Mechanisms of Lateral Inhibition in the Olfactory Bulb: Efficiency and Modulation of Spike-Evoked Calcium Influx into Granule Cells

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The Journal of Neuroscience, August 20, 2003, 23(20):7551-7558

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Mechanisms of Lateral Inhibition in the Olfactory Bulb: Efficiency and Modulation of Spike-Evoked Calcium Influx into Granule Cells
Veronica Egger, Karel Svoboda, and Zachary F. Mainen
Cold Spring Harbor Laboratory, Cold Spring Harbor, New York 11724

   Abstract

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Granule cells are axonless local interneurons that mediate lateral inhibitory interactions between the principal neurons of theolfactory bulb via dendrodendritic reciprocal synapses. Thisunusual arrangement may give rise to functional propertiesdifferent from conventional lateral inhibition. Although granulecells spike, little is known about the role of the action potentialwith respect to their synaptic output. To investigate the signals that underlie dendritic release in these cells, two-photon microscopyin rat brain slices was used to image calcium transients ingranule cell dendrites and spines. Action potentials evokedcalcium transients throughout the dendrites, with amplitudesincreasing with distance from soma and attaining a plateaulevel within the external plexiform layer, the zone of granulecell synaptic output. Transient amplitudes were, on average,equal in size in spines and adjacent dendrites. Surprisingly,both spine and dendritic amplitudes were strongly dependenton membrane potential, decreasing with depolarization and increasingwith hyperpolarization from rest. Both the current-voltagerelationship and the time course of inactivation were consistentwith the known properties of T-type calcium channels, and the voltage dependence was blocked by application of the T-typecalcium channel antagonists Ni²⁺ and mibefradil. In addition,mibefradil reduced action potential-mediated synaptic transmissionfrom granule to mitral cells. The implication of a transientlyinactivating calcium channel in synaptic release from granulecells suggests novel mechanisms for the regulation of lateralinhibition in the olfactory bulb.

Key words: olfactory bulb; granule cell; lateral inhibition; action potential; T-type calcium channels; calcium imaging

   Introduction

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Granule cells (GCs) are axonless inhibitory interneurons thatconstitute the majority of neurons in the vertebrate olfactorybulb (OB). They provide the main source of interaction betweenthe principal excitatory neurons of the bulb, the mitral andtufted cells (M/TCs) (Shepherd and Greer, 1998). GCs are centralto major aspects of OB function, yet their role within olfactoryprocessing is still poorly understood. First, they may providea "spatial" contrast mechanism that sharpens the tuning ofM/TC odorant receptive fields, analogous to the role of lateralinhibition in the visual system (Yokoi et al., 1995; Urban,2002) (but see Laurent, 1999). Next, the reciprocal M/TC-GCsynapse may be a site for olfactory plasticity (Kendrick etal., 1992; Wilson and Sullivan, 1994; Hendin et al., 1997).GCs have been implicated in the generation of OB oscillationsand synchrony of M/TC firing (Buonviso et al., 1996; MacLeodand Laurent, 1996; Desmaisons et al., 1999), possibly relevantfor odor discrimination (Stopfer et al., 1997). Finally, GCsreceive the majority of cortical feedback to the bulb (Priceand Powell, 1970c).
GCs interact with M/TCs via reciprocal dendrodendritic synapses.On the GC, both presynaptic and postsynaptic specializationsare found in large spines. This unusual arrangement gives riseto three different GC output modes: (1) Self-inhibition: asingle M/TC activates a GC spine, which in turn releases GABAback onto the same M/TC (Jahr and Nicoll, 1980, 1982; Isaacsonand Strowbridge, 1998). (2) Local lateral inhibition: MT/Csactivate one or more spines in a local region of a GC. Subthresholdactivity spreads between spines to cause mutual lateral inhibitionbetween M/TCs (Jahr and Nicoll, 1982; Woolf et al., 1991b; Isaacson and Strowbridge, 1998). (3) Global lateral inhibition:Several M/TCs activate a GC strongly enough to elicit an actionpotential (AP). Presumably, this AP propagates through thedendritic tree, causing widespread lateral inhibition (Chenet al., 2000).
Little is known about the role of the AP in GC signaling. Robust self-inhibition can be produced without GC APs (Jahr and Nicoll, 1980, 1982), yet in vivo recordings demonstrate that GCs doindeed spike in response to odorants (Mori and Takagi, 1977; Wellis and Scott, 1990; Luo and Katz, 2001; Margrie and Schaefer,2003; Cang and Isaacson, 2003), and APs can evoke calciumtransients in GCs (Hall and Delaney, 2002). Most experimentsstudying OB dendrodendritic inhibition have investigated self-inhibitionin the presence of TTX (Isaacson and Strowbridge, 1998; Schoppaet al., 1998; Chen et al., 2000; Halabisky et al., 2000;Isaacson, 2001), and none has isolated GC AP-mediated lateralinhibition. The relative predominance of AP-independent (local)lateral inhibition and AP-dependent (possibly global) lateralinhibition will depend on several factors, including the efficacyof dendritic AP propagation, the types of voltage-dependentcalcium channels within spines, and modulatory mechanisms.
Calcium influx into GC dendrites is both an indicator of thespread of neuronal activity and tightly coupled to GC output.Thus, we chose to image AP-evoked GC calcium dynamics at thelevel of individual spines, using two-photon microscopy.

