0.19 nA) in one CBI-5/6 resulted in a similar plateau potential in the other (Fig. 1E), presumably attributed to strong electrical coupling. Likewise, when the plateau potential was terminated in one CBI-5/6, the other also reverted to the resting state. However, in most experiments spikes were not synchronous in each cell, either during positive current injection or during the plateau potential. Instead spikes in one cell were reflected by brief spike-like depolarizations in the other. The amplitude of the true action potentials in CBI-5/6 was quite small (5-20 mV; Figs. 1E, 2) and may be caused by an inexcitable soma, a feature seen in another pair of plateau-generating neurons in Aplysia, B31/B32 (Hurwitz et al., 1994
Mechanism of plateau potential generation
Plateau potentials are often the result of the activation of a slow, voltage-sensitive inward current, so we investigated the ionic requirements for the maintenance of the plateau in CBI-5/6. When the ASW bathing the cerebral ganglion was replaced with a solution containing 0 Na+, the plateau potentials could no longer be generated (Fig. 2A). Indeed no regenerative membrane properties were observed under these conditions, despite using a range of current pulse amplitudes and durations from a variety of initial membrane potentials. However, the plateau potential was not affected when the ASW was replaced with a solution containing nominally 0 Ca2+ and 1 mM EGTA (Fig. 2B). In solutions containing zero Ca2+ and 11 mM Co2+ (a potent Ca2+ channel blocker) the plateau potential was reduced in both duration and amplitude (Fig. 2B). Assuming that Co2+ does not have nonspecific effects on Na+ channels, these results indicate that the current responsible for maintaining the plateau potential is carried predominantly by Na+, although some Ca2+ entry may be required to generate the full plateau potential. The plateau potential was also not affected by bathing the ganglion in ASW containing 100 µM TTX (Fig. 1C), a concentration that abolished fast action potentials in CBI-5/6 as well as the full-sized spikes in neighboring neurons. Because the plateau potential is still present in solutions with TTX or zero Ca2+, this suggests it is an endogenous property of CBI-5/6 and does not require transmitter release from other neurons.
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Figure 2. The current responsible for the plateau potential in CBI-5/6 was carried mainly by Na+. A, In normal ASW a plateau potential was generated by a brief depolarizing current pulse and terminated by hyperpolarization. The ability to generate plateau potentials was abolished in a solution with 0 mM Na+, despite using several different amplitudes of current pulse from three different starting membrane potentials. The plateau potential returned in wash. B, The plateau potential was unaffected in a solution containing 0 mM Ca2+ and 1 mM EGTA but was reduced in amplitude and duration by 0 mM Ca2+ and 10 mM Co2+ and returned to normal during wash. C, TTX (100 µM) abolished spiking in CBI-5/6 but had no effect on the plateau potential. Some action potentials return during wash. The scale is the same in all sections.
Local cerebral interactions of CBI-5/6
To better characterize CBI-5/6, we investigated the connections it makes within the Aplysia feeding system, both with individual neurons and with networks responsible for generating feeding-related motor programs. In this section we will describe interactions with neurons in the cerebral ganglion, in which the soma of CBI-5/6 is located. In the following section we will detail connections with neurons and circuitry in the buccal ganglion, in which CBI-5/6 has numerous distal processes.
Electrical coupling
As well as being coupled to each other, each CBI-5/6 was strongly electrically coupled to a neighboring E-cluster cell (coupling ratio, 0.25:0.40; Fig. 3B). Injections of 5(6)-carboxyfluorescein revealed a cell body approximately the same size as CBI-5/6 and in a similar location. However, this neuron had an axon projecting to the cerebral-to-pedal connective rather than the CBC and had extensive dendritic branching in both the E- and M-clusters (Fig. 3A). Until more formal nomenclature exists, we will refer to this neuron as cerebral-pedal neuron (CPN1). During plateau potentials in CBI-5/6, CPN1 was driven above threshold by the electrotonic transfer of excitation (Fig. 3C). When neurons are electrically coupled in this way, it is difficult to determine which neurons actually have the potential to generate plateau potentials, and which are passive followers. We found that from rest, a brief positive current could produce characteristic regenerative responses in CBI-5/6, regardless of the membrane potential of CPN1 (Fig. 4A). However, if CBI-5/6 was hyperpolarized, current injected into CPN1 no longer possessed any regenerative properties (Fig. 4B). From this we conclude that the CBI-5/6 neurons possess the currents responsible for generating plateau potentials, whereas CPN1 passively follows these responses because of the tight electrical coupling.
