Statistical Model Relating CA3 Burst Probability to Recovery From Burst-Induced Depression at Recurrent Collateral Synapses

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Statistical Model Relating CA3 Burst Probability to Recovery From Burst-Induced Depression at Recurrent Collateral Synapses

Kevin J. Staley, Jaideep S. Bains, Audrey Yee, Jennifer Hellier, and J. Mark Longacher

Departments of Pediatrics and Neurology, University of Colorado Health Sciences Center, Denver, Colorado 80262

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Staley, Kevin J., Jaideep S. Bains, Audrey Yee, Jennifer Hellier, and J. Mark Longacher. Statistical Model Relating CA3 Burst Probability to Recovery From Burst-Induced Depression at Recurrent Collateral Synapses. J. Neurophysiol. 86: 2736-2747, 2001. When neuronal excitability is increased in area CA3 of the hippocampus in vitro, the pyramidal cells generate periodic burstsof action potentials that are synchronized across the network.We have previously provided evidence that synaptic depressionat the excitatory recurrent collateral synapses in the CA3 networkterminates each population burst so that the next burst cannotbegin until these synapses have recovered. These findings raisethe possibility that burst timing can be described in terms ofthe probability of recovery of this population of synapses. Herewe demonstrate that when neuronal excitability is changed in theCA3 network, the mean and variance of the interburst intervalchange in a manner that is consistent with a timing mechanismcomprised of a pool of exponentially relaxing pacemakers. Therelaxation time constant of these pacemakers is the same as thetime constant describing the recovery from activity-dependentdepression of recurrent collateral synapses. Recovery was estimatedfrom the rate of spontaneous transmitter release versus time elapsedsince the last CA3 burst. Pharmacological and long-term alterationsof synaptic strength and network excitability affected CA3 bursttiming as predicted by the cumulative binomial distribution ifthe burst pace-maker consists of a pool of recovering recurrentsynapses. These findings indicate that the recovery of a poolof synapses from burst-induced depression is a sufficient explanationfor burst timing in the in vitro CA3 neuronal network. These findingsalso demonstrate how information regarding the nature of a pacemakercan be derived from the temporal pattern of synchronous networkactivity. This information could also be extracted from less accessiblenetworks such as those generating interictal epileptiform dischargesinvivo.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

One goal of synaptic physiology is to understand the working of neural networks in terms of the properties of the synapsesthat connect the member neurons. However, the complexity of realneural networks (Churchland and Sejnowski 1992; Hampson et al.1999; Marder 1998) makes it difficult to determine how varioussynaptic properties (Bains et al. 1999; King et al. 1999; Malenkaand Nicoll 1999; Markram et al. 1998; Martin et al. 2000) affectnetwork ouput. One approach to the complexity problem is to analyzesynaptic influences on very simple modes of network behavior,such as the periodic, synchronous discharge of all neurons inthe network. This "bursting" mode of activity is amenable to analysisbecause the outputs of all neurons in the network are so similarthat to a first approximation they can be considered identical(Traub and Miles 1991). Further, the network activity can be simplifiedto two states: all neurons firing at high frequencies during theburst versus no or low-frequency firing between bursts (Cohenand Miles 2000).

The analysis of network bursts is further simplified because this mode of network operation does not depend on intact inhibitoryconductances. Blockade of postsynaptic inhibition is one of themost robust ways to initiate burst activity in the CA3 networkof the adult hippocampus (Traub and Miles 1991), and spontaneousbursts occur in CA3 during the developmental period during whichthe postsynaptic actions of GABA are excitatory (Leinekugel etal. 1997). In bursting networks studied to date, bursts appearto be terminated by activity-dependent depression at recurrentexcitatory synapses (reviewed in Feller 1999; O'Donovan and Rinzel1997) rather than postsynaptic feedback inhibition or calcium-activatedpotassium conductances (Robinson et al. 1993; Staley et al. 1998).Although the dissipation of inhibitory conductances can modulatethe interburst interval, the period between discharges is primarilydetermined by the time required for the synapses to recover fromdepression (as proposed by O'Donovan and Rinzel 1997; Staley etal. 1998; modeled in Tabak et al. 2000; Tsodyks et al. 2000).Thus burst timing should reflect synaptic recovery in thenetwork.

In this paper, we consider whether the recovery of a network of recurrent collateral synapses from burst-induced depression(Selig et al. 1999) could be a sufficient explanation for thetiming of synchronous CA3 bursts. Periodic CA3 network burstsare readily elicited in the CA3 hippocampal network when neuronalexcitability is increased (Johnston and Brown 1986; Traub andWong 1982) due to the degree of positive feedback mediated byrecurrent collateral glutamatergic synapses (King et al. 1999;Miles and Wong 1986; Traub and Miles 1991). The next CA3 burstbegins when synapses recover sufficiently to generate spontaneousexcitatory postsynaptic potentials (EPSPs) at a rate that triggersaction potentials in some neurons (Chamberlin et al. 1990; Trauband Dingledine 1990). With each CA3 cell that reaches action potentialthreshold, the probability of recruiting subsequent CA3 cellsincreases due to additional action potential-dependent glutamaterelease. It follows that the probability of recruiting additionalpyramidal cells must be at a minimum when the number of pyramidalcells firing synchronous action potentials is at a minimum; thusthe time dependence of this probability should determine the timingof the nextburst.

The probability of initiating and propagating the first synchronous action potentials should be highest at strong synapses,synapses whose postsynaptic neurons are close to action potentialthreshold, and synapses with high release probabilities (Bainset al. 1999; Dobrunz and Stevens 1997; Markram et al. 1998; Martinet al. 2000). If there are N such synapses, then the "depressionrecovery" hypothesis predicts that a burst will be initiated onlywhen a sufficient number of these N synapses have recovered fromthe depression induced by the last burst. If K represents thissufficient number of synapses, then the probability of a networkdischarge at any point in time should be directly linked to theprobability that K of N synapses have recovered from synapticdepression. Because the time course of synaptic recovery can bemeasured (Dittman et al. 2000; Markram et al. 1998; Stevens andWesseling 1998), comparison of the time course of synaptic recoveryto the mean and variance of the burst interval permits estimationsof both N and K.

