Modulation of Long-Term Synaptic Depression in Visual Cortex by Acetylcholine and Norepinephrine

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The Journal of Neuroscience, March 1, 1999, 19(5):1599-1609

Modulation of Long-Term Synaptic Depression in Visual Cortex by Acetylcholine and Norepinephrine
Alfredo Kirkwood¹, Carlos Rozas¹, John Kirkwood², Fernanda Perez², and Mark F. Bear²
¹ Mind Brain Institute, Johns Hopkins University, Baltimore, Maryland 21218, and ² Department of Neuroscience, Howard Hughes Medical Institute, Brown University, Providence, Rhode Island 02912

  ABSTRACT

Top
Abstract
Introduction
References

In a slice preparation of rat visual cortex, we discovered that paired-pulse stimulation (PPS) elicits a form of homosynapticlong-term depression (LTD) in the superficial layers when carbachol(CCh) or norepinephrine (NE) is applied concurrently. PPS by itself,or CCh and NE in the absence of synaptic stimulation, producedno lasting change. The LTD induced by PPS in the presence of NEor CCh is of comparable magnitude with that obtained with prolongedlow-frequency stimulation (LFS) but requires far fewer stimulationpulses (40 vs 900). The cholinergic facilitation of LTD was blockedby atropine and pirenzepine, suggesting involvement of M₁ receptors.The noradrenergic facilitation of LTD was blocked by urapidiland was mimicked by methoxamine, suggesting involvement of $alpha$ 1receptors. $beta$ receptor agonists and antagonists were without effect.Induction of LTD by PPS was inhibited by NMDA receptor blockers(completely in the case of NE; partially in the case of CCh),suggesting that one action of the modulators is to control thegain of NMDA receptor-dependent homosynaptic LTD in visual cortex.We propose that this is a mechanism by which cholinergic and noradrenergicinputs to the neocortex modulate naturally occurring receptivefieldplasticity.

Key words: visual cortex; development; synaptic plasticity; long-term potentiation; long-term depression; acetylcholine; norepinephrine

  INTRODUCTION

Top
Abstract
Introduction
References

It is well established that synapses in sensory neocortex can be modified by experience. For example, brief deprivation ofnormal vision during early postnatal development can lead to adepression of synaptic transmission that renders visual corticalneurons unresponsive to retinal stimulation. This type of synapticplasticity obviously depends on information of retinal origin.However, there is evidence that experience-dependent plasticityalso requires that animals be awake, alert, and paying attentionto sensory stimuli (for review, see Singer, 1995). Thus, issuesof great interest are the mechanisms of experience-dependent synapticplasticity and their modulation by behavioralstate.

Extrathalamic inputs convey information to the cortex about behavioral state. Attention has focused mainly on the inputs arisingfrom the locus coeruleus and the basal telencephalon that usenorepinephrine (NE) and acetylcholine (ACh), respectively, asneurotransmitters. In one early study, it was shown that partialdestruction of the noradrenergic or the cholinergic inputs alonedid not disrupt deprivation-induced synaptic depression in visualcortex. However, their combined destruction produced a large deficitin this form of experience-dependent plasticity (Bear and Singer,1986). The results of this experiment suggested that both of theseinputs to visual cortex facilitate synaptic plasticity. Furthermore,because the simultaneous loss of both noradrenergic and cholinergicinputs was required to produce the defect in plasticity, the suggestionwas made that these two modulators may substitute for one anotherand act via a common molecularmechanism.

The notion that ACh and NE modulate naturally occurring cortical plasticity has received ample support (Kasamatsu and Pettigrew,1979; Gordon et al., 1990; Juliano et al., 1991; Gu and Singer,1993; Osterheld-Haas et al., 1994; Bakin and Weinberger, 1996;Baskerville et al., 1997; Kilgard and Merzenich, 1998; Sachdevet al., 1998; Zhu and Waite, 1998). The important question thatremains, of course, is precisely how these neurotransmitters affectthe cortical synapses that carry detailed information about sensoryexperience.

Over the past several years, slice preparations of visual neocortex have been used in an effort to clarify the elementarymechanisms of activity-dependent synaptic plasticity. One hypothesisthat derived from this work is that modulation of inhibition inthe cortex might be a way in which ACh and NE control plasticity(Kirkwood and Bear, 1994a). Because the state of functional inhibitionin the cortex can be assayed by recording layer III responsesto paired-pulse stimulation (PPS) of the white matter (Luhmannand Prince, 1991; Metherate and Ashe, 1994), we set out to examinethe effects of ACh and NE on responses to PPS. In the course ofthis investigation we made the unexpected discovery that PPS inthe presence of ACh or NE triggers a form of long-term synapticdepression (LTD). Here we report that ACh, acting via M₁ receptors,and NE, acting via $alpha$ 1 receptors, dramatically facilitate NMDAreceptor-dependent homosynaptic LTD in visual cortex. We suggestthat this reflects a mechanism whereby these modulators facilitateexperience-dependent synaptic plasticity in sensoryneocortex.

