Quantification of Cardiac Sac Network Effects on a Movement-Related Parameter of Pyloric Network Output in the Lobster

doi:10.1152/jn.00631.2002

Quantification of Cardiac Sac Network Effects on a Movement-Related Parameter of Pyloric Network Output in the Lobster

Jeff B. Thuma and Scott L. Hooper

Neuroscience Program, Department of Biological Sciences, Irvine Hall, Ohio University, Athens, Ohio 45701

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Thuma, Jeff B. and Scott L. Hooper. Quantification of Cardiac Sac Network Effects on a Movement-Related Parameter of Pyloric Network Output in the Lobster. J. Neurophysiol. 89: 745-753, 2003. Cardiac sac network activity (cycle period tens of seconds to minutes) has long been known to alter pyloric network activity(cycle period approximately 1 s), but these effects have not beenquantified. Some pyloric muscles extract cardiac sac timed variationsin pyloric motor neuron firing, and consequently produce cardiacsac timed movements even though no cardiac sac neurons innervatethem. Determining pyloric behavior therefore requires detaileddescription of cardiac sac effects on pyloric neural output. Pyloricmuscle activity correlates well with motor neuron overall spikefrequency (OSF, number of spikes per burst divided by cycle period).We therefore quantified the effects of cardiac sac activity onthe OSF of all pyloric neurons in the lobster, Panulirus interruptus.The ventricular dilator (VD) neuron had a biphasic response, withits OSF first increasing and then decreasing during cardiac sacbursts. Lateral pyloric (LP) neuron OSF decreased during cardiacsac activity. The pyloric (PY) neurons had two responses, withOSF either decreasing or increasing just after the beginning ofcardiac sac activity. The pyloric dilator (PD) neurons had a triphasicresponse, with OSF increasing slightly at the beginning of cardiacsac activity, decreasing during the cardiac sac burst, and stronglyincreasing after cardiac sac activity ended. The inferior cardiac(IC) neuron had a biphasic response, with OSF decreasing at thebeginning of cardiac sac activity and strongly increasing whencardiac sac activity ceased. These data provide the quantitativedescription of cardiac sac effects on pyloric activity necessaryto predict pyloric movement from pyloric neuraloutput.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

The pyloric network of the stomatogastric nervous system of decapod crustacea is a well-established model system for studyingneural network activity (Harris-Warrick et al. 1992). The neuralpattern the network produces, and many of the cellular and networkproperties underlying its activity, are well described. However,the movements the network produces remain unknown due to the internalposition and small size of the pylorus. In the absence of otherinformation, it was long assumed that the rapid (approximately1 Hz), triphasic pyloric neural pattern resulted in a similarlyrapid, triphasic movement pattern (Kennedy and Marder 1992; Maynardand Selverston 1975; Selverston et al. 1976; Turrigiano and Heinzel1992).

However, recent work has shown that many pyloric muscles relax much too slowly to accurately follow the pyloric neural pattern(Ellis et al. 1996; Harness et al. 1998; Koehnle et al. 1997;Morris and Hooper 1998a), and that some of these muscles extractlow-frequency changes in pyloric motor neuron firing that occurin-phase with another stomatogastric neural network, the cardiacsac network (Morris et al. 1999, 2000). These data indicate thatfor some pyloric muscles, cardiac sac timed contractions are alarge component of muscle output and thus add a previously unrecognizedimportance to these inter-networkinteractions.

Russell and Hartline (1981) first described the effects of an input to the pyloric network (the inferior ventricular nervethrough fibers, ivnTF) that alters pyloric cycle period and pyloricdilator (PD) neuron spike frequency. These ivnTF are part of thecardiac sac network (Dickinson and Marder 1989) and make a varietyof synapses onto pyloric network neurons (Claiborne and Selverston1984; Sigvardt and Mulloney 1982). Although this work showed thatcardiac sac activity profoundly alters pyloric network activity,these changes were not quantitatively described. We have quantitativelyanalyzed the effects of cardiac sac activity on one measure ofneuronal firing $---$ overall spike frequency (OSF, burst spike numberdivided by cycle period) $---$ that strongly correlates with muscleactivity (Morris and Hooper 1998a,b). This analysis shows thatcardiac sac activity alters the activity of all pyloric neuronsand provides the quantitative data necessary for predicting pyloricmovement from pyloric neuralactivity.

A preliminary report of these data has appeared in abstract form (Thuma and Hooper 1999).

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Panulirus interruptus (500-1,000 g) were obtained from Don Tomlinson Commercial Fishing (San Diego, CA) and maintained inaquaria with chilled (13-15°C), circulating, artificial seawater.Stomachs were dissected in the standard manner (Selverston etal. 1976), and preparations were continuously superfused with13-15°C Panulirus saline. Extracellular nerve recordings of pyloricnetwork activity were made using stainless steel pin electrodesand an A-M Systems amplifier. Intracellular neuronal recordingswere made with glass microelectrodes (filled with 0.55 M K₂SO₄,0.02 M KCl, resistance 10-20 M $Omega$ ) and an Axoclamp 2A or 2B. Datawere recorded on a MicroData Instruments DT-800 digital data recorderand transferred to computer using a Cambridge Electronics Design1401plus interface. Data were analyzed using scripts written inSpike II (Cambridge Electronics Design) and plotted using Kaleidagraph(Synergy Software). Figures were prepared in Canvas (Deneba Systems)and data interpolation was done with Origin 6 (Microcal). Allerror bars are standard deviation (SD) of the mean. The data shownhere are from sixexperiments.

