Interneuronal Projections to Identified Cilia-Activating Pedal Neurons in Hermissenda

doi:10.1152/jn.01047.2002

Interneuronal Projections to Identified Cilia-Activating Pedal Neurons in Hermissenda

Terry Crow and Lian-Ming Tian

Department of Neurobiology and Anatomy, University of Texas Medical School, Houston, Texas 77030

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Crow, Terry and Lian-Ming Tian. Interneuronal Projections to Identified Cilia-Activating Pedal Neurons in Hermissenda. J. Neurophysiol. 89: 2420-2429, 2003. Neural networks have been shown to support the generation of more than one behavioral motor act. In the nudibranch molluskHermissenda, Pavlovian conditioning results in light, the conditionedstimulus (CS), evoking both inhibition of locomotion and footcontraction. The synaptic organization of the eyes and optic ganglionis well documented; however, the characterization of the neuralnetwork mediating visually modulated behaviors is incomplete.We have now characterized synaptic connections between identifiedphotoreceptors and a newly identified interneuron (II_b), identifiedsynaptic projections from type I and type II interneurons to aninhibitory interneuron (III_i) and to two newly identified pedalneurons, VP1 and VP2. Here we show that VP1 activates ciliarymovement on the anterior foot and VP2 innervates the anteriorfoot and ventral tentacle. Stimulation of the photoreceptors withlight produced two effects on the activity of VP1 and VP2. First,light inhibits type I_i and II_i interneurons and disinhibits VP1and VP2. Depolarization of type II_e interneurons also disinhibitsVP1 and VP2. Second, the light-elicited depolarization and increasedtonic activity of VP1 and VP2 is produced by excitatory synapticinput from ipsilateral and contralateral type II_b interneurons.Pedal neurons VP1 and VP2 receive similar synaptic input fromtype I, II, and III_i interneurons; this is in agreement with previousresearch showing that the visual pathway influences both ciliarylocomotion and foot movement. The organization of the visual systemin Hermissenda provides for the expression of cellular and synapticplasticity supporting learning without altering the networks abilityto carry out the requirements for normal visualprocessing.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

A general conclusion derived from studies of motor systems is that the expression of diverse motor acts may be supported bythe same neural circuit (for reviews, see Getting 1989; Kupfermannand Weiss 2001; Marder and Calabrese 1996; Pearson 1993). In someexamples from invertebrates, multiple behaviors supported by thesame neural circuit appear to be quite different. For example,in Tritonia, activation of the swim central pattern generator(CPG) contributes to both escape swimming and ciliary locomotion(Audesirk 1978a; Popescu and Frost 2002). The serotonergic As1-4neurons in the swim network of Pleurobranchaea also excite pedalG neurons supporting ciliary locomotion (Jing and Gillette 2000).Escape swimming is muscular and rhythmic in contrast to ciliarymovement, which is a nonmuscular and nonrhythmic gliding formof locomotion in mollusks (for discussion, see Copeland 1919,1922; Gainey 1976). In addition to the requirement for selectivityof different motor programs from the same network, both modifiedand unmodified behaviors must also be expressed in examples wherelearning alters the activity of a neural circuit supporting differentbehaviors. As an example in Hermissenda, Pavlovian conditioningresults in conditioned stimulus (CS)-elicited inhibition of locomotion(Crow and Alkon 1978, 1980) and CS-elicited foot contraction (Lederhendleret al. 1986). However, these two apparent dissimilar motor actsare not incompatible, and coactivation may help to explain thebehavioral consequences of CS presentation in conditionedanimals.

The synaptic organization of primary and secondary components of the visual system of Hermissenda has been characterized anddescribed in considerable detail (Akaike and Alkon 1980; Alkon1973a,b; Alkon and Fuortes 1972; Alkon et al. 1978; Crow and Tian2000, 2002a; Crow et al. 1979). However, the neural network supportingthe generation of visually modulated behaviors such as ciliarylocomotion and foot contraction has not been identified. In thisreport, we have identified and characterized two pedal neuronswith different behavioral functions. Pedal neuron VP1 activatescilia on the anterior foot, and pedal neuron VP2 innervates theanterior foot and ventral tentacle. Axonal processes of pedalneurons VP1 and VP2 in pedal nerve P2 were verified by elicitingorthodromic spikes and recording concomitant extracellular spikesin P2 and recording antidromic spikes in VP1 and VP2 elicitedby stimulation of nerve P2. We characterized synaptic connectionsbetween type I, II, and III interneurons and recently identifiedpedal neurons VP1 and VP2. Here we show that pedal neurons VP1and VP2 receive visual input from a polysynaptic pathway consistingof identified photoreceptors, type I_i, II_i, I_e, and II_e interneurons,and recently identified type II_b and III_i interneurons. Inhibitoryand excitatory synaptic input from type I and II interneuronswere found to project to both VP1 and VP2. Activation of the visualpathway with light results in an increase in the tonic activityof both VP1 and VP2 produced by a combination of disinhibitionmediated by type III_i interneurons and excitatory synaptic inputfrom type II_b interneurons. The organization of polysensory interneuronalsynaptic projections to neurons in the motor network controllingciliary locomotion and foot movement may explain how cellularand synaptic modifications associated with Pavlovian conditioningcan co-exist with the requirement for normal visual processingexpressed by thenetwork.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Adult Hermissenda crassicornis were used in the experiments. The animals were obtained from Sea Life Supply, Sand City, CA,and maintained in closed artificial seawater aquaria at 14 ± 1°Con a 12-h light-dark cycle. All electrophysiological procedureswere conducted during the light phase of the light/darkcycle.