  MATERIALS AND METHODS

The experiments described in this paper were performed on transverse slices prepared from the visual cortex of 3- to 5-week-oldLong-Evans rats. Each animal was deeply anesthetized by exposureto methoxyflurane vapors and was decapitated soon after the disappearanceof any corneal reflexes. The brain was rapidly removed and immersedin ice-cold dissection buffer containing (in mM): sucrose, 212.7;KCl, 5; NaH₂PO₄, 1.25; MgSO₄, 3; CaCl₂, 1; NaHCO₃, 26; dextrose,10; and kynurenate, 10. A block of visual cortex was removed andsectioned in the coronal plane into 0.4-mm-thick slices usinga microslicer (DTK 1000; Ted Pella, Redding, CA). The slices weregently transferred to an interface storage chamber containingartificial CSF (ACSF) and maintained at room temperature for atleast an hour before recording. The ACSF was saturated with 95%O₂/5% CO₂ and contained (in mM): NaCl, 124; KCl, 5; NaH₂PO₄, 1.25;MgCl₂, 1; CaCl₂, 2; NaHCO₃, 26; and dextrose, 10. The experimentswere performed on submerged slices continuously perfused at arate of 2 ml/min with 30°C ACSF saturated with 95% O₂/5% CO₂.Microelectrodes were filled with ACSF (1-2 M $Omega$ ) for extracellularrecording or 3 M potassium acetate (80-120 M $Omega$ ) for intracellularrecording. Only cells with resting membrane potentials more negativethan $-$ 70 mV and input resistances >20 M $Omega$ were studied. A sitein the middle of the cortical thickness, confirmed histologicallyto correspond to layer IV and upper layer V, was stimulated toevoke field potentials (FPs) in layer III, as described previously(Kirkwood and Bear, 1994a,b). The amplitude of the maximum negativeFP in layer III was used as a measure of the evoked populationexcitatory synaptic current. Changes in the amplitude of the maximumnegative FP reflect changes in the magnitude of a synaptic currentsink (Mitzdorf, 1985; Aizenman et al., 1996) and correlate withchanges in the initial slope of EPSPs recorded intracellularlyin layer III neurons (Kirkwood and Bear, 1994a,b). Baseline responseswere obtained every 15 sec with a stimulation intensity that yieldeda half-maximal response. PPS was used throughout the experimentunless stated otherwise. At least 10 min of stable baseline recordingswere made before drugs were applied. When NE was applied, 40 µMsodium ascorbate was included in the ACSF to prevent oxidationof the drug. Sodium ascorbate was also included with the applicationof noradrenergic agonists and antagonists. Carbachol and atropinewere purchased from Sigma (St. Louis, MO); all other drugs werepurchased from Research Biochemicals (Natick,MA).

Only data from slices with stable recordings (<3% change over the baseline period) were included in the analysis. The datawere analyzed as follows: (1) the maximum negative FP amplitudedata for each experiment were expressed as percentages of thepreconditioning baseline average; (2) the time scale in each experimentwas converted to time from the onset of conditioning, and thefour responses recorded in each minute were averaged; and (3)then, the time-matched, normalized data were averaged across experimentsand expressed as the means (± SEM). Within each group, the statisticalsignificance of a change produced by conditioning stimulationwas assessed with a paired t test, comparing values immediatelybefore the application of neuromodulators with those 30 min afterthe end of the application. Statistical significance across groupswas assessed with an unpaired ttest.

  RESULTS

Visual cortical slices were prepared from 3- to 5-week-old rats. Initially, layer III synaptic responses were evoked withstimulation applied to the underlying white matter. Our originalgoal was to study the effects of cholinergic and noradrenergicstimulation on paired-pulse suppression, i.e., the attenuationof the synaptic responses when two pulses are given in rapid succession.In these experiments, the stimulation consisted of two pulses(40 msec apart) delivered repetitively every 15 sec throughoutthe experiment. To activate cholinergic receptors, we bath applied50 µM carbachol (CCh), and to activate noradrenergic receptors,we bath applied 40 µM NE in ascorbate (40 µM). When we realizedthat the PPS in the presence of these modulators caused LTD, weshifted the stimulating electrode to layer IV to activate a lesscomplex circuit. All the data presented below were obtained withthis stimulation-recordingconfiguration.

Paired-pulse stimulation in carbachol induces a long-lasting depression of the synaptic responses

Figure 1 illustrates the effects of a 10 min application of 50 µM CCh on the FP responses to paired pulses. Under controlconditions, the response amplitude to the second pulse is usuallysomewhat smaller than the response amplitude to the first pulse.In the experiments shown in Figure 1, the ratio of the secondresponse to the first response is 0.59 ± 0.08 (n = 11). Exposureto CCh strongly reduced the response to the first pulse (64 ±4% of control measured at 10 min of CCh), but it had a smallereffect on the response to the second pulse. Thus, paired-pulsesuppression was virtually eliminated in the presence of CCh; theratio of the second to the first response was 0.99 ± 0.14 at theend of the 10 min of CCh perfusion.

