Multiple and Opposing Roles of Cholinergic Transmission in the Main Olfactory Bulb

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The Journal of Neuroscience, November 1, 1999, 19(21):9180-9191

Multiple and Opposing Roles of Cholinergic Transmission in the Main Olfactory Bulb
Pablo E. Castillo¹^,², Alan Carleton¹, Jean-Didier Vincent¹, and Pierre-Marie Lledo¹
¹ Centre National de la Recherche Scientifique, Institut Alfred Fessard, 91198 Gif-sur-Yvette Cedex, France, and ² Departamento de Fisiologia, Facultad de Medicina, Universidad de la Republica, 11800 Montevideo, Uruguay

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The main olfactory bulb is a critical relay step between the olfactory epithelium and the olfactory cortex. A marked featureof the bulb is its massive innervation by cholinergic inputs fromthe basal forebrain. In this study, we addressed the functionalinteraction between cholinergic inputs and intrinsic bulbar circuitry.Determining the roles of acetylcholine (ACh) requires the characterizationof cholinergic effects on both neural excitability and synaptictransmission. For this purpose, we used electrophysiological techniquesto localize and characterize the diverse roles of ACh in mouseolfactory bulb slices. We found that cholinergic inputs have asurprising number of target receptor populations that are expressedon three different neuronal types in the bulb. Specifically, nicotinicacetylcholine receptors excite both the output neurons of thebulb, i.e., the mitral cells, as well as interneurons locatedin the periglomerular regions. These nicotine-induced responsesin interneurons are short lasting, whereas responses in mitralcells are long lasting. In contrast, muscarinic receptors havean inhibitory effect on the firing rate of interneurons from adeeper layer, granule cells, while at the same time they increasethe degree of activity-independent transmitter release from thesecells onto mitralcells.
Cholinergic signaling thus was found to have multiple and opposing roles in the olfactory bulb. These dual cholinergic effectson mitral cells and interneurons may be important in modulatingolfactory bulb output to central structures required for drivenbehaviors and may be relevant to understanding mechanisms underlyingthe perturbations of cholinergic inputs to cortex that occur inAlzheimer'sdisease.

Key words: mitral cells; inhibitory interneurons; basal forebrain; GABA; nicotinic receptors; muscarinic receptors; olfaction

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Considerable evidence exists for an extrinsic cholinergic influence in the maturation and function of the main olfactory bulb(Halász and Shepherd, 1983; Le Jeune et al., 1996). It is alsowell established that a number of neurodegenerative disordersrelated to cholinergic systems are accompanied by olfactory dysfunctions(Serby et al., 1985; Kovacs et al., 1998) (for review, see Doty,1991; Quirion, 1993; Kasa et al., 1997). Indeed, the presenceof cholinergic centrifugal fibers originating from the magnocellularbasal forebrain nuclei [the substantia innominata and the medialpart of the horizontal limb of the diagonal band of Broca (HDB)]has been revealed in the olfactory bulb (Shute and Lewis, 1975;Macrides et al., 1981). In vertebrates, the olfactory bulb isthe first relay for olfactory processing, receiving informationfrom the olfactory epithelium and conveying it to higher brainstructures via its principal neurons, the mitral and tufted cells.These neurons interact with two classes of local inhibitory interneurons:(1) periglomerular cells that make synapses onto the primary dendritesof mitral/tufted cells, and (2) granule cells that release GABAonto mitral cell secondary dendrites (Ribak et al., 1977; Nowyckyet al., 1981; Jahr and Nicoll, 1982). Cholinergic inputs wereonce thought to terminate predominantly onto granule spines, leadingto the conclusion that the main role of acetylcholine (ACh) isto modulate granule cell inhibition of mitral cells (for review,see Halász and Shepherd, 1983; Macrides and Davis, 1983). However,more recent anatomical observations have reported significantcholinergic innervation of several layers of the olfactory bulb(Kasa et al., 1995), which led us to hypothesize far more variedroles forACh.

Although behavioral studies have stressed the importance of cholinergic inputs in olfactory memory (Ravel et al., 1994; Lévyet al., 1995), the sites and mechanisms of cholinergic actionhave not been clearly defined. Electrophysiological experimentshave yielded contradictory results. For example, electrical stimulationof the HDB in vivo was reported either to depress (Nickell andShipley, 1988b) or to increase (Kunze et al., 1991) mitral cellfiring through cholinergic modulation of GABAergic inhibition.In addition, application of ACh in vivo either decreased or increasedmitral cell firing activity (Ravel et al., 1990; Elaagouby andGervais, 1992).

The effects of ACh in the CNS were long thought to be mediated only by muscarinic ACh receptors (mAChRs), because their pharmacologicalblockade results in serious disruption of multiple brain functions(Ghonheim and Mewaldt, 1975) (for review, see Hagan and Moris,1989). However, nicotinic AChRs (nAChRs) have been shown in recentyears to play major roles in the CNS as well (Levin, 1992; Changeuxet al., 1998). In this study, we took advantage of the slice preparationto explore the effects of the activation of both nicotinic andmuscarinic ACh receptors on cell excitability and synaptic transmissionin the olfactory bulb network. We report opposite effects of cholinergicmodulation of excitability of mitral and granule cells. We havealso found opposite modulatory action of ACh on GABAergic synapticinputs onto granule and mitral cells; the latter may be criticalfor olfactory processing and learning (Shepherd and Greer, 1998).All of these cholinergic actions in conjunction with correlatedanatomical findings suggest specific roles of the cholinergicsystem in odor processing as well as in olfactorylearning.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Slice preparation. Experiments were performed on olfactory bulb slices obtained from 2- to 5-week-old C57/Bl6 mice. Bulbswere rapidly removed and immediately placed in 4°C oxygenatedartificial CSF (ACSF) containing (in mM): 124 NaCl, 3 KCl, 2 CaCl₂,1.3 MgCl₂, 25 NaHCO₃, 1.25 NaH₂PO₄, 10 D-glucose, pH 7.3, whenbubbled with 95% O₂/5% CO₂ (310 mOsm). Horizontal slices (300µm) were cut with a vibrating microslicer (Vibratome 1000; TPI,St. Louis, MO) and kept in oxygenated ACSF at 32°C for ~30 min.Subsequently, the slices were stored at room temperature (20-22°C)for 4-6 hr. Individual slices were then transferred to a submerged-slicerecording chamber where they were superfused with oxygenated ACSF(same composition as above) at a rate of 2-3 ml/min. The horizontalplane was chosen because this orientation preserves the primaryand secondary dendrites of mitralcells.

