Modulation of Neuronal Activity by Glial Cells in the Retina

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The Journal of Neuroscience, June 1, 1998, 18(11):4022-4028

Modulation of Neuronal Activity by Glial Cells in the Retina
Eric A. Newman and Kathleen R. Zahs
Department of Physiology, University of Minnesota, Minneapolis, Minnesota 55455

  ABSTRACT

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Glial-neuronal communication was studied by monitoring the effect of intercellular glial Ca²⁺ waves on the electrical activity of neighboring neurons in theeyecup preparation of the rat. Calcium waves in astrocytes andMüller cells were initiated with a mechanical stimulus appliedto the retinal surface. Changes in the light-evoked spike activityof neurons within the ganglion cell layer occurred when, and onlywhen, these Ca²⁺ waves reached the neurons. Inhibition of activity was observedin 25 of 53 neurons (mean decrease in spike frequency, 28 ± 2%).Excitation occurred in another five neurons (mean increase, 27± 5%). Larger amplitude Ca²⁺ waves were associated with greater modulation of neuronal activity.Thapsigargin, which reduced the amplitude of the glial Ca²⁺ increases, also reduced the magnitude of neuronal modulation.Bicuculline and strychnine, inhibitory neurotransmitter antagonists,as well as 6-Nitro-7-sulphamoylbenzo[f]quinoxaline-2,3-dione (NBQX)and D( $-$ )-2-amino-7-phosphonoheptanoic acid (D-AP7), glutamateantagonists, reduced the inhibition of neuronal activity associatedwith glial Ca²⁺ waves, suggesting that inhibition is mediated by inhibitory interneuronsstimulated by glutamate release from glial cells. The resultssuggest that glial cells are capable of modulating the electricalactivity of neurons within the retina and thus, may directly participatein information processing in the CNS.

Key words: calcium waves; glial cells; astrocytes; Müller cells; neurons; ganglion cells; retina; modulation; glial-neuronal interaction

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Intercellular Ca²⁺ waves have been observed in various cell types, including glial cells of the CNS (Finkbeiner, 1993). TheseCa²⁺ waves are transient increases in intracellular Ca²⁺ concentration ([Ca²⁺]_i) that propagate through networks of cells coupled togetherby gap junctions. They are initiated by various types of focalstimuli.

Intercellular Ca²⁺ waves in glial cells have been observed in a number of in vitro preparations (Finkbeiner, 1993). They havebeen recorded in syncytia of cultured astrocytes (Cornell-Bellet al., 1990; Charles et al., 1991; Cornell-Bell and Finkbeiner,1991; Enkvist and McCarthy, 1992) and in glial cells of organotypichippocampal slices (Dani et al., 1992). The waves can be initiatedby mechanical stimuli or application of neurotransmitters (Finkbeiner,1993).

Recently, we demonstrated that intercellular Ca²⁺ waves can also be propagated through networks of glial cells in situ in thefreshly isolated mammalian retina (Newman and Zahs, 1997). Thesewaves are initiated by electrical or mechanical stimuli as wellas focal application of neurotransmitters. The waves travel outconcentrically across the retinal surface and travel synchronouslyin astrocytes and Müller cells, the two principal glial cellsof the mammalian retina.

These glial Ca²⁺ waves could have several possible functions. The waves could serve as a signaling mechanism permitting glialcells to communicate with each other over long distances. Suchcommunication could serve to coordinate glial cell activity. Calciumwaves might also represent a mechanism by which glial cells communicatewith and modulate the activity of neighboring neurons.

Support for such communication between glial cells and neurons has come from work in cell culture. When glial Ca²⁺ waves are initiated in co-cultures of astrocytes and neurons,increases in neuronal [Ca²⁺]_i are seen as Ca²⁺ waves are propagated through the underlying glial cells (Nedergaard,1994; Parpura et al., 1994; Hassinger et al., 1995). A fascinatingrecord showing the electrical excitation of a neuron, initiatedby a glial Ca²⁺ wave, has also been reported (Hassinger et al., 1995). In thesecell culture experiments, glial modulation of neuronal activityis thought to be mediated by the release of glutamate from astrocytes,because glutamate antagonists block the increases in neuronal[Ca²⁺]_i associated with the glial Ca²⁺ waves (Parpura et al., 1994; Hassinger et al., 1995).