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Figure 1. The cholinergic agonist CCh induces a lasting depression of the layer III synaptic responses to layer IV stimulation. A, B, Effects of a brief (10 min) bath application of CCh (50 µM; open horizontal bar in B) on the field responses evoked with paired-pulse stimulation [interstimulus interval (ISI) = 40 msec] are shown. A, FPs are from an experiment in which the CCh application resulted in a clear depression of the response to the first pulse but had virtually no effect on the response to the second pulse. The traces were recorded immediately before (control) and during the application of CCh and 30 min after washout of the drug. B, Time course of the average of 11 experiments is shown. Solid circles are responses to the first pulse; open circles are responses to the second pulse. C, Prolonged paired-pulse stimulation alone has no effect on the FPs (n = 9). D, E, The effects of CCh on FPs correlate with changes in simultaneously recorded intracellular EPSPs. D, Traces are averages of four consecutive intracellular (top) and extracellular (bottom) responses recorded before (control) and 30 min after washout of CCh. E, Average time course of seven similar experiments is shown. Top, Changes in FP amplitude (open circles) and initial slope of the EPSP (filled triangles) are presented. Bottom, Changes in the membrane potential are shown.

These acute effects of CCh $---$ that is, the transient and reversible reduction of the synaptic responses and the reduction inpaired-pulse suppression $---$ have been reported previously (Vakninand Teyler, 1991; Murakoshi, 1995). These effects are likely toreflect a reduced probability of glutamate release (Markram andTsodyks, 1996; Gil et al., 1997), probably because of the actionof CCh on cholinergic receptors located on glutamatergic presynapticterminals (Valentino and Dingledine, 1981; Segal, 1982; Dodt etal., 1991; Vaknin and Teyler, 1991). An unexpected result, however,was that after removal of CCh the responses to the first stimulationpulse never returned to the original level. After an initial partialrecovery, the response magnitude reached a stable level 20 minafter washing out the CCh and remained depressed (80 ± 6% of control)even after an additional 30 min of washout. The LTD was a specificconsequence of the CCh, because prolonged PPS by itself had noeffect on the FPs (Fig. 1C).

To confirm that the changes in the FP reflect changes in excitatory synaptic transmission, we repeated the experiment usingintracellular recording. Simultaneous recordings were made ofthe evoked FP in layer III and the EPSP in a nearby layer IIIneuron. PPS during CCh resulted in a reduction of FP amplitude(70 ± 6%) that was paralleled by a comparable reduction in theinitial slope of the EPSPs (73 ± 8%; n = 7), indicating that areduction of the synaptic responses of layer II/III cells is reflectedin the reduction of the field responses. The application of CChalso produced a modest depolarization that was rapidly reversedafter removal of the drug. Thus the LTD of FP responses is notcaused by a tonic depolarization of postsynaptic neurons. To determinewhether the slight depolarization of the neuron by CCh duringPPS was the cause of LTD, we injected current intracellularlythat yielded similar levels of depolarization (10 mV for 12 min;n = 3). However, in no case was LTD observed, suggesting thatthe depolarization alone (at least in the cell soma) is not sufficientto cause expression of theLTD.

The LTD induced by PPS in 50 µM CCh was very reliable, so this procedure was used to characterize the phenomenon. However,we did examine the CCh dose-response relationship. By the useof a 20 min application during PPS, LTD of increasing magnitude(measured 30 min after washout) was observed with 0.1 µM (94 ±2% of baseline; n = 7), 1 µM (81 ± 3%; n = 7), 10 µM (84 ± 3%;n = 7), 50 µM (72 ± 3%; n = 8), and 100 µM CCh (68 ± 4%; n =7).

Synaptic depression induced in the presence of carbachol requires synaptic stimulation and is input specific

An important issue to be resolved concerned the role of synaptic activation in the depression induced with CCh. Thus we askedwhether CCh applied alone, without concurrent synaptic activation,would be sufficient to produce LTD. Figure 2 shows that in theabsence of stimulation, CCh application has minor effects on thesynaptic responses (97 ± 4% of baseline; paired t test, p > 0.2;n = 5). However, subsequent administration of CCh in the sameslices during PPS did result in substantial depression (78 ± 4%;p < 0.02). These results indicate that CCh permits or facilitatesan activity-dependent form of synaptic depression. These findingsalso eliminate the possibility that the lasting depression iscaused by tonic activation of ACh receptors (i.e., incompletewashout of CCh).

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Figure 2. Synaptic depression induced with CCh requires synaptic stimulation. A, Left, In the absence of stimulation, CCh failed to produce any significant change in the FP responses. Right, Subsequently, depression was reliably produced when CCh was applied with PPS. In both panels the responses were normalized with respect to the average response during the initial baseline period before CCh application. The time that elapsed between the last data point on the left and the first data point on the right varied but was not >30 min. B, The depression induced by CCh is input specific. Right, The stimulation-recording configuration used to assess input specificity is shown. Layer IV was stimulated on either side of a radial cut that extended from the white matter (WM) through layer IV. Left, The graph shows that CCh application induces depression only on the side that was stimulated. In all experiments designed to test for input specificity, responses from the two inputs showed summation and were of similar amplitudes.