   Materials and Methods

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Preparation, solutions, and instrumentation. In all experiments, we prepared sagittal olfactory bulb brain slices (thickness350 µm) of juvenile Sprague Dawley rats [postnatal day10 (P10)-P16]. The preparation was performed in accordancewith Cold Spring Harbor Laboratory guidelines for animal care.The intracellular solution contained (in mM): 130 K-methylsulfate,10 HEPES, 4 MgCl₂, 4 Na₂ATP, 0.4 NaGTP, 10 Na phosphocreatine,and 2 ascorbate, pH 7.2. For imaging, 100 µM of the calcium-sensitivedye OGB-1 (Molecular Probes, Eugene, OR) was added. The extracellularACSF was bubbled with carbogen and contained [mM]: 127 NaCl,25 NaHCO₃, 1.25 NaH₂PO₄, 25 glucose, 2.5 KCl, 1 MgCl₂, and2 CaCl₂. The junction potential was -5 mV. Pharmacologicalagents used in some experiments were APV, CNQX, bicuculline(all from Tocris Cookson, Bristol, UK), TTX (Sigma, St. Louis,MO), and mibefradil (gift from Hoffman-La Roche, Basel, Switzerland).When applying TTX, we increased current injection to obtainthe same somatic AP waveform as in control conditions. All experiments were performed at room temperature (21°C), unlessstated otherwise.
Neurons were visualized with infrared differential interferencecontrast optics. Two-photon excitation at 810 nm was providedby a Ti: Sapphire solid-state laser system (Mira/Verdi; Coherent,Santa Clara, CA). For a more detailed description of the custom-builttwo-photon microscope, see Mainen et al. (1999). Somatic whole-cell patch-clamp recordings were performed with an Axopatch 200B(Axon Instruments, Foster City, CA). The pipette resistancewas R_P = 5-8M ${Omega}$ , and the series resistance was R_S = 15-40 M ${Omega}$ .APs were elicited by a short current injection in current-clampmode from resting potential, i.e., -70 mV, unless stated otherwise.After a filling time of $~$ 10 min, calcium transients were imagedin line-scan mode at different locations along the apical dendriteof granule cells and within its spines (Fig. 1 A,B). The smallsize of granule cells promoted fast filling, but also requiredquick experimentation because cells tended to deteriorate ratherabruptly after 25-45 min.

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Figure 1. Action potentials produce calcium transients in granule cell dendrites. A, Experimental design. The left panel shows a dendrite of the cell in C, with the line scan position indicated by the gray vertical line. The middle panel shows the line scan across the dendrite (top), the voltage trace of the corresponding action potential (middle; white/black) evoked by current injection (bottom) to the granule cell soma. The right panel shows the fluorescence transient resulting from this line scan. B, ( ${Delta}$ F/F)_AP amplitudes do not decrease with distance from the soma. The top traces represent averaged calcium transients imaged at increasing distance from the soma in the cell shown in C. The bottom graph shows dendritic ( ${Delta}$ F/F)_AP amplitudes versus distance from the soma and their linear fit. C, Scan of the corresponding granule cell at the same scale. Arrows indicate the measurement locations.

For the experiments on synaptic transmission between granulecells and mitral cells, glass electrodes filled with ACSF (R_P ${approx}$ 1-4 M ${Omega}$ ) and connected to an Isoflex stimulator (A.M.P.I., Jerusalem, Israel) were placed near granule cell somata. Stimulation strengthsjust sufficient for AP generation in granule cells were determinedby test experiments in which granule cells were patched inthe whole-cell mode and then extracellularly stimulated.
Data analysis. Imaging and electrophysiological data were recorded and analyzed with custom software based on Matlab (Mathworks,Natick, MA; Pologruto et al., 2003) and Igor (Wavemetrics,Lake Oswego, OR). To measure changes in calcium, fluorescencewas collected while scanning in a line that intersected the region or regions of interest. Fluorescence, F(t), was then averaged over the region or regions of interest. Baseline fluorescence, F₀, was measured for 50 msec before the stimulus, and ${Delta}$ F/F wascalculated as ( ${Delta}$ F/F)(t) = (F(t) - F₀)/F₀. ( ${Delta}$ F/F)_AP correspondsto the fluorescence transient evoked by stimulation with asingle AP.
For the collective representation of cells, data of individualexperiments were normalized to their transient amplitude atthe level of the mitral cell layer (MCL). If there was no datapoint close to the interception of dendrite and MCL, the respectivetransient amplitude was interpolated. Only neurons with atleast three amplitude data points along the apical dendritewere included in the analysis.
To describe voltage dependence of calcium transients, we usedtwo different measures. Data with sufficiently strong voltagedependence and little noise in the individual fluorescencetransient amplitudes were fitted with a Boltzmann function.Because this type of fit is not meaningful if applied to datawith little voltage dependence or high levels of noise, itwas not applicable to the whole population and also not usefulto determine block of voltage dependence. Therefore, we evaluatedvoltage dependence for all measurements in terms of the slopeof a linear fit to the data. In any case, based on our Boltzmannanalysis yielding an average V ${approx}$ -76 mV and k ${approx}$ 10 mV, a linearfit is a fairly good approximation of the data in the rangeof -90 to -60 mV.
To assess statistical significance levels, the nonparametricWilcoxon matched-pairs signed-ranks test was applied for comparingdata sets, and the Spearman correlation coefficient for establishingcorrelations. All data are given ± SD, unless statedotherwise.

