Long-Term Neuromodulatory Regulation of a Motor Pattern-Generating Network: Maintenance of Synaptic Efficacy and Oscillatory Properties

doi:10.1152/jn.00482.2001

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Long-Term Neuromodulatory Regulation of a Motor Pattern-Generating Network: Maintenance of Synaptic Efficacy and Oscillatory Properties

Muriel Thoby-Brisson and John Simmers

Laboratoire de Neurobiologie des Réseaux, Université Bordeaux 1 and Centre National de la Recherche Scientifique, Unité Mixte de Recherche 5816, 33405 Talence, France

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Thoby-Brisson, Muriel and John Simmers. Long-Term Neuromodulatory Regulation of a Motor Pattern-Generating Network: Maintenance of Synaptic Efficacy and Oscillatory Properties. J. Neurophysiol. 88: 2942-2953, 2002. Rhythm generation by the pyloric motor network in the stomatogastric ganglion (STG) of the spiny lobster requires permissiveneuromodulatory inputs from other central ganglia. When theseinputs to the STG are suppressed by cutting the single, mainlyafferent stomatogastric nerve (stn), pyloric neurons cease toburst and the network falls silent. However, as shown previously,if such a decentralized quiescent ganglion is maintained in organculture, pyloric network rhythmicity returns after 3-4 days and,although slower, is similar to the motor pattern expressed whenthe stn is intact. Here we use current- and voltage-clamp, primarilyof identified pyloric dilator (PD) neurons, to investigate changesin synaptic and cellular properties that underlie this transitionin network behavior. Although the efficacy of chemical synapsesbetween pyloric neurons decreases significantly (by $<=$ 50%) afterSTG decentralization, the fundamental change leading to rhythmrecovery occurs in the voltage-dependent properties of the neuronsthemselves. Whereas pyloric neurons, including the PD, lateralpyloric, and pyloric cell types, are unable to generate burst-producingmembrane potential oscillations in the short-term absence of extrinsicmodulatory inputs, in long-term decentralized ganglia, the samecells are able to oscillate spontaneously, even after experimentalisolation in situ from all other elements in the pyloric network.In PD neurons this reacquisition of rhythmicity is associatedwith a net reduction in outward tetraethylammonium-sensitive ioniccurrents that include a delayed-rectifier type potassium current(I_Kd) and a calcium-dependent K⁺ current, I_KCa. By contrast, long-term STG decentralization causedenhancement of a hyperpolarization-activated inward current thatresembles I_h. These results are consistent with the hypothesisthat modulatory inputs sustain the modulation-dependent rhythmogeniccharacter of the pyloric network by continuously regulating thebalance of membrane conductances that underlie neuronaloscillation.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

The operation of central neural networks responsible for the generation of rhythmic motor behavior derives from an interplayof the intrinsic membrane properties of constituent neurons andtheir synaptic interactions (Marder and Calabrese 1996). As wellas producing basic network rhythmicity, these cellular and synapticproperties are targets of extrinsic neuromodulatory inputs that,via their actions on a wide array of both classical synaptic conductancesand voltage-dependent channels implicated in neuronal oscillation,are able to shape network activity to satisfy immediate and changingbehavioral demands (Calabrese 1998; Harris-Warrick and Marder1991; Stein et al. 1997).

In addition to such short-term adaptive instruction, modulatory inputs may exert long-term regulatory effects on their targetnetworks. In the developing nervous system, for example, modulatoryinputs have been found to play a critical role in the maturationof motor networks, either by facilitating the progressive emergenceof adult neuronal properties (Sillar et al. 1992) or by activelyrepressing the adult circuit phenotype until appropriate stagesin development (Le Feuvre et al. 1999).

There is also strong evidence, derived mainly from the experimental suppression of innervating pathways, that presynapticinputs continue to exert persistent and long-term regulatory influenceson their postsynaptic targets in the mature nervous system. Inaddition to the well-described innervation-dependent regulationof receptor/channel expression and distribution in muscle (Angelides1986; Fambrough 1979; Lupa et al. 1995), synaptic inputs havebeen found to regulate transmitter/receptor biosynthesis (Hyatt-Sachset al. 1993; Kirsch and Betz 1998), neuronal structure (Kosselat al. 1997), and gene expression (Fawcett et al. 2000; Martinouand Merlie 1991; Weiser et al. 1994). Furthermore, recent evidencesuggests that central synaptic and neuromodulatory inputs alsoplay an important role in regulating and maintaining the bioelectricalproperties of neurons in the adult networks they modulate. Forexample, in the spinal cord of the adult turtle, the membraneproperties of deafferented motoneurons gradually alter and revertto an embryonic phenotype after several days in organ culture(Perrier and Hounsgaard 2000). The persistent extrinsic regulationof intrinsic excitability that this implies under normal conditionscould be mediated by two different but complementary mechanisms:either indirectly by altering the ongoing activity of target neuronsto allow activity-dependent regulation of their membrane conductances(Desai et al. 1999; Golowasch et al. 1999; Turrigiano et al. 1995)or directly via a trophic control of second messenger cascadesthat ultimately lead to changes in ion channel expression in theseneurons (Jonas and Kaczmarek 1999).

In the stomatogastric nervous system (STNS) of the adult spiny lobster, Jasus lalandii, the well-described pyloric motor networkin the stomatogastric ganglion (STG) falls silent when modulatoryinputs from anterior ganglia are eliminated by cutting or blockingthe STG input nerve. However, after 3-4 days in organ culture,the decentralized network gradually recovers a pattern-generatingcapability that no longer depends on these inputs (Thoby-Brissonand Simmers 1998, 2000; see also Golowasch et al. 1999). Thusthe prolonged absence of central modulatory inputs to the pyloricnetwork allows the emergence of a modulation-independent rhythmogenicproperty that is maintained in a modulation-dependent state whenthese inputs are present. The reacquisition of network rhythmicityrequires new gene transcription occurring in a critical periodat the time the modulatory inputs are first eliminated (Thoby-Brissonand Simmers 2000), and recent evidence from the lobster Homarusgammarus has indicated that pyloric circuit decentralization inducesneuron-specific alterations in gene expression of at least oneion channel, the transient potassium current, I_A (Mizrahi et al.2001).