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Figure 3. CBI-5/6 was strongly electrically coupled to a neighboring cerebral-to-pedal neuron (CPN1). A, Morphology of CPN1, which had extensive branches in the cerebral ganglion, and an axon leaving via the CPC. B, Negative current (solid bars) injected into each of the CBI-5/6s or CPN1 produced a smaller hyperpolarization in the other two cells. C, Driving a plateau by current injection into CBI-5/6 depolarized CPN1 above firing threshold.
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Figure 4. CBI-5/6, but not CPN1, had regenerative membrane properties. A, Positive current pulses injected into CPN1 depolarized both CPN1 and CBI-5/6 with indications in both of regenerative membrane properties. CBI-5/6 was then hyperpolarized, and CPN1 brought back to the resting potential. Current injected into CPN1 now produced a passive depolarization in both neurons. B, Brief positive current injected into CBI-5/6 depolarized both CPN1 and CBI-5/6 with indications in both of regenerative membrane properties. CPN1 was then hyperpolarized, and CBI-5/6 brought back to the resting potential. The depolarizations in both neurons during current injection still had regenerative characteristics.
Input from the lips
To investigate the types of feeding-related stimuli to which CBI-5/6 respond, we recorded from these neurons in a preparation consisting of the cerebral ganglion with the head and lips attached via the anterior tentacular and lower and upper labial nerves (Rosen et al., 1991bC2 is a cerebral mechanoafferent for the inner lips and makes widespread connections with cerebral feeding circuitry (Chiel et al., 1986
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Figure 5. Inputs from the lips to CBI-5/6. A, Lip mechanoafferent C2 produced a biphasic excitation of CBI-5/6, which was not blocked in a high-divalent solution. B, Longer stimulation of C2 drove CBI-5/6 into a plateau potential (terminated by a hyperpolarizing current pulse indicated by the bar). C, In a preparation of the head and cerebral ganglion, chemical stimuli (seaweed extract) applied to the lips strongly excited CBI-2 but had little effect on CBI-5/6. D, A brief mechanical stimulus to the lips briefly depolarized CBI-2 and drove CBI-5/6 into a plateau (terminated by a negative current pulse indicated by the solid bar).
Input during the cerebral motor program
It has recently been shown that excitation of neuron C15 can activate a central pattern generator (CPG) in the isolated cerebral ganglion (Perrins and Weiss, 1996
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Figure 6. Input to CBI-5/6 during the CMP. A, The CMP was driven by injecting tonic depolarizing current into C15 (solid bar). The input to CBI-5/6 consisted of barrages of fast PSPs that were one-for-one with the fast IPSPs in lip motoneuron C12 (time-expanded bottom trace). B, A brief depolarizing current pulse in CBI-5/6 gave rise to a plateau potential that spontaneously terminated after 54 sec, and the next two plateau potentials terminated early (after 13-14 sec), after PSPs received during one cycle of the CMP driven by depolarization of C15 (shown by bar). A forth plateau terminated spontaneously after 62 sec. Records are consecutive. C, An example in which the plateau potential in CBI-5/6 could be both terminated and terminated by E/IPSPs during the CMP. A first cycle of the CMP produced by current in C15 (first bar) resulted in depolarizing E/IPSPs in CBI-5/6 that drove it into a plateau. A second cycle (second bar) terminated the plateau. The faster time base records to the right show that the E/IPSPs (the first three PSPs of each CMP cycle are indicated by the arrowheads) were depolarizing from rest (
Connections of CBI-5/6 with buccal feeding circuitry
We investigated the presynaptic and postsynaptic connections of CBI-5/6 with a number of buccal neurons involved in feeding behaviors. Firing in the buccal-to-cerebral interneurons (BCIs) (Rosen et al., 1990
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Figure 7. A, Spikes in buccal-to-cerebral interneuron B19 produced fast one-for-one EPSPs in CBI-5/6. At 37 Hz, the EPSPs summate sufficiently to drive CBI-5/6 into a sustained plateau potential (terminated by a hyperpolarizing current pulse indicated by the bar). Note that CBI-5/6 did not fire during the plateau. B, Spikes in buccal-to-cerebral interneuron B18 produced fast EPSPs in CBI-5/6 that could also drive it into the plateau (data not shown).
