Modulators with Convergent Cellular Actions Elicit Distinct Circuit Outputs

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The Journal of Neuroscience, June 1, 2001, 21(11):4050-4058

Modulators with Convergent Cellular Actions Elicit Distinct Circuit Outputs
Andrew M. Swensen and Eve Marder
Volen Center and Biology Department, Brandeis University, Waltham, Massachusetts 02454

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Six neuromodulators [proctolin, Cancer borealis tachykinin-related peptide Ia, crustacean cardioactive peptide (CCAP), redpigment-concentrating hormone, TNRNFLRFamide, and pilocarpine]converge onto the same voltage-dependent inward current in stomatogastricganglion (STG) neurons of the crab C. borealis. We show here thateach of these modulators acts on a distinct subset of pyloricnetwork neurons in the STG. To ask whether the differences incell targets could account for their differential effects on thepyloric rhythm, we systematically compared the motor patternsproduced by proctolin and CCAP. The motor patterns produced inproctolin and CCAP differed quantitatively in a number of ways.Proctolin and CCAP both act on the lateral pyloric neuron andthe inferior cardiac neuron. Proctolin additionally acts on thepyloric dilator (PD) neurons, the pyloric (PY) neurons, and theventricular dilator neuron. Using the dynamic clamp, we introducedan artificial peptide-elicited current into the PD and PY neurons,in the presence of CCAP, and converted the CCAP rhythm into arhythm that was statistically similar to that seen in proctolin.This suggests that the differences in the network effects of thesetwo modulators can primarily be attributed to the known differentialdistributions of their receptors onto distinct subsets of neurons,despite the fact that they activate the samecurrent.

Key words: stomatogastric ganglion; crab; Cancer borealis; proctolin; CCAP; RPCH; CabTRP; FLRFamide-related peptides

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

All nervous systems use a large number of different signaling molecules as neurotransmitters and neuromodulators. In principle,voltage-dependent and ligand-gated channels, chemical synapses,and electrical synapses are all subject to neuromodulation, resultingin changes in circuit activity and output (Marder and Calabrese,1996). The large number of potential sites for neuromodulationwithin a circuit often makes it difficult to understand exactlyhow modulation of one or more currents in one or more neuronswithin a circuit results in altered circuit activity. Understandinghow modulation at the cellular level translates into altered circuitoutput can be profitably studied in relatively small nervous systems,in which the number of neurons involved allows the investigatorto identify the neurons that are direct targets of modulation(Marder and Eisen, 1984b; Flamm and Harris-Warrick, 1986; Hooperand Marder, 1987). The stomatogastric ganglion (STG) of crabscontains only 26-27 neurons (Kilman and Marder, 1996) but is modulatedby 15-20 different substances (Marder, 1987; Christie et al.,1995; Marder et al., 1995). This raises a series of issues abouthow multiple neuromodulators can act on the same circuits to producea variety ofbehaviors.

Recently we found that six modulators [proctolin, Cancer borealis tachykinin-related peptide Ia (CabTRP), TNRNFLRFamide, crustaceancardioactive peptide (CCAP), red pigment-concentrating hormone(RPCH), and the muscarinic agonist pilocarpine] that elicit distincteffects on the rhythmic output of the STG (Marder and Hooper,1985; Marder and Weimann, 1992) converge onto the same voltage-dependentcurrent (Swensen and Marder, 2000). This is in contrast to theamines serotonin and dopamine that modulate a variety of differentcurrents in STG neurons (Kiehn and Harris-Warrick, 1992a,b; Harris-Warricket al., 1995a,b, 1998; Zhang and Harris-Warrick, 1995; Zhang etal., 1995; Kloppenburg et al., 1999).

How can a network produce divergent outputs in response to multiple substances that converge onto the same current? To answerthis question, we first determined which neurons of the pyloricnetwork of the STG responded to each of the convergent modulatorsand found that each of the convergent modulators acts on a differentsubset of neurons. This suggests that the differential distributionof receptors onto distinct subsets of target neurons may be responsiblefor the divergent effects of these modulators on network activity.To test this hypothesis, we used the dynamic clamp (Sharp et al.,1993a,b) to introduce an artificial peptide current into specificneurons, to attempt to convert the motor patterns from those characteristicallyproduced by one set of neuronal targets to those produced by another.Specifically, we found that by introducing an artificial peptide-activatedcurrent into two cells that do not respond to CCAP but do respondto proctolin we could convert the CCAP rhythm into a proctolin-likerhythm. This would suggest that major differences in circuit outputcan result from modulators that act on the same current if theyact on different subsets of circuitneurons.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animals. C. borealis were obtained from Commercial Lobster (Boston, MA) and maintained in artificial seawater untilused.

