Long-Lasting Inhibitory Synaptic Depression is Age- and Calcium-Dependent

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Web of Science (29)

Citing Articles via Google Scholar

Google Scholar

Articles by Kotak, V. C.

Articles by Sanes, D. H.

Search for Related Content

PubMed

PubMed Citation

Articles by Kotak, V. C.

Articles by Sanes, D. H.

Pubmed/NCBI databases
Compound via MeSH
Substance via MeSH
Hazardous Substances DB
CALCIUM COMPOUNDS
CALCIUM, ELEMENTAL

Previous Article  |  Next Article

The Journal of Neuroscience, August 1, 2000, 20(15):5820-5826

Long-Lasting Inhibitory Synaptic Depression is Age- and Calcium-Dependent
Vibhakar C. Kotak¹ and Dan H. Sanes¹^,²
¹ Center for Neural Science and ² Department of Biology, New York University, New York, New York 10003

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The developmental refinement of excitatory synapses is often influenced by neuronal activity, and underlying synaptic mechanismshave been suggested. In contrast, few studies have asked whetherinhibitory synapses are reorganized during development and whetherthis is accompanied by use-dependent changes of inhibitory synapticstrength. The topographic inhibitory projection from the medialnucleus of the trapezoid body (MNTB) to the lateral superior olive(LSO) undergoes synapse elimination during development (Sanesand Takács, 1993). To determine whether there is an associatedperiod of synaptic plasticity, whole-cell recordings were obtainedfrom developing LSO neurons of gerbils in a brain slice preparation.In current-clamp recordings, low-frequency stimulation of theMNTB led to a decline in IPSP amplitude by 43%. In voltage-clamprecordings, hyperpolarized LSO neurons also exhibited a long-lastingdepression of MNTB-evoked inhibitory synaptic currents (34%) afterlow-frequency stimulation. When LSO neurons were depolarized,low-frequency stimulation of the MNTB produced a significantlylarger inhibitory synaptic depression (59%). This synaptic plasticitydeclined dramatically by postnatal days 17-19. Similar to wellstudied forms of excitatory synaptic plasticity, inhibitory depressiondepended on postsynaptic calcium. We propose that such activity-dependentsynaptic depression may support the developmental rearrangementof inhibitory terminals as they compete with neighboring excitatoryand/or inhibitoryinputs.

Key words: LTD; LSO; inhibition; development; synaptogenesis; calcium

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The refinement of excitatory projections has been well described in systems as diverse as the neuromuscular junction and thevisual cortex. Furthermore, the formation and elimination of excitatoryconnections depend, in part, on synaptic transmission. Thus, whenneural activity is blocked or altered in the developing visualpathway, excitatory terminals may innervate inappropriate targets(Constantine-Paton et al., 1990; Shatz, 1990). The mechanism thatmediates excitatory synaptic refinement is not yet known, althoughthere is strong evidence that NMDA receptors are involved in theactivity-dependent stabilization of glutamatergic connectionsin the CNS (Constantine-Paton and Cline, 1998). At the vertebrateneuromuscular junction, excitatory synapse elimination may relyon a calcium-dependent depression mechanism (Lo and Poo, 1994;Cash et al., 1996; Colman et al., 1997). Despite these tremendousadvances in our understanding of excitatory synaptic plasticityin developing systems, there is little information about the activity-dependentrefinement of central inhibitory connections. In the present study,we demonstrate use-dependent depression at a set of inhibitorysynapses that are known to be refined via a process of synapseelimination (Sanes and Takács, 1993).

One reason that motor neuron and retinal ganglion cell afferents have been so well studied is that they form pure excitatoryprojections. To test selectively the role of inhibitory transmissionduring development, it seemed important to identify a similarkind of projection. The lateral superior olivary nucleus (LSO)is a central auditory structure that encodes interaural leveldifferences, an acoustic cue that is used for sound localization.LSO neurons perform this computation by integrating excitatoryinputs driven by the ipsilateral ear with inhibitory inputs drivenby the contralateral ear (see Fig. 1A). Inhibitory afferents fromthe medial nucleus of the trapezoid body (MNTB) form a tonotopicprojection in LSO that is aligned with the ipsilateral excitatoryprojection (Sanes and Rubel, 1988). During postnatal development,individual MNTB arbors become ~30% more restricted along the frequencyaxis (Sanes and Siverls, 1991). Furthermore, if MNTB neurons arefunctionally denervated by removal of the contralateral ear, thenthe arbors remain in their expanded state, suggesting the involvementof an activity-dependent mechanism (Sanes and Takács, 1993).Recently, it has been found that inhibitory terminals on anotherbinaural nucleus, called the medial superior olivary nucleus (MSO),also undergo a period of synaptic pruning (Kapfer et al., 1999).In this case, inhibitory synapses are initially spread out alongMSO dendrites but are restricted to the soma during development,a process that also appears to require activity. Taken together,these data suggest that MNTB synapses may compete with inhibitoryand/or excitatory terminals for postsynaptic space during earlypostnatal development. Therefore, we asked whether inhibitoryafferent activity influences the strength of their inhibitorysynapses within the LSO. Specifically, we were interested in exploringwhether activation of MNTB afferents at low levels could decreaseinhibitory transmission in the LSO, because low-frequency stimulationof excitatory afferents has been shown to produce a decline inexcitatory synaptic strength (Dudek and Bear, 1992).

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

MNTB-LSO slice preparation. Gerbils (Meriones unguiculatus) aged postnatal day 7 (P7)-P12 or P17-P19 were used to generate300 µm transverse brain slices through the LSO and medial nucleusof the trapezoid body (Sanes, 1993). The artificial CSF (ACSF)contained (in mM): 125 NaCl, 4 KCl, 1.2 KH₂PO₄, 1.3 MgSO₄, 26NaHCO₃, 15 glucose, 2.4 CaCl₂, and 0.4 L-ascorbic acid, pH = 7.3when bubbled with 95% O₂/5% CO₂. ACSF was continuously superfusedin the recording chamber at 5 ml/min at room temperature (23-24°C).