Firing in CBI-5/6 produced by current injection at the soma resulted in PSPs in a variety of buccal neurons (Fig. 8; see Fig. 12). Fast EPSPs were observed in the putative pattern generator neuron B64 (Hurwitz and Susswein, 1996
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Figure 8. CBI-5/6 makes synapses onto buccal motor and premotor neurons involved in feeding-related motor programs. A, Spikes in CBI-5/6 were followed one-for-one by fast EPSPs in premotor neurons B4 and B64. B, A hyperpolarizing current pulse injected into B4 resulted in hyperpolarization of CBI-5/6. This electrical coupling was probably strong in the buccal ganglion, but the signal was weakened while traveling along the axon of CBI-5/6 from buccal to cerebral ganglia. C, Spiking in CBI-5/6 produced fast IPSPs in an unidentified buccal motoneuron (bMN). D, Spiking in CBI-5/6 produced fast EPSPs in B19. E, Spiking in CBI-5/6 produced fast EPSPs in buccal motoneuron B15. For D and E note that the regularly occurring IPSPs in B19 and B15 were briefly eliminated by firing in CBI-5/6. For all records CBI-5/6 was held hyperpolarized from rest to prevent the activation of a plateau potential after current injection. Note for records in C-E that it is difficult to judge whether the PSPs are one-for-one with spikes in CBI-5/6 because of multiple spike-like events caused by electrical coupling to other neurons. Scale bars: CBI-5/6 in A, C-E, B4 in B, 40 mV; all buccal neurons in A, C, D, CBI-5/6 in B, 10 mV.
At the motoneuron level orthodromic firing in CBI-5/6 produced fast EPSPs and IPSPs in several neurons in the ventral motoneuron cluster of the buccal ganglion. Figure 8C shows examples of IPSPs in an unidentified motoneuron and EPSPs received by B15. The fast PSPs observed in buccal neurons could occasionally be seen to be one-for-one with spikes in CBI-5/6 (Fig. 8A), although more often this was difficult to determine because of the multiple spike-like potentials resulting from the electrotonic transfer of spikes in the neighboring CBI-5/6 and CPN1 (Fig. 8C-E).
Activity of CBI-5/6 during BMPs
Because CBI-5/6 made connections with elements of buccal and cerebral feeding circuitry, we investigated the activity of CBI-5/6 during two distinct evoked BMPs to discover at what phase during feeding these synapses may be active. An ingestive-like BMP was driven by intracellular excitation of CBI-2 (Rosen et al., 1991b
Phase 1
During the phase associated with protraction of the radula in both BMPs CBI-5/6 received a barrage of PSPs. These increased in amplitude when CBI-5/6 was hyperpolarized (Fig. 9). As with the PSPs recorded during the CMP, these PSPs were depolarizing from rest but hyperpolarizing from the plateau (Fig. 9) and are thus E/IPSPs. The summation of these E/IPSPs was decreased by hyperpolarization attributed to inward rectification in CBI-5/6 that reduced EPSP fall time. The E/IPSPs were chemical in nature, because they were blocked when a solution containing zero Ca2+ and 10 mM Co2+ was applied to the cerebral ganglion (Fig. 10).
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Figure 9. Input onto CBI-5/6, recorded from the soma, during an ingestive-like BMP. A, Three cycles of a BMP were driven by injecting constant current into CBI-2 (bar). This incorporated rhythmic firing in buccal neurons B4 and B8. CBI-5/6 received input during the BMP that could be divided into three phases (labeled 1-3). Phase 1 coincided with the buildup of excitation in B8. Phase 2 took place during firing in B4, and phase 3 coincided with a period of little activity in either neuron. CBI-5/6 remained in the plateau of the final phase 3 for 30 sec after the BMP stopped. B, With CBI-5/6 hyperpolarized by 50 mV, a BMP could still be driven by CBI-2. Each phase of input to CBI-5/6 was altered in a characteristic way by hyperpolarization. The potentials in phase 1 were increased in amplitude, whereas those in phase 2 were reduced in amplitude. No activity or input could be seen in CBI-5/6 during phase 3. The activity of CBI-5/6 in each phase is seen best in the bottom time-expanded record in C. Dashed lines in C represent the membrane potential before the start of the BMP.