Simultaneous intracellular recordings from identified type B photoreceptors, interneurons, and/or pedal neurons were collectedfrom isolated nervous systems. Extracellular recordings were obtainedfrom suction electrodes containing pedal nerve P2. Anatomicaland electrophysiological criteria were used to identify type-Bphotoreceptors within the eyes as described previously (Alkonand Fuortes 1972; Crow and Tian 2000; Frysztak and Crow 1994).The isolated nervous systems were incubated in a protease solution(Sigma Type VIII; 0.67 mg/ml, 5 min) to facilitate microelectrodepenetration of photoreceptors. Surgical desheathing of a smallarea of the cerebropleural and pedal ganglion was conducted toexpose the cell bodies of interneurons and pedal neurons. As previouslyreported (Crow and Tian 2000), the criteria for identifying interneuronsconsisted of soma size, cell layer, location in the cerebropleuralganglion, electrophysiological responses to light, and extrinsiccurrent stimulation of photoreceptors. In isolated circumesophagealnervous systems, pedal neurons were identified based on size,position along the anterior-ventral edge of the pedal ganglion,and electrophysiological responses to light and extrinsic currentstimulation of pedal nerves and interneurons. In semi-intact preparations,pedal neurons VP1 and VP2 were identified by depolarization withextrinsic current and simultaneous video recording of ciliarymovement and/or movement of the anterior foot and ventraltentacle.

The partially desheathed circumesophageal nervous systems were pinned to a silicone elastomer (Sylgard; Dow Chemical) stagein a recording chamber filled with artificial seawater (ASW) ofthe following composition (in mM) 460 NaCl, 10 KCl, 10 CaCl₂,and 55 MgCl₂, buffered with 10 mM HEPES and brought to pH 7.46with dilute NaOH. The ASW in the recording chamber was monitoredby a thermistor and held at 15 ± 0.5°C. Illumination of the eyeswas provided by a tungsten halogen incandescent lamp attachedto a fiber optic bundle mounted underneath the recording chamber.Maximum light intensity was attenuated with neutral density filtersexpressed in negative log units. Photoreceptors, interneurons,and pedal neurons were impaled with microelectrodes filled with4 M KAc. Micoelectrodes were connected to the two headstages ofan Axoclamp 2A (Axon Instruments, Foster City, CA). Standard intracellularand extracellular recording and stimulation techniques were employed.Digitized data were analyzed and plotted using Spike 2 software(Cambridge Electronic Design). Single spikes elicited by briefextrinsic current pulses and trains of action potentials elicitedby current steps were applied in the dark through a bridge circuit.Depolarizing generator potentials were evoked by light steps ofvariable duration that followed appropriate periods of dark adaptation.Synaptic connections between photoreceptors, interneurons, andpedal neurons were examined in normal ASW. Evidence for monosynapticconnections between interneurons and pedal neurons was providedby PSPs with relatively short and constant latencies and a one-for-onerelationship between interneuron action potentials and PSPs recordedfrom pedal neurons in normal ASW and in ASW containing high-divalentcations (3× Ca²⁺ and 3× Mg²⁺).

Semi-intact preparations were prepared by cooling the animals to between 0 and 1°C followed by isolation of the circumesophagealnervous system from the buccal crest and body leaving an intactpedal nerve P2. The foot was positioned ventral side up adjacentto the isolated circumesophageal nervous system. The exposed nervoussystem and anterior foot were visualized in infrared illuminationprovided by a 45-W tungsten/halogen light source projected bya light guide through an infrared filter (Schott model RG-850).A dissecting microscope formed an image of the nervous systemin the infrared light on a Dage MTi video camera connected toa video monitor and video recorder. Ciliary movement was assessedindirectly in infrared illumination by video imaging of the movementof small dried ink particles on the anterior region of the footduring depolarization of VP1 with extrinsic current. Ciliary activityevoked by stimulation of VP1 was quantified by measuring particlemovement during the depolarizing current step on a transparencyattached to the video monitor. Movement of the anterior foot wasvideotaped during depolarization of VP2 and quantified by measuringfoot displacement from prestimulus baseline positions on the transparencycovering the video monitor screen. To rule out the possible contributionof indirect activation of other central neurons to ciliary movement,VP1 and VP2 were depolarized and ciliary movement and anteriorfoot displacement videotaped with nervous systems exposed to ASWsolutions containing high divalent cations (3× Ca²⁺ and 3× Mg²⁺).

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

A neural network diagram showing the synaptic connections among photoreceptors, interneurons, and pedal neurons VP1 and VP2is shown in Fig. 1. The network represents previously identifiedand newly identified synaptic connections reported in this paper.

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Fig. 1. Neural network depicting components of the Hermissenda visual pathway. Diagram of synaptic connections between identified photoreceptors, photoreceptors, and interneurons, and interneurons and pedal neurons VP1, VP2, VP3 and VCMN. Photoreceptors are designated as lateral A (LA), medial A (MA), lateral B (LB), central B (CB) and medial B (MB). Previously identified interneurons designated as type I_e, I_i, type II_e, II_i, and newly identified interneurons designated as type II_b, type III_i and ventral pedal neurons (VP1, VP2, VP3, and VCMN). $triangle$ , excitatory synapses; $black-triangle$ , inhibitory synapses. $---$ , established monosynaptic connections; - - -, polysynaptic connections with potential interneurons not yet identified.