Figure 1A is a schematic of the lobster stomach and stomatogastric nervous system (gray). The inset identifies the four regionsof the stomach: the esophagus, cardiac sac, gastric mill, andpylorus. The cardiac sac serves as a storage chamber for largepieces of food that are then passed to the gastric mill for chewing.The pylorus then filters the food for absorption, excretion, orrechewing. The somata of all pyloric neurons are located in thestomatogastric ganglion (STG). The neurons of the pyloric networkwere monitored either by intracellular recording from the neuron'ssoma or by extracellular recordings from the nerves in which theiraxons run (ventricular dilator (VD) and inferior cardiac (IC)neuron activity in the medial ventricular nerve (mvn), lateralpyloric (LP) neuron activity in the lateral ventricular nerve(lvn), and PD neuron activity in the pyloric dilator nerve (pdn)).Pyloric (PY) neuron activity was always recorded intracellularlybecause individual PY neuron activity cannot be distinguishedin extracellular recordings. Figure 1B shows the network connectionsbetween the cardiac sac and the pyloric networks. The ivnTF makean excitatory synapse onto the VD neuron which causes the VD neuronto fire with the cardiac sac network. The ivnTF have a complexsynapse onto the PD neurons that produces a compound PSP consistingof a fast excitatory postsynaptic potential (EPSP) followed bya slow inhibitory postsynaptic potential (IPSP) followed by aneven slower increase in burst amplitude and cycle period (Russelland Hartline 1981; Sigvardt and Mulloney 1982).

View larger version (20K):
[in this window]
[in a new window]

Fig. 1. The lobster stomach with nerves (gray) (A) and cardiac sac and pyloric synaptic connectivity diagrams (B). A: the stomach consists of 4 regions (inset), the esophagus, cardiac sac, gastric mill, and pylorus; lvn, lateral ventricular nerve; mvn, medial ventricular nerve; pdn, pyloric dilator nerve. B: ball and stick connections represent ionotropic inhibitory synapses; triangle and stick connections, ionotropic excitatory synapses; resistors, electrical coupling; diodes, rectifying electrical coupling. The cardiac sac network makes an excitatory ionotropic synapse onto the VD neuron and a complex synapse onto the PD neurons that produces a compound postsynaptic potential (PSP) consisting of a fast excitatory postsynaptic potential (EPSP) followed by a slow inhibitory postsynaptic potential (IPSP) followed by an even slower increase in burst generation properties. Abbreviations: AB, anterior burster; VD, ventricular dilator; PD, pyloric dilator; LP, lateral pyloric; PY, pyloric; IC, inferior cardiac; ivnTF, inferior ventricular nerve through fibers; CD1, CD2, Cardiac Dilator 1 and 2.

Figure 2A shows simultaneous recordings of the VD neuron and the cardiac sac network. The top two traces are extracellularivn and mvn recordings and show a cardiac sac burst; the medium-sizedspikes on the ivn are from the ivnTF and the large spikes on themvn from the VD neuron. Between cardiac sac bursts, the VD neuroncycles rhythmically with the pyloric network (left portion, mvntrace). The ivnTF excite the VD neuron, and strong ivnTF firinginduces the VD neuron to stop cycling rhythmically with the pyloricnetwork and fire a long tonic burst. The ivnTF show a variable,low-level firing activity between their high spike-frequency burstsand these bursts begin with a period of slowly increasing spikefrequency. The fibers also sometimes show low spike-frequency"bursts" that appear to slightly alter pyloric activity, but donot induce a long, nonpyloric burst in the VD neuron. To overcomethese difficulties, we used the beginning of the long VD neuronburst induced by cardiac sac activity to define cardiac sac bursts.In our experiments this change was unambiguous, and it establisheda threshold level of cardiac sac network activity necessary toqualify as a cardiac sac burst. Thirty pyloric cycles before andafter each cardiac sac burst were taken for data analysis. Thestart of the cardiac sac induced VD neuron burst was designatedas cycle 0 (triangle). The cycles before cycle 0 were numberedsequentially starting with $-$ 1 (closed circle) and the cycles aftercycle 0 were numbered sequentially starting with 1 (square). TheOSF of each cycle was calculated by dividing the number of spikesin the VD neuron burst by VD neuron cycle period. The inset showsan example: there are 11 spikes in the burst and the period is0.732 s. OSF for this burst is therefore 11/0.732 or 15 Hz. OSFwas similarly calculated for all pyloric neurons, with each neuron'sactivity being used to define its cycle period.

View larger version (35K):
[in this window]
[in a new window]

Fig. 2. Analysis of cardiac sac effects on VD neuron activity. A: extracellular recordings of ivnTF (medium-sized spikes) and VD neuron (large spikes) from the ivn and mvn, respectively. Cardiac sac activity was defined as beginning when the VD neuron began to fire tonically (cycle 0, triangle here and in B and C). Pyloric cycles were numbered sequentially ( $-$ 1, circle; 1, square) relative to cycle 0. Inset: overall spike frequency (OSF) calculation. For each cycle period (as defined by the neuron's own activity), OSF equals burst spike number divided by cycle period. B: OSF vs. cycle number. Note that, since the varying durations of the various cycles are not being accounted for, this plot is not equivalent to OSF vs. time relative to cardiac sac beginning. C: OSF vs. time relative to cardiac sac beginning. D and E: plots of VD neuron OSF in 6 cardiac sac bursts vs. cycle number (D) and time relative to cardiac sac beginning (E). In both plots the cycle 0 data points are marked with open circles. See METHODS for explanation of averaging in and across experiments.