In this paper, we derive expressions relating N and K to burst timing. It was not possible to test these expressions directlyby independent measurements of N and K. Instead, we tested theutility of these expressions by pharmacologically manipulatingthe strength of recurrent synapses, measuring the consequent changesin CA3 burst timing, fitting the interburst time interval distributionsto the expressions for N and K and determining whether the changesin N and K predicted by the expressions are consistent with thepharmacological effects on synapticfunction.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Recordings

Hippocampal slices were prepared from adult rats as described previously (Staley et al. 1998). Recordings were performed inartificial cerebrospinal fluid (ACSF) at 35°C. ACSF was saturatedwith 95% O₂-5% CO₂ and included (in mM) 126 NaCl, 2.5 KCl, 26NaHCO₃, 2 CaCl₂, 2 MgCl₂, 1.25 NaH₂PO₄, and 10 glucose. Wholecell pipette solutions contained (in mM) 123 cesium methylsulfonate,2 MgCl₂, 8 NaCl, 1 potassium ethylene glycol-bis(b-aminoethylether) N, N,N',N'-tetraacteic acid (EGTA), 4 potassium ATP, 0.3sodium GTP, and 1 N-(2,6-dimethylphenylcarbamoylmethyl) triethylammoniumbromide (QX314) (for current-clamp experiments, Cs was replacedby K and QX314 was omitted). Whole cell solutions were bufferedwith 16 mM KHCO₃ and saturated with 95% O₂-5% CO₂. Extracellularrecordings were performed using ACSF-filled whole cell pipettesplaced in stratum pyramidale. Bursting in CA3 was induced by eitherincreasing the K to between 4.5 and8.5 mM as noted in the text, or by one-time tetanic stimulation(100 Hz for 1 s) of the recurrent collateral system using a bipolarelectrode placed in s. pyramidale (Staley et al. 1998). When burstswere induced by tetanic stimulation, final ACSF ionic concentrationswere as described by Stasheff et al. (1989): (in mM) 1.3 Ca²⁺, 0.9 Mg²⁺, and 3.3 K⁺. Long-term depression (LTD) of the recurrent synapses was inducedby temporary partial block of the N-methyl-D-aspartate (NMDA)receptor during spontaneous network discharges using 40-100 µMDL-amino-5-phosphonovaleric acid (APV) (Bains et al. 1999). Evokednetwork discharges (Fig. 7, A and B) were triggered after everythird spontaneous discharge by electrical stimulation in the pyramidalcell layer at an intensity that was sufficient to trigger a populationspike prior to initiation of periodic discharges. Excitatory postsynapticcurrents (EPSCs) were identified using a rectangular window (amplitude× duration), with amplitude set by eye to exclude baseline noise.Recordings were performed with an Axoclamp 2B amplifier (AxonInstruments, Foster City, CA) and digitized at 2-kHz using a PCI-DAS1602/16 (Computer Boards, Middleboro, MA) and software writtenin visual basic 6.0. Drugs were obtained from Sigma (St. Louis,MO) and applied bybath.

Some of the experimental data in Figs. 4, 9, 10, and 11 have been previously published in aggregate form (Bains et al. 1999;Staley et al. 1998).

Data analysis

The cumulative probability of recovery from short-term depression at an individual synapse (p₁) has been derived in a numberof preparations by fitting the response to evoked transmitterrelease to an exponential function (Dittman et al. 2000; Markramet al. 1998; Stevens and Wesseling 1998)

<IT>p</IT><IT>1</IT><IT>=1−</IT><IT>e</IT>(<IT>−</IT><IT>t</IT><IT>/&tgr;</IT>) (1)

where $tau$ is the time constant describing the recovery rate, and t is the time since the onset of depression. The same expressionhas also been derived by considering that the rate of recoveryis proportional to the remaining number of empty release sites(Staley et al. 1998). Because the rate of recovery at each synapsemay not be identical (Stevens and Wesseling 1998), in this studywe estimated a population-average recovery rate from the rateof spontaneous EPSCs. Then Eq. 1 can be considered to be the probabilitythat a synapse has recovered sufficiently, if the average recoveryrate is 1/ $tau$ and synaptic recovery proceeds as a Poisson process(Bethea et al. 1995: the cumulative Poisson probability is alsodescribed by Eq. 1). For Poisson recovery, the probability ofrecovery is constant during a given interval of time so that asmore time intervals elapse, the probability that a synapse hasrecovered increases with time constant $tau$ .

The number of synapses that are capable of participating in burst initiation is denoted by N, and the number that must recoverto initiate a burst is denoted by K. We assumed that all N synapsesare uniformly depressed at the end of each burst, which seemsreasonable given the high probability of transmitter release duringaction potential bursts (Selig et al. 1999). This uniform postburstdepression implies that the current interburst interval is independentof prior intervals. If the N synapses recover from depressionas described by Eq. 1, then we can greatly simplify the calculationof the probability of recovery of K of N synapses during the interburstinterval by using the binomial distribution to estimate the probabilitythat K synapses from a candidate pool of size N have recovered

<IT>P</IT>(<IT>N</IT><IT>, </IT><IT>K</IT><IT>, </IT><IT>p</IT><IT>1</IT>)<IT>=</IT><FENCE><FR><NU><IT>N</IT><IT>!</IT></NU><DE><IT>K</IT><IT>!×</IT>(<IT>N</IT><IT>−</IT><IT>K</IT>)<IT>!</IT></DE></FR></FENCE>(<IT>p</IT><IT>1</IT>)<IT>K</IT>(<IT>1−</IT><IT>p</IT><IT>1</IT>)(<IT>N</IT><IT>−</IT><IT>K</IT>) (2)

The binomial distribution applies to binary (true/false) variables; we are considering synapses to be in two states, eitherrecovered sufficiently to be capable of releasing transmitterduring burst initiation, or not (Debanne et al. 1996).