The glial-neuronal signaling observed in cell culture is intriguing and suggests an important modulatory role for glial cellsin the CNS. The results must be interpreted with caution, however,because cultured glial cells are known to differ from cells insitu in important respects (Barres et al., 1990; Duffy and MacVicar,1995; Porter and McCarthy, 1995a,b). It remains to be shown thatsimilar glial-neuronal signaling occurs in intact CNS tissue.We have examined this issue in the present work by studying glial-neuronalsignaling in the freshly excised eyecup preparation of the rat.We have investigated whether the propagation of intercellularCa²⁺ waves in retinal glial cells results in the modulation of thefiring rate of neighboring retinal neurons. Our results suggestthat glial cells can indeed modulate neuronal activity.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Eyecup preparation. Male Long-Evans rats (250-400 gm) were deeply anesthetized with sodium pentobarbital administered intraperitoneally,and the eyes were removed. The posterior one-third of the eyeswas everted over a Plexiglas dome and held in place with a stainlesssteel retaining ring. Most of the vitreous humor was removed bysuction, and the eyecups were incubated in Calcium Green-1 AM(70 µg/ml; Molecular Probes, Eugene, OR) and pluronic acid (4.7mg/ml) in Ringer's solution for 35 to 60 min at 22°C. After incubation,eyecups were perfused with HCO₃-buffered Ringer's at 24°C. The Ringer's solution, containing117 mM NaCl, 3 mM KCl, 2 mM CaCl₂, 1 mM MgSO₄, 0.5 mM NaH₂PO₄,15 mM dextrose, and 26 mM NaHCO₃, was equilibrated with 5% CO₂in O₂, pH 7.4. In contrast to earlier experiments (Newman andZahs, 1997), neither ATP nor glutamate was added to the Ringer'ssolution to potentiate Ca²⁺ waves.

Imaging of intracellular Ca²⁺. Incubation of rat eyecups with Calcium Green-1 AM selectively labeled astrocytes and Müllercells but left retinal neurons essentially unlabeled (Fig. 1).Calcium Green-1-labeled cells were viewed with a video-rate NoranOdyssey Confocal scanner (Middleton, WI) and a BX60 Olympus microscopewith a 20×, 0.5 numerical aperture water immersion objective.Calcium Green-1 fluorescence was monitored with 488 nm argon excitationand a 515 nm long-pass barrier filter. Averaged images (averageof 16 frames) were acquired every 2.55 sec, with the laser excitationsource turned on for 1.10 sec during each acquisition cycle. MetaMorphsoftware (Universal Imaging, West Chester, PA) was used to acquire,store, and analyze images.

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Figure 1. Confocal fluorescence image of the retinal surface of the eyecup labeled with Calcium Green-1. Astrocytes (arrows) and Müller cell endfeet (dim, diffuse fluorescence) were labeled. Calcium waves were initiated by advance of a micropipette (left). Extracellular activity of single neurons within the ganglion cell layer was recorded with a metal microelectrode (right). Calcium Green-1 fluorescence was measured within a 15 µm diameter region near the microelectrode tip (open circle). Scale bar, 50 µm.

Calcium waves were monitored to determine whether, in a particular trial, a wave reached the neuron being recorded. CalciumGreen-1 fluorescence from glial cells within a circular region15 µm in diameter, positioned just past the tip of the recordingmicroelectrode (Fig. 1, open circle), was measured off-line. Normalizedfluorescence values, the change in fluorescence divided by thebaseline fluorescence ( $Delta$ F/F), are reported.