P2 nerve recordings: projections of VP1 and VP2

Pedal motor neurons that innervate the foot and contribute to locomotion project to postsynaptic targets through identifiedpedal nerves P1 and P2 (Hodgson and Crow 1991; Richards and Farley1987). Extracellular recordings from pedal nerve P2 in isolatednervous systems revealed several extracellular spikes whose tonicfiring frequency was increased by illumination of the eyes. Previously,backfills of P2 with Ni-Ly labeled a number of candidate pedalmotor neurons (data not shown). Two of the labeled pedal neuronsdesignated VP1 and VP2 were examined in the present experiments.Pedal neuron VP1 receives ipsilateral and contralateral polysynapticinput from photoreceptors. As shown in Fig. 2A1, light produceda depolarization and increased tonic firing of pedal neuron VP1that was associated with an increase in the smaller amplitudeextracellular spike activity recorded from nerve P2 (Fig. 2B1).The increase in extracellularly recorded spikes is reflected byan increase in light-evoked baseline amplitude (B1). On a fastertime scale shown in Fig. 2, A2 and B2, the VP1 spike is associatedone-for-one with an extracellular spike recorded from P2 ( $up-arrow$ ; B2).In addition to light-elicited activity of VP1, the largest amplitudeextracellular spikes recorded from nerve P2 reflect light-elicitedactivity generated in pedal neuron VP2. As shown in Fig. 2C, lightelicited a depolarization and increase in spike activity in pedalneuron VP2 and a concomitant large-amplitude extracellular spikerecorded from pedal nerve P2 ( $up-arrow$ , Fig. 2D). The large-amplitudeextracellular spike followed the action potentials recorded fromVP2 one-for-one (Fig. 2D).

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Fig. 2. Simultaneous recordings from pedal neurons VP1 and VP2 and nerve P2 during illumination of the eyes. Light elicited an increase in tonic firing of VP1 (A1) and a corresponding increase in extracellular spike activity recorded in P2 (B1). The same recording on a faster time scale showed that the action potential recorded in VP1 (A2) is associated with an extracellular spike ( $up-arrow$ ) 1-for-1 in the recording from nerve P2 (B2). The large amplitude extracellular spike in B2 is associated with spike activity in pedal neuron VP1. Action potentials recorded in VP2 (C) are associated 1-for-1 ( $up-arrow$ ) with the large amplitude extracellular spike recorded from verve P2 (D).

Extracellular spike activity recorded in nerve P2 followed VP1 and VP2 spike activity with a brief latency as shown in Fig.3. A current-elicited spike generated in VP1 (Fig. 3A) resultedin a short-latency extracellular spike recorded from nerve P2(Fig. 3B). In the same preparation, stimulation of nerve P2 withextrinsic current elicited a short-latency antidromic spike recordedin VP1 (Fig. 3C). Antidromic spikes exhibited a short and constantlatency after stimulation of nerve P2 as shown by the three superimposedspikes in Fig. 3D. Similar results were obtained from recordingsof pedal neuron VP2 as shown by the examples of orthodromic andantidromic spikes in Fig. 3, E-G. A spike in VP2 elicited by extrinsiccurrent was associated with a brief latency extracellular spikerecorded from nerve P2 (Fig. 3F). A short-latency antidromic spikerecorded in VP2 followed stimulation of nerve P2 (Fig. 3G).

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Fig. 3. Pedal neurons VP1 and VP2 project axonal processes in pedal nerve P2. A single spike elicited by an extrinsic current pulse in VP1 (A) is followed by a brief and constant latency extracellular spike recorded in nerve P2 (B). An antidromic spike recorded in VP1 (C) followed stimulation of nerve P2. Antidromic spikes recorded in VP1 exhibited a brief and constant latency following stimulation of nerve P2 as shown by the 3 superimposed VP1 antidromic spikes in D. A single spike elicited by an extrinsic current pulse in VP2 (E) is followed by a brief and constant latency extracellular spike recorded in nerve P2 (F). Stimulation of nerve P2 elicited an antidromic spike recorded from VP2 (G).

VP1 stimulation activates cilia on the anterior foot and stimulation of VP2 elicits movement of the anterior foot and ventral tentacle in semi-intact preparations

Depolarization of VP1 with a 10-s extrinsic current pulse elicited ciliary movement on the anterior foot in a semi-intactpreparation. Figure 4A shows an example of increased tonic firingof VP1 elicited by extrinsic current and the concomitant movementof small dried ink particles on the anterior foot analyzed fromvideotape data (B). The foot was imaged in infrared illuminationduring activation of VP1 in normal ASW (Fig. 4A) and in a preparationwhose nervous system was exposed to a high-divalent cation ASWsolution (Fig. 4C). The high-divalent cation ASW solution didnot block ciliary activation during depolarization of VP1 (Fig.4D), indicating that VP1 does not indirectly activate cilia throughpolysynaptic connections with central neurons. As shown in Fig.5 depolarization of VP2 in semi-intact preparations produced movementof the anterior foot measured from videotape recordings. Circumesophagealnervous systems exposed to the high-divalent cation ASW solutioncould still express anterior foot movement elicited by depolarizationof VP2 (Fig. 5, B and C), indicating that indirect activationof central neurons was not contributing to anterior foot movementselicited by stimulation of VP2.

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Fig. 4. Depolarization of VP1 evoked activation of cilia on the anterior foot in semi-intact preparations. A: intracellular recording from VP1 during depolarization with a 10-s 0.8-nA extrinsic current pulse. Movement of dried ink particles on the anterior foot in arbitrary units during the 10-s depolarization of VP1 in normal artificial seawater (ASW; B). C: depolarization of VP1 (1 nA) in a circumesophageal nervous system exposed to a high-divalent cation solution (3× Ca²⁺ and 3× Mg²⁺). Movement of dried ink particles on the anterior foot during the 10-s depolarization of VP1 in a high-divalent cation solution (D).