We are interested in the probability that K or more synapses have recovered. The cumulative binomial probability distributiongives the probability that less than K synapses have recovered.The survival function, which is equal to one minus the cumulativebinomial distribution (Hastings and Peacock 1975), therefore givesthe probability that K or more of the N synapses have recovered.Thus the cumulative probability of a burst in the interval (0,t) is given by

<IT>P</IT><IT>discharge</IT><IT>=</IT><IT>P</IT>(<IT>N</IT><IT>, </IT>≥<IT>K</IT><IT>, </IT><IT>p</IT><IT>1</IT>)<IT>=1−</IT><LIM><OP>∑</OP><LL><IT>X</IT><IT>=1</IT></LL><UL><IT>X</IT><IT>=</IT><IT>K</IT><IT>−1</IT></UL></LIM> <IT>P</IT>(<IT>N</IT><IT>, </IT><IT>X</IT><IT>, </IT><IT>p</IT><IT>1</IT>) (3)

This is the probability that K or more of N synapses have recovered. The value of p₁ increases with time (Eq. 1), so theprobability that K of N synapses have recovered also changes withtime (Fig. 1).

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Fig. 1. Relationship between probability of recovery of 1 synapse vs. the probability of recovery of a pool of synapses. Middle: the probability of recovery of one synapse based on Eq. 1. Top and bottom: the probability of recovery of a fraction of a pool of 30 such synapses. For the top panel, the cumulative probability of recovery of 9 of 30 synapses is illustrated using Eq. 3. The bottom panel illustrates the cumulative probability that 20 of 30 synapses have recovered. - - -, for a given probility of recovery at an individual synapse, the probability that a fraction of a pool of such synapses has recovered is strongly dependent on the size of the fraction.

How unique are the solutions provided by particular values of K and N? At any one point in time, for example 2 s after thelast burst, many different values of N and K might provide a reasonableburst probability. However, to fit the experimental data, Eq.3 must be fit to the burst probability using the same values ofN and K at every time interval using the corresponding value ofp₁ calculated from Eq. 1. This severely constrains the acceptablevalues of N and K because the rate at which Eq. 3 changes withtime (which corresponds to the variance of the burst interval)depends on the difference between K and N (Fig. 2B), while thepoint at which the probability becomes significant (which correspondsto the mean burst interval) depends on the ratio of K to N (Fig.2A).

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Fig. 2. Behavior of the survival function. A time constant of 8 s is used in these examples. A: the difference between N and K determines the slope of the survival function. When (N $-$ K) is constant, variations of N and K shift the curve to the left or right without changing the slope. B: the ratio of K to N determines the position of the curve on the ordinate. When (N/K) is constant, varying N and K changes the slope but has minor effects on the position of the rising portion curve. C: changing $tau$ affects both the position of the survival function on the ordinate and the shape of the survival function. $tau$ was fixed at 8 s in all fits of experimental data.

Equation 3 was fit to the cumulative probability plots of the interburst intervals using 50-100 time increments and least-squaresestimates of goodness of fit to the cumulative probability ofthe burst interval. The incomplete beta function was used to calculatethe cumulative binomial distribution (Press et al. 1997). Equation1 was fit to EPSC rates at postburst intervals before the probabilityof a subsequent discharge became significant (Fig. 6B) and theEPSC rate became unstable (Fig. 6, B and C), using the least-squaresmethod. Equation 1 was also used to fit the length of bursts evokedat variable intervals after a spontaneous burst to assay the degreeof synaptic recovery (Staley et al. 1998), a method analogousto compound EPSC amplitude measurements in paired pulse paradigms(Markram et al. 1998). This fit was only relevant when the stimuluswas sufficiently large to preclude burst initiation failure (Fig.7B).

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Probability distribution of interburst intervals

We induced stable periodic population bursts in hippocampal area CA3 in vitro by either long-term potentiation (LTP) of recurrentcollateral synapses (Bains et al. 1999) or by increasing the concentrationof extracellular potassium (K) above4.5 mM (Fig. 3, A and B; n = 145 slices). The intervals betweenbursts were normally distributed for all conditions (Fig. 3, Cand D) (Robinson et al. 1993). Increasing network excitabilityby increasing K from 5.5 to 10.5 mMaltered the frequency of bursts by over 6 octaves, from <0.05Hz in 5.5 mM K to 1 Hz in 10.5 mM K(Fig. 4, A and B). For each change in K,the corresponding burst intervals were normally distributed aboutthe mean (Fig. 4B) and the variance of the intervals increasedwith the third power of the mean (Fig. 4C).

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Fig. 3. The intervals between CA3 population bursts are normally distributed. A, left: a whole cell recording from a pyramidal cell demonstrating the temporal pattern of spontaneous CA3 discharges in 8.5 mM K. Right: paired recordings from a pyramidal cell (IC) and the pyramidal cell layer (EC) demonstrating that the CA3 network discharges are a synchronous, all-or-none process. B: plot of the intervals between spontaneous CA3 population bursts demonstrates a stable mean burst interval over 30 min. C: intervals in B are normally distributed: a histogram of intervals binned at 100-ms intervals is well fit by the normal distribution ( $---$ ). D: unbinned cumulative probability plot of the data shown in C and the cumulative normal distribution ( $---$ ).

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Fig. 4. The mean vs. variance of the interburst interval. A: interval between CA3 network discharges vs. K ( $---$ ). The level of neuronal excitability alters the interval. B: intervals from the experiment shown in B are normally distributed for each level of K. $---$ , fit normal distributions. C: variance of the discharge intervals shown in B and C increase with the 3rd power of the mean ( $---$ : variance = 0.007 × mean^3.3).