Neuronal recording. Extracellular recordings from neurons were made with metal-in-glass microelectrodes plated with gold andplatinum (Dowben and Rose, 1953). The recordings were from cellsomata, as indicated by the recorded action potential waveforms,which often displayed both axonal and somatal components. Recordingswere made in the ganglion cell layer within a few micrometersof the retinal surface.

Stimulation of the retina. Glial Ca²⁺ waves were initiated by a mechanical prodding of single glial cells at the retinal surfacewith the tip of a micropipette. The micropipette was advanced15 µm for 10 msec, under the control of a piezoelectric actuator(Burleigh Instruments, Fishers, NY). The heat-sealed pipette wasfilled with a fluorescent dye to make it visible under confocaloptics.

Neurons within the retina were stimulated by repetitive light flashes of the confocal laser excitation source. During an experimentaltrial, the laser was turned on for 1.10 sec every 2.55 sec. Theexcitation source illuminated a square region ~300 µm on a side.

Analysis. Results are given in the form mean ± SEM (number of samples). Statistical significance between samples was assessedusing the Student's t test (unpaired samples).

  RESULTS

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

The two principal types of macroglial cells within the mammalian retina are astrocytes and Müller cells (Ramon y Cajal, 1995).Astrocytes are confined largely to the nerve fiber layer at theinner retinal boundary, whereas radial Müller cells extend fromthe inner retinal surface to the photoreceptors in the outer retina.When Ca²⁺ waves are initiated at the retinal surface, increases in intracellularCa²⁺ are observed in astrocyte somata and processes as well as inMüller cell endfeet and processes within the ganglion cell andinner plexiform layers (Newman and Zahs, 1997).

In the present study, Ca²⁺ waves in retinal eyecups were initiated by mechanically stimulating astrocyte somata or Müller cellendfeet. The resulting Ca²⁺ waves, traveling through astrocytes and Müller cells, were similarto those observed previously in the isolated retina (Newman andZahs, 1997), although the propagation velocities were somewhatslower: 13.8 ± 0.4 µm/sec (57) compared with 23.1 µm/sec in theisolated retina (where the bathing solution was supplemented withglutamate and ATP). In the eyecup, the largest Ca²⁺ waves attained a diameter of ~400 µm. We studied the effect ofthese Ca²⁺ waves on neuronal activity by recording the spike activity ofsingle neurons in the ganglion cell layer while simultaneouslymonitoring the propagation of glial Ca²⁺ waves at the retinal surface.

Light-evoked neuronal activity

More than 90% of all of the neurons recorded within the ganglion cell layer responded to flashes of light. Cells were classifiedinto three groups according to their responses to the on and offof the light stimulus: ON, ON-OFF, and OFF cells. Peristimulustime histograms of three representative cells are illustratedin Figure 2.

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Figure 2. Peristimulus time histograms of the light-driven activity of an ON (A), an ON-OFF (B), and an OFF (C) neuron, each representative of one of the three response classes observed. Open and closed bars above the histograms indicate periods of light ON and OFF, respectively. Activity was recorded during control periods, before initiation of Ca²⁺ waves.

Modulation of neuronal activity

The light-evoked activity of a neuron was frequently altered when a glial Ca²⁺ wave traveled past the cell. One example of this change in activityis illustrated in Figure 3. The activity of the neuron, an ONcell, is indicated in traces 1 and 2, and the Calcium Green-1fluorescence within glial cells adjacent to the neuron is shownin trace 3. After a 30 sec control period, a Ca²⁺ wave was initiated by a mechanical stimulus (arrow). After adelay of ~3 sec, the Ca²⁺ wave arrived at the neuron. An increase in the firing rate ofthe neuron occurred after a similar delay. A movie illustratingthis experimental trial can be viewed at http://enlil.med.umn.edu/www/phsl/work/caw.htm#neuron.