The aim of the present study was to further explore the electrophysiological basis for the recovery of pyloric network operationfollowing long-term decentralization. Specifically, to assessthe extent to which modulatory inputs might normally sustain theconditional nature of pyloric network operation, we examined theeffects of modulatory input deprivation on pyloric neuron propertiesin organ cultures of the spiny lobster STNS by comparing theseproperties in short- and long-term isolated STG. In addition toanalyzing decentralization-induced changes in synaptic conductanceswithin the pyloric network, alterations in membrane propertiesof individual pyloric neurons were assessed through voltage clampinvestigation of three currents known to play crucial roles inshaping oscillatory membrane behavior in a number of neuronalnetworks (Calabrese 1998): a sustained voltage-activated K⁺ current (I_Kd), a calcium-activated K⁺ current (I_KCa), and a hyperpolarization-activated inward current(I_h). Our data indicate that the pyloric network responds to theprolonged absence of extrinsic modulatory innervation by a substantialdecrease in the strength of its synaptic connections and selectiveconductance changes that lead to an overall increase in the intrinsicoscillatory capacity of individual pyloricneurons.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Experiments were performed on adult J. lalandii purchased from commercial suppliers and kept in laboratory tanks of freshcirculating sea water until used. Before dissection, lobsterswere cold anesthetized in ice for 30 min. To set up in vitro preparationsof the STNS (Fig. 1A), the STG, still attached via the stomatogastricnerve (stn) to the esophageal (OG) and bilateral commissural ganglia(CoG), was dissected from the foregut wall and pinned out underlobster saline in an silicone elastomer-lined (Sylgard 184; DowCorning) petri dish, as previously described (Thoby-Brisson andSimmers 1998). The saline composition consisted of (in mM) 480NaCl, 12.75 KCl, 3.9 MgSO₄, 13.7 CaCl₂-2H₂O, 5 HEPES, pH 7.45.For long-term in vitro survival of preparations, the saline wassterile-filtered and contained glucose (1 g/l), penicillin (35µg/ml), and streptomycin (50 µg/ml). Such organ cultures, whichremained viable for $>=$ 8-10 days, were maintained at 15°C and thebathing saline was renewed daily. The STG was disconnected fromextrinsic modulatory inputs arising in the OG and CoGs by cuttingthe stn at the approximate midpoint between STG and OG.

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Fig. 1. The lobster stomatogastric nervous system (STNS) and pyloric neural network. A: schematic of isolated STNS. B: pyloric neurons and their synaptic connections. Resistance symbols indicate electrotonic synapses; stick and ball symbols: filled, glutamatergic inhibitory synapses; clear, cholinergic inhibitory synapses. Numbers of each cell type are indicated. Hatching denotes main pyloric neurons. IC and VD neurons control the cardiopyloric valve. AB, anterior burster interneuron; Ach, acetylcholine; CoG, commissural ganglion; Glu, glutamate; IC, inferior ventricular neuron; LP, lateral pyloric neuron; lp-pyn, nerve with LP and PY axons; OG, esophageal ganglion; PD, pyloric dilator neuron; pdn, nerve with PD axons; PY, pyloric neuron; STG, stomatogastric ganglion; stn, stomatogastric nerve; VD, ventricular dilator neuron.

Electrophysiological procedures were as routinely used for the STNS in vitro (Harris-Warrick et al. 1992). Extracellular recordingswere made from motor nerves with Vaseline-isolated platinum electrodeswhile intracellular recordings were made from somata within thedesheathed STG with glass microelectrodes (tip resistance 10-20M $Omega$ ) filled with 3 M KCl. Single electrode recordings and currentinjection were achieved via the bridge circuits of WPI electrometers.In a series of experiments, an Axoclamp 2A amplifier (Axon Instruments)was used for both current-and voltage-clamp recordings. Voltage-clampexperiments were performed in two-electrode mode using pClamp6 software from Axon Instruments. The degree of space clamp obtainedin these neurons under our conditions is unknown, although thefinding that the rate and voltage-dependence of the conductanceswe investigated were smooth and continuous functions of the membranepotential suggested that sufficient clamp was obtained to avoidserious error. Conventional techniques were used for display,storage, and transcription of recordeddata.

Impaled STG neurons were identified according to their peripheral axonal projections, firing patterns, and synaptic interactionswith other pyloric neurons. Sketching the somata layout withina ganglion allowed the same neuron(s) to be recognized and penetratedrepeatedly in a given organ culture experiment. In most cases,pairs of pre- and postsynaptic pyloric neurons were impaled toassess the strength of synaptic connections. To isolate neuronsof primary interest from their partners within the pyloric network,known cholinergic presynaptic elements (Fig. 1B) were photoablatedwith blue light illumination after intrasomatic injection of Luciferyellow (Miller and Selverston 1979) and remaining glutamatergicinputs were suppressed with bath-applied picrotoxin (PTX, 10⁵ M) (Bidaut 1980).

In two-electrode voltage-clamp experiments, TTX (10⁷ M) to block action potential generation and tetraethylammonium (TEA, 10mM) to block combined outward K⁺ currents (delayed rectifier I_Kd plus Ca²⁺-activated current I_KCa) were introduced to the bathing medium.All averaged data are given as mean ± SD, unless otherwise stated.Student's t-tests were used to assess statistical difference.Significances were accepted at P < 0.05.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Recovery of pyloric network rhythmicity after long-term STG decentralization

The pyloric network in the STG of the combined STNS in vitro (Fig. 1) is continuously active, generating a basic output patternthat includes sequential bursting in the lateral pyloric (LP),pyloric (PY), and pyloric dilator (PD) motoneurons (Fig. 2A).In Jasus, pyloric rhythm generation depends strictly on permissivemodulatory substances released from stn axon terminals, since,after STG inputs from the OG and CoG are prevented by cuttingthe stn, pyloric network rhythmicity ceases within 10 min (Fig.2B) (see also Bal et al. 1988). However, as reported previously(Thoby-Brisson and Simmers 1998, 2000), when such decentralizedSTG are maintained 3 to 5 days in organ culture, a pyloric motorpattern is gradually reexpressed, which, although slower, is comparablein terms of general burst phase relations to that generated bythe intact STNS (compare Fig. 2C with 2A). Moreover, in all isolatedSTG in which rhythm recovery occurred (77% of 93 preparations),spontaneous activity persisted for the remaining survival time(maximum 15 days) of the preparation. Thus, in long-term decentralizedSTG, the pyloric network is capable of functional recovery fromthe loss of central inputs on which its activity normally depends.