The nonlinear relationship between the variance and the mean of the discharge interval (Fig. 4C) is not easy to reconcilewith a single pacemaking mechanism whose probability changes withnetwork excitability. Neither a Poisson nor a binomial distributioncan describe the observed relationship between the mean and thevariance of the burst intervals (Bethea et al. 1995; cf. Reidand Clements 1999). Rather, this relationship supports the ideathat a process such as recovery from synaptic depression (Eq.1) of a population of synapses is the primary determinant of theburst interval: because the probability of recovery of a singlesynapse (Eq. 1) increases rapidly at short time intervals andmore slowly at longer time intervals (Fig. 5A), the survival function(Eq. 3) has a very tight time distribution for short time intervalsand a much broader distribution at longer intervals for any givenN and K (Fig. 5, B and C). In fact, the probability of recoveryof K synapses from among a candidate pool of size N has the samerelationship between the variance and the mean as the experimentallyobserved probability of a burst (Fig. 4B vs. 5C; the data in Fig.4B are fit by Eq. 3 in Fig. 11A).

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Fig. 5. The survival function has the same relationship between the mean and the variance as the CA3 burst interval distribution. A: plot of Eq. 1, the cumulative probability of recovery from depression at a single synapse. The rate of recovery (time derivative of Eq. 1) is maximal for small time intervals. Time is plotted as multiples of the time constant $tau$ . B: plot of survival function (= 1 $-$ cumulative probability distribution; Eq. 3) for a population of n = 100 and the values of K noted in the figure. C: the mean and variance of the probability density of the survival function (derived by differentiation from the cumulative probability distributions shown in B) change in a manner similar to the network discharge probability density (Fig. 4B).

Estimating the time constant for recovery from synaptic depression

To determine the time constant for recovery from depression at individual synapses (Eq. 1), we measured the rate of spontaneoustransmitter release (Liu and Tsien 1995; Otis et al. 1996; Stevensand Wesseling 1998). The frequency of spontaneous EPSCs was measuredas a function of time after a burst (Fig. 6, A and B). Althoughthe postburst spontaneous EPSC rate should reflect a variety ofprocesses such as diminishing facilitation (Dittman et al. 2000),the monoexponential increase suggests that the EPSC rate is dominatedby recovery from depression. At short postdischarge intervals,the frequency of EPSCs increased with a time constant of 8 ± 2.3(SD) s (n = 8 cells; Fig. 6B). The measured EPSC recovery rateis similar to the rate of recovery in single-synapse studies ofthese neurons (Stevens and Wesseling 1998) and is of the sameorder of magnitude as the intervals between spontaneous bursts(e.g., Fig. 4B). The EPSC rates at longer intervals from the lastburst discharge fluctuated widely, consistent with action-potential-dependenttransmitter release (Fig. 6, B and C) as a consequence of thepositive feedback mediated by the recurrent collateral synapses(Traub and Dingledine 1990; Traub and Miles 1991). There was nocorrelation between the EPSC recovery rate measured from a singlecell recording and the interburst interval in the slice from whichthe cell was recorded, consistent with the idea that synapticrecovery does not vary from slice to slice so that the variationin the measured EPSC recovery rate represented sampling error(1 pyramidal cell of the thousands in the slice) rather than asystematic difference in synaptic recovery rates between slices.We used a fixed recovery time constant of 8 s to fit the datain all subsequent experiments.

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Fig. 6. Synaptic recovery assayed by spontaneous synaptic activity. A: an example of excitatory postsynaptic currents (EPSCs) recorded between network discharges at a holding potential of $-$ 60 mV after induction of discharges by a single tetanization. Clusters of EPSCs occur near the start of a network discharge (Traub and Dingledine 1990

). Afterhyperpolarizations were antagonized by 20 µM norepinephrine in these experiments (Staley et al. 1998

), and GABA_A receptors were blocked with 100 µM picrotoxin. B: the frequency of EPSCs is plotted vs. the time elapsed since the end of the last discharge. $---$ , a fit of Eq. 1 to the initial 12 s of data with $tau$ = 6 s. The EPSC frequency becomes unpredictable at intervals closer to the average discharge interval, which was 20 s in this experiment. EPSCs recorded at a potential of $-$ 60 mV after induction of CA3 discharges using a tetanic stimulation. C: the charge transfer (area) of the EPSCs plotted in B shows a greater increase with time than the EPSC frequency, consistent with action potential-dependent amplification [the increase in EPSC amplitude is not due to postburst changes in dendritic space clamp (Staley and Mody 1992

) because input resistance returned to within 95% of preburst baseline within 3 s after a burst, n = 3 cells (Robinson and Deadwyler 1981

; Staley et al. 1998

)].