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Figure 3. Modulation of neuronal activity in an ON neuron. Cell activity is plotted as a spike display in trace 1 (vertical lines represent single action potentials) and as a frequency plot in trace 2 (abscissa represents the running average of spike frequency, i.e., a leaky integrator with a linear decay to 0% at 10 sec; 0 frequency is indicated at left end of the trace). Trace 3, Calcium Green-1 fluorescence in a circular region near the recording microelectrode tip. Trace 4, light stimulus, indicating periods of light ON (open segments) and OFF (closed segments). Arrow indicates initiation of the Ca²⁺ wave. Open and closed bars above trace 1 indicate control and test periods, respectively, during which average spike frequency was measured. Neuron spike frequency and glial cell fluorescence increase concurrently several seconds after initiation of the glial Ca²⁺ wave. Calibration bars: trace 2 (spike frequency), three spikes/sec; trace 3 (Calcium Green-1 fluorescence), 20% $Delta$ F/F; time, 10 sec.

The majority of the neurons we monitored showed changes in their firing rate that were correlated with the arrival of glialCa²⁺ waves. Modulation of the light-evoked responses of neurons, aswell as neuronal spontaneous activity, was observed. The modulationwas either excitatory or inhibitory, depending on the neuron beingrecorded.

An example of excitatory modulation is illustrated in Figure 4A, where records from three sequential trials in an ON neuronare shown. In all three trials, a mechanical stimulus initiateda glial Ca²⁺ wave. The Ca²⁺ wave reached the neuron in trials 1 and 3. In trial 2, the wavedied out before reaching the cell. As shown in Figure 4A, thefiring rate of the neuron increased in those trials when the Ca²⁺ wave reached the cell but remained unchanged when the wave failedto reach the cell.

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Figure 4. Excitatory and inhibitory modulation of neuronal activity. A frequency plot of cell activity (top trace) and glial cell Calcium Green-1 fluorescence (bottom trace) are shown for each trial. A, Excitatory modulation in an ON neuron. Spike frequency increases in those trials (1 and 3) in which [Ca²⁺]_i in neighboring glial cells also increases. B, Inhibitory modulation in an ON-OFF neuron. Spike frequency decreases when glial [Ca²⁺]_i increases. The peristimulus time histograms of cells in A and B are shown in Figure 2, A and B, respectively. Calibration bars are the same as in Figure 3.

An example of inhibitory modulation in an ON-OFF neuron is illustrated in Figure 4B. A decrease in the firing rate of theneuron occurred when the glial Ca²⁺ wave reached the cell (trials 1 and 3). When a Ca²⁺ wave was initiated but failed to reach the cell (trial 2), thefiring rate of the neuron remained unaltered.

Although changes in neuronal firing rate were associated with increases in glial Ca²⁺, the onset and decline of neuronal modulation did not necessarilyfollow the time course of changes in glial Ca²⁺ precisely. The neuronal firing rate sometimes recovered towardcontrol levels even as glial Ca²⁺ levels remained elevated (e.g., Fig. 3).

Magnitude of neuronal modulation

Changes in the firing rate of neurons were quantified by comparing the average frequency of spike activity in a control period,before initiation of a Ca²⁺ wave, to activity in a test period during propagation of thewave. The control period spanned the eight on-off light cyclesimmediately preceding initiation of the Ca²⁺ wave (Fig. 3, open bar above trace 1). The test period consistedof the two light cycles centered at the peak of the Ca²⁺ wave (Fig. 3, closed bar). For trials in which the Ca²⁺ wave did not reach the neuron being monitored, the test periodwas determined by estimating when the wave would have arrivedif it had propagated past the neuron (based on its propagationvelocity). Modulation of the neuronal firing rate was expressedas the percentage change in average spike frequency:

The relation between the change in neuronal firing rate and Ca²⁺ levels in adjacent glial cells was analyzed for a total of 53neurons. For each neuron tested, 9-14 trials were conducted. Insome of these trials, the glial Ca²⁺ wave propagated past the neuron (defined as a $Delta$ F/F fluorescencechange of >22% in the glial cells adjacent to the neuron). Inother trials, a Ca²⁺ wave was initiated but failed to reach the neuron ( $Delta$ F/F < 1%).For each neuron, the average value of neuronal modulation wascalculated for those trials in which the Ca²⁺ wave reached the cell and for those trials in which the wavefailed to reach the cell.