   Results

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Whole-cell recordings were made in horizontal slices of theolfactory bulb from small cells ( $~$ 8 µm diameter soma)in the granule cell layer. Because cells were filled with calcium-sensitivefluorescent dye via the pipette, we could identify GCs by thepresence of an apical dendrite ascending into the externalplexiform layer (EPL) studded with large dendritic spines, also called "gemmules," and a brush of shorter basal dendrites, but lack of an axon (Fig. 1C) (Valverde, 1965; Price and Powell, 1970a).
On average, GC input resistance was 0.81 ± 0.35 G ${Omega}$ (mean ± SD; n = 72; Schoppa et al., 1998), the membrane timeconstant was 30 ± 14 msec (n = 15), and the restingmembrane potential was -69.3 ± 5.2 mV (n = 32), similarto previous in vitro and in vivo data (Wellis and Scott, 1990;Schoppa et al., 1998; Margrie and Schaefer, 2003). Brief,depolarizing current pulses (3 msec; 30-60 pA) elicited singlespikes followed by large afterdepolarizations (ADPs) (Fig.1A). Longer current steps produced characteristic late-onsetfiring at low current intensities and a "plateau" pattern athigher intensities, probably reflecting I_A and I_CAN, respectively(Schoppa and Westbrook, 1999; Hall and Delaney, 2002). Wevery rarely observed bursting or rebound APs from hyperpolarizingcurrent steps.
Action potential-evoked dendritic calcium transients
Fluorescence was measured using line scans across dendritesand spines (Fig. 1A). Single spikes evoked detectable fluorescencetransients, ( ${Delta}$ F/F)_AP, in almost all cell locations imaged (367dendrites and 158 spines in 102 cells). Long trains of 20 APsat 50 Hz resulted in plateau calcium levels 3.5 ± 1.6times the amplitude of ( ${Delta}$ F/F)_AP (range, 1.5-6.8; n = 30 in13 cells), indicating that single APs did not saturate the indicator (100 µM OGB-1). Dendritic calcium transients required Na⁺-dependent APs, as they were blocked by bath applicationof TTX (1 µM; n = 8 locations in seven cells; see Materials and Methods). The decay of dendritic calcium transients wasslow ( ${tau}$ = 780 ± 380 msec; n = 145 locations). Althoughthe kinetics became faster at physiological temperature (T= 34-36°C; ${tau}$ = 410 ± 120 msec, n = 15; p < 0.005for paired experiments, n = 10; Wilcoxon signed-ranks testfor all comparisons), these values are still relatively highcompared with transients in pyramidal neurons recorded undersimilar buffering conditions ( ${tau}$ ${approx}$ 400 msec at physiological temperaturevs ${tau}$ ${approx}$ 100 msec: neocortical L5, 100 µM CG-1, Markram etal., 1995; ${tau}$ ${approx}$ 200 msec: CA1, 100 µM OGB-1, Sabatini etal., 2002). Possible mechanisms for such slow kinetics includea large endogenous buffer capacity, a slow calcium extrusionrate, and calcium-induced calcium release.
Action potentials produce robust dendritic calcium transients
We quantified the amplitudes of dendritic calcium transientsalong the apical dendrite of each GC (Fig. 1). In contrastto observations in pyramidal neurons (see Discussion), these( ${Delta}$ F/F)_AP amplitudes did not decrease with distance from thesoma (Fig. 1B). We examined the amplitude of dendritic ( ${Delta}$ F/F)_APat different positions along individual dendrites with respectto the border of the EPL, as demarcated by the mitral celllayer. This analysis revealed that an amplitude plateau wasoften reached at the beginning of the EPL, as depicted in Figure2A. This observation was consistent across the GC population,resulting in a characteristic profile of the relative ( ${Delta}$ F/F)_APamplitude with respect to the EPL shown in Figure 2B (n =98 cells; see Materials and Methods). A systematic gradientin indicator concentration caused by incomplete loading couldproduce apparent amplification of transients with distancefrom the soma, but such a gradient would not be expected toproduce a plateau in ( ${Delta}$ F/F)_AP amplitude. Moreover, ( ${Delta}$ F/F)_APdecay time constants did not decrease with distance (Fig. 2C) as would occur if transients were subject to inhomogeneousbuffering by the indicator (Neher and Augustine, 1992; Helmchenet al., 1996).