Modulators. Proctolin (Sigma, St. Louis, MO), CabTRP Ia (gift from A. E. Christie and M. P. Nusbaum), CCAP (Bachem, Torrance,CA), RPCH and TNRNFLRFamide (American Peptide Company, Sunnyvale,CA), and pilocarpine (Sigma) were dissolved in saline and eitherpressure applied using a Picospritzer (5-15 psi; 50-1000 msec)with 100-500 µM (proctolin, CabTRP, CCAP, TNRNFLRFamide, and RPCH)or 10-50 mM (pilocarpine) in the pressure pipette or bath appliedat the concentrations indicated in the text and figurelegends.

Solutions. C. borealis physiological saline was composed of (in mM): NaCl, 440; KCl, 11; CaCl₂, 13; MgCl₂, 26; Trizma base,11; and maleic acid, 5, pH 7.4-7.5.

Recordings. The stomatogastric nervous systems were dissected out of the animals and pinned out in dishes containing Sylgard(Dow Corning, Midland, MI). During the experiments, the nervoussystems were continuously superfused with chilled (11-14°C) physiologicalsaline. Extracellular recordings from nerves were made using stainlesssteel pin electrodes. Intracellular recordings were made usingthe Axoclamp 2A and 2B amplifiers (Axon Instruments, Foster City,CA) in either two-electrode current clamp, single-electrode currentclamp, or two-electrode voltage clamp (TEVC). Microelectrodesused for intracellular recordings and injections contained 0.6M K₂SO₄ and 20 mM KCl, and electrode resistances ranged from 20to 40 M $Omega$ . Data were collected and analyzed using pCLAMP software(Axon Instruments).

For the experiments performed to identify the cell targets of the various modulators and for the dose-response curves, neuronswere pharmacologically isolated using 10 µM picrotoxin (PTX; Sigma)to block the inhibitory glutamatergic synapses in the STG (Bidaut,1980; Marder and Eisen, 1984a), 0.1 µM tetrodotoxin (TTX; AlomoneLabs, Jerusalem, Israel) to block action potential generation,and, in some cases, 10 mM tetraethylammonium chloride (TEA; Sigma)to block some of the K⁺ currents. Photoinactivation was used to eliminate electricallycoupled neurons (Miller and Selverston, 1979). For photoinactivation,cells were filled for 45 min with Lucifer yellow (10%) in an electrodebackfilled with 1 M LiCl ( $-$ 4 to $-$ 8 nA pulses). Cells sat for anadditional 30-60 min before irradiation to allow the Lucifer yellowto diffuse to the outerprocesses.

For the experiments performed to compare the network effects of CCAP and proctolin, the STG was isolated from anterior modulatoryinputs by blocking the stomatogastric nerve with a well containingsucrose (750 mM). Data analyses of the phase relationships andcell activity measurements were done using DataMaster, version2.0, by William Miller. Phase relationships were calculated bydividing the time of burst onset (or offset) by the cycle period.The onset of the pyloric dilator (PD) neuron was defined as time0 for eachcycle.

Dynamic clamp. Artificial currents were introduced into neurons using a version of the dynamic clamp (Sharp et al., 1993a,b)developed by Farzan Nadim, Yair Manor, and William Miller withLabView/CVI software (National Instruments, Austin, TX). The artificialcurrents were described by the equation: I = g*m*(V $-$ E_r), wherem = 1/(1 + exp((V $-$ V_m)/K_m)), E_r is the reversal potential, V_mis the half-maximal activation, and K_m is the slope of the logisticfunction at V_m. For the artificial current in the PD neuron, E_r= $-$ 22 mV, V_m = $-$ 21 mV, and K_m = $-$ 8 mV. For the pyloric (PY) neuron,these values were E_r = 9 mV, V_m = $-$ 18 mV, and K_m = $-$ 10mV.

Current-voltage curves. To obtain current-voltage curves, cells were voltage clamped and typically ramped from $-$ 90 to 0 mVat 75 mV/sec (1.2 sec total). The currents elicited under controlconditions were then subtracted from those obtained in the presenceof the pressure-applied modulator. This difference current wasplotted versus voltage to yield the current-voltage curves (Swensenand Marder, 2000).