Electrophysiological recordings. Recordings were performed using the patch-clamp technique in the cell-attached and whole-cellconfigurations with a RK300 patch-clamp amplifier (BiologicalScience Instruments, Claix, France). Cells were recorded undervisual control with an upright Zeiss Axioskop microscope (40×water immersion objective lens; 0.75 numerical aperture) and infrareddifferential interference contrast videomicroscopy (IR-DIC; filter,850 nm). Images of neurons were captured and processed with animage processor (PXC200 Precision Color, Imagination). Mitralcells, periglomerular interneurons, and granule cells were easilydiscriminated based on morphology and location (Shepherd and Greer,1998). To confirm visual identification of recorded neurons, asubset of cells was filled with Lucifer yellow (lithium salt fromSigma, St. Louis, MO) in the whole-cell recording configuration.The morphology of the patched cells was then sketched after recordings.All experiments were performed at room temperature (22-24°C).Microelectrodes with access resistance of ~6 and 12 M $Omega$ were usedto record mitral and granule cells, respectively. An internalsolution of the following composition was used (in mM): 123 Cs-gluconate,10 CsCl, 8 NaCl, 1 CaCl₂, 10 Cs-EGTA, 10 Na-HEPES, 10 D-glucose,0.3 GTP, 2 Mg-ATP, 0.2 AMPc, pH 7.3 (280 mOsm). Unless indicatedotherwise, IPSCs were recorded either in the presence of the AMPAreceptor antagonist 1,2,3,4-tetrahydro-6-nitro-2,3-dioxobenzo[f]quinoxaline-7-sulfonamide(NBQX; 10-20 µM), with the NMDA receptor antagonist D,L-2-amino-5-phosphonopentanoicacid (D,L-APV; 100 µM), or in the presence of a nonspecific ionotropicglutamate receptor antagonist, kynurenic acid (5 mM).

Data analysis. Synaptic responses were filtered at 1-5 kHz with an eight-pole Bessel filter, digitized at 4 kHz on a TL-1interface (Axon Instruments, Foster City, CA), and collected onan IBM-compatible computer. On- and off-line data analyses wereperformed with Acquis1 (Gérard Sadoc, Centre National de la RechercheScientifique-Agence Nationale pour la Valorisation de la Recherche,Paris, France). The frequency and amplitude of IPSCs were determinedoff-line, and our detection threshold was set at a di/dt of 10pA/msec with minimum and maximum rise times set at 0.1 and 4 msec,respectively. The minimal acceptable amplitude for a miniatureevent was 6 pA. Statistical significance of differences betweenmeans was assessed using Student's t test. Kolmogorov-Smirnovstatistics were used to determine whether there were statisticallysignificant changes in the frequency and amplitude of IPSCs. Thelevel of significance was set at p < 0.05 unless indicatedotherwise.

To investigate cholinergic effects in the cell-attached mode, a stable frequency of firing was recorded for at least 100 secto establish a baseline expressed as mean firing rate (definedas 100%). During drug applications, effects were then quantifiedas a maximum firing frequency relative to baseline for mitralcells and mean for frequency relative to baseline for interneurons.For whole-cell recordings, the reported membrane potentials werecorrected for junction potentials, which were measured to be 11mV, for the solutions used. During all experiments, the accessresistance (R_a) and the input membrane resistance (R_m) were constantlymonitored, and acquisition was terminated when these parameterschanged more than 15%. Capacitance compensation was used to decreasethe charging time of the pipette. Because of the small voltageerror from the R_a, no series resistance compensation was used.Group measurements were expressed as mean ±SEM.

Solution and drugs. Drug solutions were bath-applied using a gravity-driven perfusion system, and maximally effective concentrationsof the drugs were achieved within 30 sec (see Fig. 1B for timecourse of wash-in). NBQX, D,L-APV and oxotremorine were from Tocris;all other drugs and salts were purchased fromSigma.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

During the course of this study, whole-cell or cell-attached patch-clamp recordings were performed on 142 mitral cells (principalneurons) and different subtypes of interneurons: 9 bipolar periglomerularcells, 6 monopolar periglomerular cells, and 75 granule cells.Successfully patched mitral cells and interneurons were held forperiods ranging from 15 min to >1 hr. Membrane resistances rangedfrom 89 to 325 M $Omega$ (mean of 153 ± 10 M $Omega$ ) for mitral cells and weretwo- to eightfold higher in interneurons (mean of 703 ± 46 M $Omega$ ).The location and morphometric features used here to characterizeeach interneuron were consistent with previous morphological classifications(Schneider and Macrides, 1978) (for review, see Mori, 1987; Shepherdand Greer, 1998).

Activation of nicotinic receptors increases mitral cell firing frequency

To determine whether cholinergic receptor activation modulates neuronal excitability in the main olfactory bulb, we firstassessed the firing activity of mitral cells in the cell-attachedmode, and the effects of different cholinergic agonists were evaluated(Fig. 1A; see the recording arrangement). All recordings fromthe somata of visually identified mitral cells showed spontaneousfiring activity under our standard conditions (Fig. 1B). The firingrates for mitral cells ranged from 1 to 11 Hz, with a mean of5.5 ± 1.3 Hz (n = 7), in good agreement with previous in vivoreports (Pager, 1983; Motokizawa, 1996). The application of 10µM NBQX, 100 µM D,L-APV, and 20 µM bicuculline methiodide (BMI),to block AMPA, NMDA, and GABA_A receptors, respectively, only slightlyreduced the basal firing rate of mitral cells, indicating thatmitral cells were able to fire action potentials spontaneouslyeven in the absence of fast glutamatergic and GABAergic synapticinputs (n = 28). The broad-spectrum cholinergic receptor agonistcarbachol was bath-applied to olfactory bulb slices at concentrationsranging from 10 to 100 µM. As illustrated in Figure 1B,D, applicationof 50 µM carbachol caused a dramatic increase in the frequencyof spontaneous action potential discharge of all neurons recordedin standard conditions (a mean rate of 5.5 Hz, range 1-11 Hz incontrol conditions and a mean of 28 Hz, range 9-54 Hz in the presenceof cholinergic agonist; p < 0.015; n = 8). This carbachol-inducedresponse was fully reversible with washout of the drug (Fig. 1B).Previous studies have shown that cholinergic receptors can causethe release of neurotransmitters through the activation of AChreceptors on the presynaptic terminals (Wonnacott, 1997). We soughtto determine whether the carbachol responses we observed werecaused by the direct activation of postsynaptic receptors or indirectlythrough the release of neurotransmitter onto the mitral cells.Blocking ionotropic glutamate receptors (NBQX, 10 µM and D,L-APV,100 µM) and GABA_A receptors (BMI, 20 µM) did not inhibit carbacholresponses (n = 5; p > 0.05), suggesting a direct effect onto mitralcells (Fig. 1D). In the presence of these synaptic blockers, applicationof 30 µM nicotine (Fig. 1C) mimicked the carbachol effect (n =8). The mean frequency was increased from 6 Hz (range 0.9-10 Hz)to 58 Hz, (range 19-95 Hz; n = 8) after nicotinic application(Fig. 1D). Because there are many subtypes of neuronal nicotinicreceptors in the CNS (for review, see Wonnacott, 1997; Changeuxet al., 1998), we used the nicotinic receptor antagonist mecamylamineat a concentration unlikely to distinguish between these differentsubtypes. We found that 50 µM mecamylamine completely blockedthe enhancing actions of carbachol or nicotine on mitral cellfiring frequency (n = 4) (Fig. 1D). Moreover, oxotremorine (50µM), used as a specific mAChR agonist, did not change the cellfiring rate (n = 4; data not shown).