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Figure 2. Calcium transients are robust in the external plexiform layer. A, Calcium transient amplitudes attain a plateau in the EPL. The top graph represents dendritic ( ${Delta}$ F/F)_AP amplitude data of the individual cell shown below at the same scale versus relative distance to the MCL. The soma of this cell was located at 120 µm below the MCL. Amplitude data are shown with SD. B, Normalized ( ${Delta}$ F/F)_AP amplitudes averaged over all cells also attain a plateau in the EPL. The graph represents the average amplitudes of all granule cells with at least three dendritic data points (n = 98 cells) binned into 50 µm intervals, again versus their relative distance to the MCL. Before averaging, data from individual cells were normalized to the amplitude at the MCL border. Data are shown with SEM. C, The decay time constant of ( ${Delta}$ F/F)_AP does not depend on distance from the soma. Dendritic data (n = 145) with linear fit (r = 0.11) is shown. Similar results were obtained for spine measurements (r = 0.03; n = 63; data not shown).

Therefore, dendritic calcium transients provide robust and fairlyuniform effects throughout the EPL, where the reciprocal spinesare located.
Spine calcium transients
Transmitter release from granule cells is thought to occur exclusivelyfrom dendritic spines within the EPL (Price and Powell, 1970b;Woolf et al., 1991a). Spines and dendrites could show differentcalcium transient properties caused by differential clearance,buffering, or distribution of calcium channel types. We thereforeimaged calcium transients in spines and compared them withthe parent dendritic shaft using simultaneous line scans throughboth structures (Fig. 3A). Throughout the EPL, transients wereas robust in spines as in dendrites. The average ratio of spineto dendrite ( ${Delta}$ F/F)_AP amplitude was close to unity: 1.08 ±0.49 (Fig. 3B) (n = 152 pairs of spine and adjacent dendrite;p > 0.5). In response to AP trains, spines and dendrites also showed a similar transient amplitude, with the dendriticmagnitude slightly larger (ratio S/D 0.90 ± 0.14; n= 21; p < 0.01). However, the decay of ( ${Delta}$ F/F)_AP was significantlyfaster in spines than in adjacent dendrites (Fig. 3C) ( ${tau}$ = 640 ± 50 msec vs ${tau}$ = 750 ± 50 msec; SEM; n = 52; p< 0.002), indicating that the similarity in ( ${Delta}$ F/F)_AP amplitudesis not simply caused by rapid equilibration of calcium betweenspine and dendrite.

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Figure 3. AP and synaptically mediated calcium transients are observed in spines. A, Spine and dendritic ( ${Delta}$ F/F)_AP transients are similar. The scan shows a large spine/gemmule, located at 111 µm from the cell soma. Below, the averaged filtered transients in dendrite (gray) and spine (black) are shown, as measured in the regions with respective colors indicated below the scan. The horizontal line scan was aligned with the spine. B, Similar ( ${Delta}$ F/F)_AP amplitudes are observed in dendrites and spines. The scatterplot shows transient amplitudes in spines versus transient amplitudes in the adjacent dendrite. The dotted line represents the diagonal x = y, and the straight line a linear fit to the data. The inset shows a histogram of amplitude ratios spine/dendrite. C, Slightly faster ( ${Delta}$ F/F)_AP decay is seen in spines than in dendrites. The scatterplot shows transient decay constants in spines versus transient decay time constants in the adjacent dendrite, with details similar to B. D, Spontaneous synaptic events occur. The synaptic transient shown was measured in the spine from A, with identical scaling. The top trace shows the voltage recording with truncated evoked AP and spontaneous EPSPs. The bottom shows corresponding calcium signals in the spine (black) and adjacent dendrite (gray). Note that the AP evokes a transient both in spine and dendrite, whereas the spontaneous transient is localized to the spine and coincides with a spontaneous EPSP. E, Synaptic and AP-evoked ${Delta}$ F/F amplitudes are similar. The scatterplot shows mean synaptic versus AP-evoked ${Delta}$ F/F amplitudes in each spine where spontaneous synaptic events were observed (n = 12). The open diamond represents the population mean ± SD. F, Synaptic calcium is not observed in the adjacent dendrite. The plot shows mean synaptic ${Delta}$ F/F amplitudes in all spine/dendrite pairs where spontaneous synaptic events were observed (n = 12). Mean values are represented by open diamonds.