Next we wished to determine whether this form of depression is input specific, that is, whether the reduction in synapticefficacy was confined to the stimulated inputs only. To addressthis question, separate inputs to layer III were isolated by makinga radial cut in the slice that extended from the white matterto layer IV, and baseline stimulation was applied in layer IVon each side of the cut. During CCh, PPS was applied to only oneinput, the other serving as an unstimulated control. The results,summarized in Figure 2B, showed that only inputs receiving stimulationduring CCh show the LTD (stimulated path, 82 ± 6% of baseline;control path, 98 ± 1%; n = 5). Thus, cholinergic stimulation promotesLTD only in activeinputs.

The results described above indicate that CCh in conjunction with paired-pulse stimulation induces an activity-dependent andhomosynaptic form of LTD. We were interested to know whether theCCh effect is specific to inputs receiving PPS or whether CChexerts a more general facilitation of homosynaptic LTD mechanisms.In hippocampal and visual cortical slices, a homosynaptic formof LTD can also be reliably induced with low-frequency stimulation(LFS; typically 1 Hz), but only if this stimulation is prolonged[usually 10-15 min (Dudek and Bear, 1992; Kirkwood et al., 1993)].To see whether CCh can facilitate LFS-induced LTD, we combinedapplication of the drug with brief epochs of LFS (1 Hz for 5 min;Fig. 3). When the brief LFS was applied alone, little or no LTDwas induced (94 ± 3%; n = 11). However, when brief LFS was appliedin conjunction with CCh, substantial LTD was induced (81 ± 3;n = 17; p < 0.005; Fig. 3C). These results indicate that CCh applicationfacilitates the induction of homosynaptic LTD with LFS, as wellas with PPS.

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Figure 3. CCh promotes the induction of LTD with a LFS. A, Results from an experiment in which a brief epoch of LFS (300 pulses at 1 Hz; solid horizontal bar) failed to induce LTD under control conditions but did produce LTD when it was subsequently applied in the presence of CCh. The baseline was collected with single-pulse stimulation delivered every 15 sec. B, Changes in the FP amplitude induced by LFS alone (open circles; n = 11) and by LFS in the presence of 50 µM CCh (filled circles; n = 17). C, Cumulative probability distribution of the changes induced by LFS in the absence (dashed line) and in the presence (solid line) of CCh. The percentage change over the baseline was measured at 30 min after conditioning. Data are from the same experiments shown in B.

Involvement of NMDA receptors and M₁ receptors in the induction of synaptic depression in the presence of carbachol

The induction of one prominent form of homosynaptic LTD in visual cortex requires the activation of NMDA receptors (Kirkwoodand Bear, 1994b). To test whether this is also the case for thesynaptic depression promoted by CCh, we attempted to block itsinduction with the NMDA receptor antagonist 2-amino-5-phosphonovalericacid (AP5). Figure 4, A-C, illustrates the effects of bath-applied100 µM AP5 on the induction of depression in CCh. In three cases,one of them shown in Figure 4A, AP5 completely blocked LTD inducedwith the aid of CCh, and this blockade was relieved after removalof AP5. On average, LTD induced by PPS in the presence of CChwas significantly reduced but not eliminated by AP5 (AP5, 91 ±9%; n = 12; control, 77 ± 12; n = 10; p < 0.01; Fig. 4C). Thedata indicate that cholinergic activation promotes the inductionof an NMDA receptor-dependent form of LTD. However, the fact thatthe inhibition of LTD with AP5 is incomplete suggests that anNMDA receptor-independent form of LTD may also be promoted byCCh. In this regard, it is worth mentioning that in the CA1 regionit has been demonstrated that two forms of LTD can be inducedat the same synapses (Oliet et al., 1997).

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Figure 4. Synaptic depression induced by PPS in CCh is partially dependent on NMDA receptor activation. A, Results are from one of the three experiments in which application of 100 µM AP5 reversibly blocked the depression induced with CCh. B, On average, application of 100 µM AP5 reduced the depression induced with CCh. The graph shows the effects of CCh on the first response in the presence (filled circles; n = 10) and in the absence (open circles; n = 12) of 100 µM AP5. C, Cumulative probability distribution of the changes in the field potential amplitude measured 30 min after washout of CCh is shown. Experiments were done in the presence of AP5 (solid line) and in the absence of AP5 (dashed line). Data are from the same experiments shown in B.

In adults, cholinergic terminals and muscarinic receptors are distributed throughout the depth of the visual cortex. Nicotinicreceptors, in contrast, are confined to the middle layers. Itseemed reasonable to assume, therefore, that the effects of CChon layer III synaptic responses depend on the activation of muscarinicreceptors. To test this assumption, we studied the effects ofthe muscarinic antagonist atropine on the synaptic depressioninduced with CCh. In the presence of 5 µM atropine, the applicationof CCh failed to produce either the transient or the lasting depressionof the field responses (98 ± 3.4% of baseline; n = 6), whereassubstantial depression was induced in the interleaved controls(87 ± 2; n = 7; Fig. 5A). A major postsynaptic muscarinic receptortype is the M₁ receptor (Mrzljak et al., 1993; Wang and McCormick,1993), and this receptor has been implicated in the regulationof visual cortical plasticity (Gu and Singer, 1993). As shownin Figure 5B, in the presence of the selective M₁ antagonist pirenzepine(50 µM), application of CCh failed to induce LTD [98 ± 3% of baseline(n = 10) as compared with 80 ± 4% (n = 10) in the interleavedcontrols]. In contrast, the M₂ receptor antagonist gallamine (50µM) had no effect (79 ± 3% of baseline 30 min after CCh; n = 7;data not shown). Thus, facilitation of LTD by CCh depends, atleast in part, on M₁ receptor activation coincident with synapticactivation of NMDA receptors.