Statistics. The SigmaPlot and SigmaStat software packages (Jandel Scientific, San Rafael, CA) were used for statisticalanalyses.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We demonstrated previously that six modulators (proctolin, CabTRP, CCAP, RPCH, TNRNFLRFamide, and pilocarpine) converge ontothe same voltage-dependent current (Swensen and Marder, 2000).This current is an inward nonspecific cation current that showsstrong outward rectification (Golowasch and Marder, 1992). Thepeak inward current is elicited at voltages ranging from $-$ 40 to $-$ 20 mV depending on the cell type (Swensen and Marder, 2000).We showed that although the lateral pyloric (LP) neuron respondedto all six modulators, the ventricular dilator (VD) neuron respondedto only a subset of the modulators (Swensen and Marder, 2000).To account for the effects of these neuromodulators on the entirenetwork, it is necessary to determine which cell types respondto each substance. Therefore, we assayed the remaining pyloricnetwork neurons to determine which modulators act on each celltype.

The PD neurons respond to proctolin, CabTRP, and pilocarpine

There are two PD neurons in each STG. Figure 1A shows an example of the current-voltage curves for proctolin, CabTRP, andpilocarpine in an isolated PD neuron. Note the similarity in thecurves and that, for each modulator, the voltage at which thepeak inward current was elicited (V_peak) was approximately $-$ 35mV. The PD neurons responded to proctolin (n = 7), CabTRP (n =8), and pilocarpine (n = 7) but not to TNRNFLRFamide (n = 4),CCAP (n = 5), or RPCH (n = 3). The mean V_peak values for proctolin,CabTRP, and pilocarpine were statistically indistinguishable (one-wayANOVA, p = 0.162). The mean V_peak value for all PD neurons was $-$ 30 ± 1 mV (n = 8).

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Figure 1. Modulators acting on the PD and PY neurons. A, Convergence of proctolin, CabTRP, and pilocarpine onto the PD neuron. All three modulators yield similar current-voltage curves with V_peak values of approximately $-$ 35 mV. Recordings were made from the same PD neuron. The PD neuron was isolated from the electrically coupled AB and LPG neurons by photoinactivation. B, Two of the response types exhibited by PY neurons. The responses of the PY neuron fell into three categories: those that responded to only TNRNFLRFamide (type I; top), those that responded to TNRNFLRFamide, proctolin, and pilocarpine (type II; bottom), and those that responded to TNRNFLRFamide, proctolin, pilocarpine, and CabTRP (type III; data not shown). Note that all three modulators converging onto the type-II neurons yield similar current-voltage curves with V_peak values at approximately $-$ 20 mV. Recordings were all made in TEVC. Modulators were pressure applied for 100 msec at 500 µM (proctolin, CabTRP, or TNRNFLRFamide) or 50 mM (pilocarpine). The bath contained 10 µM PTX to block the inhibitory glutamatergic synapses, 0.1 µM TTX to block action potential generation, and 10 mM TEA to block some of the K⁺ currents.

PY neurons fall into three categories

In the lobster Panulirus interruptus, there are eight PY neurons that have been divided into two classes on the basis of theirfiring patterns and synaptic connections (Hartline et al., 1987).In the crab C. borealis, there are approximately five PY neurons(Kilman and Marder, 1996), which are also likely to be heterogeneousin terms of synaptic connectivity. Figure 1B shows the current-voltagecurves for two PY neurons that responded to different subsetsof the modulators. The PY neurons responding to only TNRNFLRFamide(4 of 14) were classified as type-I PY neurons. The other PY neuronsresponded either to TNRNFLRFamide, proctolin, and pilocarpine(type II; 6 of 14) or to TNRNFLRFamide, proctolin, pilocarpine,and CabTRP (type III; 4 of 14). None of the PY neurons testedresponded to either CCAP (n = 14) or RPCH (n = 14). In three offour experiments in which we recorded from two PY neurons in thesame preparation, we found that the PY neurons fell into differentcategories on the basis of their modulator responses. This suggeststhat these different PY neuron subtypes are expressed in eachindividual animal and are not simply a result of animal-to-animalvariability. The mean V_peak values for type-I ( $-$ 18 ± 6 mV; n =3), type-II ( $-$ 21 ± 7 mV; n = 5), and type-III ( $-$ 19 ± 6 mV; n =4) PY neurons were statistically indistinguishable (one-way ANOVA,p = 0.777). In addition, the pooled V_peak values for each individualmodulator (TNRNFLRFamide, proctolin, pilocarpine, and CabTRP)across all PY neurons were not statistically different (one-wayANOVA, p = 0.587).

The inferior cardiac neuron responds to five of the six modulators

There is one inferior cardiac (IC) neuron in each STG. The IC neuron responded to proctolin (n = 7), CabTRP (n = 7), CCAP(n = 5), TNRNFLRFamide (n = 7), and pilocarpine (n = 5) but notto RPCH (n = 4). The V_peak measurements for the different modulatorsacting on the IC neuron were not statistically different (one-wayANOVA, p = 0.617). The mean V_peak value for all IC neurons was $-$ 29 ± 5 mV (n =7).