Whole-cell electrophysiology and pharmacological manipulations. Initially, whole-cell current-clamp recordings were performedin LSO to examine the influence of prolonged MNTB stimulation(see Fig. 1B; n = 10). Recording electrodes were fabricated fromborosilicate glass microcapillaries (1.5 mm outer diameter), andtheir resistance ranged from 5 to 10 M $Omega$ . Access resistance wasbalanced throughout the recordings and generally ranged between15 and 40 M $Omega$ . The internal patch solution contained (in mM): 127.5potassium gluconate, 0.6 EGTA, 10 HEPES, 2 MgCl₂, 5 KCl, 2 ATP,and 0.3 GTP, pH = 7.2.

In the majority of experiments, whole-cell voltage-clamp recordings were obtained from LSO neurons at a holding potentialof $-$ 55 to $-$ 90 mV (see Fig. 2; n = 10) or 0 mV (see Fig. 3; n =21), while electrical stimuli were delivered directly to the MNTB(see Fig. 1A). The wide range of hyperpolarizing holding potentialswas chosen to record IPSCs at an operational resting potentiallevel or, if the ISPCs were small, at more hyperpolarized levelsto increase the driving force and thus enhance their baselineamplitude. The internal patch solution contained cesium gluconate(127.5 mM) to block most potassium channels, and QX-314 (5 mM)was added to block voltage-dependent sodium channels. The restof the constituents (in mM) were the same as those in currentclamp (pH = 7.2). To decrease postsynaptic free calcium, BAPTA(20 mM) was added to the recording pipette solution in some experiments.This solution was made separately, and the pH was adjusted to7.2. A Warner Instruments PC-501A was used for recordings, and~70% of the access resistance wascompensated.

After a whole-cell voltage-clamp recording was obtained (Kotak et al., 1998), a modified ACSF with kynurenic acid (5 mM; pHadjusted to 7.3) was superfused for 6 min before adjusting theholding potential either to $-$ 55 to $-$ 90 mV or to 0 mV for the durationof the recording. Under these conditions, MNTB-evoked maximumIPSCs were recorded as inward or outward currents, respectively(Kotak et al., 1998). The voltage pulse (200 µsec) that evokedthe maximum amplitude IPSC was used for the remainder of the experiment.During a 15 min control period, MNTB-evoked IPSCs were acquiredevery minute for the first 5 min and then at 10 and 15 min. MNTBwas then activated with low-frequency stimulation (LFS; 1 Hz for15 min). This protocol was chosen because it has been shown previouslyto induce long-term depression (LTD) of excitatory synapses inthe hippocampus (Dudek and Bear, 1992). In addition to hyperpolarizedpotentials, a holding potential of 0 mV was selected because asimilar pairing of depolarization and 1 Hz stimulation was usedto study age-dependent plasticity of excitatory connections inbarrel cortex (Crair and Malenka, 1995) and robust IPSCs freeof EPSCs were recorded previously (Kotak et al., 1998). A smallnumber of P7-P12 neurons (n = 6) exhibited a significant and rapidreduction of MNTB-evoked IPSCs during the initial 15 min controlperiod, and these neurons were excluded from the analysis becausewe believed this behavior indicated a sudden decline inviability.

Immediately after LFS, MNTB-evoked IPSCs were recorded every minute for the first 5 min and then every 5 min for the nexthour. The total duration of the experiments was therefore typically90 min. In some cases, recording was extended for an additionalhour. The IPSC amplitudes and their slopes were analyzed off-lineusing custom software (Sanes, 1993). In some neurons, to see theeffect of the absence of LFS and the interim afferent activityduring the 90 min data acquisition, five IPSCs were recorded beforeand 90 min after holding the cells at V_HOLD = $-$ 80 mV (n = 6) orV_HOLD = 0mV.

To assess the effect of a potent [Ca²⁺]_i chelator, a separate group of recordings were performed with 20 mM BAPTA (MolecularProbes, Eugene, OR) in the internal recording solution at V_HOLD $<=$ $-$ 55 mV (n = 7) or V_HOLD = 0 mV (n =12).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Current-clamp recordings were obtained from LSO neurons without any pharmacological manipulations, while electrical stimuliwere delivered directly to the MNTB (Fig. 1A). LFS (1 Hz for 15min) of the MNTB produced long-lasting depression of the evokedIPSPs. At 60 min after LFS, the IPSP amplitude declined by 43± 7% (n = 10; mean ± SEM) when compared with the initial IPSPamplitude (Fig. 1B). The membrane potential of some neurons changedby up to 6 mV after LFS. Therefore, to determine whether depolarizationitself could generate a similar IPSP reduction, we raised membranepotential by 10-15 mV (n = 5). Before LFS, the IPSP amplitudeincreased by 3.2 ± 0.3 mV during membrane depolarization. AfterLFS, the increase in IPSP amplitude was 1.1 ± 0.3 mV (mean ± SEM).Thus, in both control and depressed conditions, the increasedIPSP amplitude during membrane depolarization was approximatelyproportional to the IPSP amplitude at rest.

View larger version (23K):
[in this window]
[in a new window]
Figure 1. Long-lasting depression of inhibitory synapses in the LSO. A, Schematic of the inhibitory pathway from MNTB to LSO used in the present study is shown. LSO neurons receive a direct inhibitory projection from several MNTB neurons and excitatory inputs from several ipsilateral ventral cochlear nucleus (VCN) neurons. MNTB neurons also project to the MSO. B, IPSPs were recorded from the medial limb of the LSO, while electrical stimuli were delivered to the MNTB. In this P9 LSO neuron, IPSP amplitude remained fairly stable during the first 15 min recording period (the time at which each IPSP was obtained is shown beneath each trace). LFS (1 Hz for 15 min; gray bar) was then provided to the MNTB at a stimulus intensity that evoked a maximum amplitude IPSP. IPSPs were depressed during the 1 hr period after LFS. The bottom dashed line indicates the initial resting membrane potential. During the pre-LFS period, the amplitude of an IPSP recorded at a $-$ 40 mV membrane potential (+0.02 nA) was augmented by ~3 mV, and a similar depolarization 1 hr after LFS increased the depressed IPSP by ~1 mV.