Figure 2B shows OSF plotted against cycle number for each VD neuron cycle in Fig. 2A. Although this plotting method accuratelyportrays OSF as a function of cycle number, it does not do soas a function of time because cycle period is not constant and,more importantly, because of the very long VD neuron burst thatoccurs during cardiac sac activity (in the example at hand, cycle0 occurs only 1 s after cycle $-$ 1, but cycle 1 occurs 12 s aftercycle 0). The OSF of each cycle was therefore plotted vs. timerelative to the beginning of cardiac sac activity Fig. 2C. Figure2D shows the OSF for six cardiac sac bursts from one experimentplotted against cycle number; Fig. 2E shows the same data plottedvs. time relative to the beginning of cardiac sac activity. Onceall cardiac sac bursts had been plotted, average OSF and timerelative to cardiac sac beginning in each experiment were foundby averaging the OSFs and relative times of equal numbered cycles(i.e., the OSFs and relative times of all cycle 0s were averaged,of all cycle 1s, etc.).

Calculating each neuron's overall average across experiments required several additional steps. First, it was necessary tonormalize the data since different experiments had different baselineOSFs. Each experiment's average baseline OSF was determined byaveraging OSF across cycles $-$ 30 to $-$ 15. This average was subtractedfrom all data in that experiment to normalize OSF to 0 Hz. Second,in different experiments individual cycles occurred at differenttimes relative to cardiac sac beginning (for instance, in oneexperiment, cycle 1 might occur 10 s after cardiac sac beginning,and in another, cycle 1 might occur 14 s after cardiac sac beginning).To obtain a complete set of data points at each time to average(that is, to have data from all experiments at time 0, 0.1, 0.2s, etc.), we linearly interpolated (step size 0.1 s) between eachexperiment's datapoints.

Third, in different experiments the most salient response of the neuron might occur at different times after the beginningof cardiac sac activity (except for the VD neuron because itsactivity was used to define cardiac sac activity). For instance,for the PY neurons that responded to cardiac sac activity withexcitation (Fig. 5A), in one experiment the increase might occur0 s after the beginning of cardiac sac activity, but in anotherat 0.5 s after the beginning. Given the steepness of the responsesof many of the pyloric neurons, this would have resulted in peakvalues in one experiment being averaged with baseline values ofanother. To overcome this difficulty, the appropriate value wasadded to all the time points of each experiment to make the mostsalient feature of their response occur at time 0 (for the PD,IC, and excited PY neurons, the maximum of the excitation; forthe LP and inhibited PY neurons, the minimum of the inhibition).This procedure resulted in the OSF plot of each experiment beingput into register such that the most salient feature of the responseoccurred at the same time. The interpolated OSF values at eachtime point were then averaged. The average was then placed relativeto cardiac sac activity by averaging the values that had beenadded to each experiment's time axis to make the time of the mostsalient feature zero. For example, the four experiments that comprisethe LP overall average had to be adjusted -0.54, +2.45, +0.66,and -0.89 s to make the minima of the LP neuron response in eachexperiment's average occur at time 0. The mean of those timesis 0.42 ± 1.5 s. Therefore the minimum of the LP inhibition occurredat an average time of 0.42 s after the beginning of cardiac sacactivity. The horizontal error bar present in each neuron's averageplot is the SD of these times and shows the variation with whichthe neuron response occurred relative to the beginning of cardiacsac activity. This procedure is the equivalent of the pattern-basedanalysis performed in Thuma and Hooper (2002). However, becausethe delay to most salient response feature was constant insideeach individual experiment, it did not need to be performed oneach cardiac sac burst, but only to average the data acrossexperiments.

Fourth, due to the different VD neuron burst lengths during the cardiac sac bursts and the different pyloric cycle periodspresent in the various experiments, ±30 cycles correspond to differentduration ranges in different experiments. For instance, in experimentA ±30 cycles might correspond to a duration range of $-$ 19 s to+20 s, while in experiment B ±30 cycles might correspond to aduration range of $-$ 25 s to +25 s. Experiment A thus has no datato average with the data from time $-$ 25 to $-$ 19 s, and time +20to +25 s, in experiment B. Therefore in the across experimentaverages, OSFs and relative times were averaged only for interpolationpoints that had data from at least four of the six experiments.The average baselines of all experiments were then averaged andthis value was added to the normalized average OSF to give thetrue averageOSF.

The statistical significance of pyloric neuron responses to cardiac sac activity were assessed by Student's t-test (paireddata) comparison performed in Kaleidagraph between the data pointat the time of interest (e.g., the peak VD neuron OSF in Fig.3B) and an average of several seconds of control data before thecardiac sac burst.

View larger version (27K):
[in this window]
[in a new window]

Fig. 3. VD neuron response to cardiac sac activity is an OSF increase followed by a decrease. A: extracellular VD neuron recording from the ventricular dilator nerve (vdn). B: across experiment average of VD neuron OSF vs. time relative to cardiac sac beginning.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

We measured the OSF of all pyloric neurons for 30 pyloric cycles before cardiac sac activity, during the cardiac sac burst,and for 30 pyloric cycles after the burst, using the long, high-frequencyburst induced in the VD neuron by ivnTF firing as a monitor ofcardiac sac activity. The VD neuron had a biphasic response, withits OSF first increasing and then decreasing during cardiac sacbursts. Figure 3A shows an extracellular recording from the ventriculardilator nerve (vdn), a branch of the mvn containing only the VDneuron's axon; Fig. 3B shows the VD neuron across experiment OSFaverage (n = 5, 27 cardiac sac bursts). VD neuron OSF significantlyincreased from a baseline value of 16 to 25 Hz at the beginningof cardiac sac activity (P < 0.004).