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Figure 5. Synaptic depression induced by CCh is dependent on the activation of M₁ muscarinic receptors. A, Time course of the effects of CCh applied in the absence (open circles; n = 6) and presence (filled circles; n = 7) of the muscarinic antagonist atropine (5 µM). B, Time course of the effects of CCh applied in the absence (open circles; n = 10) and presence (filled circles; n = 10) of the specific M₁ muscarinic antagonist pirenzepine (50 µM).

Norepinephrine induces a long-lasting depression of the synaptic responses

The suggestion has been made from lesion studies in vivo that ACh and NE might have similar modulatory effects on synapticplasticity in visual cortex (Bear and Singer, 1986). Therefore,we investigated whether NE can also promote synaptic plasticityof layer III synaptic responses in visual cortical slices. Inthese experiments we used the same stimulation paradigms usedin the CCh experiments. Figure 6, A and B, shows that applicationof 40 µM NE for 10 min results in an acute reduction of the responsesto PPS. The ratio of the second to the first response, which was0.90 ± 0.05 (n = 8) at the beginning of the experiments, grewto 0.98 ± 0.06 during NE application and remained at that value(1.00 ± 0.05) after the washout of NE. As was the case for CCh,when NE was removed the response to the first pulse remained depressedfor as long as the response was recorded (82 ± 2% of control at60 min after NE). Simultaneous intracellular and extracellularrecordings revealed that NE reduced the EPSP (90 ± 2%; n = 11)and the field potential (88 ± 3%) to a similar extent and causeda slight and transient depolarization (Fig. 6C,D) that disappearedafter washout of the drug. Thus, the lasting depression of thefield responses induced with the aid of NE reflects, at leastin part, changes in synaptic efficacy.

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Figure 6. PPS in the presence of NE induces a lasting depression of the layer III synaptic responses to layer IV stimulation. A, B, Effects of a brief (10 min) bath application of NE (40 µM) on the field responses evoked with paired-pulse stimulation (ISI = 40 msec) are shown. A, FPs were recorded immediately before (control) and during the application of NE and 30 min after washout of the drug. B, Time course of the average of nine experiments is shown. Solid circles are responses to the first pulse; open circles are responses to the second pulse. C, D, The effects of NE on FPs correlate with changes in simultaneously recorded intracellular EPSPs. C, Traces are averages of four consecutive intracellular (top) and extracellular (bottom) responses recorded before and 30 min after washout of NE. D, Average time course of 11 similar experiments is shown. Top, Changes in FP amplitude (open circles) and initial slope of the EPSP (filled triangles) are presented. Bottom, Changes in the membrane potential are shown.

Norepinephrine promotes an activity- and NMDA receptor-dependent form of LTD

The striking similarity of the long-term effects of CCh and NE led us to examine further whether LTD induced with the aidof NE also requires synaptic activity. In these experiments westimulated and recorded simultaneously from two independent sitesin the same slice (see Fig. 7). Stimulation at one site was suspendedduring the application of NE and resumed 5 min after washout ofthe drug; the other site was stimulated throughout the experimentand served as a control. As shown in Figure 7, very little depressiondeveloped in the nonstimulated site (99 ± 3%; n = 5), whereasrobust depression was observed in the control site (83 ± 6%).

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Figure 7. Synaptic depression induced with NE requires synaptic activity. Left, Time course of the changes induced by NE on the amplitude of the first response in two sites recorded simultaneously in the same slices (n = 5). One site was stimulated throughout the experiment (solid circles), whereas in the other site stimulation was suspended during NE application and resumed 5 min after washout (open circles). Right, Stimulus-recording arrangement.

Next we investigated the involvement of NMDA receptors in the induction of LTD by PPS in the presence of NE, using the NMDAreceptor antagonist AP5. As shown in Figure 8, in the presenceof 100 µM AP5, PPS in NE failed to induce LTD (103 ± 3%; n = 6),but it did induce substantial LTD after washout of the antagonist(84 ± 3%; p < 0.005). Taken together, these results support theconclusion that noradrenergic activation, like cholinergic activation,facilitates the induction of homosynaptic LTD in visual cortex.

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Figure 8. Synaptic depression induced with NE is reversibly blocked by the NMDA receptor antagonist AP5. Left, In the presence of AP5 (100 µM), NE failed to produce any change in the FP response to test stimulation. Right, After washout of the drug, however, depression was reliably produced. In both panels the responses were normalized with respect to the average response during the initial baseline period before NE application. The time that elapsed between the last data point on the left and the first data point on the right varied but was not >30 min.