To better assess long-lasting depression of MNTB-evoked inhibitory transmission, we performed the remainder of the experimentsunder voltage-clamp conditions, while ionotropic glutamate receptorswere blocked pharmacologically. At a holding potential of $-$ 55to $-$ 90 mV, when MNTB was directly stimulated, IPSCs were recordedas inward currents (Fig. 2A). At these hyperpolarized potentials,LFS (1 Hz for 15 min) of the MNTB produced long-lasting depressionof the evoked IPSCs (Fig. 2B). At 60 min after LFS, the IPSC amplitudedeclined by 34% when compared with the initial IPSC amplitude(Fig. 2B). To determine whether synaptic depression was causedby the LFS and in absence of any afferent activation, recordingswere obtained for an equivalent amount of time (90 min) withoutany stimulation of the MNTB (Fig. 2B, asterisks). The LFS treatmentinduced a significant depression when compared with these controlrecordings.

View larger version (28K):
[in this window]
[in a new window]
Figure 2. Long-lasting depression of inhibitory synapses in the LSO at a holding potential of $-$ 55 mV or less (voltage clamp). A, Representative recordings from a P10 LSO neuron show a maximum amplitude IPSC recorded at V_HOLD = $-$ 80 mV at the beginning of the experiment (0 min) and its post-LFS depression at the end of the experiment (90 min). B, Long-lasting depression of IPSCs for all recorded LSO neurons at P7-P12 is shown. Means (± SEM) of IPSCs show that synaptic depression was significant after LFS (black circles). Age-matched control neurons that did not receive any LFS or intermediary MNTB stimulation (asterisks) did not get depressed. See Figure 6 for statistics.

In a separate set of recordings, we determined whether inhibitory synaptic depression was influenced by postsynaptic membranepotential. LSO neurons were held at 0 mV, and electrical stimuliwere once again delivered to the MNTB while IPSCs were recordedas outward currents. As shown for one P9 neuron in Figure 3A,MNTB-evoked IPSCs were ~110 pA during the first 15 min of recordingbut decreased to ~50 pA after LFS. All 21 neurons recorded fromP7 to P12 slices displayed a depression whose magnitude was significantlygreater than that recorded at hyperpolarized potentials (see Fig.6). As shown in Figure 3B, the IPSC amplitude decreased by over55% at 50-60 min after LFS. There was also a complementary declinein IPSC slope (before LFS, 7.4 ± 0.7 pA/msec; after LFS, 3.5 ±0.4 pA/msec), indicating that the peak IPSC amplitude and itstime to peak had both decreased concomitantly. In five neurons,the recording continued for 2 hr after LFS, and the synaptic depressionpersisted during this period. When recordings were obtained for90 min in the absence of LFS to the MNTB (but with continued acquisitionof IPSCs), a 21% decrease in IPSC amplitude was observed (Fig.3B). In addition, there was a small (~15%), but significant, declinein IPSC amplitude in the absence of any interim MNTB activity(see Figs. 3B, 6). The IPSC amplitude in LFS-treated neurons wassignificantly reduced compared with both control groups (see Fig.6). The effect was not caused by the particular glutamatergicantagonist used (kynurenic acid) because depression was also observedin the presence of 20 µM CNQX and 40 µM AP-5 (62% depression at60 min after LFS; n = 2).

View larger version (21K):
[in this window]
[in a new window]
Figure 3. Long-lasting depression of inhibitory synapses in the LSO at a holding potential of 0 mV. A, Long-lasting depression of inhibitory transmission for an individual P9 LSO neuron is shown. Top, Representative MNTB-evoked IPSCs are shown before (left) and after (right) LFS. Bottom, The amplitude of IPSCs in one neuron declined dramatically after LFS, and this depression persisted for 1 hr. B, Long-lasting depression of IPSCs for all recorded LSO neurons at P7-P12 is shown. Means (± SEM) of IPSCs show that synaptic depression was profound after LFS (black circles). Age-matched control neurons in which LFS was not delivered (white circles) or without LFS and intermediary MNTB stimulation (asterisks) displayed a smaller, but significant, decrease in amplitude.

If inhibitory synaptic depression is a developmental mechanism that is specifically involved in the refinement of inhibitoryMNTB synapses, then we might expect to see a decline in plasticityafter anatomical refinement has been primarily completed (Sanesand Siverls, 1991). Therefore LSO neurons were recorded at V_HOLD= 0 mV in P17-P19 slices to test the age dependence of synapticdepression. As shown in Figure 4, although LFS produced a declinein IPSC amplitude at P17-P19, this decrease was significantlyless when compared with the depression in IPSCs in the P7-P12group otherwise treated under similar conditions (see Fig. 6).

View larger version (30K):
[in this window]
[in a new window]
Figure 4. Long-lasting synaptic depression was age-dependent. Top, MNTB-evoked IPSCs in a P17 neuron before LFS (left) and 60 min after LFS (right). Bottom, A comparison of summary data from P17 to P19 LSO neurons that were treated with LFS (white squares) with data from P7 to P12 neurons (gray circles). The magnitude of synaptic depression in the older age group is much reduced (see Fig. 6 for statistics).

We next asked whether postsynaptic calcium was necessary to elicit inhibitory synaptic depression. A calcium chelator (BAPTA,20 mM) was added to the pipette solution and allowed to equilibratefor 5 min before the experiment commenced. We performed the BAPTAmanipulation experiments at both hyperpolarized and depolarizedholding potentials because depression was recorded in either condition.As shown in Figures 5 and 6, this manipulation completely eliminatedinhibitory synaptic depression after LFS in P7-P12 neurons. Infact, we observed potentiation of MNTB-evoked IPSCs after LFSin 6 of the 12 neurons recorded at V_HOLD = 0 mV.