We occasionally observed spontaneous synaptic transients ( ${Delta}$ F/F)_syn (Fig. 3D,E)(n = 12 spines, except for two all within the EPL;n = 27 events). Such transients were localized to the spinehead, coincided with an EPSP (Fig. 3D) and did not invadethe parent dendrite (Fig. 3F) [mean ( ${Delta}$ F/F)_syn amplitude spinevs dendrite 41 ± 11 vs 1 ± 3% ${Delta}$ F/F; p < 0.001].Therefore, as in pyramidal cells (Svoboda et al., 1996), thespine neck provides a substantial barrier to diffusion overthe time scale of 100 msec. The average rise time of ( ${Delta}$ F/F)_synevents was considerably longer than that of ( ${Delta}$ F/F)_AP (70 ±37 msec vs 16 ± 6 msec; n = 12; p < 0.005), whereasthe mean ( ${Delta}$ F/F)_syn amplitude in spines was similar to thatof ( ${Delta}$ F/F)_AP in the same spines (Fig. 3E) (41 ± 11 vs34 ± 17% ${Delta}$ F/F; n = 12; p > 0.25). If synaptic andAP-evoked calcium had the same access to the release machinery,this observation would imply a similar efficiency of the twopathways with respect to causing release and thus inhibition(see Discussion).
Voltage dependence of calcium transients
Although AP-evoked calcium transients were highly robust, weobserved a striking susceptibility of transient amplitudesto the membrane holding potential, being attenuated with depolarizationand enhanced with hyperpolarization (Fig. 4A,B, left panels).The average voltage dependence in all dendrites, as describedby the linear slope (see Materials and Methods) was -1.20 ±0.86 (% ${Delta}$ F/F)/mV (n = 75 in 43 neurons) (Fig. 4C) and strongerfor spines than for their adjacent dendrites [-2.07 ±1.71 vs -1.26 ± 1.04 (% ${Delta}$ F/F)/mV; n = 27 in 19 neurons;p < 0.01]. The voltage dependence of ( ${Delta}$ F/F)_AP amplitudeswas not caused by changes in the width or peak amplitude ofthe somatic AP, because both increased slightly with depolarization(n = 5). Furthermore, voltage dependence was not dependenton the distance of the measurement location from the soma (r= -0.12/-0.03 for dendrites/spines; n = 67/27) (Fig. 4D). SpikeADP amplitude was inversely dependent on the membrane potentialin a manner closely paralleling the effect on calcium transients (Fig. 4A, right panel), suggesting a calcium dependence ofthe conductance underlying the ADP.

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Figure 4. Calcium transient amplitudes are regulated by membrane potential. A, Both ( ${Delta}$ F/F)_AP and ADP amplitude are voltage-dependent. The left panel shows representative individual calcium transients at a fixed location ordered at increasingly hyperpolarized pre-pike membrane potentials, the right panel the corresponding APs (truncated) and ADPs. B, Voltage dependence obeys a Boltzmann relationship. ( ${Delta}$ F/F)_AP amplitudes (left panel; from individual experiment also shown in A) and corresponding ADP amplitudes (right panel; calculated as difference between prespike potential and maximum within the shaded interval in A) are shown as a function of the prespike membrane potential. The Boltzmann fits yield V_0.5 = -80.5 mV, k = 8.9 mV for ( ${Delta}$ F/F)_AP and V_0.5 = -80.3 mV, k = 10.2 mV for the ADPs. C, Histograms of all locations. The data are represented as histograms of the slopes of linear fits to the transient amplitudes from dendrites (n = 75; black solid bars) and spines (n = 31; gray open bars). D, Voltage dependence is independent on distance from soma. The slopes of linear fits to voltage dependence are shown versus distance of measurement from the soma. Black solid and gray dashed lines are linear fits to dendrite (filled circle) and spine (open triangle) data, respectively.

The voltage dependence of both ADP and, in locations with sufficiently large voltage dependence, ( ${Delta}$ F/F)_AP, could be fitted with Boltzmannfunctions (Fig. 4B). This fit yielded a mean half-inactivationvoltage V_0.5 = -76.1 ± 7.4 mV and a Boltzmann slopefactor, k = 9.8 ± 5.1 mV for calcium transients (n =25 locations; n = 13 cells), and V_0.5 = -78.1 ± 5.3mV and k = 8.1 ± 1.9 mV for ADPs in the same 13 cells.This voltage dependence is similar to the characteristic profilefor inactivation of low voltage-activated (LVA) or T-type calciumchannels (T-channels; Huguenard, 1996).
Role of low voltage-activated channels in regulation of calcium transients
LVA calcium currents have not been previously described in GCs,but the calcium channel ${alpha}$ subunits that encode T-channels areknown to be expressed richly in these cells (Talley et al.,1999). We tested the effect of two T-channel antagonists. Applicationof Ni²⁺ (100 µM) caused a significant reduction in boththe amplitudes (to 50 ± 16% of control) and the voltagedependence of calcium transients (Fig. 5A,B) [control, -1.68± 0.91; drug, -0.29 ± 0.41 (% ${Delta}$ F/F)/mV; n = 12locations in 6 cells; p < 0.002 for both; dendrites andspines pooled]. Dendrite and spine data are shown separatelyin Figure 5, B and D. Similarly, the more specific, activity-dependentT-channel blocker mibefradil (1-10 µM; Bezprozvanny andTsien, 1995; Lacinova et al., 2000) reduced both ( ${Delta}$ F/F)_AP amplitudes(49 ± 12% of control) and their voltage dependence (Fig. 5C,D) [control, -1.20 ± 1.00; drug, -0.29 ±0.28 (% ${Delta}$ F/F)/mV; n = 14 locations in five cells; p < 0.001for both]. The high concentrations of the T-channel blockersused and the negligible voltage dependence of the remaining50% of the calcium signal imply that this remaining signalwas not carried by LVA calcium channels. Both blockers alsoabolished or reduced the ADP (Fig. 5A,C) without affectingthe rise time of calcium transients (n = 10). Given the slowtime course of the ADP (decay time constant ${tau}$ = 80 ± 50msec; n = 15; V_m = -70 mV), the lack of sensitivity of ( ${Delta}$ F/F)_APrise time to ADP blockade indicates that the ADP reflects aCa²⁺-activated current rather than the T-current itself. Finally,mibefradil had no effect on GC spiking (data not shown): itdid not change the amount of current required to elicit singleAPs (n = 5), or the number of spikes in response to 500 msec depolarizing current steps (n = 3) or oscillatory current injections (n = 5).