VD neuron OSF decreased to 10 Hz at the end of cardiac sac activity, but this decrease was not significant when the OSF valuesof the individual experiments at the time of the minimum in theaveraged data were compared with control values. However, in oneof these experiments the cardiac sac burst was longer than inthe others. As a consequence, the trough of this experiment wasat a later time than those of the other experiments, and, thetrough shown thus underestimates the true magnitude of the decrease(note large error bars on the trough data points). For the statisticalcomparison of trough and control values, when the true minimumOSF of the experiment with the long cardiac sac burst was used,the trough differed from control (P < 0.006). VD neuron OSF didnot return to baseline for 20-150 s (mean, 53 ± 33s).

LP neuron OSF decreased during cardiac sac activity. Figure 4A shows an extracellular lvn recording of LP neuron activity(all non-LP neuron spikes have been removed for clarity). Thebar above the trace represents cardiac sac activity. For the LPneuron, as well as the PY, PD, and IC neurons, cycle 0 (asterisk)was defined as the first cycle after the beginning of cardiacsac activity. Figure 4B shows the LP neuron across experimentOSF average (n = 4, 22 cardiac sac bursts). LP neuron OSF sharplyand significantly (P < 0.006) decreased from 12 to 7 Hz at thebeginning of cardiac sac activity and returned to baseline valueswithin 10 s after the end of cardiac sac activity.

View larger version (23K):
[in this window]
[in a new window]

Fig. 4. LP neuron response to cardiac sac activity is an OSF decrease. A: extracellular LP neuron recording from the lvn. Bar represents cardiac sac burst. For this neuron and the PY, PD, and IC neurons, cycle 0 (asterisk) was defined as the first cycle after the beginning of cardiac sac activity. B: across experiment average of LP neuron OSF vs. time relative to cardiac sac beginning.

Two PY neuron responses to cardiac sac activity (Fig. 5A, bars) were observed. The first was to fire a long, high-frequencyburst during the cardiac sac burst (Fig. 5A, left); the otherwas to be inhibited during cardiac sac activity (Fig. 5A, right).Figure 5B shows the across experiment OSF averages for both typesof PY neurons (n = 5, 8 cardiac sac bursts for the excited PY;n = 4, 22 cardiac sac bursts for the inhibited PY); the excitedPY neuron's OSF increased from 8 to 12 Hz and the inhibited PYneuron's OSF decreased from 7 to 2 Hz during cardiac sac activity.Both changes were significant (P < 0.007 and P < 0.03, respectively).

View larger version (38K):
[in this window]
[in a new window]

Fig. 5. PY neurons had two responses to cardiac sac activity, an OSF increase (left) and a decrease (right). A: intracellular PY neuron recordings. Bars represent cardiac sac bursts. B: across experiment averages of PY neuron OSF vs. time relative to cardiac sac beginning.

The PD neurons also had two responses to cardiac sac activity (bars, Fig. 6, A and B). In the first, PD neuron cycle periodand intra-burst spiking were altered during the cardiac sac burstbut the pyloric rhythm nonetheless continued (Fig. 6A); OSF decreasedfrom 11 to 4 Hz at the onset of cardiac sac activity and stronglyincreased to 22 Hz immediately after it (Fig. 6A, plot). Figure6B shows the second response, in which the PD neurons stoppedfiring during cardiac sac activity and then fired a large reboundburst on cardiac sac cessation; OSF decreased from 10 to 3 Hzat the onset of cardiac sac activity and strongly increased to20 Hz immediately after (Fig. 6B, plot). Thus, despite the differentvisual appearances of these two responses, with respect to theOSF changes at the start and end of cardiac sac activity, theywere very similar.

View larger version (18K):
[in this window]
[in a new window]

Fig. 6. PD neurons had 2 visually different, but OSF similar, responses to cardiac sac activity. A: PD neuron continues to burst throughout cardiac sac burst (bar). OSF decreases early in the cardiac sac burst and then increases. B: PD neuron stops firing during the cardiac sac burst (bar). OSF again decreases early in the cardiac sac burst and then increases. In both A and B the top panel is an intracellular PD neuron recording and the bottom panel is the corresponding OSF vs. time relative to cardiac sac beginning plot.

VD, LP, and PY neuron cardiac sac responses correlated well with the beginning of cardiac sac activity. However, the responsesof the PD and IC neurons did not. Figure 7A shows the responsesof a PD neuron for all cardiac sac bursts in one experiment (left)and the average across the experiment (right) when plotted againsttime relative to the beginning of cardiac sac activity. The peaksand troughs for each trace are not well aligned. Consequently,averaging the data in this reference frame averaged peaks withtroughs, which resulted in an underrepresentation of the individualresponses and large SD (Fig. 7A, right). This was true of theIC neuron as well (data not shown). Using the end of cardiac sacactivity as a reference point resulted in the peaks and troughsof the data aligning very well (Fig. 7B, left), and an averagethat better reflected the individual responses and had much smallerSD (Fig. 7B, right).