View larger version (23K):
[in this window]
[in a new window]
Figure 5. Long-lasting synaptic depression was calcium-dependent. A, Bottom, Comparison of synaptic depression in P7-P12 neurons at holding potentials of less than or equal to $-$ 55 mV recorded with normal pipette solution [gray circles (from Fig. 2)] or with pipette solution containing 20 mM BAPTA (black squares). Synaptic depression was abolished by intracellular perfusion with BAPTA (see Fig. 6 for statistical comparisons). Top, Representative current traces for one BAPTA-treated P9 neuron. B, Bottom, Comparison of synaptic depression in P7-P12 neurons at a holding potential of 0 mV recorded with normal pipette solution [gray circles (from Fig. 3)] or with pipette solution containing 20 mM BAPTA (gray squares). Synaptic depression was abolished by intracellular perfusion with BAPTA (see Fig. 6 for statistical comparisons). Top, Representative current traces for one BAPTA-treated P9 neuron. Note that the mean size of IPSCs in BAPTA-treated neurons became larger after LFS, although the variance was high.

View larger version (23K):
[in this window]
[in a new window]
Figure 6. Comparison of percent change of IPSC amplitude at 90 min in each experimental group. At V_HOLD $<=$ $-$ 55 mV, LFS produced a significant change in IPSC amplitude as compared with no stimulation (No Stim; p < 0.05; t = symbol 45 2.16; df = 14) or LFS + BAPTA (p < 0.05; t = 2.1; df = 15). At V_HOLD = 0 mV, LFS at P7-P12 produced a significant change in IPSC amplitude as compared with no LFS (p < 0.0005; t = symbol 45 3.6; df = 29), no stimulation (p < 0.05; t = symbol 45 3.6; df = 29), LFS at P17-P19 (p < 0.0005; t = symbol 45 4.14; df = 28), or LFS + BAPTA (p < 0.0001; t = 3.6; df = 31). Finally, LFS induced a significantly greater reduction in IPSC amplitude when delivered at V_HOLD = 0 as compared with V_HOLD $<=$ $-$ 55 (p < 0.05; t = 2.23; df = 29). The mean percent change was calculated by comparing the average IPSC amplitude recorded at 50-60 min after LFS with the initial IPSC amplitude.

Finally, we considered the possibility that two factors could contribute to synaptic depression: a general change in the postsynapticexcitability or a depolarizing shift in E_IPSC. Alteration of postsynapticmembrane properties could not have produced the depression becausethe minor change in holding current (I_HOLD) during the periodof recording was nearly identical for both LFS-treated and controlneurons. In fact, the I_HOLD decrease was slightly greater forcontrol neurons (control, $-$ 48 ± 10 pA; LFS, $-$ 35 ± 7 pA; t = 1.019;p = 0.32). Nonetheless, to determine whether I_HOLD contributedto depression, IPSCs were reanalyzed after the holding currentwas adjusted to its pre-LFS value. This manipulation did not changeIPSC amplitude significantly (before LFS, 128 ± 10 pA; after LFS,56 ± 8 pA; after LFS with adjustment of I_HOLD , 74 pA ± 11 pA;t = 2.0; p = 0.16; n = 9). The E_IPSC also depolarized slightlyduring the course of the experiments (before LFS, E_IPSC = $-$ 40± 1.5 mV; after LFS, E_IPSC = $-$ 33 ± 2.6 mV; t = 2.0; p = 0.02;n = 11). However, we found that there was a significant declinein the inhibitory conductance after LFS, suggesting that the drivingforce (E_HOLD $-$ E_IPSC) played only a minor role in depression (beforeLFS, 4.7 ± 0.8 pS; after LFS, 2.3 ± 0.2 pS; t = 2.08; p = 0.05;n = 11). In fact, inhibitory depression of >50% was observed inthree LSO neurons without any shift in E_IPSC.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Our study attempts to bridge previous data showing that inhibitory synapses are rearranged in the developing central auditorysystem (Sanes and Takács, 1993) with a candidate mechanism, long-lastingdepression of synaptic transmission. There are several lines ofevidences that synaptic depression contributes to the developmentalreduction of polyneuronal innervation at the nerve-muscle junction.Electrical stimulation of one set of motor axons can speed upthe process of synapse elimination and produce a weakening ofunstimulated terminals (O'Brien et al., 1978; Ridge and Betz,1984; Balice-Gordon and Lichtman, 1994; Lo and Poo, 1994). Thismechanism appears to be dependent on a postsynaptic rise in calcium(Connold et al., 1986; Cash et al., 1996). LTD of excitatory synapsesis also well characterized in the CNS (Linden and Connor, 1995),and an age-dependent decline of excitatory LTD has been demonstrated(Battistin and Cherubini, 1994; Dudek and Friedlander, 1996; Feldmanet al., 1998). For example excitatory LTD is present in layerIV of the visual cortex in juvenile cats and guinea pigs but isvirtually absent in adult animals (Dudek and Friedlander, 1996).

In the LSO, several experimental findings suggest that spontaneous inhibitory activity influences the maturation of neuronalmorphology and physiology within the LSO, including the expressionof NMDA receptors (Sanes et al., 1992; Kotak and Sanes, 1996;Sanes and Hafidi, 1996). The present results are broadly consistentwith the remodeling of inhibitory synaptic pathways during development(Sanes and Siverls, 1991; Sanes and Takács, 1993). Inhibitorydepression recorded under either current- (Fig. 1) or voltage-clamp(Figs. 2-6) conditions, and at different holding potentials, supportsthe hypothesis that this phenomenon may be an integral elementof inhibitory synaptogenesis. In other forms of inhibitory plasticitythat decrease GABAergic transmission, glutamate may mediate depolarization-inducedsuppression of inhibition via a metabotropic signaling at theinterneuron-Purkinje cell synapse (Glitsch et al., 1996) or atthe hippocampal CA1 neurons (Morishita et al., 1998). In our experiments,inhibitory depression was maximized by a postsynaptic depolarizationand high intracellularcalcium.