Shorter time constant obtained by measuring evoked release

The 8-s time constant for synaptic recovery assayed by EPSC frequency is longer than the time constant of recovery assayedusing osmotically and electrically evoked transmitter release(Staley et al. 1998). When bursts were evoked at various timeintervals following a spontaneous burst, synaptic recovery asassayed by the evoked burst length was too rapid to explain theinterval between discharges: evoked burst length was already maximalwhen the probability of a spontaneous burst was still negligible(Fig. 7A). It has recently been demonstrated that during recoveryfrom synaptic depression, large stimuli can evoke transmitterrelease when small stimuli cannot (Stevens and Wesseling 1998;Wu et al. 1999; modeled in Mateev and Wang 2000). Thus one explanationfor the difference in spontaneous versus evoked recovery may bethe size of the depolarization and the number of cells that aresynchronously depolarized by the electrical stimulus versus aspontaneous EPSP. If this was true, then it would be expectedthat smaller external stimuli should be less effective at triggeringbursts at short postburst time intervals. This effect is illustratedin Fig. 7B: stimuli of two different amplitudes were deliveredthrough the same electrode using the same protocol as for theexperiment illustrated in Fig. 7A. The large stimulus was sufficientto evoke the maximum-amplitude population spike before the inductionof bursting. The smaller stimulus was sufficient to evoke a just-detectablepopulation spike. The duration of the burst evoked by either ofthese two stimuli, each delivered at random intervals after aspontaneous burst, is plotted in Fig. 7B. The smaller stimuliresulted in more failures of burst initiation when delivered atshort intervals following a spontaneous burst. The resulting sigmoidal,rather than exponential, relationship between evoked burst lengthand the interval since the last burst resembled the cumulativeprobability distribution of spontaneous burst initiation (Fig.7, A and B; see also Figs. 3D and 4B), as well as the probabilityof evoking a burst when a single neuron is stimulated (Miles andWong 1983). Thus the rate of recovery from depression varies asa function of the stimulus used to measure it as demonstratedin other systems (Stevens and Wesseling 1998; Wu et al. 1999;modeled in Mateev and Wang 2000). Because spontaneous bursts areinitiated by EPSPs (Chamberlin et al. 1990; Traub and Dingledine1990), we used the 8-s time constant established by the experimentsshown in Fig. 6 for our calculations.

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Fig. 7. Synaptic recovery assayed by evoked network discharges. A: comparison of the recovery rate assayed by evoked CA3 burst length vs. the cumulative probability of a spontaneous burst. The degree of synaptic recovery was assayed by the length of a burst evoked at various time intervals after a spontaneous burst (

), and fit to Eq. 1 ( $---$ ; $tau$ = 1.2 s). The synaptic recovery assayed in this way was essentially complete when the probability of a spontaneous CA3 burst ( $open circle$ ) was still minimal. B: the time course of synaptic recovery approaches the cumulative probability of spontaneous burst intervals as the stimulus strength is decreased. Synaptic recovery was assayed by the duration of evoked bursts as in A.

, duration of bursts evoked at random intervals following the last burst by a large stimulus. Line fit to large stimulus data using Eq. 1, $tau$ = 500 ms.

, duration of bursts evoked at random intervals following the last burst by a smaller stimulus. · · · , SEs. The SE for the smaller stimulus is maximal on the rising portion of the curve due to the mixture of burst initiation failures and successes. Small stimulus burst lengths were fit using a polynomial, because neither Eq. 1 nor 3 was appropriate to fit evoked burst lengths with failures. $open circle$ , cumulative probability of intervals between spontaneous bursts. $---$ , Eq. 3 fit to the interval data with K = 10, n = 11. (The stimulation protocol cannot be accurately extended to intervals that overlap with the spontaneous burst interval because under such conditions a second spontaneous burst may occur in the interval between the initial burst and the evoked burst, resulting in additional synaptic depression.)

Fitting interburst interval probability distributions to the survival function

Once the time course of synaptic recovery is known (Fig. 6B and Eq. 1), it should be possible to predict the probability ofa burst from the probability of recovery of the appropriate numberof synapses (i.e., the probability that K synapses from a poolof N candidate synapses have recovered, Eq. 3). The best testof this idea would be to experimentally determine the value ofK and N and then use these values to predict the burst probability.In the absence of a means to determine K or N directly, we testedthe validity of Eq. 3 by fitting it to the burst probability,thereby deriving the values of K and N. Although there is no directmethod to test whether these fitted values correspond to the actualnumbers of synapses involved in burst initiation, we can testtwo predictions that follow from the idea that CA3 bursts occurwhen a sufficient number of the pool of initiating synapses haverecovered from depression. First, the size of the initiating poolshould be directly reflected in the probability of a CA3 discharge.Second, manipulations of either neuronal excitability or synapticstrength should change N, the number of synapses at which transmitterrelease significantly increases the probability of successfulinitiation of a burst. Manipulations of either neuronal excitabilityor synaptic strength should also produce a corresponding changein K, the number of synapses whose recovery is necessary to initiateaburst.

To test these predictions, synaptic strength was decreased up to 50% using either low concentrations of the competitive non-NMDAantagonist 6,7-dinitroquinoxaline-2,3(1H,4H)-dione (DNQX) (Andreasonet al. 1989; Chamberlin et al. 1990) (n = 7; Fig. 8, A and B),decreasing release probability with baclofen (Scanziani et al.1992; Swartzwelder et al. 1987) (n = 8; Fig. 9, A and B), or bylong-term depression (LTD) of the recurrent synapses (Bains etal. 1999; Cummings et al. 1996; Lisman et al. 1989) (n = 4; Fig.10, A and B). All three methods of decreasing the synaptic strengthincreased the mean and variance of the burst interval. These changeswere well-fit by Eq. 3 ( $---$ in Figs. 8, A and B; 9, A and B; and10, A and B). The fit values of N and K are shown in Figs. 8C,9C, and 10C.

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Fig. 8. The probability of network output is changed when synaptic strength is decreased by low concentrations of an AMPA antagonist. Synaptic strength was altered by decreasing the postsynaptic receptor availability with 6,7-dinitroquinoxaline-2,3(1H,4H)-dione (DNQX). A: the cumulative burst interval probability is plotted for control conditions (8.5 mM K), during bath application of 0.2 µM DNQX and during application of 0.4 µM DNQX. B: the corresponding probability densities for the data shown in A. $---$ in A and B are best fits of Eq. 3 to the data. C: the fit values of K and N vs. the DNQX concentration.

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Fig. 9. The probability of network output is changed by decreasing the probability of transmitter release with baclofen. A: the cumulative burst interval probability is plotted for control conditions (8.5 mM K), during bath application of 1 µM baclofen and during application of 2 µM baclofen. B: the corresponding probability densities for the data shown in A. $---$ in A and B are best fits of Eq. 3 to the data. C: the fit values of K and N vs. the baclofen concentration.