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Fig. 2. Functional recovery of pyloric network rhythmicity after long-term STG decentralization in vitro. A: top, STNS with STG connected via the stn to anterior ganglia. Bottom: pyloric rhythm recorded extracellularly on motor nerves carrying the axons of LP, PY (lp-pyn) and PD (pdn) neurons, and intracellularly from their somata (LP, PY, and PD). B: same recordings 1 h after stn transection. Pyloric neurons no longer burst. C: same recordings from the same preparation after 4 days in organ culture. Spontaneous network rhythmicity has reappeared.

Since extrinsic factors, such as regeneration of input pathways or residual activity in axotomized STG terminals do not underliethis restoration of pyloric rhythmicity (Thoby-Brisson and Simmers1998), the recuperative process must derive from the pyloric networkitself, and specifically from modifications either in the synapticinteractions between pyloric neurons and/or in their intrinsicmembraneproperties.

Decentralization-induced changes in synaptic connectivity

Fundamental changes in synaptic wiring within the pyloric network did not occur in the 5-day period after STG decentralization.First, the maintenance of coordinated phase relations betweenLP, PY, and PD neuron bursts, indicating functionally significantsynaptic inhibition between these cells, was clearly evident inthe pyloric motor pattern reexpressed by long-term disconnectedSTG. As seen in Fig. 2C, each PD neuron burst was again associatedwith synchronous hyperpolarization of postsynaptic LP and PY neurons,with the latter cells tending to fire in alternation (LP neuronbursts again preceding those of the PY neuron) due to their reciprocalinhibitory connection (see Fig. 1B). Second, routine examinationwith pair-wise intracellular recordings confirmed that all previouslyestablished network synaptic connections were conserved and nonew synapses werefound.

However, closer inspection of synaptic relations did reveal a substantial decline in synaptic strength throughout the decentralizedpyloric network. This is illustrated in Fig. 3 where graded synapticinhibition between PD and PY neuron pairs was examined in thepresence and long-term absence of STG inputs. To prevent spike-mediatedtransmission and membrane oscillations, these experiments wereperformed in saline containing 10⁷ M TTX. In each case the membrane potential of the presynapticneuron (PD in Fig. 3) of a stn-intact pyloric network was currentclamped to $-$ 50 mV, and then 3 s depolarizing pulses incrementingin 10 mV steps and repeating at 4 s intervals were applied througha second electrode until the neuron's membrane potential reached+20 mV (Fig. 3A2). The graded inhibitory synaptic potential (GSP)was measured with a third electrode placed in the postsynapticneuron soma (PY in Fig. 3). Examples of control day 1 recordingsare illustrated in the lower left panels of Fig. 3, A1 and B1where two different presynaptic PD neurons were step depolarizedfrom $-$ 50 to $-$ 10 mV. As for graded synaptic inhibition in STG neuronsin general (Graubard 1978; Johnson and Harris-Warrick 1990; Manoret al. 1997), an early peak component that decays to a lower sustainedlevel is evident in the postsynaptic PY neuron responses. In Fig.3, A1 and B1 for example, the peak and persistent component amplitudesof control PY neuron GSPs on day 1 in vitro were 3.0 and 1.5 mV,respectively. After TTX washout, eight such preparations, includingfour freshly decentralized STG, were placed in organ culture.After 4 further days in vitro, these preparations were again placedunder TTX and the same PD and PY neurons were reimpaled and identicalpresynaptic voltage steps were reapplied (see lower right panelsof Fig. 3, A1 and B1). The amplitude of the PY neuron GSP didnot change significantly in the four long-term stn-intact preparations(Fig. 3, A1 and A2), suggesting that synaptic efficacy in thepyloric network with intact modulatory inputs was maintained underour organotypic conditions. In contrast, in long-term decentralizedSTG, both the peak and persistent component of the PY neuron responseshowed a significant decrease in amplitude at all presynapticvoltages. In the experiment of Fig. 3B1, the peak amplitude ofthe PY neuron's response to PD neuron voltage steps from $-$ 50 to $-$ 10 mV decreased from 3.11 to 0.85 mV, and, as seen from the normalizeddata in Fig. 3B2, the mean decline in the PY neuron response tothe same presynaptic voltage step was ca. 46% (from 64.3 ± 11.3%of maximal GSP amplitude on day 1 to 17.6 ± 6.6% on day 5 postdecentralization;P = 0.023, n = 4).

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Fig. 3. Postdecentralization decrease in strength of the graded synapse from the PD to PY neurons. A: PD neuron-evoked graded synaptic potential (GSP) in PY neurons in stn-intact STG on day 1 and day 5 in vitro. A1: inhibitory responses of the same PY neuron to a 40 mV depolarization (from $-$ 50 to $-$ 10 mV) of a presynaptic PD neuron on day 1 (left) and on day 5 (right). A2: input-output curves (peak PY neuron GSP amplitudes normalized to their respective values at +20 mV, plotted against presynaptic PD potential) pooled from 4 preparations measured on day 1 (open circles) and day 5 (filled circles). B: PD-PY GSP in 4 further STG on day 1 (open circles) and day 5 after STG decentralization (filled circles). B1 and B2: same data treatment as in A1 and A2. ^*Mean ± SD corresponding to the single responses illustrated in A1 and B1, respectively.