Inhibitory synaptic depression was strongest in P7-P12 LSO neurons (Figs. 1-3), near the onset of response to airborne sound(Finck et al., 1972; Harris and Dallos, 1984; Woolf and Ryan,1985; Sanes and Siverls, 1991). By P17-P19, the magnitude of inhibitorydepression had declined to less than one-half the magnitude observedin younger animals (Fig. 4). Thus, the age at which inhibitorydepression was observed correlates rather precisely with the periodof normal inhibitory synapse elimination (Sanes and Siverls, 1991).If use-dependent synaptic depression is to have an effect on inhibitorysynaptogenesis, then it is important to determine whether neuralactivity exists during the period of inhibitory synapse elimination.We have shown previously that spontaneous activity is presentin the developing gerbil auditory nervous system, but at a relativelylow level (Kotak and Sanes, 1995). In vivo recordings confirmthat inhibitory synaptic drive is present by postnatal day 13(Sanes and Rubel, 1988). In addition, the rate of spontaneousinhibitory synaptic currents can be dramatically enhanced by serotonin(Fitzgerald and Sanes, 1999). Thus, inhibitory depression couldbe elicited by either spontaneous or driven inhibitory synapticactivity in vivo.

Inhibitory synaptic depression occurred after a relatively brief (1 Hz; 15 min) train of stimuli to the entire MNTB afferentpopulation. As shown in Figure 2, the effect was observed whenLSO neurons were held at a potential equal to, or more hyperpolarizedthan, their normal resting membrane potential (less than or equalto $-$ 55 mV). The depression was clearly related to synapse activityin that nonstimulated preparations displayed no depression after90 min of recording (Fig. 2). Therefore, it is possible the inhibitorysynapses compete with one another on the basis of their abilityto evoke a postsynaptic response. When LSO neurons were depolarizedto 0 mV, LFS produced a significantly greater depression of theevoked IPSCs (Fig. 3). This result suggests that excitatory synapticactivity may actually facilitate the inhibitory depressionmechanism.

Intracellular free calcium was a necessary component of inhibitory synaptic depression, evoked at either hyperpolarized ordepolarized membrane potentials (Fig. 5). Addition of the calcium-chelatingagent BAPTA to the pipette solution resulted in the complete absenceof depression after LFS. In fact, there was some indication thatvery low postsynaptic calcium levels were associated with a potentiationof the evoked IPSC. A 20% increase in the IPSC amplitude was observedat 90 min when LFS was delivered in the presence of intracellularBAPTA (Fig. 5).

Although calcium was involved in synaptic depression at 0 or less than or equal to $-$ 55 mV, it is likely that the mechanismof calcium entry or mobilization differs under these two conditions.For example, neonatal inhibitory synapses have been shown to evokedepolarizing postsynaptic potentials because the chloride extrusionmechanism is not yet mature (Payne et al., 1996; Plotkin et al.,1997; Backus et al., 1998; Ehrlich et al., 1999; Kakazu et al.,1999; Lu et al., 1999; Rivera et al., 1999; Williams et al., 1999).Depolarizing IPSPs only are observed until approximately P7 inthe rat LSO (Kandler and Friauf, 1995). In this study, persistentactivation of inhibitory synapses does not lead to an inversionof the chloride gradient because IPSPs remained hyperpolarizingeven after LFS (Fig. 1). A direct increase of postsynaptic calciumby inhibitory activity (Connor et al., 1987; Ben-Ari et al., 1989;Ito and Cherubini, 1991; Obrietan and Van den Pol, 1995; Boehmet al., 1997; Lo et al., 1998; Kullman and Kandler, 1999) afterP8 in the gerbil LSO thus appears an unlikely mechanism for calcium-mediateddepression, although the blockade of depression by BAPTA suggeststhat intracellular free calcium is a necessary element (Fig. 5).

Although the inefficient space clamp of distal LSO neuron dendrites during hyperpolarizing holding potential commands at thesoma must be kept in mind, it is difficult to explain how theLSO calcium concentration could be increased when the membranepotential is held at a hyperpolarized level. One other possibilityis that the inhibitory synapses activate a metabotropic pathway.For example, we have reported previously that inhibitory synapsesare predominantly GABAergic at P3-P5 and become primarily glycinergicby P16 (Kotak et al., 1998). Furthermore, functional GABA_B receptorsare present during the ages when GABA is released. It is alsoknown that MNTB neurons contain BDNF and that LSO neurons expressthe cognate receptor TrkB during development (Hafidi et al., 1996;Hafidi, 1999). Although we have no firm candidate at this time,it seems plausible that inhibitory synapses may do more than simplyopen ligand-gated chloridechannels.

Modulation of inhibitory synaptic strength has been reported in several systems. For example, there is short-term facilitationor depression of IPSPs in P20-P40 auditory cortex (Buonomano andMerzenich, 1998) and inhibitory long-term potentiation (LTP) andLTD in the hippocampus (Morishita and Sastry, 1991). In goldfish,inhibitory inputs show LTP (Oda et al., 1995, 1998). Althoughthere are a few accounts of inhibitory synaptic plasticity inthe developing nervous system (Komatsu, 1994), these are not knownto be associated with a developmental rearrangement of inhibitoryterminals. Furthermore, it is not clear how the timing of excitatoryand inhibitory events might influence the strength of either afferentprojection. The relative timing of excitatory synaptic eventscan influence whether excitatory LTD or LTP is observed. In theXenopus retinotectal system, an EPSC that occurs ~20 msec beforea postsynaptic action potential is potentiated, whereas an EPSCthat occurs ~20 msec after the action potential is depressed (Zhanget al., 1998).

We therefore propose that inhibitory terminals become stabilized when they are active during low postsynaptic calcium. Lowintracellular calcium levels could exist because of the lack ofexcitatory activity, because of the ability of inhibitory terminalsto hyperpolarize the membrane potential during brief activation(Callaway et al., 1995; Lo et al., 1998), or in much older animals(>P20) because their intracellular calcium-buffering efficacycould be greater (Friauf, 1994; Lohmann and Friauf, 1996; Parkset al., 1996; Zettel et al., 1997; Caicedo et al., 1998; Henkeland Brunso-Bechtold, 1998; Iwasaki and Takahashi, 1998). If excitatoryterminals are activated first, the subsequent transmission atinhibitory terminals may lead to inhibitory synapse withdrawal.Although the MNTB-evoked IPSC became depressed, we do not yetknow whether this represents the selective depression of someinhibitory synapses or the widespread depression of themall.