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Fig. 10. The probability of network output is changed by long-term depression (LTD), the strength of the recurrent collateral synapses. LTD was induced by application of 40 µM of the competitive N-methyl-D-aspartate (NMDA) antagonist, D,L-APV during spontaneous CA3 bursting that had been induced by tetanization (Bains et al. 1999

; Cummings et al. 1996

; Lisman 1989

). A: the cumulative burst interval probability is plotted before and after LTD. B: the corresponding probability densities for the data shown in A. $---$ in A and B are best fits of Eq. 3 to the data. C: the fit values of K and N before and after LTD.

Baclofen and DNQX both decreased the average synaptic strength and thus decreased N, the number of synapses capable of participatingin burst initiation. These agents had different effects on K,however. One way to interpret the differential effect on K isin terms of the effects of baclofen and DNQX on inter-burst depression.Depression should be similar at the end of a burst for both agentsdue to the degree of facilitation of release during a burst (Seliget al. 1999). However, between bursts baclofen decreases the probabilityof release (Debanne et al. 1996) and thus the degree of ongoingdepression from spontaneous EPSCs; thus the network may be moreable to respond to an initiating EPSP, which would be reflectedin decreased values of K.

Neuronal excitability was altered by changing K (Fig. 11, A and B; n = 7). Decreasing the networkexcitability produced a corresponding decrease in the size ofthe pool of synapses that were capable of initiating a burst andincreased the fraction of the pool that needed to recover (Fig.11B). When network excitability is increased, bursts are more likelyto be initiated at shorter interburst intervals (Fig. 11, A andB) when the degree of synaptic recovery is less complete. Thisdecreased recovery should be reflected in the burst duration,as is the case for evoked bursts (Fig. 7). Figure 11C plots theduration of spontaneous bursts versus the interval since the lastburst for the experiment in which Kwas varied. The burst duration increases with a time constantof 6 s, close to the rate of synaptic recovery measured from theEPSC rates (Fig. 6B). There is no relationship between spontaneousburst length and interburst interval for any given K(Fig. 11C, insets). This indicates that recovery from depressionis the timing mechanism for burst intervals: if burst durationwere determined by the degree of synaptic recovery, but an independenttiming mechanism (such as dissipation of inhibition) determinedburst intervals, then for any given experimental condition theburst duration versus interval plots (Fig. 11C, insets) would showthe same relationship between burst interval and duration as dothe independently timed evoked bursts in Fig. 7, A and B.

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Fig. 11. Effect of network excitability on burst probability. A: Eq. 3 ( $---$ ) fit to the network output intervals plotted in Fig. 4, A and B. B: the values of N and K for the fits shown in A. The pool size (N) varies from a few dozen to several thousand, and the number required to recover (K) varies from >90 to <20% of N. C: the rate of synaptic recovery can be estimated from the duration of the spontaneous bursts (plotted in A) vs. the interburst interval. Insets: there is no relationship between the interburst interval and the spontaneous burst length for any single level of excitability. The highest (10.5 mM K) and lowest (4.5 mM K) network excitabilities are shown.

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

We conclude that a under a variety of experimental conditions, the temporal pattern of CA3 network output can be accuratelyfit using a pool of exponentially relaxing pacemakers. The timeconstant describing the relaxation of these pacemakers is thesame as the time constant describing the recovery of recurrentcollateral synapses from activity-induced depression. Long andshort-term determinants of synaptic strength and the level ofnetwork excitability affect the distribution of CA3 interburstintervals as predicted if these manipulations affected the totalnumber of synapses in the pacemaking pool (i.e., N, the synapsescapable of participating in burst initiation), and the numberof synapses in the pacemaking pool that must recover before anotherspontaneous burst is possible (K).

Physiological significance of the fit parameters

In the experiment illustrated in Fig. 7B, the calculated number of synapses capable of initiating a burst discharge is 11.If these 11 synapses could be selectively blocked, bursts mightcontinue, but at a somewhat lower frequency. This is because Ncan only be determined for a specific experimental condition anddoes not reflect the number of intact recurrent collateral connectionsin the slice except perhaps as a limit at maximal excitability(Fig. 11, B and C). Further, N may not represent the very strongestsynapses or those with the highest probability of release: ongoingtransmitter release during the interburst interval (Fig. 6A) re-depressesthe synapses that release transmitter too far in advance of burstinitiation. These synapses could be stronger or have a higherprobability of release than the N synapses that actually participatein burstinitiation.

K, the number of synapses that need to recover to initiate a burst, also changes with experimental conditions. Immediatelyafter a burst, synapses are depressed and excitability is correspondinglylow, so K is large. For example in Fig. 7B, most smaller stimulifailed to initiate bursts for the first second after a spontaneousburst. This indicates that during the first second after a bursttime interval, K was larger than the number of synapses activatedby the smaller stimulus. As synapses recover and excitabilityincreases, the number of synapses that are needed to initiatea burst decreases, so the smaller stimulus became sufficient toinitiate a burst. It is important to note in terms of the assumptionsunderlying the derivation of Eq. 3 that this decrease in K iscomplete by the time a spontaneous burst is likely (in Fig. 7,the postburst time interval at which small stimuli trigger burstsas efficiently as large stimuli is shorter than the shortest spontaneousinterburst interval). This result is not an artifact of the choiceof stimulus sizes because Miles and Wong obtained similar resultswith single-cell stimulation (Miles and Wong 1983).

The tendency of K to change in the same direction as N (Figs. 8-11 and 12A) may seem counterintuitive. As network excitabilityincreases, more synapses are capable of initiating a burst, soN increases; it seems that with increasing excitability thereshould be a corresponding decrease in the number of synapses neededto initiate a burst (K). The fraction of synapses in the initiatingpool that need to recover does indeed decrease with increasingexcitability (Fig. 12B). However, the absolute number of synapsesrequired increases due to the increase in the size of the initiatingnetwork of synapses.