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Figure 1. Activation of nicotinic receptors enhances mitral cell firing frequency in the main olfactory bulb. A (left), Infrared image of a mitral cell visualized in cell-attached mode under IR-DIC microscopy (arrow indicates the location of the patch electrode) and schema (right) illustrating the location of the recording pipette and the major cell types analyzed in the present study. MC, Mitral cell; GC, granule cell; PG_mono, monopolar periglomerular cell; PG_bi, bipolar periglomerular cell. B (left), Extracellular recording in cell-attached mode from a mitral cell, in normal conditions (STD), during carbachol (CCh, 50 µM) application, and after drug washout (Wash). Single action potentials are shown on the right side of each trace at an expanded time scale (note the different time calibration bar). B (right), The time courses for changes in action potential frequency (bin size: 10 sec) and amplitude after bath application of CCh are shown (numbers indicate the times of traces chosen for illustration in the left panel). C, Mitral cell firing activity in the presence of BMI (20 µM), NBQX (10 µM), and D,L-APV (100 µM) was increased after bath application of 30 µM nicotine. This nicotine-induced effect was reversible on washout of the drug (Wash). D, Average of the firing frequency changes induced by cholinergic drug applications in different treatments and normalized to the control responses. Changes in frequency were compared between control conditions and drug applications using a paired t test. Ago: 50 µM carbachol or 30 µM nicotine (*p < 0.05; **p < 0.01).

The spike amplitude reduction observed after nAChR activation (Fig. 1B, right) strongly suggested that the firing activityenhancement was caused by a membrane potential depolarization.In agreement with this interpretation, bath application of nicotineat concentrations ranging from 10 to 100 µM always elicited aninward current accompanied by an increase in noise (Fig. 2) (n= 42). In standard medium, the mean maximum amplitude of the responseinduced by nicotine application (30 µM) was $-$ 645 ± 138 pA (rangefrom $-$ 238 to $-$ 1382 pA; n = 11) at $-$ 80 mV. As illustrated in Figure2A, these responses were dose dependent and specifically blockedby mecamylamine (50 µM; n = 4). Rundown of the nicotine-inducedcurrent was not observed during the course of these experimentsusing our pipette medium (Fig. 2A1). This nicotine-induced currentwas also mimicked by 50 µM carbachol application (data not shown)and was revealed to be a direct response of mitral cells. Hence,nicotine (30 µM) still evoked a significant inward current (rangefrom $-$ 113 to $-$ 570 pA; n = 17) in the presence of BMI and NBQX-APV(Fig. 2B1), as well as in the presence of blockers of voltage-dependentsodium channels (TTX, 1 µM) and voltage-dependent calcium channels(200 µM Cd²⁺ plus a mixture of external high Mg²⁺/0 Ca²⁺ ratio) (mean current: $-$ 244 ± 41 pA; n = 15) (Fig. 2B2), arguingfor a direct effect on mitral cells. Altogether, these findingssupport the existence of functional nicotinic receptors on mitralcells that enhance their firing activity by directly depolarizingthe membrane potential.

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Figure 2. Characterization of nicotine-induced inward currents in mitral cells. A, Repeated applications of nicotine consistently elicited an inward current. Two consecutive bath applications of 100 µM nicotine showed no evidence of rundown (1). This current showed dose dependency (2) and was blocked by 50 µM mecamylamine (3). Sample recordings were taken from three different cells bathed in standard medium. B, The nicotine-induced current was also observed in the presence of a cocktail that included 20 µM BMI, 10 µM NBQX, and 100 µM D,L-APV (1), or on a different cell bathed with extracellular Ca²⁺ substituted with Mg²⁺ and containing 1 µM TTX (2). C, Long applications of nicotine revealed a slow decay. Inward currents were obtained from two different mitral cells (1 and 2) and showed identical decay kinetics when scaled (1 + 2). For all cells shown in A-C, V_h = $-$ 80 mV. D, Subtraction of currents elicited during a voltage ramp without and with nicotine application reveals the voltage dependence of nicotine-induced current. The recording was performed in the BMI-NBQX-APV mixture supplemented with TTX (1 µM) and Cd²⁺ (200 µM) (top trace). The corresponding current-voltage relationship (bottom) shows inward rectification.

As illustrated in Figure 2C, a long (up to 400 sec) application of nicotine (30 µM) showed a slow decay, with a mean half-decaytime ranging between 160 and 285 sec (247 ± 18 sec; n = 6). Thistime constant was relatively independent of the peak current amplitude(Fig. 2C, bottom traces). To further characterize this slowlydecaying current, voltage-ramp commands were applied to evaluateits relationship with voltage (Fig. 2D). Neuronal nAChRs havepreviously been shown to have inwardly rectifying current-voltagerelationships, passing little outward current and having zerocurrent between 0 and +20 mV (for review, see Role, 1992). Consistentwith previous findings, voltage ramps given in the absence andpresence of nicotine (30 µM) revealed a reversal potential (E_rev)ranging from $-$ 5 to + 10 mV (a mean value of 3.2 ± 2.7 mV; n =6) and an inward current, which strongly rectified such that outwardcurrent was not observed for positive membrane potential values,up to +50 mV (Fig. 2D). Thus, the current-voltage relationshipof the slowly decaying nicotinic response is consistent with theactivation of neuronalnAChRs.