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Figure 10. Effects of blocking chemical transmission in the cerebral ganglion on the input to the soma of CBI-5/6. A, Three cycles of an egestive-like BMP were driven by repetitive electrical stimulation of the esophageal nerve (at 2.5 Hz; open bar). This BMP incorporated firing in B8 and B4. As with the ingestive-like BMP, three phases in input to CBI-5/6 can be distinguished, with phase 2 coinciding with firing in B4. Phase 2 in CBI-5/6 from the third cycle is shown at a faster time base in the lowest trace, as it also is for B and C. B, The cerebral ganglion was bathed in a solution containing 0 mM Ca2+ and 11 mM Co2+ to block chemical transmission. Because transmission in the buccal ganglion was unaffected, the BMP could still be driven by esophageal nerve stimulation, and a similar pattern of firing to control occurred in B8 and B4. In CBI-5/6, however, the potentials of phase 1 and the firing during phase 3 were completely blocked. The barrage of fast-depolarizing potentials during phase 2 remained largely unaffected, although they appear to be more regular than in control, indicating that some chemical input may have been blocked. The remaining potentials probably represent A-spikes originating in the buccal ganglion (see Results for details). C, When CBI-5/6 was hyperpolarized by 33 mV, there was still no observable input during phases 1 and 3, and the potentials of phase 2 were reduced in amplitude, although their frequency was not affected. D, All three phases of input to CBI-5/6 were clearly seen again during wash.
Phase 2
During the phase associated with radula retraction, the soma of CBI-5/6 received a series of potentials that had a similar appearance to chemical PSPs. However, unlike the E/IPSPs, these potentials were reduced in amplitude when the soma of CBI-5/6 was hyperpolarized (Figs. 9, 10). Additionally, when a solution with zero Ca2+ and 10 mM Co2+ was applied to the cerebral ganglion, this second phase remained (Fig. 10), indicating that the potentials were not due to transmitter release in the cerebral ganglion. In zero Ca2+ and 10 mM Co2+ these potentials were again reduced by hyperpolarization of CBI-5/6. These results suggest that phase 2 consists of a barrage of axon spikes (A-spikes) arriving antidromically from the distal processes in the buccal ganglion. Similar potentials could be obtained using electrical stimulation of the CBCs, which were also reduced by hyperpolarization (Fig. 11A) and not blocked in zero Ca2+ and 10 mM Co2+. Although the amplitude of the potentials during phase 2 could be reduced by hyperpolarization, their frequency was not altered (maximum of 20-25 Hz; Fig. 11B1,B2). This was probably because the buccal spike initiation site was too distant to be affected by current injected into the soma. We attempted to use en passant suction electrode on the CBC to identify one-for-one extracellular spikes with the potentials of phase 2. Although we could identify orthodromic spikes after current injected into the cell body of CBI-5/6, there was too much activity in the CBC (from BCIs and other CBIs) during BMPs to distinguish antidromic spikes extracellularly during phase 2.
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Figure 11. The characteristics of A-spikes in CBI-5/6 in response to electrical stimulation of the cerebral-to-buccal connective (CBC). A, The CBC was stimulated at 0.5 Hz (a small stimulus artifact can be seen as a downward deflection in the CBI-5/6 trace), producing A-spikes in CBI-5/6. Hyperpolarization of CBI-5/6 (bar) resulted in a dramatic reduction in the amplitude of these A-spikes. Chemical EPSPs generally get larger on hyperpolarization, as they are taken farther from their reversal potential. B1, A train of stimuli to the CBC (at 5 Hz) led to summation of the A-spikes. The resulting depolarization was sufficient to drive CBI-5/6 into a plateau potential after termination of stimulation. B2, The transition from phase 2 to phase 3 from a CBI-2-induced BMP in a different preparation is shown at the same scale for comparison with B1. The potentials of phase 2 resemble the A-spikes, whereas phase 3 has a similar amplitude and firing frequency to the plateau potential.