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Figure 5. T-type calcium channels underlie voltage dependence of calcium transients. Black traces represent control data and gray traces data with drug applied (100 µM NiCl₂, 1-10 µM mibefradil). A, B, NiCl₂ reduces ( ${Delta}$ F/F)_AP amplitude voltage dependence and blocks the ADP. C, D, Mibefradil also reduces ( ${Delta}$ F/F)_AP amplitude voltage dependence and blocks the ADP. The three panels in A and C show individual experiments. The traces were recorded at prespike potentials of -65 and -85 mV, respectively, and the AP at -70 mV. B and D show the average linear slope of voltage dependence (see Materials and Methods) in dendrites and spines before and after drug application (error bars indicate SEM; NiCl₂: n = 9 dendrites, n = 3 spines; mibefradil: n = 9 dendrites, n = 5 spines).

Time course of calcium transient modulation
To investigate the time course of calcium transient modulationby voltage, we applied a timed 20 mV depolarizing or hyperpolarizingprepulse to inactivate or deinactivate LVA calcium channels (Fig. 6A) (Magee et al., 1995). We varied the duration ofthe prepulse and calculated the ratio of ( ${Delta}$ F/F)_AP amplitudesat depolarized and hyperpolarized potentials, R_D/H (Fig. 6B).After 500 msec, R_D/H was 0.66 ± 0.18 (n = 32) and almostsaturated, corresponding to a time constant of $~$ 290 msec. Thistime course is consistent with reported time constants forT-channel inactivation and deinactivation at these membranepotentials (Huguenard, 1996; Randall and Tsien, 1997; Lacinovaet al., 2000).

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Figure 6. Voltage dependence of calcium transients develops rapidly. In all panels, thick traces mark hyperpolarization to approximately -90 mV, and thin traces depolarization to approximately -50 mV. Before the prepulse, cells were held at approximately -70 mV. A, Depolarizing versus hyperpolarizing 500 msec prepulses lead to a pronounced difference in ( ${Delta}$ F/F)_AP amplitudes. The traces from a representative experiment show the injected current (top, schematic), the recorded somatic voltage (middle), and the respective calcium transients (bottom). B, Voltage dependence evolves with a time constant of $~$ 300 msec. Cumulative data from all experiments. Average data are plotted as ratios of transient amplitudes for depolarization and hyperpolarization, R_D/H, versus duration of the polarization interval (100, 250, 500, and 1000 msec). Data are shown ± SD. The dotted line corresponds to a single exponential fit ( ${tau}$ = 290 msec). C, Close-to-spiking-threshold depolarization results in considerable calcium influx. Dashed traces mark strong depolarization. Again, the polarization interval was 500 msec. Note the characteristic hump in the dashed voltage recording.

Larger amplitude depolarizing pulses to just below AP threshold(mean depolarization, -40.9 ± 6 mV) resulted in substantialcalcium influx ( ${Delta}$ F/F)_-40mV (Fig. 6C). The average ( ${Delta}$ F/F)_-40mVlevel achieved with 500 msec of depolarization was 42.3 ±20.6% ${Delta}$ F/F (n = 23). This activation voltage is consistent withT-type calcium channels (Randall and Tsien, 1997). Indeed,the ( ${Delta}$ F/F)_-40mV amplitude was reduced substantially by 10 µMmibefradil (27 ± 10% of control; n = 9; p < 0.005).These observations also indicate that subthreshold depolarizationcan produce calcium influx through T-channels that may leadto local lateral inhibition (see Discussion).
Role of T-type calcium channels in synaptic release
Do T-type calcium channels participate in AP-mediated transmitterrelease from granule cells? Their involvement seems likely,given our finding that T-channel blockers reduced the ( ${Delta}$ F/F)_AP amplitude in dendrites and spines by 50%. To test this moredirectly, we first sought to examine the effect of depolarizationor hyperpolarization on GC output using paired recordings ofgranule and mitral cells (n >100). However, this approachwas precluded by an extremely low success rate in finding connectedpairs (cf. Isaacson, 2001). We therefore evoked APs in GCsusing extracellular stimulation and recorded in whole-cell mode from mitral cells (Fig. 7A). To prevent triggering ofthe polysynaptic local lateral inhibition pathway (which doesnot involve GC spiking) via stimulation of mitral cell axons,we blocked transmission from mitral cells to GCs with APV andCNQX (50 µM; 10 µM; Chen et al., 2000). Under these conditions, small (0.83 ± 0.51 mV; n = 6), short-latencyIPSPs with a slow decay time constant ( ${tau}$ = 300 ± 200msec; n = 6) could be evoked in some mitral cells. Mibefradil(10 µM) reduced these evoked IPSPs by 48 ± 6%(p < 0.025) (Fig. 7B,C). This decrease is unlikely to becaused by a change in stimulation efficiency or input resistance,because neither GC excitability in whole-cell recordings (seeResults above) nor the amplitude and kinetics of spontaneousIPSPs (n = 3) were affected by mibefradil application. Subsequent application of bicuculline (50 µM) abolished the IPSPin all cases tested (n = 3), demonstrating that the IPSPs weremediated by GABA-A receptors. Mibefradil-sensitive calciumchannels therefore contribute at least half of the effect ofglobal (AP-mediated) lateral inhibition.