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Fig. 12. Relationship between the size of the initiating pool of synapses (N), the number of synapses required to recover to initiate a network output (K), and the probability of network output. A: the range of values of N and K computed for the experiments shown in Figs. 8-11: DNQX ( $down-triangle$ ), baclofen ( $open circle$ ), LTD ( $black-lozenge$ ), and K (

). The average ratio of K to N was 0.55 ± 0.19. B: the fraction of the pool required to recover to initiate a burst (K/N) increases as the probability of network output decreases (increased interval between network outputs, corresponding to decreased network excitability). Pooled data from the experiments shown in Figs. 8-11; symbols as in A. $---$ fit by Eq. 1 with $tau$ = 8 s.

There are many potential biological correlates of N and K. For instance, the decay of inhibitory conductances is a candidatedeterminant of burst probability (Traub and Miles 1991). Becauseblocking these conductances does not alter burst probability significantly,we favor the idea that synaptic depression terminates bursts andrecovery from depression limits the probability of burst initiation(Staley et al. 1998). The large impact of small alterations ofsynaptic strength on the burst probability (Figs. 8-10) (Bains etal. 1999) supports the idea that recovery from synaptic depressionis an important determinant of the probability of network discharge(modeled in Tabak et al. 2000; Tsodyks et al. 2000). For instance,if a pacemaker current was the sole determinant of burst timing,altering synaptic strength should have a more significant effecton burst duration (as in Fig. 7) (see also Staley et al. 1998)rather than the interval between bursts (Fig. 11C, insets).

How EPSP amplitude, resting membrane potential (RMP), and action potential threshold influence N and K is unknown. Understandingthe number of coincident EPSPs that are necessary to trigger anaction potential would clarify burst initiation, but this willrequire a more detailed knowledge of dendritic EPSP algebra (Mageeet al. 1998). Such information would help elucidate how postsynapticinhibition by increasing the number of EPSPs required to initiatean action potential (Miles et al. 1996) modulates the probabilityof synchronous networkactivity.

Limitations

The binomial analysis is based on the related assumptions that the outcome of any one trial does not depend on the others,that the probability of success (p₁) is the same for all N trialsand that all trials are identical. Trials here correspond to theburst probability for each time increment. Because the numberof active neurons in one time interval affects the number of activeneurons in the next, trial-to-trial independence implies thatin this model N does not represent the number of spontaneouslyactive neurons (Butts et al. 1999). The assumption that p₁ isidentical for all trials is strictly true only as a populationaverage because the rate of recovery of individual synapses mayvary (Stevens and Wesseling 1998). The assumption that all trialsare identical implies that any combination of K or N synapsescan initiate bursts. However, there may be circuits in which somesynapses are more important than others, which would violate thisassumption.

This analysis assumes that variation in burst timing is a consequence of variation in the recovery probability of K synapses;the variation in the time required for the recovered synapsesto initiate a burst is neglected. If the time between recoveryand burst initiation is substantial, it would lead to an inaccurateestimate of K (e.g., Fig. 2A). The frequency of EPSCs (Fig. 6)and action potentials (Cohen and Miles 2000) in the intervalsbetween bursts suggests that adequate stimuli for burst initiationare continuously present. The similarity in the variance in CA3burst initiation failures when a known population of synapsesis activated (Miles and Wong 1983) (Fig. 7B) versus the varianceof spontaneous intervals (e.g., Fig. 7, A and B) also suggeststhat synaptic recovery is the main source of variation, but thisneeds to be studied systematically. For instance, Eq. 1 couldbe modified to a more general expression of the probability ofachieving sufficient interburst synaptic strength, where synapticstrength is the product of the degree of depression, the baselineprobability of release, and the postsynaptic effect. The lasttwo terms can be combined as a term multiplying Eq. 1: A_o × (1- e ^-t/). Then if synapses are substantially weakened either pre- orpostsynaptically, full recovery of p₁ would still leave the probabilityof achieving full synaptic strength at <1 (Fig. 1, middle) becauseA_o would be <1; under those conditions, much longer interburstintervals can be accommodated, but at the cost of another fittedvariable. Verification would require dual recordings of synapticallyconnected pyramidal cells to ascertain A_o.

We have not considered variations in $tau$ , the time constant for recovery from synaptic depression at a single synapse, as anexplanation for burst timing. Although $tau$ clearly affects Eqs.1-3 (Fig. 2C), $tau$ was fixed at 8 s for two reasons. First, we wishedto limit the number of free variables in the fits. Second, themanipulations shown in Figs. 9-11 affect burst interval but do notaffect $tau$ (e.g., Fig. 6D of Staley et al. 1998). However, otherexperimental manipulations, such as alterations of calcium homeostasisin the synaptic terminal, might affect $tau$ (Dittman et al. 2000;Stevens and Wesseling 1999).

The information provided by this model, the burst probability as a function of time, is much more limited than informationprovided by models that describe the activity of every cell inthe network (Traub and Miles 1991) or the spatial distributionof network activity (Butts et al. 1999). The limited predictionsof this model allow the number of free parameters to be limitedto the experimentally determined synaptic recovery rate and thefit parameters N and K. More detailed network models should provideadditional insights into relationship of network behavior andthe degree of synaptic depression and recovery as well as themost accurate physiological correlates of theseparameters.

Definitive proof of the depression recovery model of burst timing requires measurement and manipulation of N and K to testwhether the manipulations affect burst timing as Eq. 3 predicts.This could be approached qualitatively by sectioning the CA3 networkand comparing burst interval distribution to the size of the remainingnetwork (Miles et al. 1984). This issue might be studied quantitativelyin autaptic cell cultures, where high degrees of synaptic positivefeedback produce discharge patterns similar to CA3 bursts (Segaland Furshpan 1990). In the autaptic preparation, the number andactivity of feedback synapses can be quantified (Prange and Murphy1999) and manipulated (Liu et al. 2000).