These data therefore suggest that, in long-term organ culture, the strength of synapses between PD and PY neurons decreasesspecifically as a result of prolonged modulatory input suppression.Similar observations were also made for the reciprocal inhibitorysynapses between the cholinergic PD and glutamatergic LP neurons.The LP neuron response to $-$ 50 to $-$ 10 mV PD neuron voltage stepsdeclined by 49% with decentralization (from 64.2 ± 16.0% of day1 maximal GSP to 15.5 ± 14.6% on day 5 postdecentralization, P= 0.018, n = 3), while the LP to PD synapse weakened by ca. 47%(from 76.0 ± 20.3 to 29.9 ± 19.2%, P = 0.016, n = 4), thereforeindicating that decentralization results in a very similar declinein synaptic efficacy between these chemically connected pyloricneurons. It is noteworthy finally that recordings from four PDneuron pairs indicated that STG decentralization did not modifysignificantly (P > 0.15 for comparison at all voltage steps between $-$ 120 and +20 mV from a holding potential of $-$ 50 mV) the strengthof electrical coupling, at least between the two PD celltypes.

Decentralization-induced changes in oscillatory properties

The second site from which functional network recovery might arise is the intrinsic excitability of pyloric neurons themselvesand, specifically, the extent to which their burst-generatingproperties remain dependent on modulatory inputs. To explore thispossibility we compared the bursting capability of pyloric neuronsin stn-intact STG and after short- and long-term network decentralization.Moreover, to eliminate any contribution of synaptic input to recoveredneuronal bursting in the absence of modulatory inputs, we examinedindividual neurons after further experimental isolation from allother pyloric circuit members (see Fig. 1A). For example, to isolatea PD neuron, its electrically coupled ventricular dilator, anteriorburster (AB), and PD network partners were photoablated and theglutamatergic synapse with the LP neuron was blocked with 10⁵ M PTX (see schematic Fig. 4A). After such in situ isolation,but with modulatory inputs still intact, the PD neuron (n = 10)oscillates spontaneously as in the intact network (Fig. 4A, lowerpanels). Moreover as for neuronal oscillators in general, thisactivity is strongly voltage dependent in that cycle frequencyincreased with tonic depolarizing current injection (top and middletraces) and the phase of oscillation could be reset by brief currentpulses (bottom). In contrast, soon after modulatory inputs tothe STG were eliminated (Fig. 4B), the same isolated PD neuronnow ceased to oscillate, even in response to tonic or pulsed currentinjection. This is consistent with the cessation of activity inthe intact pyloric network immediately following STG decentralizationas seen in Fig. 2B and further attests to the modulator dependenceof pyloric neuron oscillations (see also Bal at al. 1988).

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Fig. 4. Transition from conditional to endogenous PD neuron bursting after long-term STG decentralization. A: oscillatory properties of an in situ-isolated PD neuron in a STG with intact modulatory inputs. The PD neuron was isolated by photoablating electrically coupled VD, AB neurons, and the second PD cell and blocking glutamatergic synapses with PTX (see schematic). The isolated cell oscillated spontaneously (second trace), its frequency increased with depolarizing current injection (top), and the phase of oscillation was reset by injecting a brief positive current pulse (bottom; squares indicate the expected time of oscillation peaks in the absence of injected current). B: 5 h after STG decentralization the same PD neuron has ceased to oscillate, either spontaneously (middle) or in response to tonic (top) and pulsed depolarization (bottom). C: a different PD neuron after in situ isolation in a 5-day decentralized STG. The cell expresses strong endogenous oscillatory properties.

However, in eight further preparations that had been previously decentralized on day 1 in vitro and then maintained 4 daysin organ culture, six of eight PD neurons continued to expressstrong spontaneous membrane potential oscillations when furtherisolated on day 5 from all detectable synaptic input (Fig. 4C).The frequency of these oscillations again displayed voltage-dependent,regenerative responsiveness to continuous and pulsed current injection.These findings thus confirmed previous evidence from the intactpyloric circuit (Thoby-Brisson and Simmers 2000) that the postdecentralizationrecovery of PD neuron rhythmicity derives from a modificationin intrinsic properties, involving a switch from a conditionalburster that is unable to operate without permissive modulatoryinput (Fig. 4, A and B) into a chemo-independent burster thatoscillates freely without modulatory input (Fig. 4C).

This transition to endogenous bursting seen in isolated PD neurons also occurred in other pyloric cell types. In Fig. 5, forexample, which is from a 5-day decentralized STG, a recorded PYneuron was transiently isolated from presynaptic LP and PD neuronsby holding the latter silent with tonic hyperpolarizing currentinjection. In this experiment, moreover, the AB interneuron, whichis electrically coupled to the PD neurons, had been previouslyphotoablated following migration of Lucifer yellow into the stncut stump (note, this procedure also photoablates modulatory stninput terminals in the STG; see Thoby-Brisson and Simmers 1998).Under these conditions, and again in striking contrast to thesituation in short-term decentralized STG, the PY neuron continuedto oscillate and burst at its inherent frequency, and the phaseof its rhythm could be easily reset by brief current pulse injection.When released from hyperpolarization (Fig. 5, right), however,the LP and PD neurons immediately resumed their own oscillatoryactivity and, via their inhibitory synaptic relations, the threecells again became locked into a coordinated activity pattern.Similar evidence for the acquisition of an endogenous oscillatorycapability in the long-term absence of modulatory inputs was obtainedfor four of five PY neurons examined.

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Fig. 5. Endogenous bursting properties in a PY neuron after long-term STG decentralization. Intracellular recordings of three main types of pyloric neuron (LP, PY, and PD) in a 5-day disconnected ganglion. In this preparation the AB interneuron had been previously photoablated on day 2 in vitro (see text). The PY neuron was "isolated" by hyperpolarizing the LP and PD neurons with negative current injection ( $-$ 2 nA), during which time the PY cell continued to oscillate spontaneously and the phase of oscillation could be reset with a brief hyperpolarization (black squares indicate rhythm phase in absence of resetting). Note that the flat membrane potentials of the PD and LP neurons during experimental hyperpolarization indicate that the second PD neuron had also ceased to oscillate during the current injection.