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Figure 7. Action potential-mediated synaptic transmission from granule cells to mitral cells is reduced by a T-type calcium channel antagonist. A, Experimental stimulation and recording scheme. Granule cells are stimulated extracellularly, whereas a mitral cell is being recorded from in whole-cell mode. B, Mibefradil reduces synaptic transmission. Traces from an individual experiment show averaged data ( $~$ 20 sweeps each) of the baseline IPSP (thick trace) and 15 min after application of 10 µM mibefradil (thin trace). C, Average reduction of synaptic transmission by mibefradil (n = 6 for control and mibefradil application, n = 3 for bicuculline application). Data are shown with SD.

   Discussion

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Our results indicate that somatically evoked APs cause calciumtransients throughout the GC dendritic tree. These calciumtransients are particularly robust in the output zone of GCsand thus appear well suited to evoke transmitter release frommost or all release sites. Thus, we refer to this GC outputmode as "global lateral inhibition" (Chen et al., 2000). Wefind that AP-evoked calcium transients are subject to voltage-dependentmodulation, apparently because of the contribution of T-typecalcium channels, giving rise to novel mechanisms for regulationof lateral inhibition.
Action potential-evoked calcium transients in dendrites
In contrast to many other cell types studied (e.g., CA1 pyramidalneurons, Spruston et al., 1995; neocortical layer (L) 2/3pyramidal neurons, Svoboda et al., 1999; L2/3 interneurons,Kaiser et al., 2001) AP-evoked GC calcium transients were robustin even the most distal regions of the dendritic tree imagedand in the large spines in the EPL that are the site of dendritictransmitter release. Data from OB MCs (Xiong and Chen, 2002)(but see Margrie et al., 2001), retinal amacrine cells (Euleret al., 2002), and thalamic GABAergic interneurons (Munschet al., 1997), are consistent with the idea that upregulationof calcium influx within output regions may be a general rulefor cell types with dendritic release. The factors that determineGC dendritic calcium transient amplitudes remain to be elucidated,but could involve spatial gradients in calcium channel distributions(Christie et al., 1995) or effects of passive dendritic electricalproperties on AP propagation (Spruston et al., 1995; Vetteret al., 2001).
Voltage-dependent calcium transients mediated by T-channels
Whereas axonal spikes and bouton calcium transients are essentiallyall or none (Mackenzie et al., 1996; Cox et al., 2000; Koesterand Sakmann, 2000), GC dendritic calcium transients were stronglymodulated by membrane potential. Several lines of evidencesupport the idea that T-type calcium channels underlie thismodulation. First, the voltage dependence and its time course were consistent with characteristics of T-channel inactivation (Huguenard, 1996; Lacinova et al., 2000). Second, the R- andT-channel blocker Ni²⁺ and the more selective T-channel antagonistmibefradil (Bezprozvanny and Tsien, 1995; Lacinova et al.,2000) abolished the voltage dependence and partially blockedthe calcium transients. Third, although the T-channel antagonistsused may also block high voltage-activated (HVA) calcium channels,in particular R-type (Bezprozvanny and Tsien, 1995; Jimenezet al., 2000), and inactivation relationships of T- and R-channelsmay be similar (Randall and Tsien, 1997), subthreshold depolarizingpulses, which will not activate R-channels, caused considerablecalcium influx. Finally, GCs express the mRNA transcripts ofall three known subtypes of T-channels at high levels ( ${alpha}$ 1G,H, I; Talley et al., 1999).
The resting potential of GCs (-70 mV) is well suited to allowfor T-channel based modulation of calcium dynamics in bothdirections of polarization. Although we did not observe electrophysiologicalhallmarks of T-channels such as rebound spikes or bursting,the strong A-type potassium conductance in GCs (Schoppa andWestbrook, 1999) may obscure these effects, as described indendritically releasing thalamic GABAergic interneurons (Papeet al., 1994).
The coupling of calcium to transmitter release
Release from axonal boutons is triggered by calcium influx viaseveral types of HVA calcium channels (Fisher and Bourque,2001). In granule reciprocal spines however, calcium entryvia NMDA receptors has also been linked to release (Schoppaet al., 1998; Chen et al., 2000; Halabisky et al., 2000) (but see Isaacson, 2001). Our data have added another potentialpathway for release, calcium entry via LVA channels, whichhave only been known to play a role in graded release from retinal bipolar neurons so far (Pan et al., 2001). Becausethe resolution of our fluorescence measurements does not revealdirectly the calcium signal available to the release machinery,the precise nature of this coexistence of pathways remains to be elucidated. The coupling of diverse calcium sources torelease could be simply attributable to the proximity of allthese sources to the release machinery. It is also conceivablethat release from granule cells is sensitive to lower levelsof calcium, and hence there is an extended spatial domain for calcium entry from which release may be triggered, allowingfor a larger variety of calcium sources to contribute to release(but see Isaacson, 2001). The latter scenario could help toexplain the phenomenon of asynchronous release from granulecells (Isaacson and Strowbridge, 1998; Schoppa et al., 1998).Asynchronous release underlies the slow decay of IPSCs and IPSPs generally observed in self- and lateral inhibition andis consistent with the slow time course of IPSPs evoked byextracellular stimulation of GCs. The relatively slow kineticsof GC calcium transients we observed may also contribute toan extended time window for release.