Phase 3
During this phase most other neurons recorded were silent, and this probably represents the pause between each cycle of activity. In 3 of 15 preparations the membrane potential of CBI-5/6 returned to the resting potential, and no obvious inputs were observed. In the remaining cases a plateau potential was generated during phase 3. The level of depolarization and firing rate of CBI-5/6 during phase 3 was similar to that recorded during current-evoked plateau potentials (Fig. 11B1 and B2). Constant hyperpolarizing current injected into CBI-5/6 resulted in complete blockage of the plateau potential during phase 3. Under these conditions no synaptic inputs were observed during this phase, suggesting that the plateau potential is a result of intrinsic cellular properties after the A-spikes.
DISCUSSION
Is CBI-5/6 part of the feeding rhythm generating circuitry?
We have three strong lines of evidence that activity in CBI-5/6 is important during feeding-related motor programs: (1) CBI-5/6 is excited by feeding-related stimuli; (2) CBI-5/6 synapses onto buccal motor and premotor circuitry; and (3) CBI-5/6 is phasically active during BMPs.
CBI-5/6 produces EPSPs in B64, B4, B15, and B19, and it spikes antidromically at high frequencies in phase with the peak excitation in these neurons during BMPs. It therefore seems likely that spiking in the buccal processes of CBI-5/6 contributes to the excitation in these buccal neurons during BMPs.
Although antidromic firing rates of up to 25 Hz (Fig. 11) were recorded during feeding-like BMPs, depolarizing current injections at the soma failed to elicit firing at >10 Hz (Fig. 8A). In addition, strong hyperpolarization of the soma had little effect on antidromic spike frequency, despite the dramatic reduction in spike amplitude (Figs. 9, 10). This is presumably because of the distance between the spike-initiating zones and the site of current injection. Although such features serve to emphasize the compartmentalized nature of this neuron, it limited the range of firing frequencies open to experimental manipulation from recordings at the soma. Therefore, although we found no effects of current-induced firing or hyperpolarization of CBI-5/6 on overall buccal motor output (either in the quiescent state or during ongoing BMPs), this does not rule out profound influences of CBI-5/6 on buccal circuitry at the natural firing frequencies observed during BMPs, especially during phase 2 (up to 25 Hz). Interestingly, the intrinsic properties of CBI-5/6 are quite distinct from those of other CBIs. Indeed, they have more in common (plateau potentials, electrically coupled followers, and nonovershooting spikes observed in the soma) with neurons thought to be involved in the buccal CPG of Aplysia, such as B31/B32 (Susswein and Byrne, 1988
Spike initiation in CBI-5/6
The orthodromic spikes in CBI-5/6 recorded from the soma were quite small, perhaps caused by a cerebral spike initiation zone of CBI-5/6 at a relatively large distance from the soma, which itself is inexcitable. Why is this the case, when the majority of Aplysia neurons have active somata? If the main role of the plateau potential is to produce an even depolarization in CPN1 and other electrically coupled neurons, then the electrotonic transfer of full soma spikes in CBI-5/6 would disrupt this (B31/B32; Hurwitz et al., 1994
The antidromic spikes observed during phase 2 of BMPs indicate that there is also a spike initiation zone even farther from the soma, probably in the distal processes of CBI-5/6 in the buccal ganglion. The axon of CBI-5/6 thus conveys spikes in both directions during BMPs. We have called these orthodromic and antidromic, because the only possible terms, somatopetal and somatofugal (Nagy et al., 1981
Compartmentalization of information processing in CBI-5/6
The combination of inputs, outputs, and intrinsic properties of CBI-5/6 leads to a number of possible modes of information flow, summarized in Figure 12.