$alpha$ 1 receptors are involved in the noradrenergic facilitation of LTD

NE can activate a variety of adrenergic receptors in the superficial layers of visual cortex, including $alpha$ 1-, $alpha$ 2-, and $beta$ -adrenergicreceptors. To determine the receptor subtype involved in the facilitationof LTD, we investigated the effect of a battery of receptor-specificantagonists andagonists.

Figure 9, A and B, shows that $beta$ -adrenergic receptors are unlikely to be involved in the facilitation of LTD. PPS in the presenceof the $beta$ -adrenergic receptor agonist isoproterenol (40 µM) producedno LTD (97 ± 4%; n = 6), and application of the $beta$ receptor antagonistpropranolol (40 µM) had no effect on the induction of LTD in thepresence of NE (74 ± 4%; n = 5). These results contrast with theeffects of $alpha$ 1 receptor agonists and antagonists (Fig. 9C,D). PPSduring application of the $alpha$ 1 receptor agonist methoxamine (40µM) caused a sustained depression of the synaptic responses (84± 3; n = 8) that mimicked the LTD induced with NE (Fig. 9C). Moreover,the $alpha$ 1 antagonist urapidil (40-80 µM) effectively blocked theeffects of NE (98 ± 3%; n = 12) as compared with interleaved controls(85 ± 2%; n = 12; Fig. 9D). Together, these data indicate that $alpha$ 1, but not $beta$ , receptors are involved in the facilitation of LTDby NE.

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Figure 9. Noradrenergic facilitation of LTD is mediated by the activation of $alpha$ 1 receptors. A, The $beta$ -adrenergic receptor agonist isoproterenol (40 µM; ISO) fails to facilitate LTD. B, Application of the $beta$ -adrenergic receptor antagonist propranolol (40 µM) does not block the facilitation of LTD by NE. C, The $alpha$ 1-adrenergic agonist methoxamine (40 µM; METHOX) mimics NE. D, The $alpha$ 1-adrenergic antagonist urapidil (40 µM) blocks the effects of NE (open symbols, NE + urapidil; filled symbols, NE controls). E, Bath application of the $alpha$ 2-adrenergic agonist clonidine (40 µM) transiently potentiates the response to synaptic stimulation. F, Application of the $alpha$ 2-adrenergic antagonist yohimbine (40 µM) depresses the synaptic responses.

The pharmacological manipulation of $alpha$ 2 receptors produced some perplexing results. The $alpha$ 2 agonist clonidine had the oppositeeffect of NE; PPS in clonidine produced a large, but transient,potentiation of the synaptic responses (130 ± 8% at 20 min ofclonidine application). After clonidine was removed, the responsesslowly came back to control levels (103 ± 3% at 50 min of washout;n = 4; Fig. 9E). The $alpha$ 2 antagonist yohimbine (40 µM) mimickedthe effects of NE and profoundly reduced the field responses.When the drug was removed, the responses recovered only partially,reaching a stably depressed level (70 ± 4%; n = 7; Fig. 9F). Theparadoxical results obtained with yohimbine and clonidine mightbe attributable, at least in part, to their effects on presynaptic $alpha$ 2 inhibitory autoreceptors. By blocking the autoreceptors, yohimbinemight enhance the release of endogenous NE and facilitate theinduction ofLTD.

Differential effects of neuromodulators in visual cortex and hippocampus

Previous studies indicate that synaptic plasticity evoked in visual cortical layer III and synaptic plasticity evoked in theCA1 region of the hippocampus share crucial similarities in theirmechanism of induction (Kirkwood et al., 1993). Therefore, itwas of interest to investigate the effect of the neuromodulatorson the CA1 synaptic responses. In these experiments, the responsesto PPS were recorded simultaneously in visual cortex and hippocampususing slices that contained both structures (Fig. 10A). Duringthe CCh application, the CA1 responses were the most affected(Fig. 10B). After removal of the drug, however, the responses inboth visual cortex and hippocampus stabilized at a similar, depressedlevel (82 ± 7% in visual cortex; 89 ± 4% in CA1; n = 8). On theother hand, whereas during the application of NE both CA1 andvisual cortex were depressed to the same level (Fig. 10C), onlythe visual cortical responses remained depressed after the removalof the drug (82 ± 3% in visual cortex; 103 ± 6% in CA1; n = 10).

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Figure 10. Differential effects of CCh and NE in hippocampus and visual cortex. A, The drawing depicts the electrode configuration used for simultaneous recording in CA1 and visual cortex. B, Application of CCh yields comparable LTD in CA1 and visual cortex. Top, The traces are averages of four consecutive recordings taken before (thick line), during (dotted line), and 30 min after the application of CCh (thin line). Bottom, The graph shows the time course of the changes induced in the first response recorded simultaneously in the CA1 region of the hippocampus (initial slope of the field potential; open circles) and in the visual cortex (field potential amplitude; filled circles). C, The time course of the changes induced by bath application of NE is shown. PPS in the presence of NE failed to produce LTD in the hippocampus.