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Fig. 5. Depolarization of VP2 evoked movement of the anterior foot. A: intracellular recording from VP2 in normal ASW during a 10-s depolarization (2 nA). B: depolarization of VP2 (5 nA) in a circumesophageal nervous system exposed to a high-divalent cation solution. C: group data (mean ± SE) of anterior foot movement evoked during the 10-s depolarization in normal ASW and nervous systems exposed to a high-divalent cation solution (n = 4).

Synaptic projections from photoreceptors and interneurons

We next examined synaptic input to VP1 and VP2 from previously identified components of the visual pathway. Evidence showingpolysynaptic input to VP1 from an identified type-B photoreceptoris shown in Fig. 6. Stimulation of a medial type-B photoreceptorwith extrinsic current (Fig. 6A) resulted in an increase in tonicfiring of pedal neuron VP1 (Fig. 6B) and an increase in extracellularspike activity recorded in nerve P2 as indicated by an increasein prestimulus baseline amplitude (Fig. 6C). The increase in thedischarge frequency of the largest amplitude extracellular spikerecorded in nerve P2 suggests that the medial type-B photoreceptoralso projects to both VP1 and VP2 (see preceding text).

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Fig. 6. Identified type B photoreceptors exhibit polysynaptic projections to pedal neuron VP1. Simultaneous recordings from a medial type B photoreceptor, pedal neuron VP1 and pedal nerve P2. A depolarizing extrinsic current step applied to a medial type B photoreceptor (A) elicited an increase in tonic firing of pedal neuron VP1 (B) and an increase in extracellularly recorded spikes of different amplitudes recorded from pedal nerve P2 (C).

We previously showed that identified photoreceptors exhibited monosynaptic projections to two aggregates of interneurons designatedas type I_e and type I_i, and polysynaptic connections to type II_eand type II_i interneurons (Crow and Tian 2000, 2002a). Here weshow that synaptic projections from photoreceptors to pedal neuronsVP1 and VP2 involve previously identified type I and type II interneurons.An example of a light-elicited depolarization and increase intonic spike frequency in an identified type I_e interneuron isshown in Fig. 7A1. Depolarization of the same type I_e interneuronwith extrinsic current (Fig. 7A2) elicited an increase in extracellularspike activity recorded from nerve P2 (Fig. 7B). The increasein the discharge frequency of the large-amplitude extracellularspike suggests that the type I_e interneuron also projected bypolysynaptic pathways to pedal neuron VP2. As shown previously,the increase in light-elicited extracellular spike activity recordedfrom nerve P2 is associated with increased tonic firing of bothpedal neurons VP1 and VP2.

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Fig. 7. Identified type I_e interneurons project to pedal neurons with axonal processes in nerve P2. The type I_e interneuron was identified by a characteristic light-elicited depolarization and increase in tonic firing (A1). Stimulation of the same type I_e interneuron shown in A1 with an extrinsic depolarizing current pulse (A2) resulted in an increase in the firing of extracellularly recorded spikes of different amplitudes in nerve P2.

Convergence of type I and II interneuron synaptic input

A characteristic of the synaptic activity recorded in pedal neuron VP1 is the generation of inhibitory postsynaptic potentials(IPSPs) recorded in the dark and a decrease in IPSP frequencyduring illumination. The average IPSP frequency of VP1 pedal neuronsin the dark (n = 20) was 3.0 ± 0.17 and 1.9 ± 0.19 during thelight step. The decrease in IPSP frequency of VP1 neurons evokedby light was statistically significant (t₁₉ = 5.6; P < 0.001).An example of a simultaneous recording from a type I_i interneuronand pedal neuron VP1 in the dark and during a light step is shownin Fig. 8, A and B. The light step elicited a characteristic complexIPSP recorded from the type I_i interneuron (Fig. 8A). At the onsetof light and during the light step, IPSP frequency decreased inpedal neuron VP1 as shown in Fig. 8B. During the period of illumination,the presentation of an extrinsic depolarizing current pulse inthe type I_i interneuron increased the frequency of IPSPs recordedin VP1 (Fig. 8B). After the termination of the light step, IPSPfrequency increased in VP1 to prelight baseline levels. Lightand extrinsic current stimulation of type I_i interneurons producedsimilar effects on IPSP frequency recorded from VP2 pedal neurons(Fig. 8, C and D). The average IPSP frequency of VP2 pedal neuronsrecorded in the dark (n = 10) was 3.2 ± 0.34 and 2.1 ± 0.27 duringthe light step. The decrease in IPSP frequency of VP2 neuronsevoked by light was statistically significant (t₉ = 6.1; P < 0.001).Light hyperpolarized and decreased activity in the type I_i interneuronand the depolarizing extrinsic current pulse applied during thelight step increased IPSP frequency recorded in VP2 (Fig. 8D).These results indicate that type I_i interneurons project to interneuronsthat inhibit VP1 and VP2 pedal neurons, and light results in adisinhibition of VP1 and VP2 pedal neurons as a result of light-elicitedinhibition of spike activity in type I_i interneurons. The effectof light on changes in IPSP frequency recorded from VP1 and VP2pedal neurons and extrinsic current depolarization on IPSP frequencyrecorded from VP1 and VP2 neurons is summarized in the group datashown in Fig. 8, E and F. The analysis of the group data revealedthat light produced a significant decrease in IPSP frequency inVP1 (t₁₉ = 6.0; P < 0.001) and VP2 (t₉ = 6.2; P < 0.001) as comparedwith prelight baseline activity. In addition, the depolarizingcurrent pulse applied to the I_i interneurons produced a significantincrease in IPSP frequency recorded in VP1 (t₆ = 4.1; P < 0.006)and VP2 (t₅ = 2.4, P < 0.05) during the light step (Fig. 8F).A similar finding was detected in type II_i interneurons as shownin Fig. 9. A light step elicited a decrease in type II_i spikeactivity (Fig. 9A1) and a decrease in IPSP frequency recordedin VP1 (Fig. 9B1). Stimulation of the same type II_i interneuronwith depolarizing extrinsic current (Fig. 9A2) elicited an increasein IPSP frequency recorded in VP1 during the current pulse (Fig.9B2).