Activation of muscarinic receptors decreases granule cell firing frequency

Because granule cells constitute the largest neuronal population in the main olfactory bulb, these interneurons are extremelyinfluential in the control of olfactory bulb circuitry (for review,see Mori, 1987). We thus investigated whether they were subjectedto cholinergic modulation. When recorded in the cell-attachedconfiguration with BMI and NBQX-APV, some granule cells were alsofound to be spontaneously active (Fig. 3B,C), with a mean firingrate of 6.0 ± 1.3 Hz (n = 7). Bath application of carbachol (50-100µM) reduced spike discharge of granule cells (a mean reductionof 58 ± 11%; n = 4) (Fig. 3B,D). A dose-dependent effect was foundwithin the range of 10-100 µM of carbachol (n = 5), and the reductionof granule cell firing activity was slowly reversible on washoutof the agonist (Fig. 3B). The muscarinic nature of this carbacholeffect on granule cell firing was revealed by oxotremorine (50µM) (Fig. 3C,D) (n = 4), whereas nicotine (up to 50 µM) treatmentdid not affect their firing frequency (Fig. 3D) (n = 4). The reductionof spike discharge induced by muscarinic receptor activation mayresult from a membrane potential hyperpolarization because theamplitude of currents generated by action potentials was increased(Fig. 3B, right).

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Figure 3. Muscarinic receptor activation decreases granule cell firing frequency. A, A granule cell visualized under IR-DIC microscopy with the arrow indicating the cell dendrite (left); right, schema of a recorded cell filled with Lucifer yellow. B (left), Extracellular recording in cell-attached mode from a granule cell recorded before, during, and after CCh (50 µM) (Wash). Single action potentials are shown on the right (note different time calibration bars). B (right), The time course for changes in action potential frequency (bin size: 10 sec) and amplitude during CCh treatment is shown (numbers indicate when traces were extracted for illustration in the left panel). C, Oxotremorine (50 µM) decreased the firing frequency; this effect was reversible on washout (Wash). All granule cells were recorded in a mixture that included BMI (20 µM), NBQX (10 µM), and D,L-APV (100 µM). D, Average of the firing frequency changes induced by cholinergic drug applications in different treatments and normalized to the control responses. Changes in frequency were compared between control medium and drug applications using paired t test (*p < 0.05).

Altogether, these findings demonstrate that ACh modulates, in opposite directions, the spontaneous firing of mitral and granulecells through the activation of nicotinic and muscarinic receptors,respectively. Moreover, because these dual effects were also seenafter blockade of ionotropic glutamatergic and GABAergic synaptictransmission, these two cholinergic actions probably result fromdirect membrane potential changes. It is noteworthy that our findingsdo not support a direct nicotinic effect on granule cells, whereasothers have reported nicotine-induced responses in olfactory bulbinterneurons (Alkondon and Albuquerque, 1994; Alkondon et al.,1996). We therefore decided to further investigate the nicotinicactions on other olfactory bulb interneuronsubtypes.

Whole-cell nicotinic currents in interneurons

To examine a direct effect of nicotinic receptor activation on olfactory bulb interneurons (i.e., monopolar periglomerularcells, bipolar periglomerular cells, and granule cells), whole-cellrecordings were performed with patch electrodes containing Luciferyellow. This dye was used to determine whether the effects inducedby cholinergic receptor activation could be correlated with distinctcell morphology and location. For all interneuron subtypes recorded,only bipolar periglomerular cells were sensitive to nicotine (30µM). In the presence of BMI and NBQX-APV, a nicotine-induced currentwas observed from four of four recorded cells ( $-$ 113 ± 84 pA) (Fig.4A,B), but up to 100 µM nicotine application failed to inducea response from all tested monopolar periglomerular (n = 6) andgranule cells (n = 4) (Fig. 4A). Bipolar periglomerular cell firingactivity was also dramatically enhanced during nicotine treatmentin the presence of BMI and NBQX-APV (data not shown). Figure 4also shows that the response to nicotine (30 µM) progressivelydecays during prolonged application of the agonist; as reportedfor mitral cells, the decay time was independent of the amplitude(Fig. 4B). This amplitude independence allowed us to compare therate of decay across cell types. As depicted in Figure 4C, thedecay was found to be faster in interneurons than in mitral cells(mean times to half-decay of 94 ± 7 and 247 ± 18 sec for fourbipolar periglomerular cells and six mitral cells, respectively;p < 0.001). This discrepancy could result from different compositionsof nAChR subunits. Indeed, similarly fast decay time constantshave been reported for nicotinic responses recorded in culturedolfactory bulb interneurons expressing the $alpha$ 7-subunit (Alkondonand Albuquerque, 1994); it is this $alpha$ 7 subunit that has been foundto be highly expressed in the glomerular layer (Le Jeune et al.,1995). With the finding that functional nAChRs and mAChRs arepresent in the olfactory bulb network and that activation of thesereceptors strongly modulates neuronal excitability, we then analyzedin detail the ability of cholinergic receptors to control GABArelease from interneurons.

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Figure 4. Selective responses of nicotine on olfactory bulb interneurons. The effect of bath application of nicotine was examined for three interneuron subtypes: monopolar periglomerular cell (PG_mono), bipolar periglomerular cell (PG_bi), and granule cell (GC). These cells were identified by their location, morphology, and pattern of electrophysiological activity. A, Membrane current traces of individual interneurons showed that only bipolar periglomerular cells respond to nicotine application. Insets, Camera lucida drawings of the Lucifer yellow-filled interneurons performed after whole-cell recordings. B, Inward currents obtained from two different periglomerular interneurons (1 and 2) showed identical decay kinetics when scaled (1 + 2). C, Long applications of nicotine revealed a faster decay for a periglomerular cell (PG) than for a mitral cell (MC) shown in Fig. 2C₂. The holding potential was $-$ 80 mV for all recordings.

Spontaneous and glutamate-evoked GABA release onto mitral cells

Spontaneous synaptic inputs onto mitral cells were measured in the whole-cell recording configuration. Excitatory and inhibitorysynaptic activities were distinguished under control conditionsby using a low-chloride internal solution to separate the reversalpotentials of excitatory and inhibitory synaptic currents. Underthese conditions, spontaneous IPSCs were seen as inward at $-$ 80mV and outward at 0 mV (the reversal potential for excitatorysynaptic events) (Fig. 5A). As expected, these spontaneous eventsreversed at the chloride equilibrium potential (E_Cl of $-$ 48 mV)and were completely and reversibly blocked by bicuculline (20µM; n = 6), indicating that they were mediated by activation ofGABA_A receptors (Fig. 5A). It is noteworthy that during the courseof these recordings, GABAergic events remained stable even afterlong periods of recording in control conditions. This lack ofrundown contrasts with the receptors observed in hippocampal cells(Stelzer et al., 1988).