  DISCUSSION

The principal finding of our study is that cholinergic or noradrenergic receptor activation dramatically facilitates the inductionof homosynaptic LTD in layer III of visual cortex. In fact, whenPPS is used, the neuromodulators enable induction and expressionof synaptic plasticity that otherwise would not be observed. Thus,our results provide strong support for the view that ACh and NEcan serve as "enabling factors" for activity-dependent corticalplasticity (Singer, 1979, 1995; Dykes et al., 1990; Dykes, 1997).Because this robust modulation of plasticity can be observed undercontrolled conditions in vitro, the paradigm we describe heremay be useful for the further dissection of the molecular mechanismof experience-dependent cortical plasticity and its modulationby behavioralstate.

Properties of LTD induced in the presence of ACh and NE

In recent years, it has become clear that many synapses in the CNS can undergo activity-dependent LTD. In the hippocampusand neocortex, LTD can be induced reliably with prolonged (e.g.,15 min), low-frequency (e.g., 1 Hz) synaptic stimulation. LTDinduced in this way occurs only at the stimulated synapses andthus is said to be homosynaptic. In the CA1 region of hippocampusand in layer III of visual cortex, homosynaptic LTD evoked withLFS requires NMDA receptor activation under most experimentalconditions (e.g., Dudek and Bear, 1992; Kirkwood et al., 1993).

The properties of LTD in visual cortex induced by PPS in the presence of NE suggest that it uses a similar induction mechanism.In particular, the LTD is completely blocked by application ofAP5, an NMDA receptor antagonist. Thus, NE may act as a sort ofgain-control mechanism for NMDA receptor-dependent homosynapticLTD. The situation for ACh, however, may be more complicated.Although the LTD induced by PPS in the presence of CCh was inputspecific, it was only partially blocked by AP5. Thus, in additionto facilitating NMDA receptor-dependent homosynaptic LTD, AChmay also promote other mechanisms of LTD induction. In this context,it should be noted that NMDA receptor-independent forms of homosynapticLTD have been described, both in visual cortex (Artola et al.,1990) and in hippocampus, including area CA1 (Stanton and Sejnowski,1989; Bolshakov and Siegelbaum, 1994; Oliet et al., 1997).

With PPS, a brief application of NE or CCh resulted in LTD of magnitude comparable with that obtained with prolonged LFS,the standard method to induce LTD in many laboratories. However,PPS induced LTD with far fewer stimulation pulses (40 vs 900).PPS may be a particularly efficacious stimulation regime, in partbecause it facilitates NMDA receptor-mediated responses (Metherateand Ashe, 1994). However, the facilitation of LTD by the neuromodulatorsis not unique to PPS, because we find that LFS-induced LTD isalso enhanced. In this context it should be noted that Kojic etal. (1997) reported that another neuromodulator, serotonin, couldalso greatly facilitate LFS-induced LTD in visualcortex.

The LTD induced by PPS in the presence of neuromodulators was associated with an increase in the paired-pulse response ratio.This effect was more pronounced for ACh than it was for NE. Thesefindings could be taken as support for a presynaptic expressionmechanism for LTD in the neocortex (i.e., reduced probabilityof glutamate release in response to the first pulse). However,interpretation of a change in paired-pulse responses in our preparationis not straightforward. The paired-pulse ratio depends importantlyon the magnitude of the response to the first pulse and on thestate of inhibition (Luhmann and Prince, 1991; Metherate and Ashe,1994; Frank et al., 1995). Thus, elucidation of the expressionmechanism(s) for LTD in the neocortex will require additionalexperiments, using intracellular recordings of responses to minimalstimulation of a small number of synapticinputs.

Mechanism of LTD facilitation in visual cortex

Our data suggest that the effect of CCh on LTD is mediated via muscarinic receptors of the M₁ subtype and that the effectof NE is mediated via $alpha$ receptors of the $alpha$ 1 type. Both of thesereceptor types are highly expressed in the superficial layersof visual cortex (Shaw et al., 1986; Schliebs et al., 1989), andinterestingly, both are coupled to phospholipaseC.

Although the exact site(s) of modulation and the precise mechanisms by which the modulation occurs remain to be determined,there are some obvious possibilities. The LTD triggered by PPSdepends, at least in part, on NMDA receptor activation. Becausethe NMDA receptor is voltage dependent, cholinergic and noradrenergicmodulation of LTD could occur indirectly by regulating the excitabilityof the postsynaptic neuron or by altering the properties of inhibition.In addition, the NMDA receptor itself is a phosphoprotein thatis subject to regulation (Roche et al., 1994). Finally, regulationof LTD could occur downstream of NMDA receptor activation, forexample, via release of Ca²⁺ from intracellular stores or by altering the activity of theprotein kinases and phosphatases that control synapticefficacy.