The lateral posterior gastric neurons

There are two lateral posterior gastric (LPG) neurons in each STG. All isolated LPG neurons responded to CabTRP (n = 7) butnot to proctolin (n = 7), CCAP (n = 3), TNRNFLRFamide (n = 3),or RPCH (n = 3). Two of five LPG neurons responded to pilocarpineas well. The V_peak value for CabTRP in the LPG neurons was $-$ 18± 5 mV (n =5).

The anterior burster neuron

There is one anterior burster (AB) neuron in each STG. The AB neuron is electrically coupled to the PD neurons and often hasa very small soma with a narrow neck, partially isolating thesoma from its major neurite and its electrically coupled partners.In voltage-clamped isolated AB neurons, we were not able to seeany modulator-elicited currents in response to voltage ramps.In current-clamp recordings of isolated AB neuron activity, however,the modulators increased the frequency and/or enhanced the amplitudeof the membrane potential oscillations of the AB neuron (proctolin,n = 5; CabTRP, n = 3; CCAP, n = 3; pilocarpine, n = 2; TNRNFLRFamide,n = 2; and RPCH, n = 2; data notshown).

Summary of the cellular targets for each modulator

Figure 2 summarizes the cell targets of each modulator, and Table 1 reports the measured V_peak values of the modulator responsesin each cell type. In Figure 2, neurons that displayed multipleresponse types are shaded according to the subpopulation of thoseneurons that showed responses.

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Figure 2. Pyloric circuits summarizing the target neurons (shaded) for each of the convergent modulators. Each modulator targets a different subset of cells. Neurons that exhibited multiple responses are shaded according to the percentage of the cells that did respond to a given modulator.


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Table 1. Summary of modulators converging onto each pyloric cell type

Figure 2 shows that each of the modulators acted on a different subset of the neurons in the pyloric rhythm. On one end ofthe spectrum, CabTRP activated all cell types, whereas at theother end of the spectrum, RPCH had only two cell targets. Todetermine experimentally whether the differences in cell targetscan account for differences in the motor patterns evoked by thedifferent modulators, we wanted to select a pair of substancesthat differed in cell targets sufficiently to be interesting (morethan one cell different) but were close enough so that we couldlater apply artificial peptide currents with the dynamic clamp.Therefore, we chose to compare the actions of proctolin and CCAP.The logic of the remainder of this paper is first to compare quantitativelythe motor patterns evoked by proctolin and CCAP and then to determinewhether we can convert a CCAP pattern to a proctolin pattern byapplication of the modulator current, using the dynamic clamp,to those cells that do not respond to CCAP but do respond toproctolin.

Proctolin and CCAP elicit distinct effects at the network level

The physiological actions of bath-applied proctolin and CCAP have been reported previously (Hooper and Marder, 1984; Marderet al., 1986; Nusbaum and Marder, 1989a,b; Weimann et al., 1997).However, in the previous work proctolin and CCAP were studiedseparately, and each was compared with control saline, and therewere no direct quantitative comparisons of the motor patternsevoked by these modulators. Figure 3 shows an example of proctolinand CCAP (at two concentrations) applied to the same preparation.Previous work had shown that both modulators strongly excitedthe LP neuron but that CCAP has a more potent action on the LPneuron at a given concentration (Hooper and Marder, 1984; Marderet al., 1986; Nusbaum and Marder, 1989a,b; Weimann et al., 1997).This can be seen in Figure 3, where the LP neuron is more stronglyactivated in CCAP than in proctolin at a given concentration.In 5 × 10⁷ M CCAP, the LP neuron fired at a higher spike frequency (p <0.041, paired t test) and for a longer duration (p < 0.001, pairedt test) than in 10⁶ M proctolin (n = 8 experiments). We wanted to ask whether therewere significant differences in the pyloric rhythm in the twopeptides because of effects on other target neurons, independentof differences in the activation of the LP neuron. Therefore weused LP neuron activity to normalize for potency differences betweenproctolin and CCAP and studied the rhythms at concentrations ofthe two peptides that produced equivalent spike frequency in theLP neuron.

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Figure 3. Proctolin- and CCAP-elicited pyloric rhythms at two different concentrations (10⁶ and 10⁷ M). Extracellular recordings are from STG motor nerves. These recordings show the activity of the pyloric neurons as labeled. Both sets of recordings are from the same preparation.