Comparison to "recovering pacemaker current" model

Pacemaker currents such as I_H have been proposed to underlie several oscillatory network behaviors (McCormick and Pape 1990).This model of burst timing could also be described by Eq. 3: ifthe pacemaker conductance was inactivated by the membrane depolarizationthat occurred during the CA3 burst and if the conductance recoveredfrom inactivation with first-order kinetics during the interburstinterval, then N could represent the pool of pacemaking neurons,and K could represent the subset that needed to have their pacemakingconductances reach a particular threshold of de-inactivation totrigger a burstdischarge.

A disadvantage of the "recovery to noisy threshold" model when applied to pacemaking neurons is that the recovery of the wholecell pacemaker conductance should not be probabilistic becausewhole cell recovery is the average of the recovery of a very largenumber of stochastically recovering channel proteins. Thus thetrick of equating a recovery rate to a probability (Eq. 1) isnot as easy to support for neurons as it is for individual synapses,which are known to behave in a stochastic manner (Fatt and Katz1952). A physiological disadvantage of I_H as a pacemaking conductanceis that I_H has a net inhibitory effect in hippocampal pyramidalcells (Magee 1998) and thus is not well suited to initiate CA3bursts; further, CA3 bursts proceed normally after I_H is blocked(Xiong and Stringer 1999).

Instead of a pacemaking conductance, the rate-limiting recovery process that sets the CA3 interburst interval might be thede-inactivation of a voltage-dependent depolarizing membrane conductanceto a particular threshold value. Examples might be dendritic conductancesthat amplify EPSPs, such as the dendritic sodium conductance orlow-threshold calcium conductance (Magee et al. 1998). If thethreshold to which the conductance needed to recover varied fromburst to burst, then the binomial distribution used in Eqs. 2and 3 might be replaced by a normal distribution that describesthe average value and standard deviation of this probabilisticthreshold. As shown in Fig. 13, the recovery of a membrane conductanceto a noisy threshold also fits the data.

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Fig. 13. The interburst interval distribution can be fit with a model employing relaxation of a first-order process (Eq. 1) to a noisy threshold. If the threshold's probability is normally distributed, the interburst intervals can be described by Eq. 3 with the cumulative normal distribution used instead of the cumulative binomial distribution. The LTD data shown in Fig. 9 are fitted here by least squares with a relaxation time constant of 8 s. In control conditions, the threshold = 0.85 ± 0.052, and after LTD, the threshold was 0.955 ± 0.03 (means ± standard deviaton).

A physiological disadvantage of the recovery to noisy threshold model is that there are no known pacemaking or voltage-dependentdepolarizing conductances that have an inactivation recovery timeconstant in the range (~8 s at 35°C) that fits the interburstinterval data (Magee 1998; Mickus et al. 1999), although it isconceivable that second-messenger regulation of a pacemaker conductancemight have the appropriate kinetics. Further, manipulation ofthe known candidate conductances does not produce the expectedeffects on burst intervals. For example, blocking I_A negates mostof the effects of dendritic sodium current inactivation (Colbertet al. 1997), but the intervals between CA3 bursts induced bythe I_A antagonist 4AP are similar to those induced by other means(Traub and Miles 1991). A conceptual disadvantage of the recoveryto noisy threshold model is that the threshold to which the conductancemust recover to trigger a burst is described by a mean and SDthat have no easily testable physiological interpretation (Fig.13).

Although both models can be equally well fit to the burst interval distributions, we favor the synaptic recovery model. Thismodel is based on measured recovery synaptic rates that are consistentwith the interburst intervals, and this model is based on morereadily quantifiable parameters that can be subjected to experimentaltesting.

Implications

An important result of this analysis is that spontaneous transmitter release, which appears to be noise at a single synapse(McCormick 1999; Staley 1999), has a central role in signalingthe recovery from depression and driving network output. Thuslinking synaptic properties to network behavior is not only importantfor understanding neural networks but also for understanding thesignificance of the synapticproperties.

Many neuronal oscillators use membrane conductances for positive and negative feedback. In the bursting CA3 network, positiveand negative feedback is provided by depressing recurrent collateralsynapses. Thus a network of depressing positive feedback synapsescan comprise a distributed synaptic clock (O'Donovan and Rinzel1997; Tabak et al. 2000; Tsodyks et al. 2000). Such an oscillatorcontains no pacemaker cells but rather pacemaker synapses thatcan be tuned by long-term alterations in synaptic strength (Bainset al. 1999; King et al. 1999) (Fig. 10) and synaptic input (Fig.7B).

One prediction of this analysis is that the smallest increment in burst probability is effected by the gain or loss of a singleinitiating synapse. As N approaches K (Figs. 8-10), this should bereflected in quantized values of the observed means and variancesof the burst interval as synaptic strength is varied. For example,when burst probability is already low, further small decreasesin synaptic strength produce a complete cessation of burstinginstead of a proportional decrease in the burst frequency (Bainset al. 1999).

The distribution of the intervals between the bursts of a periodically discharging neural network provides information aboutthe level of network excitability and the number of initiatingpositive feedback synapses. This method can be readily appliedto less accessible networks. For example, this analysis wouldallow an estimation of the amount of positive feedback in an epilepticfocus (Lytton et al. 1998; Prince 1999) based on the temporaldistribution of electroencepholographic interictal discharges,which might help predict the risk of spontaneousseizures.

	ACKNOWLEDGMENTS

We thank Drs. John Lisman, F. Edward Dudek, and Thomas Dunwiddie for helpful discussions and comments on themanuscript.

This work was supported by the National Institute of Neurological Disorders and Stroke and the Epilepsy Foundation ofAmerica.

	FOOTNOTES

Address for reprint requests: K. J. Staley, Depts. of Pediatrics and Neurology, B182, University of Colorado Health SciencesCenter, 4200 E. Ninth Ave., Denver, CO 80262 (E-mail: kevin.staley{at}uchsc.edu).

Received 28 December 2000; accepted in final form 6 August 2001.

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