Indeed, studies in neocortex and hippocampus have shown that activation of M₁ (Valentino and Dingledine, 1981; Markram andSegal, 1990, 1992; Behrends and Buggencate, 1993; Murakoshi, 1995;Kimura and Baughman, 1997) and $alpha$ 1 receptors (Madison and Nicoll,1988) reduces evoked GABA release by inhibitory interneurons.In addition, M₁ receptor activation increases the excitabilityof pyramidal neurons (McCormick and Prince, 1986; Dutar and Nicoll,1988) and directly enhances NMDA receptor function (Segal, 1992;Aramakis et al., 1997). Any or all of these effects could contributeto the modulation of LTD in visual cortex, and it will be of interestto investigate these possible mechanisms in future studies. Itshould be noted, however, that there is already evidence thatdecreasing inhibition can facilitate homosynaptic LTD in CA1 (Wagnerand Alger, 1995).

Neuromodulators and bidirectional synaptic plasticity

To our knowledge, our study is the first to show facilitation of LTD by ACh and NE. However, there have been many reportson the effects of ACh and NE on long-term potentiation (LTP).As is the case for LTD, there are multiple forms of LTP with differentinduction and expression mechanisms. One form, which is highlyexpressed in CA1 and in the superficial layers of neocortex (e.g.,Kirkwood et al., 1993), depends on NMDA receptor activation forits induction. This type of LTP is of particular interest becauseit is the functional inverse of NMDA receptor-dependent LTD (forreview, see Bear and Kirkwood, 1996).

As we have shown for LTD, NMDA receptor-dependent LTP is enhanced by muscarinic receptor activation (Tanaka et al., 1989;Blitzer et al., 1990; Burgard and Sarvey, 1990; Brocher et al.,1992; Huerta and Lisman, 1993; Sokolov and Kleschevnikov, 1995).In fact, Auerbach and Segal (1994, 1996) report that low concentrationsof CCh (0.25-0.75 µM) can directly trigger LTP in CA1. We didnot observe a similar effect in visual cortex,however.

Similarly, NMDA receptor-dependent LTP is enhanced by NE. However, this facilitatory effect is mediated by $beta$ receptors andnot $alpha$ receptors as is the case for LTD (Stanton and Sarvey, 1987;Brocher et al., 1992; Kato, 1993; Thomas et al., 1996; Katsukiet al., 1997). Moreover, in CA1 10 µM NE not only facilitatesLTP but also inhibits induction of LTD with LFS (Blitzer et al.,1995; Thomas et al., 1996). The apparent discrepancy between theeffects of NE on LTD in visual cortex and hippocampus could beexplained by differences in the balance of $alpha$ and $beta$ receptor activationby NE in the two preparations. Indeed, our direct comparison ofhippocampus and visual cortex revealed that synaptic transmissionin the two structures responds differently to bath-applied NE.Unlike in the visual cortex, there was no LTD induced in CA1 byPPS in the presence ofNE.

Relevance to experience-dependent cortical plasticity

The stimulus selectivity of cortical neurons is subject to experience-dependent modification, and such changes are likelyto reflect the storage of information by cortical synapses. Theoreticalstudies have shown that synaptic modifications with the propertiesof LTP and LTD are well suited to account for experience-dependentshifts in selectivity (Bienenstock et al., 1982; Bear et al.,1987; Bear, 1996). The striking facilitation by NE and ACh ofboth LTP and LTD suggests that these modulators could functiongenerally as a gain-control mechanism for the synaptic plasticitythat underlies receptive field plasticity and learning. Indeed,the notion that cortical synaptic plasticity is somehow "gated"by ACh and NE has received abundant support from studies performedin vivo on visual, auditory, and somatosensory cortex (Kasamatsuand Pettigrew, 1979; Bear and Singer, 1986; Gordon et al., 1990;Juliano et al., 1991; Kasamatsu, 1991; Gu and Singer, 1993; Edelineet al., 1994; Baskerville et al., 1997; Dykes, 1997; Kilgard andMerzenich, 1998; Zhu and Waite, 1998).

Although plasticity is an important feature of adult cortical organization, it is clearly most robust during early postnataldevelopment. A classic example of developmental plasticity inthe visual cortex is the loss of responsiveness to stimulationof an eye that has been briefly deprived of vision. Like otherforms of cortical plasticity, the deprivation-induced synapticdepression is disrupted by lesions that interrupt cholinergicand noradrenergic inputs to cortex (Bear and Singer, 1986; Gordonet al., 1990). Interestingly, although partial destruction ofeach input alone was insufficient to produce a detectable lossof deprivation-induced synaptic depression, their combined destructiondid disrupt this form of plasticity. This finding led to the suggestionthat the two inputs might be able to substitute for one anotherin the control of cortical plasticity. Our discovery that AChand NE produce a qualitatively similar facilitation of LTD isentirely consistent with this idea. Thus, the study of LTD andits modulation may provide new insights into the mechanisms ofexperience-dependent synaptic plasticity in theneocortex.

  FOOTNOTES

Received July 30, 1998; revised Dec. 10, 1998; accepted Dec. 14, 1998.

This work was partly supported by grants from the National Eye Institute, the National Science Foundation, and the CharlesA. Dana Foundation. We thank Dr. Kim Huber for helpfulcomments.
Correspondence should be addressed to Dr. Mark Bear, Howard Hughes Medical Institute and Department of Neuroscience, BrownUniversity, Providence, RI02912.

  REFERENCES

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Abstract
Introduction
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