Figure 4 shows the dose-response curves for proctolin- and CCAP-evoked currents in the LP neuron. On the basis of the bestfits, at concentrations of 10⁶ M, proctolin was at 83% of its maximal current, and CCAP wasat 94% of its maximal current. To compensate for the differencein potency, as calculated from the inward currents measured inthe peptides, we started by comparing the effects of 10⁶ M proctolin with a CCAP concentration of 3 × 10⁷ M. At these concentrations (10⁶ M proctolin and 3 × 10⁷ M CCAP) the spike frequencies of the LP neuron in the intactnetwork were approximately equivalent but still varied slightlydepending on the preparation. To compensate for this, in eachindividual experiment we adjusted the CCAP concentration untilthe LP neuron fired at the same frequency in CCAP as in 10⁶ M proctolin. The CCAP concentrations for the six experimentswere the following: 1.5 × 10⁷, 2.0 × 10⁷, 3.0 × 10⁷, 3.5 × 10⁷, 5.0 × 10⁷, and 5.0 × 10⁷ M.

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Figure 4. Dose-response curves for proctolin and CCAP in the LP neuron. The proctolin dose-response curve is adapted from Swensen and Marder (2000). For proctolin, 90% of the maximal current was reached at 1.8 × 10⁶ M, and for CCAP, 90% maximal was reached at 6 × 10⁷ M. Plotted points represent the normalized peak inward current elicited (±SE) in the LP neuron while voltage clamped to $-$ 40 mV. The bath contained 10 µM PTX and 0.1 µM TTX. Points were fit to the equation: y = (I_max)x/(K_d + x), where x is the concentration of the applied peptide, I_max is the normalized maximal current, and K_d is the dissociation constant. For proctolin, I_max = 1.06 ± 0.01, and K_d = 2.02 (± 0.01) × 10⁷ M. For CCAP, I_max = 0.99 ± 0.02, and K_d = 6.7 (± 1.1) × 10⁸ M.

Using the dynamic clamp to mimic peptide actions

The artificial peptide currents that we used were derived from currents measured in a PD and a PY neuron. Figure 5A showsthe artificial peptide currents we used for the PD and PY neuronsalong with the actual current-voltage curves from which they werefit. Examples of the artificial currents applied to a PD neuronand a PY neuron are shown in Figure 5B. The left panels show controlrecordings for a PD and a PY neuron, and the right panels showrecordings from these two cells with the addition of artificialcurrent. Below each intracellular recording is a current traceshowing the amount of artificial current being injected at anygiven time. Because of the voltage dependence of the peptide currents,the dynamic-clamp current oscillates with the voltage swings ofthe cell. Moreover, because there is more inward current whenthe cells are depolarized, the peptide current enhances the amplitudeof the oscillations and causes an increase in the number of spikesfired in each burst.

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Figure 5. The artificial peptide-elicited currents for the PD and PY neurons. A, Proctolin currents recorded from a PD and a PY neuron and the fits that were used as the artificial peptide currents. Recordings were made using TEVC in the presence of 10 µM PTX and 0.1 µM TTX. Values obtained from the fits were used in the dynamic-clamp program (see Materials and Methods). B, Left, The control activity of a PD and a PY neuron. Right, How the activity of the PD and the PY neurons change with the introduction of the artificial current. Below each intracellular trace is a current trace showing the amplitude of the artificial current being injected at any given time. The horizontal line indicates $-$ 50 mV. In these two examples the peak current values were set at $-$ 1.8 nA (PD neuron) and $-$ 1.6 nA (PY neuron).

Comparison of the proctolin, CCAP, and artificial rhythms

For these experiments, we first applied proctolin (10⁶ M) to the STG to elicit a control proctolin rhythm. After extensiverinsing, CCAP was applied to the STG to obtain a CCAP rhythm.While still in CCAP, we then used the dynamic clamp to injectvarying amounts of the artificial peptide current into the PDand PY neurons simultaneously to see how these neurons influencedthe background CCAP-elicited rhythm. We then analyzed the rhythmsproduced with these artificial peptide currents to see whetherthey had become more proctolin-like. We refer to these rhythmsas the "artificialrhythm."

To assess the extent to which the CCAP rhythm became more proctolin-like, we measured the following parameters of the motorpatterns: (1) the cycle frequency, (2) the burst duration of eachneuron, (3) the phase of onset and termination of the burst ofeach neuron, (4) for single neurons (LP and IC neurons) the spikefrequency within the burst, and (5) for neurons with multiplecopies (PD and PY neurons) the number of spikes perburst.