Recovery of oscillatory properties in long-term isolated neurons

In a further strategy, we wanted to determine whether intercellular communication, possibly involving intrinsic modulatorysignaling (Katz and Frost 1996), within the pyloric network throughoutthe decentralized period somehow contributed to the above changesin intrinsic behavior of pyloric neurons. To assess this possibilitya selected pyloric neuron was isolated from its network partnerson day 1 in vitro (Fig. 6A), and then, after stn transection and4 further days in organ culture, the same neuron was reimpaledand examined with intracellular recording. The LP neuron was themain focus for these difficult experiments since it is a singleneuron type and, of the three main cell types (i.e., PD, PY, andLP), it typically displays the weakest capacity to recover activityafter decentralization. As illustrated in Fig. 6, A and B, long-termsynaptically isolated LP neuron still acquired the ability tooscillate and burst in the prolonged absence of modulatory input.Interestingly, the voltage sensitivity of this recovered activityis similar to that of a freshly isolated LP neuron in a stn-intactSTG, where typically the cell fires tonically at resting potentialand oscillates only when slightly hyperpolarized (Bal et al. 1988).Results similar to those shown in the experiment in Fig. 6 wereobtained from three LP neurons and four long-term isolated PDneurons (although not shown, it is noteworthy that, unlike theLP type cell, long-term synaptically isolated PD neurons oscillatedspontaneously without current injection, in a manner similar toPD neurons freshly isolated on day 5 after STG decentralizationas seen in Fig. 4C). Together therefore these data indicate thatthe postdecentralization reexpression of oscillatory activityderives solely from an intrinsic membrane response of individualpyloric neurons to the lack of extrinsic modulatory inputs, withoutany significant influence from other neighboring STG neurons.

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Fig. 6. Endogenous oscillatory properties expressed by a long-term isolated and decentralized LP neuron. A: schematic indicating in situ isolation of an identified LP neuron on day 1 in vitro. The VD and 2 PD neurons were photoablated, and the PY-LP, AB-LP synapses were blocked with PTX. The STG was then disconnected from anterior ganglia and placed in organ culture. B: intracellular recordings from the same isolated LP neuron on day 5 in culture. The cell oscillated in a voltage-dependent manner when tonically hyperpolarized from resting potential (top), and the phase of its rhythm could be reset with brief negative pulses (bottom).

Changes in electrical properties

We next compared basic membrane properties of pyloric neurons before and after long-term STG decentralization. The resultssummarized in Fig. 7 were obtained from 20 PD neurons. Whereasdecentralization induced no significant modification in PD membranepotential ( $-$ 54.1 ± 1.7 mV day 1, $-$ 57.4 ± 1.1 mV day 5; P > 0.05),there was a significant decrease in oscillation amplitude (21.5± 0.9 mV day 1, 14.0 ± 0.7 mV day 5, P < 0.001), an increase inspike amplitude (5.8 ± 0.3 mV day 1, 9.6 ± 0.7 mV day 5, P < 0.001),and membrane input resistance (measured under TTX) increased from17.2 to 25.5 M $Omega$ (P < 0.001). Although the changes in oscillationand spike amplitude were possibly due to motoneuron axotomy, whichis known to induce alterations in neuronal excitability (Titmusand Faber 1995), that these changes were not observed in control5-day-old preparations with intact stns (i.e., with only motornerves axotomized) argues against this possibility (see also Thoby-Brissonand Simmers 1998).

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Fig. 7. PD neuron membrane properties before and after long-term STG decentralization. Histograms of mean membrane potential (measured under TTX 10⁷ M), amplitude of oscillations and action potentials (mV), and membrane input resistance (M $Omega$ ) of 20 PD neurons in stn-intact preparations (day 1, open bars) and 4 days after STG disconnection (filled bars). ^*Significant differences (Student's t-test, P < 0.001).

TEA-sensitive outward currents

In a further step, two-electrode voltage clamp was used to measure two potassium currents expressed by PD neurons and to comparethem before and after long-term decentralization. These previouslywell-described currents, the delayed-rectifier current (I_Kd) anda calcium-dependent K⁺ current (I_KCa), are activated together by membrane potentialdepolarization above around $-$ 40 mV, where a third potassium current,the transient A-type current, is almost completely inactivated(Golowasch and Marder 1992; Graubard and Hartline 1991; Kloppenburget al. 1999; Tierney and Harris-Warrick 1992). We did not attemptsystematically to separate the delayed rectifier and calcium-dependentK⁺ current components in our organotypic experiments; therefore,the sum of I_Kd plus I_KCa is reported throughout the remainderof this paper. To investigate this combined outward current, day1 STG were bathed with saline containing 10⁷ M TTX to prevent Na⁺ spiking and membrane oscillations and then a series of 10 mVsteps from a holding potential of $-$ 50 to +40 mV was applied toa recorded PD neuron (Fig. 8Ai). Superfusion of the STG with 10mM TEA was then used to reversibly block a large proportion ofI_Kd plus I_KCa (Fig. 8Aii) (Hille 1992). The combined TEA-sensitiveoutward current was thus measured by subtracting currents occurringunder TEA (Fig. 8Aii) from those elicited under normal saline(Fig. 8, Ai and Aiii). After washout of TTX, the STG was disconnectedfrom the rostral ganglia, maintained 4 days in vitro, and theidentical experiment was again performed on the same PD neuron.As can be seen in Fig. 8B, the TEA-sensitive outward current wasstill evident after long-term decentralization, but with a muchdecreased amplitude (compare with Fig. 8A). In six PD neuronsexamined (Fig. 8C1), the combined K⁺ current following decentralization attained no more than 50-55%of control values over the entire voltage range tested. At +40mV, for example, the outward current displayed a postdecentralizationdecrease in peak amplitude from a mean (±SD) of 15.8 ± 1.6 nAon day 1 to 8.3 ± 1.8 nA on day 5 (P < 0.01). Moreover, to assesswhether this decrease in current magnitude was uniquely a resultof PD neuron decentralization, TEA-sensitive currents were measuredin three preparations after 5 days in culture but with their stnintact. Under these conditions, the mean maximal current amplitudeelicited by voltage pulses to +40 mV was 12.5 ± 3.0 nA. This magnitudewas not significantly different from the conductance recordedon day 1 in culture (P = 0.5), although its higher value comparedwith long-term decentralized PD neurons did not reach statisticalsignificance with our small sample size 1 (P = 0.1; n = 3). Asa consequence, we are unable to reject entirely the possibilitythat the organ culture conditions per se were not also contributingto the decline in combined outward current (but see followingtext).