View larger version (26K):
[in this window]
[in a new window]

Fig. 7. PD neuron response is better averaged relative to cardiac sac burst ending. A: 6 PD neuron responses plotted vs. time relative to cardiac sac beginning (left) and their average (right). B: same 6 PD neuron responses plotted vs. time relative to cardiac sac ending (left) and their average (right). Note decreased SD, and more accurate capture of the shape of the individual responses, in B vs. A. IC neuron response was also more accurately captured when averaged relative to cardiac sac ending (data not shown). C: PD neuron response to cardiac sac activity is a triphasic increase-decrease-increase in OSF.

Figure 7C shows the PD neuron across experiment OSF average (n = 6, 32 cardiac sac bursts); both PD neuron response types(Fig. 6) were included in this average because of their similarOSF changes. PD neuron OSF increased from 9 to 11 Hz at the beginningof the cardiac sac burst, decreased to 7 Hz during the burst,and increased to 19 Hz after it. The late OSF increase was significant(P < 0.002), but the other two changes were not (P < 0.42, trough;P < 0.16, first peak). Unlike the VD neuron, this was not dueto cardiac sac burst duration changes resulting in peaks, troughs,and control data being averaged together, but because in two experimentsneither the first peak nor the trough were present. As noted inDISCUSSION, these changes in PD neuron response presumably reflectthe PD neuron's complex response to cardiac sac activity (Russelland Hartline 1981; Sigvardt and Mulloney 1982) and differencesin ivnTF firing in the differentexperiments.

The IC neuron had a biphasic response, with its OSF decreasing at the beginning of cardiac sac activity and strongly increasingwhen cardiac sac activity ceased. Figure 8A shows an extracellularrecording from the inferior cardiac nerve (icn), a branch of themvn containing only the IC neuron's axon; Fig. 8B shows the ICneuron across experiment OSF average (n = 5, 27 cardiac sac bursts).IC neuron OSF decreased from 6 to 4 Hz at the beginning of thecardiac sac activity and increased to 11 Hz afterward, takingsome 10-20 s to return to baseline. Both changes were significant(P < 0.01, P < 0.0006, respectively).

View larger version (20K):
[in this window]
[in a new window]

Fig. 8. IC neuron response to cardiac sac activity is a biphasic OSF decrease followed by an increase. A: extracellular IC neuron recording from the inferior cardiac nerve (icn). Bar represents cardiac sac burst. B: across experiment average of IC neuron OSF vs. time relative to cardiac sac ending.

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

We performed a quantitative analysis of the variation of pyloric neuron OSF as a function of cardiac sac activity. Figure9 summarizes the effects of cardiac sac activity on pyloric networkactivity; the PD and IC neuron traces have been time-shifted tocompensate for using cardiac sac ending instead of beginning astheir reference point. The numbers to the left of each trace areeach neuron's average baseline OSF; the bar at the bottom is theaverage duration of the cardiac sac bursts from the 6 experimentsused. The VD neuron has a biphasic response consisting of an initialOSF increase followed by a decrease. The LP and one type of PYneuron respond with a simple OSF decrease, and the other typeof PY neuron with a simple OSF increase. The PD neuron has a triphasicincrease-decrease-increase response and the IC neuron has biphasicresponse consisting of an OSF decrease followed by a prolongedincrease. The return to baseline OSF levels for all neurons exceptthe PY neurons is slow (10-20 s).

View larger version (19K):
[in this window]
[in a new window]

Fig. 9. Summary of all pyloric neuron responses to cardiac sac activity. PD and IC neuron responses have been time shifted to compensate for being averaged relative to cardiac sac ending. The VD neuron response is a biphasic OSF increase followed by a decrease. The LP and 1 type of PY neuron respond with an OSF decrease, and the other type of PY neuron responds with an OSF increase. The PD neuron has a triphasic increase-decrease-increase response and the IC neuron response is a biphasic OSF decrease followed by a prolonged increase. The return to baseline OSF levels for all neurons except the PY neurons takes 10-20 s.

Choice of VD neuron as a monitor of cardiac sac activity

The VD neuron is a follower of cardiac sac activity, but does not help generate the cardiac sac rhythm. We nonetheless believethat, particularly since we are concerned here with the effectsof cardiac sac activity on pyloric network output, using the VDneuron as a monitor of cardiac sac activity is highly appropriate.ivnTF bursts often begin with a variable period of low-frequencyfiring, and it is unclear when in this firing ivnTF spike frequencyis sufficient to begin to alter pyloric activity. This concernis well demonstrated in the ivn trace in Fig. 2A, in which thefirst ivnTF spike occurs almost 4 s before the VD neuron beginsto fire tonically, and there is a 2 s period of low-frequencyivnTF firing in which, although VD neuron OSF increases somewhat(Fig. 2B, cycle -1), the VD neuron does not fire tonically. Comparisonof different cardiac sac bursts shows considerable variation inthe details of ivnTF firing at the beginning of ivnTF bursts,and in when the VD neuron begins to fire tonically relative tothe first ivnTF spike. Using the first spike of ivnTF bursts asa monitor would thus induce considerable variation in which pyloriccycle was chosen as the 0 cycle, and the alternative of choosinga particular ivnTF spike frequency to define ivnTF burst beginningseemed arbitrary. Using a pyloric network neuron as a monitorof cardiac sac activity obviated these difficulties by ensuringthat, regardless of the details of ivnTF firing, we were alwaysmeasuring cardiac sac activity from the time at which cardiacsac activity was great enough to change pyloric activity. TheVD neuron was an obvious choice due to its particularly well-definedresponse (tonic firing) to cardiac sac activity. It is clear,however, that this reference point is actually slightly subsequentto the true time at which ivnTF firing becomes sufficient to alterpyloric activity, as small changes in pyloric neuron activityoccur before tonic VD neuron firing begins (Fig. 9), which correspondto the low spike-frequency portion of the ivnTFburst.