Implications for local and self-inhibition
Coexisting calcium sources for release are likely to be accessed differentially by APs and synaptic events. Whereas NMDARs wouldbe only available to a spine via direct synaptic input, LVAcalcium channels could be recruited both by APs and by synapticdepolarizations, because they do not require APs to reach activatingvoltages (Magee and Johnston, 1995; Magee et al., 1995). Indeed, subthreshold depolarizing steps were capable of producing robustcalcium transients in GC spines. Apparently, in GCs HVA calciumchannels can also be activated synaptically (i.e., in TTX: Isaacson, 2001). Consequentially the different GC output modes,self-inhibition, local and global lateral inhibition, wouldalso rely on these calcium sources in a differential manner.For example, self-inhibition appears less susceptible to blockadeby Ni²⁺ (Isaacson and Strowbridge, 1998) than global lateralinhibition. Thus, the relative balance of self-inhibition andlateral inhibition could be specifically regulated.
In addition, our observations suggest that there may be a thresholdfor local lateral inhibition. Individual spontaneous synaptictransients do not lead to calcium spread into the dendriteor adjacent spines, and subthreshold depolarizations must exceed $~$ 25 mV threshold from resting potential before calcium channelsare substantially activated. Thus, spatial or temporal summationof neighboring MC input to a local dendrite would be requiredto produce local lateral inhibition. In turn, the existenceof a threshold for local lateral inhibition suggests the involvementof a regenerative mechanism, perhaps involving voltage-dependentcalcium channels. Indeed, both full-blown spikes and spikeletsof potentially dendritic origin have been recorded in vivo(Mori and Takagi, 1978; Wellis and Scott, 1990; Luo and Katz, 2001).
Consequences of voltage-dependent lateral inhibition
Because of the voltage dependence of GC calcium influx, subthreshold depolarizing or hyperpolarizing inputs to GCs will modulatelateral inhibition in the OB. One functional consequence ofthis activity dependence is that lateral inhibition will decreaseduring periods of prolonged MC firing (Urban and Sakmann, 2002). In vivo, a marked adaptation of GC output was observed during extended odor presentation (Cang and Isaacson, 2003). In addition,GCs are the primary target of centrifugal input to the OB,including excitatory input from olfactory cortex (Price andPowell, 1970b; Nakashima et al., 1978) and inhibitory inputfrom the nucleus of the horizontal limb of the diagonal band (Kunze et al., 1992). The dependence of GC output on membranepotential provides a "gate" by which central feedback couldmodulate OB functional connectivity.
Because of the time scale of their activation and inactivation,T-channels are involved in oscillatory activity at slow frequenciesin a variety of neurons (Huguenard, 1996). In the OB, respiratoryrelated oscillatory activity at 4-10 Hz (theta rhythm) is particularlyprominent (Macrides and Chorover, 1972; Chaput, 1986; Margrieand Schaefer, 2003), and in vivo studies have linked the frequencyand phase of GC spiking with the respiratory cycle (Ravelet al., 1987; Young and Wilson, 1999; Margrie and Schaefer,2003; Cang and Isaacson, 2003). Our results suggest that subthresholdtheta frequency input to granule cells might lead to periodicoscillatory modulation of lateral inhibition in the olfactory bulb.

   Footnotes

Received Mar. 25, 2003; revised Jun. 25, 2003; accepted Jul. 3, 2003.
This work was supported by the Deutsche Forschungsgemeinschaft(V.E.), the Burroughs Wellcome Fund (Z.F.M.), the Howard HughesMedical Institute, and the National Institutes of Health (K.S.).We thank P. O'Brien and B. Burbach for technical help, Dr.B. Sabatini and T. Pologruto for programming custom software,Drs. N. Urban, T. Oertner, N. Uchida, A. Kepecs, R. Malinow,and J. Huguenard for comments on previous versions of thismanuscript, and P. Weber and Dr. E. Gutknecht (Hoffmann-LaRoche, Basel, Switzerland) for the gift of mibefradil.
Correspondence should be addressed to Dr. Veronica Egger, ColdSpring Harbor Laboratory, Marks Building, 1 Bungtown Road,Cold Spring Harbor, NY 11724. E-mail egger{at}cshl.edu.
Copyright © 2003 Society for Neuroscience 0270-6474/03/237551-08$15.00/0

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