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Figure 12. Summary of the cerebral and buccal connections of CBI-5/6. A, In the cerebral ganglion the soma of CBI-5/6 is electrically coupled to CPN1 and receives input from the cerebral CPG and from mechanical stimulation of the lips. This is likely to be in part mediated via excitation of mechanoafferent C2. The soma of CBI-5/6 is also excited by BCIs such as B19. In the buccal ganglion the distal processes of CBI-5/6 make chemical and electrical connections onto a variety of motor and premotor neurons of the feeding circuitry. The buccal processes are also excited either chemically or electrically from an unidentified source (?) to drive the antidromic spikes of phase 2 during BMPs. B-D, Different form of information flow through CBI-5/6 B, CBI-5/6 can process information through its soma yet have minimal influence on buccal events. This occurs whenever the soma is excited by cerebral inputs: during phase 1 of BMPs, in response to lip stimulation, and during the CMP. C, Input to the buccal processes generates high-frequency antidromic spiking that results in strong output in both buccal and cerebral ganglia (see Discussion for details). This occurs during phase 2 of BMPs. D, Once in the plateau potential (during phase 3 or in response to other sources of excitation to the soma), output from CBI-5/6 locally will be sustained without any inputs. Output in the buccal ganglion will again be low because of the low orthodromic firing rate.
(1) Under some conditions information flow can be largely restricted to the cerebral ganglion (Fig. 12C). Mechanical stimulation of the lips excites CBI-5/6, probably partially mediated by firing in C2, which is a mechanosensory neuron for the inner lips (Weiss et al., 1986
(2) During phase 2 of BMPs, CBI-5/6 receives input at its distal processes, resulting in high-frequency antidromic spiking (Fig. 12B). These processes in turn make chemical and electrical outputs onto buccal neurons. The antidromic spikes then arrive at, and depolarize, the soma of CBI-5/6. CBI-5/6 will therefore also make outputs in the cerebral ganglion, onto electrically coupled followers such as CPN1 (which may then transfer information to the pedal ganglion). In these circumstances, CBI-5/6 acts as a single unit, relaying information between ganglia, although interestingly the direction of spike propagation is opposite that conventionally observed in other neurons. A further possibility is that if the terminals of CBI-5/6 in the buccal ganglion are the subject of presynaptic inhibition similar to that seen in MCN1, then excitatory input to the buccal processes could lead to output from the soma only.
(3) During a plateau potential, CBI-5/6 will act as a sustained local source of output excitation to cerebral followers through the electrotonic transfer of the depolarization, without the need for further inputs either to the buccal processes or the cerebral soma (Fig. 12D). The output to buccal neurons will be minimal, because the orthodromic spiking frequency is low. Plateau potentials follow the antidromic spikes of phase 2 during BMPs. The rapid summation of A-spikes in the soma of CBI-5/6 (Fig. 11B1) means that the generation of the plateau potential of phase 3 will be relatively independent of the firing frequency in the buccal processes during phase 2 (yet another way in which events in the two ganglia can be separated). Plateau potentials also follow the excitation in response to brief mechanical stimulation of the inner lips, as well as inputs from specific presynaptic neurons such as C2 and B19.
General relevance of the properties of CBI-5/6
Plateau potentials are often thought of as providing a means of maintaining activity in a neuron after a brief stimulus or as a simple "switch" between two firing rates. This role is fulfilled by CBI-5/6, for example, during phase 3 of BMPs or after lip stimulation. However, this study has revealed another function for plateau potentials, in the compartmentalization of neuronal function. As long as the spike initiation zone is distant, a plateau in the soma can locally excite followers through electrical coupling while resulting in few, if any, axonal spikes. In the same neuron, spikes generated in processes in a different ganglion can be used to fulfill a quite separate role. Despite this, it is still possible to use a neuron with this combination of properties as a single unit, obviating the need for additional interneurons.
MCN1 receives input in both the commissural and stomatogastric ganglia, and the only known outputs are in the stomatogastric ganglion (Coleman and Nusbaum, 1994
FOOTNOTES Received Nov. 13, 1997; revised March 3, 1998; accepted March 6, 1998.
This work was supported by the Human Frontiers Science Program Grant LT-561/95 and National Institutes of Health Grants GM 32009 and MH 50235. We thank Dr. Paul Church for extremely valuable comments on this manuscript.
Correspondence should be addressed to Klaudiusz R. Weiss, Department of Physiology and Biophysics, Mount Sinai School of Medicine, Mount Sinai Medical Center, One Gustave L. Levy Place, New York, NY 10029-6574.
Dr. Perrins's present address: School of Biological Sciences, University of Bristol, Woodland Road, Bristol, BS8 1UG, United Kingdom.
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