Cellular basis of cardiac sac effects on pyloric activity

In the pyloric network, the changes an input induces in a given pyloric neuron's activity often do not occur because the inputhas direct effects on the neuron, but rather because the inputdirectly alters the activity of other pyloric neurons, and thesechanges in turn change the activity of nondirectly affected neurons(Hooper and Marder 1987; Hooper and Moulins 1990). Considerationof the known cardiac sac synaptic connections to the pyloric network,and of the pyloric network's connectivity pattern (Fig. 1), suggeststhat this may be the case for some cardiac sac effects as well.The cardiac sac effects described here on the VD and PD neuronsare consistent with the strong excitatory synapses the ivnTF makeon the VD neuron, and the complex excitatory-inhibitory-delayedslow excitatory synapses they make on the PD neurons (Claiborneand Selverston 1984; Russell and Hartline 1981; Sigvardt and Mulloney1982). No direct connections from cardiac sac neurons to any otherpyloric neuron, however, are known. Some of the cardiac sac effectson these other neurons can be explained as indirect consequencesof changes in VD and PD neuron activity. For instance, the LPand PY neurons are inhibited by the VD, PD, and AB neurons (theAB neuron fires with the PD neurons). Thus LP and PY neuron inhibitionduring cardiac sac bursts may be due to increased inhibition fromthe excitatory portions of the VD and PD neuron responses to cardiacsac activity. The IC neuron inhibition during the cardiac sacburst may similarly be due to inhibition from the VD neuron, andits initial increase in firing after the cardiac sac burst frompostinhibitory rebound. The source of its subsequent long-lastingincrease in activity, however, is unclear. The excitatory PY neuronresponse is also difficult to explain as arising from an indirect,intra-pyloric network mechanism. It is thus possible that as yetundescribed cardiac sac inputs exist to theseneurons.

Multiple PY neuron responses

Although it is clear there are two PY neuron responses, we never observed a PY neuron switch its response type. However, wealso never observed PY neurons of both response types in a singlepreparation. It is thus an open question whether the two responsesobserved arise from two classes of PY neurons or from preparation-specificchanges in PY neuron responsiveness or cardiac sac input properties.Hartline et al. (1987) identified two PY neuron types, PY earlyand PY late neurons. We routinely identify, when possible, PYneurons using the Hartline et al. classification; the differentPY neuron responses to cardiac sac input are not a function ofwhether the neuron is a PY late or earlyneuron.

Multiple PD neuron responses

Unlike the PY neurons, there is no evidence that the two PD neurons differ in terms of cellular properties and synaptic outputand input patterns. The two PD neuron responses therefore almostcertainly arise either from the PD neurons being in differentstates in different preparations or from changes in ivnTF firingin different cardiac sac bursts. Sigvardt and Mulloney (1982)noted that PD neuron responses would vary in the manner shownin Fig. 6 depending on whether the ivnTF fired at low (Fig. 6A)or high (Fig. 6B) frequency. In our data set each PD neuron expressedonly one type of response. However, in each of the experimentscardiac sac burst spike frequency and duration (as reflected inVD neuron activity) were quite regular from burst to burst, andthus differences in PD neuron response inside an experiment wouldnot be expected. Comparison across experiments of the VD neuronbursts associated with Fig. 6, A and B, responses showed no obviouscorrelation of VD neuron spike frequency or burst duration withresponse type. However, although VD neuron bursts are a good monitorof the beginning and ending of ivnTF activity, they may not befor ivnTF spike frequency. It is thus very possible that the twoPD neuron responses arise from changes in ivnTF activity thatVD neuron firing does notreflect.

On a more general level, it is important to stress again that, even though in the one case the PD neurons continue to burstduring cardiac sac activity, and in the other the neurons stopbursting, OSF variation (and thus likely muscle activity, Morrisand Hooper 1998a) is similar in both. This observation highlightsthe fact that responses that differ in some characteristics (forinstance, burst patterning) may be similar in others (OSF), andthat to assess properly whether different presynaptic activitieswill generate different postsynaptic responses it is essentialto know which characteristics determine postsynaptic partner response.For example, in the case at hand, the PD neurons make synapsesboth onto pyloric muscles and on neurons inside the pyloric network.It is thus possible that the responses in Fig. 6, A and B, couldbe identical on the muscle level (because changes in OSF, notburst patterning, primarily determine muscle response to PD neuronactivity), but nonetheless elicit different responses centrally(because the patterning of PD neuron activity, not just its OSF,helps determine response for postsynaptic neuronaltargets).

Reference frame

We have noted elsewhere the importance of correct reference frame selection for accurate representation, and even simple recognition,of neuronal activity changes (Hooper 1997; Thuma and Hooper 2002).The need in the present data to use the ending of cardiac sacactivity to accurately capture the changes in PD (Fig. 7) andIC neuron activity is another example of this phenomenon. Unfortunately,we know of no a priori method of correctly choosing a referenceframe and have always relied on comparing individual and averageddata in different reference frames to select the best frame. Thismethod is time-consuming and tedious. However, the improvementin data averaging produced by choosing the correct reference framecan be dramatic (right panels of Fig. 7, A and B) and suggeststhat reference frame selection should be a general concern inanalyzing data where multiple reference frames are possible. Onthis issue, it is also important to stress that, of course, referenceframe selection must be in some way related to the source thatis inducing the neuronal change of interest. For instance, inthe case at hand reference frame must be selected relative tocardiac sac burst, and it is essential if a repeating patternof neuron response (e.g., the triphasic PD neuron response) isused to identify the reference frame, that this response neveroccur without the source being active (which is true for all datareported here). That said, however, whether to use the beginning,middle, end, or other time relative to the burst to define thereference frame can only be chosen by determining in which referenceframe the timing of the response is mostrepeatable.