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Fig. 8. Type I_i interneurons excite interneurons that are a source for inhibitory postsynaptic potentials (IPSPs) recorded in pedal neurons VP1 and VP2. Light elicited a complex IPSP recorded from interneuron I_i (A) and a concomitant decrease in IPSP frequency recorded from pedal neuron VP1 (B). During the light step, an extrinsic current step depolarized I_i (- - -, A) and produced an increase in the number of IPSPs recorded from VP1 (B). Similar effects of light- and current-elicited depolarization were detected in simultaneous recordings from a type I_i interneuron and pedal neuron VP2. Depolarization (- - -) of the type I_i interneuron during the light step (C) in a different preparation produced an increase in IPSPs recorded in VP2 (D). IPSP frequency decreased during the light step and increased after the termination of light (D). Group data showing the mean decrease in IPSPs from baseline recorded in VP1 and VP2 elicited by the light step (E). *VP1, P < 0.001; *VP2, P < 0.001. Group data showing the significant increase in IPSP frequency elicited by the extrinsic current pulse presented during light in VP1 and VP2 (F). VP1, *P < 0.006; VP2, P < 0.05

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Fig. 9. Type II_i interneurons excite interneurons that inhibit VP1 pedal neurons. Light elicited a complex IPSP and decrease in tonic firing recorded in a type II_i interneuron (A1) and a concomitant decrease in IPSP frequency recorded in pedal neuron VP1 (B1). Stimulation of the same type II_i interneuron with a depolarizing extrinsic current pulse (- - -, A2) produced an increase in IPSP frequency recorded from VP1 (B2).

Similar synaptic connections were found between type II_e interneurons and VP1 and VP2 pedal neurons. As shown in Fig. 10, alight step resulted in a characteristic depolarization of a typeII_e interneuron, the generation of a spike, an increase in excitatorypostsynaptic potential (EPSP) frequency (Fig. 10A1), and a concomitantdecrease in IPSP frequency recorded in pedal neuron VP1 (Fig.10B1). The decrease in IPSP frequency recorded in VP1 could bethe result of light-elicited inhibition of type I_i and II_i interneurons.However, stimulation of the type II_e interneuron with depolarizingextrinsic current (Fig. 10A2) produced a decrease in IPSP frequencyrecorded in VP1 (Fig. 10B2). These results suggest that excitationof type II_e interneurons inhibit the activity of the inhibitoryinterneurons that are the source of IPSPs recorded from VP1. Inaddition, extrinsic depolarizing current applied to a type II_einterneuron (Fig. 10C) decreased IPSPs recorded from a VP2 pedalneuron (Fig. 10D). In summary, light affects two pathways projectingto VP1 and VP2. Light decreased inhibition of VP1 operating throughboth type I_i and type II_i interneurons by inhibiting the activityof interneurons that normally inhibit VP1 and VP2. The secondpathway involves excitation of type II_e interneurons that inhibitthe activity of inhibitory interneurons.

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Fig. 10. Type II_e interneurons inhibit the source of IPSPs recorded in pedal neurons VP1 and VP2. Light elicited a depolarization, a spike, and an increase in excitatory postsynaptic potentials (EPSPs) recorded from a type II_e interneuron (A1) and a concomitant decrease in IPSP frequency during the light recorded in VP1 (B1). Depolarization of the II_e interneuron (A2) with extrinsic current resulted in a disinhibition (decrease in IPSPs) of pedal neuron VP1 (B2). Depolarization of a different type II_e interneuron (C) produced a decrease in IPSP frequency and a disinhibition of pedal neuron VP2 (D).

Identification of type III inhibitory interneurons

Simultaneous recordings from VP1 and VP2 pedal neurons suggested that IPSPs may be generated by a common presynaptic source.As shown in Fig. 11, spontaneous IPSPs occurred synchronously inboth VP1 and VP2. We next examined the source of the IPSPs recordedfrom pedal neurons VP1 and VP2. Simultaneous recordings from aninterneuron designated as a type III_i and pedal neuron VP1 innormal ASW and after exposing the nervous system to a high-divalentcation solution (3× Ca²⁺ and 3× Mg²⁺) are shown in Fig. 12, A and B. A spike generated in the typeIII_i interneuron (Fig. 12A1) elicited a short-latency monosynapticIPSP recorded in VP1 (Fig. 12B1). The high-divalent cation ASWdid not block the IPSP recorded in VP1 (Fig. 12B2) elicited bythe spike in the type III_i interneuron (Fig. 12A2). The IPSPs recordedfrom VP1 followed spikes in the type III_i interneuron one-for-onewith a short and relative constant latency. As shown in Fig. 12,C and D, three consecutive superimposed IPSPs with a relativelyconstant latency recorded from VP1 followed three superimposedsingle spikes in the type III_i interneuron elicited by a briefextrinsic current pulse (Fig. 12D).