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Figure 5. GABAergic synaptic events recorded in mitral cells. A, GABAergic spontaneous synaptic currents were recorded at membrane potentials indicated at the right of the traces. Outward spontaneous currents recorded at 0 mV (middle trace) correspond to pure GABAergic IPSCs because they were completely blocked by 20 µM bicuculline methiodide (+ BMI). B, The distributions of interevent intervals were constructed from 60 sec of continuous data measured at $-$ 80 mV (thin line, 784 events) or 0 mV (thick line, 2826 events). C, Spontaneous IPSCs recorded before (STD) and during application of 10 µM NBQX with 100 µM D,L-APV. Subsequent application of BMI (20 µM) completely abolished synaptic activity (bottom traces) (V_h = 0 mV). D, Corresponding cumulative distributions of spontaneous IPSC intervals (left) and amplitudes (right). Plots were constructed from 100 sec of continuous recording. Both frequency and amplitude distributions changed significantly (Kolmogorov-Smirnov test, p < 0.001) in the presence of NBQX-APV (thick line, 305 events; thin line, 1788 events). For this cell, the mean spontaneous IPSC frequency was 17.4 and 3.1 Hz, and mean amplitude was 55 ± 32 pA (SD) and 28 ± 16 pA in STD and NBQX, APV, respectively.

GABA release from granule cells onto mitral cells is located in a structure called the dendrodendritic reciprocal synapse,consisting of an excitatory synapse directly adjacent to an inhibitorygranule-to-mitral cell synapse (Price and Powell, 1970). It hasbeen demonstrated that evoked GABA release is mediated by glutamateexcitation (Nowycky et al., 1981; Jahr and Nicoll, 1982; Isaacsonand Strowbridge, 1998; Schoppa et al., 1998). However, littleis known about spontaneous granule-to-mitral cell GABA releasein the absence of excitation. To quantify spontaneous GABA release,cells were recorded in the presence of NBQX-APV (Fig. 5C,D) orthe broad-spectrum ionotropic glutamatergic antagonist kynurenate(5 mM). Glutamatergic receptor blockers dramatically decreasedspontaneous IPSC frequency (a mean reduction of 81 ± 4%, withp < 0.0005; n = 9) as well as the number of large spontaneousIPSCs (Fig. 5D). In sum, mitral cells receive spontaneous IPSCsdriven by glutamate receptor activation that are characterizedby large amplitudes and high frequency as well as spontaneousIPSCs independent of glutamate receptor activation characterizedby smaller amplitudes and a lower frequency. Having describedthese two types of GABAergic events onto mitral cells, we theninvestigated their potential sensitivity to cholinergicmodulation.

Activation of muscarinic receptors modulates GABAergic synaptic inputs onto mitral cells

As shown in Figure 6A, bath application of carbachol in standard external medium markedly increased the frequency of spontaneousIPSCs; the relative interevent interval curve was shifted to theleft, indicating an increase of the frequency of GABAergic events(Fig. 6C, left graph). The mean baseline frequency of these spontaneousevents (5.0 ± 1.1 Hz) was increased during carbachol treatmentby an average of threefold (15.4 ± 3.2 Hz) in seven of seven mitralcells. In most of these neurons, the increase in frequency wasattributable to an increase in the number of small amplitude events,which therefore resulted in an apparent decrease of mean IPSCamplitude (Fig. 6B). As illustrated in Figure 6C (right graph),the cumulative amplitude plot indicates a reduction in the numberof large amplitude GABAergic events. However, when spontaneousIPSCs were averaged and superimposed to compare kinetics, risetimes and decay rates were unchanged (Fig. 6B). On average, nochanges in cumulative rise time distributions of spontaneous IPSCsbefore and during carbachol treatment were seen (data not shown;n = 5; p > 0.05). The carbachol effect on spontaneous IPSC frequencyreached a steady state within 20-40 sec and showed no evidenceof desensitization over an application period of up to 3 min (n= 6).

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Figure 6. Carbachol increases the frequency of both spontaneous IPSCs (A-C) and miniature IPSCs (D-F) from mitral cells. A, Sample recordings of spontaneous IPSCs are depicted in standard medium (Std) and after 50 µM carbachol application (CCh). B, Spontaneous IPSCs were averaged and scaled before (Std, 220 events) and after carbachol application (CCh, 191 events). Note that carbachol caused no change in the time course of these events. C, Cumulative probability plots of event frequency (left graph) and amplitude (right graph) were constructed from 125 sec of continuous recording (394 and 967 events in Std and CCh, respectively). CCh enhanced the frequency of spontaneous IPSCs (a mean interevent interval of 0.32 ± 0.4 (SD) sec and 0.13 ± 0.15 sec before and after bath application of carbachol, respectively). The mean spontaneous IPSC amplitude in Std was 49 ± 46 pA (SD) versus 38 ± 31 pA in CCh. Both changes were statistically significant (Kolmogorov-Smirnov test, p < 0.001). D, Sample recordings of miniature IPSCs from a different cell before (Ctrl) and during application of 50 µM carbachol (CCh) in the presence of 1 µM TTX. E, Averaged miniature IPSCs before (Ctrl, 230 events) and during carbachol treatment (CCh, 206 events). As in B, traces are superimposed and scaled on the right (Scaled) to illustrate that carbachol had no effect on the time course of miniature IPSCs. F, Cumulative probability plots of synaptic current frequency and amplitude were constructed from 80 sec of continuous recording (305 and 617 events in Ctrl and CCh, respectively). CCh enhanced the frequency of miniature IPSCs [mean interevent interval of 0.26 ± 0.25 sec (SD) and 0.13 ± 0.12 sec before and after bath application of carbachol, respectively]. The mean miniature IPSC amplitude in controls was 55 ± 54 pA versus 39 ± 29 pA in CCh. Both changes were statistically significant (Kolmogorov-Smirnov test, p < 0.001). D-F, Cells in this figure were recorded in the presence of 10 µM NBQX and 100 µM D,L-APV and voltage-clamped at 0 mV.

This carbachol-induced enhancement of spontaneous IPSC frequency could be caused by an increase in mitral cell firing or adirect increase in the dendrodendritic synaptic transmission,or both. To test this possibility, slices were bathed with glutamatergicreceptor antagonists, which should prevent this effect. Carbacholstill increased the frequency of GABAergic events in all recordedneurons (n = 4). We thus decided to explore more precisely themechanism by which carbachol could directly increase GABArelease.