On the neurobiological level, the fact that the PD and IC neurons are best analyzed with respect to the end of cardiac sacactivity, and the other neurons with respect to the beginningof cardiac sac activity, presumably reflects some difference inthe mechanisms of cardiac sac action. With respect to the changesin the various neurons that occur during the cardiac sac bursts,it is unclear to us why one frame would be better than the other.However, both the PD and the IC neurons, and only the PD and ICneurons, show large activity increases after the cardiac sac bursts.The mechanisms underlying these increases are likely different[for the PD neurons the increase is due to both postinhibitoryrebound and an increase in PD neuron intrinsic "burstiness," Russelland Hartline (1981), whereas for the IC neuron it may be due toonly postinhibitory rebound]. However, in each case neither increasecan be fully expressed until the cardiac sac burst is over (becauseof the ivnTF inhibition for the PD neurons and the VD neuron inhibitionfor the IC neurons). With respect to the late increase in PD andIC neuron OSF, it is thus not surprising that cardiac sac endingis a better referenceframe.

Implications for relating pyloric neural activity to pyloric behavior

The pyloric neural network is among the best understood of all neural networks, and yet, due to the internal location of thelobster stomach and small size of the pylorus, the behavior itgenerates is almost completely unknown. Without technical advancesin noninvasive imaging, this inability to directly measure pyloricbehavior is likely to continue. As such, at present the only meansby which pyloric neural activity and behavior are likely to belinked is by computer modeling of the pyloric anatomy and by usingdata on pyloric muscle response to neural input to simulate pyloricmotions (Geier et al. 2002; Hoover et al. 2001; Morris and Hooper1998a,b, 2001; Morris et al. 1999, 2000). We have shown that thechanges in pyloric neuron OSF reported here are sufficient tochange pyloric muscle contractions (Morris et al. 1999, 2000)and are developing models of pyloric muscles that predict contractionin response to physiological neuronal activity (Geier et al. 2002).The present quantitative description of cardiac sac effects, andearlier work quantifying gastric mill effects, on pyloric neuronalactivity (Thuma and Hooper 2002) provide the data necessary todrive these models and thus are necessary steps toward linkingneuronal activity and behavior in thissystem.

	FOOTNOTES

Address for reprint requests: S. L. Hooper, Neuroscience Program, Department of Biological Sciences, Irvine Hall, Ohio University,Athens, OH 45701 (E-mail: hooper{at}ohio.edu).