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Fig. 11. IPSPs recorded from pedal neurons VP1 and VP2 may be from a common presynaptic source. Simultaneous intracellular recordings from pedal neuron VP1 (A) and VP2 (B) show that IPSPs occur synchronously in each pedal neuron.

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Fig. 12. Type III_i interneurons directly inhibit VP1 pedal neurons. Simultaneous recordings from a type III_i interneuron and pedal neuron VP1 in normal ASW and in a high-divalent cation solution (3× Ca²⁺ and 3× Mg²⁺). A single spike generated in the type III_i interneuron by a current pulse (A1) elicited a monosynaptic IPSP recorded from VP1 (B1). Exposure of the nervous system to the high-divalent cation ASW did not block the IPSP recorded in VP1 (B2) evoked by the spike in the type III_i interneuron (A2). IPSPs recorded from VP1 followed spikes in the type III_i interneuron 1-for-1 with a brief and constant latency as shown by 3 superimposed spikes generated from a type III_i interneuron (C) and superimposed IPSPs recorded from pedal neuron VP1 (D).

Type II_b projections to pedal neurons VP1 and VP2

In addition to the disinhibition of VP1 and VP2 produced by type I_i, II_i, and II_e interneurons, newly identified type II_binterneurons also contributed to light-elicited depolarizationof VP1 and VP2 pedal neurons. Figure 13 shows a light-evoked generatorpotential recorded from a central type-B-photoreceptor (Fig. 13A1)and a depolarization and increase in EPSP frequency recorded froma type II_b interneuron (Fig. 13B1). Depolarization of the B-photoreceptorwith extrinsic current elicited spikes in the type-B photoreceptor(Fig. 13A2) and EPSPs recorded from the II_b interneuron (Fig. 13B2),indicating the central type-B photoreceptor projected to the typeII_b interneuron. Because light evoked more EPSPs than stimulationof a single type-B photoreceptor, it is likely that multiple photoreceptorsproject to a single type II_b interneuron. As shown in Fig. 14A1,light elicited an increase in the tonic spike activity of a typeII_b interneuron and a concomitant increase in the spike activityrecorded in VP1 (Fig. 14B1). Hyperpolarizing VP1 to $-$ 68 mV to blockspike activity (Fig. 14B2) showed that the light step eliciteda complex EPSP and depolarization of VP1. Stimulation of the sametype II_b interneuron with a depolarizing extrinsic current pulse(Fig. 14A3) produced an increase in spike activity recorded fromVP1 (Fig. 14B3). Hyperpolarizing VP1 to $-$ 67 mV blocked spike activityand revealed a complex EPSP and a depolarization of VP1 (Fig.14B4) elicited by the depolarizing extrinsic current pulse appliedto the type II_b interneuron (Fig. 14A4).

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Fig. 13. Synaptic connections between identified photoreceptors and type II_b interneurons are polysynaptic. A light step elicited a depolarizing generator potential in a central B photoreceptor (A1) and EPSPs recorded from a type II_b interneuron hyperpolarized to block spike activity (B1). Stimulation of the same central type B photoreceptor with extrinsic current (A2) evoked EPSPs in the type II_b interneuron (B2).

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Fig. 14. Newly identified type II_b interneurons project to VP1 pedal neurons. Light elicited an increase in tonic firing of the II_b interneuron (A1) and a concomitant increase in firing of pedal neuron VP1 (B1). Hyperpolarizing VP1 to $-$ 68 mV to block spike activity revealed that the light-elicited increase in firing of the II_b interneuron (A2) resulted in a depolarization of pedal neuron VP1 (B2). Depolarization of the same type II_b interneuron with an extrinsic current pulse (A3) produced an increase in tonic firing of VP1 (B3). Depolarization of the same type II_b interneuron with extrinsic current revealed a complex EPSP recorded from pedal neuron VP1 (B4) hyperpolarized to $-$ 67 mV to block spike generation.

We next examined synaptic input to pedal neuron VP2 from type II_b interneurons. As shown in Fig. 15, A1 and B1, light produceda depolarization of the type II_b interneuron (Fig. 15A1) and aslow depolarization and increased spike activity of pedal neuronVP2 (Fig. 15B1). A depolarizing extrinsic current pulse elicitedspikes in the type II_b interneuron (Fig. 15A2) and a slow depolarizationand single action potential recorded from VP2 (Fig. 15B2). HyperpolarizingVP2 to block spike activity showed that the spikes elicited bythe current step in the same type II_b interneuron (Fig. 15A3) producedEPSPs recorded in VP2 (Fig. 15B3). Taken collectively, the resultsprovide evidence for convergence of type II_e, II_b, and II_i synapticinput to VP1 and VP2 pedal neurons.

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Fig. 15. Newly identified type II_b interneurons project to pedal neuron VP2. Light elicited an increase in tonic firing of the type II_b interneuron (A1) and a concomitant depolarization and increased spike activity recorded from pedal neuron VP2 (B1). Depolarization of the type II_b interneuron with extrinsic current (A2) produced a slow depolarization and spike in VP2 (B2). Depolarization of the same type II_b interneuron with extrinsic current (A3) produced a depolarization and complex EPSP recorded from pedal neuron VP2 (B3) hyperpolarized to $-$ 59 mV to block spike generation.