From a functional standpoint, one of the most intriguing elements of LSO development is the manner in which excitatory andinhibitory afferents become precisely matched, both structurallyand functionally, along the tonotopic axis (Sanes and Rubel, 1988;Sanes and Siverls, 1991). Individual MNTB arbors become ~30% morerestricted along the LSO frequency axis during the third postnatalweek (Sanes and Siverls, 1991). On the basis of estimates fromintracellular recordings, the refinement of MNTB arbors correlateswith the loss of ~40% of the inhibitory inputs to each LSO neuron(Sanes, 1993). Thus, it is possible that inhibitory and excitatoryterminals compete for the same postsynaptic space. For example,when sound is located closer to the "inhibitory" ear, the MNTBterminals responding to a specific frequency are activated first,and it is these terminals that must suppress discharge in theLSO neuron. Inhibitory terminals that are activated at a longerlatency, after the excitatory terminals have depolarized the LSOneuron, may be inappropriate (for example, tuned to the incorrectfrequency), and these terminals should be eliminated. Therefore,it will be important to learn about the amount and timing of excitatoryand inhibitory synaptic transmission in the developing LSO andthe functional changes that are brought about byeach.

  FOOTNOTES

Received Jan. 18, 2000; revised April 19, 2000; accepted May 10, 2000.