In preliminary experiments we found that the artificial peptide current in the PY neuron had a pronounced effect on the burstduration of the LP neuron and that the artificial peptide currentin the PD neuron influenced the cycle frequency. Therefore, thetuning strategy we used in these experiments was first to adjustthe size of the artificial peptide-activated conductance in thePY neuron until the LP burst duration was similar to what wasobserved in proctolin. We then adjusted the size of the artificialpeptide-activated conductance in the PD neuron until the cyclefrequency was similar to the observed proctolin frequency. Theresulting rhythm was then compared with the proctolin rhythm acrossall rhythm parameters. The peak current values for the PD andPY neurons that were used in the six experiments were $-$ 1.7 ± 0.33nA (PD neuron) and $-$ 1.4 ± 0.3 nA (PY neuron). These values aresimilar to the maximal current amplitudes in the current-voltagerelationships for these cells (see Fig. 5A). The mean experimentalvalues for the peak currents elicited from pressure applicationsof the peptides were $-$ 1.2 ± 0.7 nA (n = 8) for the PD neuron and $-$ 1.1 ± 0.5 nA (n = 12) for the PY neuron. The values used forthe artificial currents are a little larger than these becausewe were introducing the artificial current into only one of thetwo PD neurons and one of the PYneurons.

Figure 6A shows a representative example of the proctolin-elicited, CCAP-elicited, and artificial rhythms. To the right ofthese traces in Figure 6A, we plotted the measurements that arestatistically different for the proctolin- and CCAP-elicited rhythmsacross all experiments (see below). Figure 6B shows the phaserelationships for the rhythms shown in Figure 6A.

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Figure 6. The proctolin-elicited, CCAP-elicited, and artificial pyloric rhythms. The artificial rhythm is the rhythm produced in the presence of CCAP while the artificial "peptide" currents were being applied to the PD and PY neurons simultaneously. A, Extracellular recordings from STG motor nerves. Spike units for the different pyloric neurons are labeled. Some of the measured values from this experiment are shown to the right. These values are averages over longer portions of the traces shown. In this experiment, the number of spikes per burst of the PY neuron was measured directly from a PY neuron. All three sets of recordings are from the same preparation. lvn, Lateral ventricular nerve; pdn, pyloric dilator nerve; mvn, medial ventricular nerve. B, Phase relationships of the PD, LP, PY, and IC neurons derived from the traces in A. Measurements are the means ± SD. For this experiment, the peak current values for the artificial peptide currents were set at $-$ 1.8 nA for the PD neuron and $-$ 1.6 nA for the PY neuron. The CCAP concentration was 2 × 10⁷ M.

Figure 7A shows the mean values for the activity-related measurements that had statistically significant differences for theproctolin- and CCAP-elicited rhythms (n = 6). These values wereas follows: the duration of the PD neuron (p < 0.03), the numberof spikes per burst of the PD neuron (p < 0.001), the durationof the LP neuron (p < 0.001), the number of spikes per burst ofthe PY neuron (p < 0.01), and the overall frequency of the rhythm(p < 0.01). After the introduction of the artificial peptide currentsinto the PD and PY neurons, these values were statistically indistinguishablefrom those of the proctolin-elicited rhythm.

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Figure 7. Comparison of proctolin-elicited, CCAP-elicited, and the artificial rhythms. A, Comparison of the activity-related measurements across all experiments. Only the values found to be significantly different for the CCAP rhythm, as compared with the proctolin rhythm, are shown. B, The phase relationships averaged across all experiments. The on-time of the PD neuron was defined as phase zero. Measurements are the means ± SD (n = 6). All comparisons were made using a paired t test. * denotes p < 0.05. The concentrations of CCAP used in the experiments were the following: 1.5 × 10⁷, 2 × 10⁷, 3 × 10⁷, 3.5 × 10⁷, 5 × 10⁷, and 5 × 10⁷ M.

The phase plot of the average values for all experiments (n = 6) is shown in Figure 7B. The phase measurements that were statisticallydifferent between the proctolin and CCAP rhythms were the following:the off-phase of the PD neuron (p < 0.01), the off-phase of thePY neuron (p < 0.01), the on-phase of the IC neuron (p < 0.005),and the off-phase of the IC neuron (p < 0.05). With the introductionof the artificial peptide currents into the PD and PY neurons,only the differences in the off-phase of the PY neuron (p < 0.05)and the off-phase of the IC neuron (p < 0.01) remained statisticallysignificant compared with the values for the proctolin-elicitedrhythm. The values that were not statistically different betweenthe proctolin- and CCAP-elicited rhythms were also not differentin the artificialrhythm.