To evaluate the contribution of action potential-independent transmitter release, synaptic events were measured in the presenceof both tetrodotoxin (TTX; 0.5-1 µM, perfused for a minimum of5 min) to block action potentials, and glutamatergic antagonists,to isolate miniature IPSCs reflecting quantal release by granulecells (n = 39 experiments) (Fig. 6D-F). The baseline frequencyof miniature IPSCs (2.0 ± 0.5 Hz; n = 12) was markedly increasedin all tested cells by carbachol treatment (4.8 ± 1 Hz; n = 12;p = 0.004), and cumulative amplitude distributions of miniatureIPSCs demonstrated significant changes in 9 of 12 cells (p < 0.001with Kolmogorov-Smirnov test) (Fig. 6D,F, left panel). In Figure6, only the small amplitude (<40 pA) synaptic events seemed tobe sensitive to carbachol. In other cells, only large synapticcurrents were affected by carbachol (data not shown). However,in any case, a correlation with a change in the rise time couldbe observed, which argues against a distinct localization of thepopulation of carbachol-sensitive GABAergic synapses that impingeon mitral cells. Thus, carbachol enhanced GABA release througha mechanism independent of the spontaneous firing of granule cellsor glutamatergic excitatory drive, indicating that carbachol directlymodulates quantal release of GABA from presynapticterminals.

The carbachol-induced enhancement of miniature GABAergic events was not reproduced by 10-30 µM nicotine (Fig. 7A) (n = 6)but could be mimicked by 50 µM oxotremorine (a mean increase of318 ± 124% of control frequency; n = 4; p < 0.001), indicatingthat this enhancement was mediated through activation of mAChRs(Fig. 7B). Activation of mAChRs could increase miniature IPSCfrequency either by a direct effect on the exocytotic machineryor by increasing calcium influx into presynaptic terminals, orboth. We therefore examined whether carbachol affected the frequencyof miniature IPSCs in the presence of the Ca²⁺ channel blocker Cd²⁺ (100-200 µM) added in the external medium. A change in the frequencydistribution was still clearly observed (Fig. 7C), with a meanincrease of 319 ± 220% (n = 4). We thus conclude that mAChRs facilitateGABA release onto mitral cells through a direct presynaptic effectthat excludes modulation of Ca²⁺ influx through voltage-gated Ca²⁺ channels.

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Figure 7. Activation of muscarinic receptors enhances the frequency of miniature IPSCs recorded in mitral cells. A, Miniature IPSCs recorded before and during bath application of 30 µM nicotine (left traces), and corresponding cumulative interval distributions are shown on the right. Nicotine (thick line) had no effect on the miniature IPSC frequency (Kolmogorov-Smirnov test, p > 0.05). B, Recordings from a different cell before and after 50 µM oxotremorine application (left traces). The corresponding cumulative display of interval distributions on the right shows that oxotremorine increased miniature IPSC frequency (Kolmogorov-Smirnov test, p < 0.001). C, Carbachol (+ CCh) still increased miniature IPSC frequency in the presence of 100 µM Cd²⁺ (Kolmogorov-Smirnov test, p < 0.001). Cells were voltage-clamped at 0 mV and recorded in normal ACSF with 10 µM NBQX, 100 µM D,L-APV, and 1 µM TTX (Ctrl).

Evidence for two distinct GABAergic synaptic events in the olfactory bulb

During cell-attached recordings of granule cells, the spontaneous firing frequency was increased when bicuculline was bath-applied(data not shown). This increase may reflect a tonic GABAergicinhibition that could protect granule cells from long-lastingdepolarization. Whether the GABA involved in this modulation isreleased from intrinsic interneurons or from centrifugal fibersis unknown. First, to characterize spontaneous inhibitory synapticinputs to granule cells, synaptic currents were recorded in thepresence of NBQX-APV (as control condition) at +30 mV. Similarto the mitral cell experiments, inhibitory postsynaptic eventswere identified as GABA_A receptor-mediated events by (1) completeblockade by bicuculline (20 µM) (n = 11) and (2) similar E_revreported for IPSCs detected in mitral cells. In all granule cells(n = 43), spontaneous GABAergic inputs were observed with a meanrate of ~1 Hz (n = 21). For comparison, the mean rate of spontaneousIPSCs recorded in mitral cells under similar conditions was higher(1.88 ± 0.31 Hz; p < 0.05; n = 9) (Fig. 8A, top traces). Becauseall granule cells showed spontaneous IPSCs, the source of GABAonto granule cells was probably neighboring interneurons ratherthan centrifugal fibers [also see Wellis and Kauer (1994)].

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Figure 8. Two distinct inhibitory synaptic responses in olfactory bulb neurons. A, Spontaneous GABAergic IPSC activity from a granule (top) and a mitral cell (bottom) recorded before and during application of TTX (1 µM). Corresponding cumulative interval distributions are depicted before (thin lines) and in the presence of TTX (thick lines) (mitral cell: 220 events before and 177 events during TTX; granule cell: 664 events before and 147 events during TTX). Note that TTX strongly reduced the frequency of IPSCs from the granule cell. Neurons were recorded in the presence of NBQX and APV and voltage-clamped at 0 mV. B, Cumulative probability distribution of the reduction of IPSC frequency induced by TTX, measured in mitral cells (MC; n = 8) and granule cells (GC; n = 7) (mean reductions of 30 ± 9 and 60 ± 10%, for mitral cells and granule cells, respectively). C, Comparison of spontaneous IPSCs (no TTX included) recorded from a granule cell (GC) and a mitral cell (MC) is shown (top and middle traces). The averaged IPSCs (180 and 250 events, respectively, for granule and mitral cells) are superimposed and scaled (granule-IPSC and mitral-IPSC decay time constants: 40 msec and 10 msec, respectively). Both cells were voltage-clamped at 0 mV.

To assess the contribution of action potentials to GABA release onto mitral and granule cells, synaptic inputs were measuredbefore and after addition of TTX (1 µM) in the presence of NBQX-APV(Fig. 8A,B). A dramatic change in the distribution of intereventintervals was observed in the cumulative distributions from agranule cell shown in Figure 8A (top panel) but not from a mitralcell (Fig. 8A, bottom panel). Hence, whereas addition of TTX tothe bathing medium decreased the frequency of spontaneous IPSCsdetected in granule cells by 60 ± 10% (n = 8), it only decreasedspontaneous IPSC frequency from mitral cells by 30 ± 9% (n = 8)(Fig. 8B). This observation indicates that most of the GABAergicinputs onto granule cells depend on cell firing, whereas the largemajority of spontaneous inhibitory events onto mitral cells dependon ionotropic glutamate receptor activation (Fig. 5C,D). We alsohave found that spontaneous IPSCs, as well as miniature IPSCsin granule cells, last longer than those inhibitory events recordedfrom mitral cells. For example, spontaneous IPSCs in granule cells(n = 11) showed a mean half-decay time of 38.2 ± 3.6 msec (Fig.8C, top traces) when compared with those from mitral cells, withfourfold faster decay rates (10.9 ± 1.1 msec; p < 0.0001; n =9) (Fig. 8C, middle traces). Altogether, these results demonstratethat spontaneous GABA_A-mediated IPSCs recorded from granule cellswere distinct from those detected in mitral cells by (1) theirlow spontaneous frequency, (2) their dependence on firing activity,and (3) their slow time course ofdecay.