This work was supported by National Institutes of Health Grant DC 00540 (D.H.S.).
Correspondence should be addressed to Dr. Dan H. Sanes, Center for Neural Science, 4 Washington Place, New York University,New York, NY 10003. E-mail: sanes{at}cns.nyu.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Backus KH, Deitmer JW, Friauf E (1998) Glycine-activated currents are changed by coincident membrane depolarization in developing rat auditory brainstem neurones. J Physiol (Lond) 507:783-794[Abstract/Free Full Text].
Balice-Gordon RJ, Lichtman JW (1994) Long-term synapse loss induced by focal blockade of postsynaptic receptors. Nature 372:519-524[Medline].
Battistin T, Cherubini E (1994) Developmental shift from long-term potentiation at the mossy fibre synapses in the rat hippocampus. Eur J Neurosci 6:1750-1755[Web of Science][Medline].
Ben-Ari Y, Cherubini E, Corradetti R, Gaiarsa JL (1989) Giant synaptic potentials in immature rat CA3 hippocampal neurones. J Physiol (Lond) 416:303-325[Abstract/Free Full Text].
Boehm S, Harvey RJ, von Holst A, Rohrer H, Betz H (1997) Glycine receptors in cultured chick sympathetic neurons are excitatory and trigger neurotransmitter release. J Physiol (Lond) 504:683-694[Abstract/Free Full Text].
Buonomano DV, Merzenich MM (1998) Net interaction between different forms of short-term synaptic plasticity and slow-IPSPs in the hippocampus and auditory cortex. J Neurophysiol 80:1765-1774[Abstract/Free Full Text].
Caicedo A, Kungel M, Pujol R, Friauf E (1998) Glutamate-induced Co²⁺ uptake in rat auditory brainstem neurons reveals developmental changes in Ca²⁺ permeability of glutamate receptors. Eur J Neurosci 10:941-954[Web of Science][Medline].
Callaway JC, Lasser-Ross N, Ross WN (1995) IPSPs strongly inhibit climbing fiber-activated [Ca²⁺]_i increases in the dendrites of cerebellar Purkinje neurons. J Neurosci 15:2777-2787[Abstract].
Cash S, Dan Y, Poo M-m, Zucker R (1996) Postsynaptic elevation of calcium induces persistent depression of developing neuromuscular synapses. Neuron 16:745-754[Web of Science][Medline].
Colman H, Nabekura J, Lichtman JW (1997) Alterations in synaptic strength preceding axon withdrawal. Science 275:356-361[Abstract/Free Full Text].
Connold AL, Evers JV, Vrbova G (1986) Effect of low calcium and protease inhibitors on synapse elimination during postnatal development in the rat soleus muscle. Dev Brain Res 28:99-107.
Connor JA, Tseng HY, Hockberger PE (1987) Depolarization- and transmitter-induced changes in intracellular Ca²⁺ of rat cerebellar granule cells in explant cultures. J Neurosci 7:1384-1400[Abstract].
Constantine-Paton M, Cline HT (1998) LTP and activity-dependent synaptogenesis: the more alike they are, the more different they become. Curr Opin Neurobiol 8:139-148[Web of Science][Medline].
Constantine-Paton M, Cline HT, Debski E (1990) Patterned activity, synaptic convergence, and the NMDA receptor in developing visual pathways. Annu Rev Neurosci 13:129-154[Web of Science][Medline].
Crair MC, Malenka RC (1995) A critical period for long-term potentiation at thalamocortical synapses. Nature 375:325-328[Medline].
Dudek SM, Bear MF (1992) Homosynaptic long-term depression in area CA1 of hippocampus and effects of N-methyl-D-aspartate receptor blockade. Proc Natl Acad Sci USA 89:4363-4367[Abstract/Free Full Text].
Dudek SM, Friedlander MJ (1996) Developmental down-regulation of LTD in cortical layer IV and its independence of modulation by inhibition. Neuron 16:1097-1106[Web of Science][Medline].
Ehrlich I, Löhrke S, Friauf E (1999) Shift from depolarizing to hyperpolarizing glycine action in rat auditory neurones is due to age-dependent Cl regulation. J Physiol (Lond) 520:121-137[Abstract/Free Full Text].
Feldman DE, Nicoll RA, Malenka RC, Issac JT (1998) Long-term depression at thalamocortical synapses in developing rat somatosensory cortex. Neuron 21:347-357[Web of Science][Medline].
Finck A, Schneck CHD, Hartman AF (1972) Development of cochlear function in the neonate Mongolian gerbil (Meriones unguiculatus). J Comp Physiol Psychol 78:375-380[Web of Science][Medline].
Fitzgerald KK, Sanes DH (1999) Serotonergic modulation of synapses in the developing gerbil lateral superior olive. J Neurophysiol 81:2743-2752[Abstract/Free Full Text].
Friauf E (1994) Distribution of calcium-binding protein calbindin-D28k in the auditory system of adult and developing rats. J Comp Neurol 349:193-211[Web of Science][Medline].
Glitsch M, Llano I, Marty AJ (1996) Glutamate as a candidate retrograde messenger at interneurone-Purkinje cell synapses of rat cerebellum. J Physiol (Lond) 497:531-537[Abstract/Free Full Text].
Hafidi A (1999) Distribution of BDNF, NT-3, and NT-4 in the developing auditory brainstem. Int J Dev Neurosci 17:285-294[Web of Science][Medline].
Hafidi A, Moore T, Sanes DH (1996) Regional distribution of neurotrophin receptors in the developing auditory brainstem. J Comp Neurol 367:454-464[Web of Science][Medline].
Harris DM, Dallos P (1984) Ontogenic changes in frequency mapping of a mammalian ear. Science 225:741-743[Abstract/Free Full Text].
Henkel CK, Brunso-Bechtold JK (1998) Calcium-binding proteins and GABA reveal spatial segregation of cell types within the developing lateral superior olivary nucleus of the ferret. Microsc Res Tech 41:234-245[Web of Science][Medline].
Ito S, Cherubini E (1991) Strychnine-sensitive glycine responses of neonatal rat hippocampal neurones. J Physiol (Lond) 440:67-83[Abstract/Free Full Text].
Iwasaki S, Takahashi T (1998) Developmental changes in calcium channel types mediating synaptic transmission in rat auditory brainstem. J Physiol (Lond) 509:419-423[Abstract/Free Full Text].
Kakazu Y, Akaike N, Komiyama S, Nabekura J (1999) Regulation of intracellular chloride by cotransporters in developing lateral superior olive neurons. J Neurosci 19:2843-2851[Abstract/Free Full Text].
Kandler K, Friauf E (1995) Development of glycinergic and glutamatergic synaptic transmission in the auditory brainstem of perinatal rats. J Neurosci 15:6890-6904[Abstract/Free Full Text].
Kapfer C, Seidl A, Schweizer H, Koch U, Grothe B (1999) Activity dependent refinement of glycinergic input to medial superior olivary neurons in the gerbil. Assoc Res Otolaryngol Abstr 273:69.
Komatsu Y (1994) Age-dependent long-term potentiation of inhibitory synaptic transmission in rat visual cortex. J Neurosci 14:6488-6499[Abstract].
Kotak VC, Sanes DH (1995) Synaptically evoked prolonged depolarizations in the developing auditory system. J Neurophysiol 74:1611-1620[Abstract/Free Full Text].
Kotak VC, Sanes DH (1996) Developmental influence of glycinergic transmission: regulation of NMDA receptor-mediated EPSPs. J Neurosci 16:1836-1843[Abstract/Free Full Text].
Kotak VC, Korada S, Schwartz IR, Sanes DH (1998) A developmental shift from GABAergic to glycinergic transmission in the central auditory system. J Neurosci 18:4646-4655[Abstract/Free Full Text].
Kullman PMH, Kandler K (1999) Glycine and GABA raise [Ca²⁺]_i in developing neurons of the lateral superior olive. Soc Neurosci Abstr 25:394.
Linden DJ, Connor JA (1995) Long-term synaptic depression. Annu Rev Neurosci 18:319-357[Web of Science][Medline].
Lo Y-J, Poo M-m (1994) Heterosynaptic suppression of developing neuromuscular synapses in culture. J Neurosci 14:4684-4693[Abstract].
Lo Y-J, Rao SC, Sanes DH (1998) Modulation of calcium by inhibitory systems in the developing auditory midbrain. Neuroscience 83:1075-1084[Web of Science][Medline].
Lohmann C, Friauf E (1996) Distribution of the calcium-binding proteins parvalbumin and calretinin in the auditory brainstem of adult and developing rats. J Comp Neurol 367:90-109[Web of Science][Medline].
Lu J, Karadsheh M, Delpire E (1999) Developmental regulation of the neuronal-specific isoform of the K-Cl cotransporter KCC2 in postnatal rat brains. J Neurobiol 39:558-568[Web of Science][Medline].
Morishita W, Sastry BR (1991) Chelation of postsynaptic Ca²⁺ facilitates long-term potentiation of hippocampal IPSPs. NeuroReport 2:533-536[Web of Science][Medline].
Morishita W, Kirov SA, Alger BE (1998) Evidence for metabotropic glutamate receptor activation in the induction of depolarization-induced depression of inhibition in hippocampal CA1. J Neurosci 18:4870-4882[Abstract/Free Full Text].
O'Brien RA, Ostberg AJ, Vrbová G (1978) Observations on the elimination of polyneuronal innervation in developing mammalian skeletal muscle. J Physiol (Lond) 282:571-582[Abstract/Free Full Text].
Obrietan K, Van den Pol AN (1995) GABA neurotransmission in the hypothalamus: developmental reversal from Ca²⁺ elevating to depressing. J Neurosci 15:5065-5077[Abstract].
Oda Y, Charpier S, Murayama Y, Suma C, Korn H (1995) Long-term potentiation of glycinergic inhibitory synaptic transmission. J Neurophysiol 74:1056-1074[Abstract/Free Full Text].
Oda Y, Kawasaki K, Morita M, Korn H, Matsui H (1998) Inhibitory long-term potentiation underlies auditory conditioning of goldfish escape behavior. Nature 394:182-185[Medline].
Parks TN, Code RA, Taylor DA, Solum DA, Strauss KI, Jacobowitz DM, Winsky L (1997) Calretinin expression in the chick brainstem auditory nuclei develops and is maintained independently of cochlear nerve input. J Comp Neurol 383:112-121[Web of Science][Medline].
Payne JA, Stevenson TJ, Donaldson LF (1996) Molecular characterization of a putative K-Cl cotransporter in rat brain. A neuronal-specific isoform. J Biol Chem 271:16245-16252[Abstract/Free Full Text].
Plotkin MD, Snyder EY, Hebert SC, Delpire E (1997) Expression of the Na-K-2Cl cotransporters developmentally regulated in postnatal rat brains: a possible mechanism underlying GABA's excitatory role in immature brain. J Neurobiol 33:781-795[Web of Science][Medline].
Ridge RM, Betz WJ (1984) The effect of selective, chronic stimulation on motor unit size in developing rat muscle. J Neurosci 4:2614-2620[Abstract].
Rivera C, Voipio J, Payne JA, Ruusuvuori E, Lahtinen H, Lamsa K, Pirvola U, Saarma M, Kaila K (1999) The K⁺/Cl cotransporter KCC2 renders GABA hyperpolarizing during neuronal maturation. Nature 397:251-255[Medline].
Sanes DH (1993) The development of synaptic function and integration in the central auditory system. J Neurosci 13:2627-2637[Abstract].
Sanes DH, Hafidi A (1996) Glycinergic transmission regulates dendrite size in organotypic culture. J Neurobiol 31:503-511[Web of Science][Medline].
Sanes DH, Rubel EW (1988) The ontogeny of inhibition and excitation in the gerbil lateral superior olive. J Neurosci 8:682-700[Abstract].
Sanes DH, Siverls V (1991) The development and specificity of inhibitory axonal arborizations in the lateral superior olive. J Neurobiol 22:837-854[Web of Science][Medline].
Sanes DH, Takács C (1993) Activity-dependent refinement of inhibitory connections. Eur J Neurosci 5:570-574[Web of Science][Medline].
Sanes DH, Markowitz S, Bernstein J, Wardlow J (1992) The influence of inhibitory afferents on the development of postsynaptic dendritic arbors. J Comp Neurol 321:637-644[Web of Science][Medline].
Shatz CJ (1990) Impulse activity and the patterning of connections during CNS development. Neuron 5:745-756[Web of Science][Medline].
Williams JR, Sharp JW, Kumari VG, Wilson M, Payne JA (1999) The neuron-specific K-Cl cotransporter, KCC2. Antibody development and initial characterization of the protein. J Biol Chem 274:12656-12664[Abstract/Free Full Text].
Woolf NK, Ryan AF (1985) Ontogeny of neural discharge patterns in the ventral cochlear nucleus of the Mongolian gerbil. Dev Brain Res 17:131-147.
Zettel ML, Frisina RD, Haider SE, O'Neill WE (1997) Age-related changes in calbindin D-28k and calretinin immunoreactivity in the inferior colliculus of CBA/CaJ and C57Bl/6 mice. J Comp Neurol 386:92-110[Web of Science][Medline].
Zhang LI, Tao HW, Holt CE, Harris WA, Poo M-m (1998) A critical window for cooperation and competition among developing retinotectal synapses. Nature 395:37-44[Medline].