REFERENCES

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Claiborne BJ, and Selverston AI. Histamine as a neurotransmitter in the stomatogastric nervous system of the spiny lobster. J Neurosci 4: 708-721, 1984[Abstract].
Dickinson PS, and Marder E. Peptidergic modulation of a multioscillator system in the lobster. I. Activation of the cardiac sac motor pattern by the neuropeptides proctolin and red pigment-concentrating hormone. J Neurophysiol 61: 833-844, 1989[Abstract/Free Full Text].
Ellis TA, Donath AS, Morris LG, Thuma JB, and Hooper SL. Motor pattern expression of a lateral pyloric constrictor muscle. Soc Neurosci Abstr 22: 131, 1996.
Geier CF, Hobbs KH, and Hooper SL. Modeling p1 (LP neuron) muscle isometric motor activity. Soc Neurosci Abstr 23: 2002, 2002.
Harris-Warrick RM, Marder E, Selverston AI, and Moulins M. Dynamic Biological Networks: The Stomatogastric Nervous System., Cambridge, MA: MIT Press, 1992.
Harness PI, Morris LG, and Hooper SL. Intrinsic pyloric muscle output predicted from constant duty cycle rhythmic neural input. Soc Neurosci Abstr 24: 1891, 1998.
Hartline DK, Gassie DV, and Sirchia CD. In: PY cell types in the stomatogastric ganglion of Panulirus. In: The Crustacean Stomatogastric System,, edited by Selverston AI, and Moulins M. Berlin: Springer-Verlag, 1987, p. 75-77.
Hooper SL. The pyloric pattern of the lobster (Panulirus interruptus) stomatogastric ganglion comprises two phase maintaining subsets. J Comput Neurosci 4: 207-219, 1997[ISI][Medline].
Hooper SL, and Marder E. Modulation of the lobster pyloric rhythm by the peptide, proctolin. J Neurosci 7: 2097-2112, 1987[Abstract].
Hooper SL, and Moulins M. Flexibility in the stomatogastric nervous system of the lobster. II. Synaptic and cellular mechanisms responsible for a long lasting restructuring of the pyloric network. J Neurophysiol 64: 1574-1589, 1990[Abstract/Free Full Text].
Hoover N, Weaver AL, Harness PI, and Hooper SL. Combinatorial and cross-fiber averaging transform muscle electrical responses with a large random component into deterministic contractions. J Neurosci 22: 1895-1904, 2002[Abstract/Free Full Text].
Kennedy MB, and Marder E. Cellular and molecular mechanisms of neuronal plasticity. In: An Introduction to Molecular Neurobiology, edited by Hall ZH. Sunderland, MA: Sinauer Associates, Inc., 1992, p. 463-495.
Koehnle TJ, Morris LG, Thuma JB, and Hooper SL. Motor activity of the pyloric and cardiac sac network-innervated cv1 muscle. Soc Neurosci Abstr 23: 477, 1997.
Maynard DM, and Selverston AI. Organization of the stomatogastric ganglion of the spiny lobster. IV. The pyloric system. J Comp Physiol 100: 161-182, 1975.
Morris LG, and Hooper SL. Muscle response to changing neuronal input in the lobster (Panulirus interruptus) stomatogastric system: slow muscle properties can transform rhythmic input into tonic output. J Neurosci 18: 3433-3442, 1998a[Abstract/Free Full Text].
Morris LG, and Hooper SL. Predicting pyloric dilator muscle contractions as duty cycle is varied. Soc Neurosci Abstr 24: 1891, 1998b.
Morris LG, and Hooper SL. Mechanisms underlying stabilization of temporally summated muscle contractions in the lobster (Panulirus interruptus) pyloric system. J Neurophysiol 85: 254-268, 2001[Abstract/Free Full Text].
Morris LG, Thuma JB, and Hooper SL. Pyloric muscles can express gastric and cardiac sac contraction patterns despite pyloric-timed motor neuron firing. Soc Neurosci Abstr 25: 1642, 1999.
Morris LG, Thuma JB, and Hooper SL. Muscles express motor patterns of non-innervating neural networks by filtering broad-band input. Nat Neurosci 3: 245-250, 2000[ISI][Medline].
Russell DF, and Hartline DK. A multiaction synapse evoking both EPSPs and enhancement of endogenous bursting. Brain Res 223: 19-38, 1981[ISI][Medline].
Selverston AI, Russell DF, Miller JP, and King DG. The stomatogastric nervous system: structure and function of a small neural network. Prog Neurobiol 7: 215-290, 1976[Medline].
Sigvardt KA, and Mulloney B. Properties of synapses made by IVN command-interneurones in the stomatogastric ganglion of the spiny lobster Panulirus interruptus. J Exp Biol 97: 153-168, 1982[Abstract/Free Full Text].
Thuma JB, and Hooper SL. Quantitative description of the changes in pyloric network output associated with gastric and cardiac sac activity. Soc Neurosci Abstr 25: 1641, 1999.
Thuma JB, and Hooper SL. Quantification of gastric mill network effects on a movement related parameter of pyloric network output in the lobster. J Neurophysiol 87: 2372-2384, 2002[Abstract/Free Full Text].
Turrigiano GG, and Heinzel H-G. Behavioral correlates of stomatogastric network function. In: Dynamic Biological Networks. The Stomatogastric Nervous System, edited by Harris-Warrick RM, Marder E, Selverston AI, and Moulins M. Cambridge, MA: MIT Press, 1992, p. 197-220.

This article has been cited by other articles:

D. Bucher, A. L. Taylor, and E. Marder
Central Pattern Generating Neurons Simultaneously Express Fast and Slow Rhythmic Activities in the Stomatogastric Ganglion
J Neurophysiol, June 1, 2006; 95(6): 3617 - 3632.
[Abstract] [Full Text] [PDF]

A. Mamiya, Y. Manor, and F. Nadim
Short-Term Dynamics of a Mixed Chemical and Electrical Synapse in a Rhythmic Network
J. Neurosci., October 22, 2003; 23(29): 9557 - 9564.
[Abstract] [Full Text] [PDF]

A. L. Weaver and S. L. Hooper
Relating Network Synaptic Connectivity and Network Activity in the Lobster (Panulirus interruptus) Pyloric Network
J Neurophysiol, October 1, 2003; 90(4): 2378 - 2386.
[Abstract] [Full Text] [PDF]

J. B. Thuma, L. G. Morris, A. L. Weaver, and S. L. Hooper
Lobster (Panulirus interruptus) Pyloric Muscles Express the Motor Patterns of Three Neural Networks, Only One of Which Innervates the Muscles
J. Neurosci., October 1, 2003; 23(26): 8911 - 8920.
[Abstract] [Full Text] [PDF]

This Article

Abstract

Full Text (PDF)

Alert me when this article is cited

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in ISI Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via ISI Web of Science (6)

Citing Articles via Google Scholar

Google Scholar

Articles by Thuma, J. B.

Articles by Hooper, S. L.

Search for Related Content

PubMed

PubMed Citation

Articles by Thuma, J. B.

Articles by Hooper, S. L.

				A. Mamiya, Y. Manor, and F. Nadim Short-Term Dynamics of a Mixed Chemical and Electrical Synapse in a Rhythmic Network J. Neurosci., October 22, 2003; 23(29): 9557 - 9564. [Abstract] [Full Text] [PDF]

				A. L. Weaver and S. L. Hooper Relating Network Synaptic Connectivity and Network Activity in the Lobster (Panulirus interruptus) Pyloric Network J Neurophysiol, October 1, 2003; 90(4): 2378 - 2386. [Abstract] [Full Text] [PDF]

				J. B. Thuma, L. G. Morris, A. L. Weaver, and S. L. Hooper Lobster (Panulirus interruptus) Pyloric Muscles Express the Motor Patterns of Three Neural Networks, Only One of Which Innervates the Muscles J. Neurosci., October 1, 2003; 23(26): 8911 - 8920. [Abstract] [Full Text] [PDF]

Quantification of Cardiac Sac Network Effects on a Movement-Related Parameter of Pyloric Network Output in the Lobster

0022-3077/03 $5.00 Copyright © 2003 The American Physiological Society