Rhythm changes because of the individual effects of the PD and PY neurons

The application of the peptide current to both the PD and PY neurons can change a CCAP-elicited rhythm into a proctolin-likerhythm. Which of the modifications in circuit output are a resultof altered activity in each of the two neurons? To address thisquestion, we also introduced the artificial peptide currents intothe PD and PY neurons individually to determine which circuitparameters each neuronaffected.

As might be expected, the introduction of the artificial current into the PD neuron (n = 6), in the presence of CCAP, significantlychanged the activity of the PD neuron. The off-phase of the PDneuron increased from 0.12 to 0.17 (p < 0.05), the burst durationof the PD neuron increased from 0.18 to 0.24 sec (p < 0.03), andthe number of spikes per burst of the PD neuron increased from3.1 to 7.0 (p < 0.001). The spike frequency of the LP neuron alsoshowed a slight decrease (26.0-25.1 Hz; p < 0.05), and the on-phaseof the PY neuron was delayed (0.59-0.67; p < 0.05). No other parameterschangedsignificantly.

Artificial current applied to the PY neuron (n = 5), in the presence of CCAP, significantly altered the measured values forthe duration of the LP neuron (0.60-0.47 sec; p < 0.03), the off-phaseof the LP neuron (0.72-0.66; p < 0.02), the duration of the PYneuron (0.42-0.57 sec; p < 0.05), and the number of spikes perburst of the PY neuron (8.3-14.8; p < 0.01).

The VD neuron was only weakly affected by proctolin in ongoing rhythms

Although the isolated VD neuron responds to proctolin, the VD neuron appeared to be affected only weakly by it during ongoingrhythms (data not shown). In 12 of 13 preparations, the VD neuronwas silent under control conditions. With the addition of proctolin,the VD neuron remained silent in six of these preparations andstarted firing weakly (one to two spikes per cycle) in the othersix. In the preparation in which the VD neuron was active undercontrol conditions, the spiking in the VD neuron only increasedfrom one to two spikes perburst.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Convergence, divergence, and redundancy

Why do nervous systems use a vast array of neuropeptides and amines to modulate the neural circuits that control behavior?The simplest assumption might be that each substance might havea dedicated role, to modulate either a certain current or synapse.It is now abundantly clear, however, that this simple assumptionis not true. In many nervous systems, multiple neuromodulatorysubstances converge onto the same current (Dunlap and Fischbach,1978; Jones, 1985; Christie and North, 1988; Nicoll et al., 1990;Brezina et al., 1994a,b; Sodickson and Bean, 1998; Swensen andMarder, 2000), and many neuromodulators have actions on multiplecurrents (Levitan, 1988, 1994; Nicoll et al., 1990; Kiehn andHarris-Warrick, 1992b; Kloppenburg et al., 1999).

To what extent are convergent neuromodulatory actions redundant for circuit dynamics? In this paper we demonstrate that anumber of neuropeptides that converge onto the same current inan individual neuron each activates a different subset of neuronswithin the pyloric circuit of the stomatogastric ganglion. A comparisonof two of these neuropeptides, proctolin and CCAP, shows thatthey evoke significantly different effects on the pyloric rhythm,as a consequence of their acting on different target neurons withinthe pyloric network. This demonstrates clearly that physiologicaleffects that appear to be redundant under certain assay conditionsmay elicit quite different actions when assayed on systems ofinteractingneurons.

Direct and indirect effects of modulator action

It is no surprise that neurons, which are directly excited by proctolin and CCAP when isolated, change their activity patternswhen these substances are applied to the whole network. For example,the LP neuron markedly increases its firing in both substances,as noted previously (Hooper and Marder, 1984; Marder et al., 1986;Weimann et al., 1997; Swensen and Marder, 2000), and is a directtarget of the peptides. However, even neurons that are not directtargets of a neuromodulator can change their activity patternas a consequence of circuit interactions (Hooper and Marder, 1987).This point is made very clearly in the dynamic-clamp experimentsin which addition of the artificial peptide current to only thePD and PY neurons results in major changes in the activity ofthe LPneuron.

Intuitively, the later off-phase of the PY neuron seen in the proctolin-elicited rhythms would appear to be caused directlyby the proctolin current in the PY neuron. Individually introducingthe artificial current into the PY neuron, however, did not haveany effect on the off-phase of the PY neuron, but the introductionof the artificial current into the PD neuron did cause a smalldelay in the off-phase of the PY neuron, although its effect wasnot strong enough to be statistically significant. The simultaneousaddition of the artificial current to both the PD and PY neuronswas necessary to get a robust delay in the off-phase of the PYneuron. This suggests that the PD and PY neurons are acting synergisticallyto bring about some of thechanges.