In 30 of the 53 neurons analyzed, there was a significant difference in the modulation of spike activity when a Ca²⁺ wave reached the cell, compared with the modulation observedwhen the Ca²⁺ wave did not reach the cell (Table 1). Twenty-five of the 53cells showed a significant decrease in firing rate associatedwith the arrival of a Ca²⁺ wave. Modulation averaged $-$ 28 ± 2% (114 trials) in these cells.Another five cells showed a significant increase in firing rateassociated with a Ca²⁺ wave. Modulation averaged 28 ± 5% (27 trials) in these neurons.There was no modulation of neuronal activity when a Ca²⁺ wave failed to reach a neuron. In these trials, modulation equaled+1 ± 2% (125 trials) for the 30 cells with Ca²⁺ wave-associated modulation and $-$ 3 ± 1% (235 trials) for all 53neurons analyzed.


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Table 1. Modulation of neuronal activity

Examples of inhibition of spike activity were seen in all three classes of neurons, ON, ON-OFF, and OFF cells. Interestingly,enhancement of spike activity was seen only in ON neurons (Table1). In trials when significant modulation of neuronal activitywas observed, the distance between the neurons and the initiationsite of the Ca²⁺ wave averaged 60 ± 1 µm (74). The distance exceeded 75 µm ineight trials.

Relation between Ca²⁺ increases and neuronal modulation

The results summarized above demonstrate that a change in neuronal firing rate is associated with the arrival of a glial Ca²⁺ wave at that neuron. In addition, the magnitude of the changein neuronal activity was correlated with the amplitude of theCa²⁺ increase. This relation was analyzed for all cells displayingsignificant inhibitory modulation (Fig. 5A). In trials in whichthe amplitude of the glial [Ca²⁺]_i increase was 0, i.e., when the wave failed to reach the neuron,neuronal modulation was near 0. As the amplitude of the [Ca²⁺]_i increase grew larger, the magnitude of inhibitory modulationalso increased (greater negative modulation).

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Figure 5. Correlation between neuronal modulation and Ca²⁺ increases. A, Relation between the magnitude of inhibition of neuronal activity and the amplitude of the Ca²⁺ wave. Points represent single trials from all cells showing significant inhibitory modulation. Points at the left of the plot ( $Delta$ F/F = 0) represent trials in which the Ca²⁺ wave failed to reach the neuron. Least-squares fit, R² = 0.42. B, Relation between the time to the peak of neuron modulation and the time to the peak of the Ca²⁺ wave. Trials in which the inhibition of activity was 25% or greater are included. The discrete Ca²⁺ wave times reflect the 2.55 sec acquisition period of fluorescence images. Least-squares fit, slope = 0.97, intercept = 3.6 sec, R² = 0.30.

The timing of the modulation of neuronal activity was correlated with the timing of the Ca²⁺ wave as well. When the time to the peak of inhibitory modulationwas plotted as a function of the time to the peak of the Ca²⁺ wave, a clear relation was evident (Fig. 5B). Such a relationwould not exist if the mechanical stimulus used to initiate theCa²⁺ wave was directly modulating the activity of the neurons.

Thapsigargin and neuronal modulation

If increases in glial [Ca²⁺]_i result in the modulation of neuronal firing, then pharmacological manipulation of the Ca²⁺ increase should alter the modulation. This was tested by applicationof thapsigargin, a compound that depletes intracellular Ca²⁺ stores (Thastrup et al., 1990) and substantially reduces themagnitude of glial Ca²⁺ waves (Newman and Zahs, 1997). Experiments were conducted onneurons that displayed prominent inhibitory modulation associatedwith increases in glial [Ca²⁺]_i. Under control conditions, the average inhibitory modulationobserved in these neurons equaled $-$ 23 ± 3% (16). Modulation wasreduced to $-$ 12 ± 3% (22) after 30 min exposure to 3.0 µM thapsigargin(p < 0.02) (Fig. 6). In the same trials, the increase in [Ca²⁺]_i measured in the glial cells was reduced from 28 ± 4% ( $Delta$ F/F)to 4 ± 1% by thapsigargin. In all trials, Ca²⁺ waves were initiated sufficiently close to the neuron being monitored,so that under control conditions the waves would have reachedthe neuron (48 ± 1 and 44 ± 1 µm from the neurons in control andtest trials, respectively).