To test whether these inhibitory synapses could also be distinguished by their sensitivity to cholinergic modulation, spontaneousinhibitory events were recorded from granule cells in the presenceof cholinergic receptor agonists. Figure 9A,B shows that 50 µMoxotremorine dramatically decreased the frequency of spontaneousIPSCs recorded in control conditions (a mean reduction of 38.8± 3.6%; n = 5), whereas nicotine application had no effect (n= 5) (Fig. 9C). This reduction could result from the decreasein granule cell firing activity reported above. To test this possibility,cells were first bathed with 1 µM TTX before application of oxotremorine.As shown in Figure 9C, in the absence of action potentials oxotremorinehas no more effect, indicating that muscarinic modulation of GABArelease onto granule cells requires firing activity. Furthermore,these results strongly suggest that GABAergic inputs onto granulecells originate from neighboring granule cells. Together, thesedata illustrate a dual modulation mediated by muscarinic receptors:on the one hand they increase the level of tonic GABAergic inhibitiononto mitral cells while also relieving inhibition onto granulecells.

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Figure 9. Activation of muscarinic receptors decreased the frequency of spontaneous IPSCs recorded in granule cells. A, Spontaneous IPSCs recorded in NBQX-APV before (Std) and during application of 50 µM oxotremorine while voltage-clamping the cell at 0 mV. B, Corresponding interval (top) and amplitude (bottom) cumulative distribution plots were constructed from 150 sec of continuous data before (442 events) and after (261 events) carbachol. The amplitude distribution remained unchanged (Kolmogorov-Smirnov test, p > 0.05; mean amplitude in control, 28.4 vs 28.7 pA in carbachol), whereas the interval distributions were significantly different (Kolmogorov-Smirnov test, p < 0.001). C, Bar graph summarizing the effect of 50 µM oxotremorine (Oxo) and 50 µM nicotine (Nic) on spontaneous IPSC (sIPSC) or miniature IPSC (mIPSC) frequency.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

This study demonstrates the presence of at least four different targets for cholinergic inputs into the main olfactory bulb.We found that ACh induces a prominent increase in the firing activityof both mitral cells and bipolar periglomerular neurons throughactivation of distinct nAChR populations. In addition, activationof mAChRs both increases GABA release from granule cells ontomitral cells and inhibits granule cell firing. We propose thatthrough varied mechanisms, including extrasynaptic ACh diffusion,receptor subunit composition differences, and subcellular compartmentalization,cholinergic inputs have multiple points of control over the olfactorybulbnetwork.

Anatomical localization of cholinergic receptors in the olfactory bulb

The olfactory bulb, like other forebrain cortical structures, receives strong cholinergic inputs from the basal forebrain(Wenk et al., 1977; Macrides and Davis, 1983; Zaborsky et al.,1986). The bulb itself is virtually devoid of intrinsic cholinergicneurons (Woolf et al., 1984; Nickell and Shipley, 1988a; Senutet al., 1989). Autoradiographic and binding studies have revealedtwo important characteristics of cholinergic receptors in theolfactory bulb: both nAChRs and mAChRs are present at high densities,and their distribution within the olfactory bulb is well segregatedwith a low degree of overlap. This segregation of muscarinic andnicotinic receptors may reflect a dual organization of the olfactorybulb cholinergic system: the glomerular and mitral cell layersare more susceptible to modulation by nAChRs, whereas deeper layers(plexiform and granule cell layers) may be modulated primarilybymAChRs.

Fine structural observations have shown that centrifugal cholinergic projections terminate primarily onto interneurons (Nickelland Shipley, 1988a; Le Jeune and Jourdan, 1994; Kasa et al., 1995).For example, when choline acetyltransferase was used to labelcholinergic axons, ultrastructural analysis revealed that cholinergicsynapses were selectively targeted onto the dendrites of periglomerularor granule cells but never on mitral cells (Le Jeune and Jourdan,1993). Because no cholinergic synapses have been observed on mitralcells, it has been thought that neuromodulatory effects of AChin the bulb are mediated only through cholinergic synapses ontointerneurons (Kasa et al., 1995). During the course of this study,however, a remarkable direct effect on mitral cells was consistentlyfound after nAChR activation, suggesting an action of extrasynapticdiffusion of ACh (seebelow).

Two distinct nicotinic currents in the main olfactory bulb

Nicotinic AChRs have been found to be restricted to glomerular and mitral cell layers (Hunt and Schmidt, 1978; Hill et al.,1993; Le Jeune et al., 1995, 1996). This specific distributionsupports the selective sensitivity to nicotinic agonists thatwe observed for periglomerular and mitral cells. Our data alsoagree with previous reports showing that ACh was able to increasethe firing of interneurons from the glomerular layer (Pager, 1983)and induce inward currents in cultured interneurons (Alkondonand Albuquerque, 1994; Alkondon et al., 1996). These reports didnot identify the cell types from which cholinergic responses wereinduced. Moreover, recordings of cultured neurons have reportedonly one type of cholinoceptive neuron (Alkondon and Albuquerque,1994; Alkondon et al., 1996). This discrepancy may result fromthe absence of mitral cells in cultures prepared from neonatalanimals (Trombley and Westbrook, 1990).

Despite the fact that cholinergic projections have not been found to form synapses onto mitral cells, these cells still respondto cholinergic activation with fast inward currents. The apparentlack of cholinergic synapses onto mitral cells suggests that AChreaches postsynaptic nAChRs by long-range diffusion (Fig. 10A).Extrasynaptic release of ACh has been proposed to occur in severalsystems in the CNS and may participate in a volume transmissionphenomenon (Agnati et al., 1995) consistent with the diffuse anatomicalorganization of cholinergic fibers (Woolf, 1991).

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Figure 10. Schematic representation of cholinergic targets in the main olfactory bulb. This schema summarizes findings from the present study and takes into account previous anatomical observations. A, Cholinergic fibers activate postsynaptic nicotinic receptors located on mitral cells (MC) where ACh may be delivered through a nonsynaptic relationship to act as a neuromodulator and also on bipolar periglomerular cells (PG_bi) by a synaptic relationship where ACh rather acts as a neurotransmitter. Through this dual effect, ACh may facilitate the sensory transfer toward upper cortical centers. B, Cholinergic inputs into plexiform layers and granule cell layer allow activation of muscarinic receptors that contribute to a tonic inhibition of output neurons and a reduction of inhibition (disinhibition) onto granule cells. MC, Mitral cell; GC, granule cell; PG_bi, bipolar periglomerular cell; O.N., olfactory nerve; HDB, the horizontal limb of the diagonal band of Broca.