Copyright © 2000 Society for Neuroscience 0270-6474/00/20155820-07$05.00/0

This article has been cited by other articles:

M. I. Chelaru and V. Dragoi
Asymmetric Synaptic Depression in Cortical Networks
Cereb Cortex, April 1, 2008; 18(4): 771 - 788.
[Abstract] [Full Text] [PDF]

Y. Ben-Ari, J.-L. Gaiarsa, R. Tyzio, and R. Khazipov
GABA: A Pioneer Transmitter That Excites Immature Neurons and Generates Primitive Oscillations
Physiol Rev, October 1, 2007; 87(4): 1215 - 1284.
[Abstract] [Full Text] [PDF]

X. Yu, D. H. Sanes, O. Aristizabal, Y. Z. Wadghiri, and D. H. Turnbull
Large-scale reorganization of the tonotopic map in mouse auditory midbrain revealed by MRI
PNAS, July 17, 2007; 104(29): 12193 - 12198.
[Abstract] [Full Text] [PDF]

F. A. Ene, A. Kalmbach, and K. Kandler
Metabotropic Glutamate Receptors in the Lateral Superior Olive Activate TRP-Like Channels: Age- and Experience-Dependent Regulation
J Neurophysiol, May 1, 2007; 97(5): 3365 - 3375.
[Abstract] [Full Text] [PDF]

V. C. Kotak, A. D. Breithaupt, and D. H. Sanes
Developmental hearing loss eliminates long-term potentiation in the auditory cortex
PNAS, February 27, 2007; 104(9): 3550 - 3555.
[Abstract] [Full Text] [PDF]

A. H. Seidl and B. Grothe
Development of Sound Localization Mechanisms in the Mongolian Gerbil Is Shaped by Early Acoustic Experience
J Neurophysiol, August 1, 2005; 94(2): 1028 - 1036.
[Abstract] [Full Text] [PDF]

P. Gubellini, Y. Ben-Ari, and J.-L. Gaiarsa
Endogenous Neurotrophins Are Required for the Induction of GABAergic Long-Term Potentiation in the Neonatal Rat Hippocampus
J. Neurosci., June 15, 2005; 25(24): 5796 - 5802.
[Abstract] [Full Text] [PDF]

E. H. Chang, V. C. Kotak, and D. H. Sanes
Long-Term Depression of Synaptic Inhibition Is Expressed Postsynaptically in the Developing Auditory System
J Neurophysiol, September 1, 2003; 90(3): 1479 - 1488.
[Abstract] [Full Text] [PDF]

V. C. Kotak, C. DiMattina, and D. H. Sanes
GABAB and Trk Receptor Signaling Mediates Long-Lasting Inhibitory Synaptic Depression
J Neurophysiol, July 1, 2001; 86(1): 536 - 540.
[Abstract] [Full Text] [PDF]

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Web of Science (29)

Citing Articles via Google Scholar

Google Scholar

Articles by Kotak, V. C.

Articles by Sanes, D. H.

Search for Related Content

PubMed

PubMed Citation

Articles by Kotak, V. C.

Articles by Sanes, D. H.

Pubmed/NCBI databases
Compound via MeSH
Substance via MeSH
Hazardous Substances DB
CALCIUM COMPOUNDS
CALCIUM, ELEMENTAL