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Fig. 8. Increase in TEA-sensitive outward currents (I_kd, I_KCa) in PD neurons after long-term STG decentralization. A: outward current measured from a PD neuron in control stn-intact preparation in 10⁷ M TTX on day 1 before (i), during (ii), and after (iii) addition of 10 mM TEA. V_h = $-$ 50 mV; V_test = $-$ 50 to +40 mV in steps of 10 mV, in TEVC. B: same protocol applied to the same cell, 4 days after STG decentralization. C1: outward current magnitude (measured at steady state after 100 ms) versus membrane potential for 6 control (open circles) and long-term decentralized (filled circles) PD neurons. Each point is mean ± SD. C2: conductance-voltage curves for activation of combined outward current. Currents measured in C1 were converted to conductances assuming a potassium reversal potential of $-$ 86 mV and normalized to the calculated maximal conductance (g_max) measured at +40 mV in each experiment. The curves are fits to a third order Boltzmann relation (Eq. 1) with a calculated V_A of $-$ 32.1 and $-$ 26.5 mV and slope values of $-$ 17.2 and $-$ 16.3 mV on day 1 and day 5, respectively.

In a further analysis, the voltage-dependence of the combined outward current activation before and after long-term decentralization(Fig. 8C2) was determined by converting the peak currents evokedby each voltage step to peak conductances, g, using the equationg = I/(V_m $-$ E_rev) (where V_m is the command potential and E_revis the potassium reversal potential taken as $-$ 86 mV) (Hartlineand Graubard 1992). and the resulting g/V curve was fitted toa third-order Boltzmann equation of the form

g/gmax<IT>=1/</IT>(<IT>1+e</IT><IT>−</IT>(<IT>V−VA</IT>)<IT>/S</IT>)<IT>n</IT> (1)

where n = 3, V_A is the voltage at which half-maximal activation of the individual gating step occurs, and s is a slope factor.The resulting Boltzmann fit to the conductance-voltage relationsgave a V_A of $-$ 32.1 ± 1.6 mV under day 1 control conditions, leadingto half-maximal activation of the peak current at $-$ 8.9 mV. Althoughthe maximal conductance of the combined outward current in PDneurons decreased significantly from a mean of 0.12 ± 0.04 µSon day 1 to 0. 07 ± 0.021 µS on day 5 postdecentralization, thevoltage-dependence of activation did not alter substantially.The small shift in V_A from $-$ 32.1 ± 7.5 mV (slope value $-$ 17.2 mV)in control to $-$ 26.5 ± 6.6 mV (s = $-$ 16.2 mV) in our 5-day decentralizedpreparations was not significant (P > 0.05; n =6).

Hyperpolarization-activated inward current

Inward currents in stomatogastric neurons are notoriously difficult to study because of their soma-distant location in combinationwith rapid activation properties (Golowasch and Marder 1992; Graubardand Hartline 1991). However, one readily accessible inward currentis the slow hyperpolarization-activated I_h current (Golowaschand Marder 1992; Kiehn and Harris-Warrick 1992) responsible fora slow depolarizing sag toward resting potential, as seen fora PD neuron under TTX and current clamp conditions in Fig. 9Ai(arrow). The expression of I_h in the same neuron under voltageclamp can be seen in Fig. 9Bi, where the current continued toactivate with increasing hyperpolarization and with little signof inactivation. On day 5 after STG decentralization, the voltageresponse of this neuron to the same current steps as in controlconditions revealed a substantially increased depolarizing sag(Fig. 9Aii, arrows). That this was indeed due to an increase inthe I_h conductance can be seen under voltage clamp (Fig. 9Bii,arrows) where the amplitude was increased and the activation kineticsof I_h were substantially faster in the long-term decentralizedneuron (compare with Fig. 9Bi). As evident in the pooled I-V measurementsfrom seven PD neurons in Fig. 10A, I_h began to activate at around $-$ 60 mV in both control and postdecentralization conditions, butthe net current (i.e., the difference between current amplitudesmeasured at the beginning and end of each voltage step) was substantiallyenhanced postdecentralization by $>=$ 55% at all membrane potentials.At $-$ 120 mV, for example, I_h measured in PD neurons on day 1 instn-intact STG was 3.5 ± 0.5 nA, while 5 days after stn sectionthe current had increased to 5.8 ± 0.6 nA (P < 0.01, n = 7). Infour further control preparations that remained 5 days in culturewith an intact stn, mean I_h measured in PD neurons was 4.0 ± 0.4nA, which was not significantly different from the current magnitudeon day 1 in culture (P > 0.05) but was significantly less thanI_h in long-term decentralized neurons (P < 0.01). This stronglysuggests, therefore, that the alteration in this current was adirect consequence of STG decentralization and not simply dueto time in culture.

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Fig. 9. Changes in hyperpolarization-activated inward I_h current in PD neurons after long-term decentralization. A: current-clamp recordings of voltage responses (bottom) of the same PD neuron to negative current steps (top) ranging from 0 to $-$ 2.6 nA (duration 10 s) on day 1 (i) in an stn-intact control STG (under 10⁷ M TTX) and on day 5 (ii) postdecentralization. Arrows indicate voltage- and time-dependent depolarizing sag, which increases after STG decentralization. B: same experimental conditions as in A. Voltage-clamp recordings of sag currents (bottom) in a different PD neuron in response to 10-s voltage steps (top) from a V_h = $-$ 50 mV to a range between $-$ 120 to $-$ 60 mV. Hyperpolarizing voltage steps elicit a slow inward current (arrows), which increases with long-term decentralization.