Numerous nAChR subunits have been described that, in various combinations, form receptors with different functional properties(Marks et al., 1986; Happe et al., 1994). For instance, $alpha$ 7-containingnAChRs rapidly desensitize (Couturier et al., 1990; Gerzanichet al., 1994; Zhang et al., 1994), whereas $alpha$ 4 $beta$ 2-containing nAChRsshow slower desensitization rates (Lindstrom, 1996; Léna andChangeux, 1997; Changeux et al., 1998). Immunohistochemical studieshave found mitral cell bodies to be exclusively and intenselystained with $beta$ 2-subunit antisera (Hill et al., 1993), whereasthe $alpha$ 7 subunit has been found mainly in the periglomerular layer(Le Jeune et al., 1996). Thus, the different decay times of nicotiniccurrents that we observed could reflect the presence of putativenAChR containing $alpha$ 4 $beta$ 2 subunits (hereafter referred to as $alpha$ 4 $beta$ 2nAChR, although the exact subunit composition remains to be determined)located on mitral cells, and $alpha$ 7 subunit located on periglomerularcells. In general, $alpha$ 7-containing nAChRs are found clustered insynaptic locations, whereas $beta$ 2-containing receptors have beenlocalized perisynaptically (for review, see Clarke, 1993; Roleand Berg, 1996). It is noteworthy that $alpha$ 4 $beta$ 2-containing nAChRsshow a high-affinity ACh binding site and therefore are more suitableto activation through paracrine ACh action. In addition, the differenttime courses of decay of nicotinic responses found in mitral andbipolar periglomerular cells suggest that nAChRs are best suitedfor mediating a tonic action in mitral cells and a phasic effectin interneurons, as recently suggested for different hippocampalinterneuron subtypes (Alkondon et al., 1999; McQuiston and Madison,1999).

By increasing firing rates of both mitral cells and periglomerular neurons, nAChRs can exert opposing effects on the finaloutput firing rate of mitral cells (Fig. 10A). Diffusion of AChfrom cholinergic terminals to mitral cells would activate theslowly desensitizing nicotinic receptors to bring the restingmembrane potential closer to the threshold for initiation of actionpotentials. At the same time, in glomeruli, ACh could indirectlyinhibit olfactory nerve inputs onto mitral cell dendrites throughactivation of periglomerular cells. Indeed, it has been proposedthat the periglomerular neurons sensitive to ACh are dopaminergicinterneurons (Nickell and Shipley, 1988a), and we have recentlyreported that dopamine receptor activation reduces the strengthof olfactory nerve inputs (Hsia et al., 1999).

Dual forms of modulation by muscarinic receptor activation on granule cells

The selective effect of muscarinic receptor activation on granule cells described here is consistent with previous anatomicalreports, which find binding for both M1- and M2-like receptorslocalized to the plexiform and granule cell layers, with relativelylittle muscarinic binding in the glomerular layer (Hunt and Schmidt,1978). We found that mAChR activation modulates the output ofgranule cells in opposing directions, depending on the subcellularlocalization of the mAChR population: somatically, by reducingexcitability of granule cells, and presynaptically, by enhancingGABA release onto mitral cells. At the level of the network, itshould also be noted that the muscarinic inhibition of granulecell firing would lead to a disinhibition of neighboring granulecells, because GABAergic inputs onto these interneurons are stronglydependent on action potentials (Fig. 8A,B).

The reduction of granule cell firing by mAChR activation may result from a membrane potential hyperpolarization caused byactivation of a potassium conductance, as shown in other brainstructures (Egan and North, 1986; McCormick and Pape, 1988) (forreview, see Brown et al., 1997). As to how mAChRs could stimulateneurotransmitter release, most studies have instead reported areduction of synaptic transmission mediated by mAChRs (for review,see Nicoll et al., 1990). Because the enhancement of GABA releaseonto mitral cells was still observed in the presence of TTX andCd²⁺, we propose that mAChR activation increases GABA release eitherby recruiting Ca²⁺ release from intracellular pools or by directly modulating exocytoticmachinery. Muscarinic receptors are therefore likely to be locatednear the transmitter release site on GABAergicterminals.

Integration of cholinergic modulation in the main olfactory bulb

A consideration of the entire network of connections in the bulb can lead to more complex interpretations. First, as mentionedabove, an indirect effect of decreasing granule cell body excitabilitywould be a decrease in the degree of inhibition $---$ a disinhibition $---$ ofneighboring granule cells. Second, a consideration of the ensembleof nicotinic and muscarinic AChR effects would be necessary tounderstand a potential role for cholinergic inputs in complextemporal and spatial patterns of circuit activity. For example,the cholinergic projection to the hippocampus has been proposedto serve as the pacemaker for the hippocampal theta rhythm. Indeed,this rhythm is present in the olfactory bulb as well and has beenshown to be phase-locked with both the sniff cycle and the hippocampaltheta during odor learning tasks (Macrides et al., 1982). Temporalcoordination of circuit activity may be critical to the olfactorysystem (Stopfer et al., 1997), which lacks the point-to-pointspatial organization of other sensorysystems.

Our characterization of four distinct targets for ACh in the olfactory bulb elucidates the critical role of cholinergic inputsin modulating various elements of this network. Because of thewidespread and opposing effects of ACh receptor activation, changesin any of these four points of control will change the state ofactivity and the output of the network. Further investigationof how these sites of cholinergic modulation interact and changeduring olfactory processing and learning should deepen our understandingof this complexcircuit.

  FOOTNOTES

Received May 18, 1999; revised June 25, 1999; accepted Aug. 11, 1999.

This study was supported by the Centre National de la Recherche Scientifique, the Institut Universitaire de France, a grantfrom Evaluation-Orientation de la Coopération Scientifique (ECOS-Uruguay),and a grant from the French Ministère de la Recherche et de l'Enseignement(A.C.). We are grateful to G. Sadoc for help with the analysisand acquisition software, to R. Gervais, F. Jourdan, and G. Shepherdfor reading this manuscript, and to A. Hsia for criticalcomments.
P.E.C. and A.C. contributed equally to thiswork.

Correspondence should be addressed to Dr. Pierre-Marie Lledo, Centre National de la Recherche Scientifique, Institut AlfredFessard, Avenue de la Terrasse, 91198 Gif-sur-Yvette Cedex, France.E-mail: Pierre-Marie.Lledo{at}iaf.cnrs-gif.fr.

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ABSTRACT
INTRODUCTION
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RESULTS
DISCUSSION
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