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Characteristics of VP1 and VP2

In this report we have identified two pedal neurons (VP1 and VP2), characterized their electrophysiological activity, anddocumented the increase in tonic-firing of the neurons by illuminationof the eyes and the role of VP1 in ciliary movement and VP2 infoot movement. Both VP1 and VP2 have axonal projections to theanterior foot through pedal nerve P2 as verified by recordingsof orthodromic and antidromic spikes generated by stimulationof VP1 and VP2 and stimulation of nerve P2. Lucifer yellow labelingof VP1 and VP2 confirmed the electrophysiological results (unpublishedresults). Activation of a single photoreceptor with extrinsiccurrent is sufficient to increase tonic firing of VP1. Stimulationof a medial type-B photoreceptor with extrinsic current was shownto produce an increase in tonic spike activity recorded from VP1with concomitant changes in extracellular activity recorded frompedal nerve P2. The increase in the discharge rate of severalextracellular spikes with different amplitudes suggests that asingle type-B-photoreceptor projects polysynaptically to multiplepedal neurons. Synaptic divergence of the visual system is furthersupported by the observation that depolarization of an identifiedtype I_e interneuron elicited an increase in the activity of severalextracellularly recorded spikes from nerve P2. This suggests thatthe same components of the neural network mediate both ciliarymovement and foot movement. While different, these two behaviorsare not incompatible, and coactivation may facilitate ciliarymovement by increasing the contact area between the foot and substrate.The control over different behaviors by the same network has beenshown in Tritonia (Popescu and Frost 2002), Pleurobranchaea (Jingand Gillette 2000), and Lymnaea (Syed and Winlow 1989).

Synaptic inhibition of VP1 and VP2

Previous research has shown that light inhibits type I_i and II_i interneurons and excitates type I_e and II_e interneurons (Crowand Tian 2000, 2002a). Here we show that light evoked a complexIPSP in type I_i interneurons and a concominant decrease in IPSPfrequency recorded from VP1 and VP2. Our evidence suggests thatthe source of the IPSPs in VP1 and VP2 is the type III_i interneuron.Depolarization of type I_i interneurons during the light step resultedin an increase in IPSP frequency recorded in both VP1 and VP2.Therefore light-evoked synaptic inhibition of type I_i interneuronsresults in a disinhibition of VP1 and VP2 due to a decrease innormal synaptic excitation of type III_i interneurons. A similarfinding was observed for both light and extrinsic current depolarizationof type II_i interneurons. Light decreased spike activity recordedin type II_i interneurons and decreased IPSP frequency recordedin both VP1 and VP2. Depolarization of type II_i interneurons inthe dark increased IPSP frequency recorded in both VP1 and VP2pedal neurons. In contrast, the effects of depolarization of typeI_e and type II_e interneurons were less clear. Light-evoked depolarizationof type II_e interneurons also decreased IPSP frequency recordedfrom VP1 pedal neurons, and depolarization with extrinsic currentof type II_e interneurons produced disinhibition of VP1, e.g.,decrease in IPSPs during the current pulse. The effect of currentdepolarization on type I_e interneurons was more variable. In someexperiments, current depolarization of type I_e interneurons producedinhibition of VP1, and in other examples, no effect on PSP frequencyor changes in tonic firing could be detected in either VP1 orVP2. The variability of type I_e depolarization on changes in tonicfiring of VP1 and VP2 may be due in part to the labeled-line organizationbetween photoreceptors and type I interneurons (Crow and Tian2000). It is suggested that because lateral type-B photoreceptorsproject to the first layer of type I_e interneurons and other Bphotoreceptors project to type I_e interneurons located in deeperlayers, not all type-B photoreceptors may have polysynaptic connectionswith VP1 and VP2 pedal neurons through type I_e and II_e interneurons.Our results show that convergence of type I_i, II_i, I_e, and II_einterneuron synaptic input is to type III_i interneurons, and typeIII_i interneurons form monosynaptic connections with VP1 and VP2pedalneurons.

Type II_b interneuron synaptic projections to VP1 and VP2

In contrast to the decrease in IPSP frequency recorded in VP1 and VP2 elicited by light, light and extrinsic current depolarizationof newly identified type II_b interneurons produced excitationof pedal neurons VP1 and VP2. However, light-elicited increasedtonic firing of II_b interneurons was more variable than observedin type II_e interneurons. Taken collectively, the neural networkmediating ciliary movement consists of two independent pathwaysfrom the photoreceptors to identified interneurons that convergeon VP1. The pathway from type I_i, II_i, I_e, and II_e interneuronsis through the type III_i inhibitory interneurons and, when activatedby light, produces a disinhibition and increased tonic firingof VP1. The excitatory pathway from type II_b interneurons producesa depolarization and increase in the tonic firing of VP1 whenactivated bylight.

Pedal neuron control of ciliary locomotion

Many gastropod mollusks locomote by the movement of pedal cilia on the sole of the foot (for examples see Audesirk 1978a,b;Copeland 1919; Popescu and Frost 2002; Willows et al. 1997). Ciliarylocomotion is a nonrhythmic, nonmuscular, smooth gliding formof movement. The neural analysis of ciliary locomotion has beenconducted in Tritonia diomedea (Audesirk 1978a,b; Popescu andFrost 2002; Popescu and Willows 1999), Pleurobranchaea (Jing andGillette 2000), and Lymnaea (Syed and Winlow 1989). Interestingly,the swim CPG network contributes to both escape swimming and ciliarylocomotion in Tritonia (Popsecu and Frost 2002). Because the footis not in contact with the substrate during swimming, ciliaryactivation and swimming are not incompatible behavioral acts.Indeed, coactivation may be beneficial because after the swimciliary locomotion is expressed as soon as the foot is in contactwith the substrate (Popescu and Frost 2002). In Pleurobranchaea,the As1-4 interneurons provide both excitation to the swim CPGand locomotor G neurons that are homologs of ciliary activatingneurons in other species (Jing and Gillette 2000).