One of the most thorny problems in systems neuroscience is trying to evaluate the extent to which changes in circuit outputare a result of specific changes in one element or component ofthe circuit. Dynamic-clamp experiments, such as those reportedhere, can provide a tool with which to assess the significanceof any one portion of a circuit for the function of that circuit.For example, the pyloric frequency is higher in proctolin thanin CCAP. The PD neurons, which are electrically coupled to theAB pacemaker neuron, are direct targets for proctolin but areinsensitive to CCAP, suggesting that the frequency differencecould be simply attributable to the difference in the peptideaction directly on the PD-AB neuron pacemaker ensemble. Injectingthe artificial current into the PD neuron individually, however,did not significantly affect the overall rhythm frequency, butsimultaneous injections into the PD and PY neurons did significantlyincrease the overall frequency. This again suggests a synergisticeffect of the activation of the PD and PY neurons on the rhythmfrequency and illustrates that the PY neurons, which have no directinput to the pacemaker, can influence its frequency by virtueof their interactions with the LP neuron and other circuitelements.

How different are the proctolin and CCAP rhythms?

Previous work on the individual effects of proctolin and CCAP on the pyloric rhythm in C. borealis found that both peptidesincrease the burst duration and the number of action potentialsper burst in the LP neuron (Marder et al., 1986; Nusbaum and Marder,1989a,b; Weimann et al., 1997). Both peptides have state-dependenteffects on the pyloric frequency, generally speeding up the rhythmfor slower initial pyloric frequencies (0-0.7 Hz) and having littleor no effect for faster initial frequencies (0.7-1.5 Hz). Despiteall these similarities, the rhythms produced by proctolin andCCAP are quantitatively different. The LP neuron is more stronglyactivated in CCAP than in proctolin, and the PD neuron is stronglyactivated only in proctolin. In this study, we normalized forthe stronger activation of the LP neuron (by adjusting the concentrationof CCAP) and quantitatively described the remaining differencesby comparing a number of rhythm parameters. Thus, the statisticaldifferences we report here for these two neuropeptides are anunderestimate of the actual differences between the two rhythmsif they were compared at the same concentrations. Nonetheless,this procedure allowed us to focus on those effects not attributablesimply to the different extent of activation of the LP neuronin the twopeptides.

Bath application of neuromodulators

In this study we used bath application of neuropeptides to evoke "canonical" peptide rhythms. To what extent are these likelyto be the same as those rhythms induced in response to physiologicalrelease of these neuropeptides? Figure 2 shows the cell targetsfor each of the convergent peptides. These cell target diagramswould be those relevant to any substances released either fromlocal neurohemal-like terminals (Kilman and Marder, 1996) or hormonallythrough the hemolymph (Christie et al., 1995). In these casesall of the target neurons within the STG will "see" the releasedmodulator. All five of the peptides studied here are present hormonally,and CCAP is not found in modulatory projection neurons to theSTG but acts only as a neurohormone (Dircksen and Keller, 1988;Christie et al., 1995; Johnen et al., 1995; Dircksen, 1997). Incontrast, proctolin is released from three pairs of identifiedmodulatory projection neurons that each evoke a characteristicand different motor pattern when active (Blitz et al., 1999).Recent work argues that these different effects are not simplyattributable to the different cotransmitters found in these cellsbut also result from differential access of proctolin to the proctolinreceptors on different neurons (Wood et al., 2000).

Conclusions

It remains puzzling that the STG contains only 30 neurons, generates relatively simple motor patterns, but is modulated byat least 20 different substances (Marder and Weimann, 1992; Marderand Calabrese, 1996; Marder et al., 2001). Understanding fullythe manner in which physiologically different motor patterns areencoded in convergent and divergent modulator action will requireconsiderably more work. Nonetheless, the present results suggestthat understanding the mechanisms by which modulators with apparentlyredundant actions influence the larger circuits found in vertebrateswill require understanding, as in the STG, when modulator actionsresult from direct actions on specific target neurons and whenchanges in circuit function are an emergent property of modulatoraction at many sites within the circuit that together accountfor the final circuitoutput.

  FOOTNOTES

Received Feb. 9, 2001; revised March 15, 2001; accepted March 16, 2001.

This research was supported by National Institutes of Health Grant NS17813 and the W. M. KeckFoundation.
Correspondence should be addressed to Dr. Andrew M. Swensen, Department of Neurobiology, Harvard Medical School, 220 LongwoodAvenue, Boston, MA 02115. E-mail: andrew_swensen{at}hms.harvard.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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