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Fig. 10. I_h characteristics in PD neurons before and after long-term decentralization. A: maximal I_h current amplitude versus membrane potential. B: I_h activation curves. Currents were converted to conductances (assuming a reversal potential of $-$ 35 mV) and normalized to the corresponding maximal conductance (g_max) measured at a voltage step to $-$ 120 mV. The data were also fitted to a first-order Boltzmann relation with a calculated V_0.5 of $-$ 91.0 and $-$ 89.5 mV and slope values of 9.0 and 9.8 mV on day 1 and day 5, respectively. C: kinetics of I_h activation. Activation time constant (calculated by fitting currents at different voltage steps to a single exponential process of the form I_t = I_ss $-$ I_maxe^t/, where I_t is the current at time t, I_ss is the steady state current, and I_max and $tau$ are the peak amplitude and time constant of the current) versus membrane potential. For all plots, measurements were made at day 1 in stn-intact STG (unfilled circles) and then on day 5 postdecentralization from the same neurons (black circles). Each value is an average ± SD for 7 different PD cells.

The voltage dependence of I_h activation before and after long-term decentralization is shown in Fig. 10B, in which peak currentswere converted to peak conductances by assuming a reversal potentialof $-$ 35 mV (Golowasch and Marder 1992). These values were thennormalized to the calculated g_max (mean 0.04 ± 0.01 µS on day1, 0.07 ± 0.01 µS on day 5 postdecentralization) and the resultingconductance-voltage curves were fitted to a first order Boltzmannequation (Eq. 1; n = 1). These Boltzmann fits (Fig. 10B) gave amean voltage for half-maximal activation of $-$ 91.0 ± 0.6 mV (witha slope value of 9.0 mV) under control conditions, which was notsignificantly different (P > 0.05) from the half-activation voltage( $-$ 89.5 ± 0.7 mV; slope value 9.8 mV) measured on day 5postdecentralization.

Whereas the voltage dependence of I_h activation remained unchanged after STG decentralization, the activation time constantfor I_h decreased uniformly by almost 20% over the voltage rangetested (Fig. 10C). As is typical for I_h (e.g., Harris-Warrick etal. 1995; McCormick and Pape 1990), the activation of this currentwas very slow and was best fitted by a single exponential functionthat produced time constant values that accelerated with increasinghyperpolarization, producing a mean value of 3.9 ± 0.2 s at $-$ 120mV under day 1 control conditions. On day 5, however, the samevoltage step activated I_h with a time constant of 2.9 ± 0.2 s,commensurate with a significantly (P < 0.01) faster activationof this inward current after long-term STGdecentralization.

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

In a previous extracellular study we reported that, in the spiny lobster, elimination of extrinsic modulatory inputs rapidlyleads the pyloric network to fall silent, but after 4-5 days thenetwork recovers the capacity to be rhythmically active (Thoby-Brissonand Simmers 1998). Therefore the prolonged absence of modulatoryinputs allows the expression of a rhythmogenic capability thatis normally maintained in a strictly conditional state when theseextrinsic influences are present. One source of recovery couldbe a fundamental reorganization of pyloric network circuitry,involving changes in the strength of preexisting connections orthe formation of entirely new synapses. Alternatively, rhythmrecovery may derive from specific changes in the membrane propertiesof individual pyloric neurons (Thoby-Brisson and Simmers 2000).The goal of the present study was to examine bothpossibilities.

Decentralization-induced modifications in synaptic efficacy

Compensatory changes in synaptic connectivity is a well-known mechanism for functional recovery following lesions to innervatingpathways. Examples range from restoration of auditory functionin cricket 4-6 days following sensory deprivation (Brodfuehrerand Hoy 1988), topographical reorganization of the cat visualcortex in response to retinal lesions (Darian-Smith and Gilbert1994), and deafferentation-induced synaptic plasticity in themotor cortices of cat (Keller et al. 1990) and humans (Ziemannet al. 1998). In these cases, restoration of function derivesfrom the formation of new functional connections and/or changesin strength or unmasking of preexistingsynapses.

Our finding that the efficacy of pyloric synapses decreases substantially after suppression of modulatory input, without theformation of new synapses, does not readily comply with a majorcontribution of changes in network interactions to pyloric rhythmrecovery. Although postdecentralization synaptic coupling clearlyremains sufficient to coordinate the typical triphasic pyloricburst pattern (see also Thoby-Brisson and Simmers 1998), the reasonfor this overall decline in strength is unclear. One possibilityis that STG decentralization eliminates certain modulatory inputsthat are normally responsible for sustaining and reinforcing synapticefficacy in the pyloric network. For example, aminergic up-modulationof synaptic connectivity is well known in both vertebrates (see,for example, Knapp and Dowling 1987; Perada et al. 1992) and invertebrates,including lobster stomatogastric circuits (Ayali et al. 1998;Johnson and Harris-Warrick 1990; Johnson et al. 1995). In thelatter, however, different STG synapses may be affected differentlyor even in opposite ways by the same or different stn input modulators,so it is difficult to see why removal of the entire modulatoryinput ensemble should uniformly decrease the strength of chemicalsynapses throughout the pyloricnetwork.

A further explanation for the postdecentralization decrease in network synaptic efficacy may reside with changes in the intrinsicmembrane properties of pyloric neurons themselves. For example,in a manner equivalent to the postdecentralization reduction involtage-dependent K⁺ currents found in the present study (see following text), anapparent decline in inhibitory synaptic strength could arise froma reduction of other ionic currents that are directly involvedin presynaptic transmitter release or postsynaptic responsiveness.An additional interesting possibility is that, as seen in mammalianneocortical cultures (Rutherford et al. 1997), the reduction insynaptic inhibition may derive from an activity-dependent decreasein neurotransmitter expression due to lowered levels of pyloricnetwork activity, particularly during the first few days afterSTGdecentralization.