Previous work has shown that pedal nerves P1 and P2 contain the axons of neurons responsible for generating locomotion inHermissenda (Hodgson and Crow 1991; Richards and Farley 1987).Richards and Farley (1987) showed that the posterior three-fourthsof the foot is innervated by nerve P1, while the remaining anteriorportion is innervated by nerve P2. Consistent with their findings,here we report that extracellular recordings from pedal nerveP2 revealed light-elicited increases in tonic firing reflectedby extracellular spikes with different amplitudes. We have identifiedVP1 and VP2 as two pedal neurons contributing to the spike activityin nerve P2. In addition, experiments conducted with semi-intactpreparations showed that depolarization of VP1 produced ciliarymovement and depolarization of VP2 produced anterior foot andventral tentacle movement. The visual network consisting of photoreceptors,type I, II, and III interneurons is presynaptic to both VP1 andVP2, thus the same circuit elements can support both light-elicitedciliary movement and light-evoked muscular foot movements in Hermissenda.Muscular and ciliary effector systems are different; however,these two behavioral acts are not necessarily incompatible becausethe lateral foot movements elicited by stimulation of VP2 mayincrease the contact area of the anterior foot and thus facilitatelocomotion in conjunction with activation of cilia on the soleof the anterior foot. Interestingly, a recently identified pedalneuron that produces a rapid contraction of the anterior footdoes not receive synaptic input from type II_e or II_i interneurons(unpublished observation). This observation suggests that Pavlovianconditioning may modify different components of the circuit supportingciliary locomotion and foot shortening(contraction).

Conditioned modification of locomotion and foot contraction

Previous studies have examined light-responsive putative motor neurons in the pedal ganglia, although progress has not beenremarkable (Crow 1981; Goh and Alkon 1984; Goh et al. 1985; Hodgsonand Crow 1991, 1992; Jerussi and Alkon 1981; Richards and Farley1987). The most extensive analysis of a possible link betweenthe visual system and motor behavior was reported by Goh and Alkon(1984). They identified a putative motor neuron in the pedal ganglion,classified as motor neuron one (MN1), that produced turning ofthe posterior half of the foot when the MN1 was stimulated withextrinsic depolarizing current. They reported that MN1 receivedindirect synaptic input from medial type A photoreceptors viaa group of identified interneurons similar to type I and II interneurons.In response to light, MN1 exhibited an increase in EPSP frequencyand an increase in the spike discharge frequency. Interneuronsin the cerebropleural ganglion that received excitatory synapticinput from the medial type A photoreceptor produced excitationof MN1 when activated by light or extrinsic depolarizing current.Previous research has shown that type B excitability is enhancedby conditioning (Crow and Alkon 1978). Therefore it was proposedthat in conditioned animals, the enhanced inhibition of the medialtype A produced by type-B-enhanced excitability in response tothe CS would result in a diminished direct excitatory synapticinput to the interneurons and decreased indirect excitation ofMN1. Consistent with this hypothesis, they found that in conditionedanimals, light elicited a significantly smaller increase in thespike frequency of MN1 as compared with normal controls or randomcontrol groups (Goh et al. 1985). Goh and Alkon (1984) furtherproposed that MN1 was involved in mediating the animal's turningbehavior toward a source of illumination, and thus decreased activityof MN1 may lead to reduced motor activity and diminished phototacticbehavior. However, it is clear that inhibition of type A photoreceptoractivity cannot account for the neural correlates of Pavlovianconditioning identified from pedal neuron recordings and extracellularactivity recorded from pedal nerves. These studies showed light-eliciteddecreases in spike frequency below baseline activity that cannotbe related to type A activity because type A photoreceptors arenot spontaneously active in the dark. Therefore inhibiting theiractivity during the presentation of the CS would not be expectedto produce inhibition of the activity of pedal neurons below theirbaseline levels (Hodgson and Crow 1992; Richards and Farley 1987).

Visually mediated behaviors that have been examined in Hermissenda include the effects of light gradients on locomotion (Lederhendleret al. 1980), positive phototactic responses (Alkon 1974), footshortening (Lederhendler et al. 1986), and the initiation of locomotion(Crow and Offenbach 1983). These examples of behaviors influencedby light and their modification by Pavlovian conditioning involve,either directly or indirectly, locomotion. The network mediatingciliary locomotion in Hermissenda expresses enhanced cellularexcitability (Sahley and Crow 1998), facilitation of monosynapticPSPs between identified photoreceptors (Frysztak and Crow 1994;Gandhi and Matzel 2000), and facilitation of PSPs between photoreceptorsand type I interneurons produced by Pavlovian conditioning (Crowand Tian 2000, 2002b). The previously identified facilitationof type I interneuron monosynaptic and complex PSPs detected afterconditioning would be expected to decrease the tonic activityof VP1 during the presentation of the CS. Neural correlates ofPavlovian conditioning in VP1 and VP2 pedal neurons are currentlyunderinvestigation.

	ACKNOWLEDGMENTS

We thank D. Parker for assistance with themanuscript.

This research was supported by National Institute of Mental Health Grant MH-58698.

	FOOTNOTES

Address for reprint requests: T. Crow, Dept. of Neurobiology and Anatomy, University of Texas Medical School, P.O. Box 20708,Houston, TX 77225 (E-mail: terry.crow{at}uth.tmc.edu).

REFERENCES

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

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Interneuronal Projections to Identified Cilia-Activating Pedal Neurons in Hermissenda

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