Decentralization-induced modifications in membrane properties

The most convincing evidence that pyloric rhythm recovery arises from changes in the intrinsic excitability of individualpyloric neurons derived from experiments performed on single cellsafter isolation in situ from all other intraganglionic input.Such acutely isolated neurons still eventually reacquired a strongburst-generating oscillatory capability, therefore indicatinga fundamental alteration in their bioelectrical character; namelythe transition from chemo-dependent (conditional) oscillatorsthat are unable to burst without central inputs into endogenous(nonconditional) oscillators that operate without extrinsic input.As previously argued by Thoby-Brisson and Simmers (1998, 2000),this response to decentralization indicates that extrinsic inputsnormally exert a continuous down-regulatory influence on neuronal,and therefore network, excitability in addition to short-termneuromodulatory control. This conclusion is further supportedby recent direct evidence that network decentralization leadsto changes in the expression of genes responsible for the biophysicalproperties of pyloric neurons (Mizrahi et al. 2001; Thoby-Brissonand Simmers 2000).

In our initial voltage-clamp experiments, which here focused on a single (PD) neuron type, we investigated postdecentralizationchanges in three conductances that have all been previously reportedin STG cells of other crustacean species (Golowasch and Marder1992; Graubard and Hartline 1991). These channels included twovoltage-dependent outward conductances, I_Kd and I_KCa, which arewell known to be potent regulators of neuronal excitability andfiring patterns (Hille 1992). Following removal of STG modulatoryinputs, the magnitude of combined TEA-sensitive I_Kd plus I_KCain PD neurons decreased to only approximately 50% of the currentlevel in stn-intact controls. This substantial decline in outwardcurrent with time in organ culture, which could partially explainthe net increase in PD neuron input resistance and would helppromote bursting following decentralization, has also been reportedin dissociated STG neurons in primary culture (Turrigiano et al.1995).

The third conductance we investigated in detail, I_h, also plays an important role in oscillatory behavior in a variety ofneural networks (for reviews, see Calabrese 1998; Lüthi and McCormick1998). This ubiquitous conductance is also found in crustaceanpyloric neurons (Golowasch and Marder 1992) where its role andshort-term modulation has been studied (Harris-Warrick et al.1995; Kiehn and Harris-Warrick 1992). In our experiments, a comparisonbetween stn intact control and long-term decentralized PD neuronsrevealed a considerable modification in the expression of I_h,including a significant increase in magnitude and an increasein its rate of activation. In contrast no change was observedin I_h voltage activation characteristics. This current is importantfor neuronal pacing by setting resting potential and the occurrenceand frequency of rhythmic bursting (Angstadt and Calabrese 1989;McCormick and Pape 1990; Thoby-Brisson et al. 2000). Thus increasingI_h and speeding its rate of activation in long-term decentralizedpyloric neurons would enhance an inward current mechanism thatopposes sustained membrane hyperpolarization and facilitates activationof other voltage-dependent conductances that contribute to membraneoscillations.

Taken together, therefore, our results indicate that prolonged deprivation of modulatory inputs to pyloric network neuronsinduces a change in electrical behavior accomplished by an increasein at least one important inward current, in parallel with a decreasedeffectiveness of TEA-sensitive outward conductances. In this way,the transition from the conditional to nonconditional oscillatorphenotype does not appear to be attributable to changes in anyone particular ion channel but rather derives from modificationsin the ensemble of preexisting conductances, which in combinationlead to the altered rhythmogenic capacity of pyloricneurons.

Our results from J. lalandii and those obtained both by Turrigiano et al. (1995) on dissociated STG neurons of the spiny lobsterPanulirus interruptus, and by Golowasch et al. (1999) from modelingstudies and STNS organ cultures of the crab Cancer borealis arequalitatively similar in a number of important ways. First, inall three cases, pyloric neuron bursting, which normally dependson the release of permissive modulatory substances from STG inputterminals, reoccurs after several days in the absence of neuromodulators.Second, the reacquisition of rhythmicity depends on a modificationin intrinsic membrane properties, such that a transition fromconditional (modulator-dependent) bursting to endogenous burstingoccurs. Third, this transition is associated with specific alterationsin a variety of membrane conductances. However, the question ofwhether rhythm recovery is an indirect, activity-dependent responseto the long-term absence of modulatory inputs (Golowasch et al.1999; Turrigiano et al. 1995) and/or is a direct consequence ofthe removal of a trophic influence from the modulators themselves(Thoby-Brisson and Simmers 1998, 2000) remains unresolved by ourdata. Nonetheless our results do add to a growing body of evidencethat modulatory inputs play a crucial long-term regulatory rolenot only in the maturation of motor network properties in thedeveloping nervous system (Scrymgeour-Wedderburn et al. 1997;Sillar et al. 1992, 1995), including the lobster STG (Le Feuvreet al. 1999), but also in controlling the expression of neuronalchannel properties in the adult STG (Mizrahi et al. 2001). Itis also interesting that, after several days in organ culture,deafferented motoneurons in the turtle spinal cord gradually losetheir adult biophysical characteristics and reacquire intrinsicresponse properties normally only seen in immature motoneurons(Perrier and Hounsgaard 2000; Perrier et al. 2000). This furthersupports the idea that, in addition to governing the short-termoperational flexibility of motor networks, central synaptic andmodulatory inputs may also be responsible, either directly orindirectly, for the "life long" maintenance of appropriate rhythmogenicproperties of their neuronal targets in the mature nervoussystem.

	ACKNOWLEDGMENTS

We thank Drs. Denis Combes and Andrew Hill for useful discussions and help with dataanalysis.

This work was partly supported by the Human Frontier Science Program and a doctoral studentship from the Ministère de l'EnseignementSupérieur et de la Recherche to M. Thoby-Brisson.

Present address of M. Thoby-Brisson: Laboratoire de Neurobiologie Génétique et Intégrative, Institut Alfred Fessard, Avenuede la Terrasse, 91198 Gif sur Yvette,France.

	FOOTNOTES

Address reprint requests to: J.Simmers.

REFERENCES

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
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