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Figure 6. Effect of thapsigargin on the modulation of neuronal activity. Thapsigargin (3.0 µM) reduces the glial Ca²⁺ increase and the inhibition of activity in an OFF neuron. Calibration bars for trials in Figures 6 and 7: spike frequency, two spikes/sec; Calcium Green-1 fluorescence, 20% $Delta$ F/F; time, 10 sec. A frequency plot of neuronal activity and Calcium Green-1 fluorescence are shown in each trial.

Transmitter antagonists and neuronal modulation

If glial cells cause the observed modulation of neuronal activity, it is possible that the modulation is mediated by the releaseof neurotransmitters from the glial cells. This appears to bethe case in cell culture where Ca²⁺-dependent release of glutamate from glial cells has been demonstrated(Parpura et al., 1994, 1995) and where neuronal [Ca²⁺]_i increases associated with glial Ca²⁺ waves are blocked by glutamate antagonists (Parpura et al., 1994;Hassinger et al., 1995). We performed a number of pharmacologicalexperiments to investigate whether glutamate or other neurotransmitterswere involved in the modulation of neuronal activity associatedwith glial Ca²⁺ waves. In these studies, only trials in which the Ca²⁺ wave reached the neuron being monitored were analyzed. Experimentswere restricted to the characterization of inhibitory modulation,because neurons showing excitatory modulation were rarely encountered.

Antagonists to the inhibitory neurotransmitters GABA and glycine were both effective in reducing the inhibition of spike activityassociated with glial Ca²⁺ waves (Table 2; Fig. 7A). The GABA_A antagonist bicuculline (5µM) and the glycine antagonist strychnine (1 µM) each reducedinhibitory modulation by more than half, whereas both antagonistsapplied together completely abolished the inhibitory modulation.The effects of both bicuculline and strychnine were largely reversible(Table 2). Neither antagonist reduced the amplitude of the Ca²⁺ waves.


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Table 2. Effect of neurotransmitter antagonists on the inhibitory modulation of neuronal activity

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Figure 7. Effect of neurotransmitter antagonists on neuronal modulation. A, Bicuculline (5 µM) and strychnine (1 µM), applied together, abolish the inhibition of activity in an ON-OFF neuron without attenuating the glial Ca²⁺ increase. B, NBQX (10 µM) and D-AP7 (200 µM) together reduce the inhibition of activity in an ON-OFF neuron without reducing the glial Ca²⁺ increase. As illustrated, light responses of neurons often changed during drug application and recovery.

Glutamate antagonists were also effective in reducing the inhibition of spike activity associated with glial Ca²⁺ waves (Table 2; Fig. 7B). The AMPA antagonist NBQX (10 µM) andthe NMDA antagonist D-AP7 (200 µM) both reduced the magnitudeof inhibitory modulation by one-half or more, and the two antagonistsapplied together nearly abolished the inhibition of spike activity.The effects of the antagonists were partially reversible, andneither antagonist reduced the amplitude of the Ca²⁺ waves.

  DISCUSSION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Glial modulation of neuronal activity

The results presented in this study suggest that the propagation of intercellular Ca²⁺ waves through glial cells in the retina results in the modulationof the firing rate of retinal neurons. Modulation of neuronalactivity was not dependent on the initiation of a glial Ca²⁺ wave, per se, but rather on whether the Ca²⁺ wave reached the neuron. In addition, the magnitude of the modulationof neuronal activity was correlated with the amplitude of theCa²⁺ increase in the glial cells adjacent to the neuron. The timingbetween the modulation of neuronal activity and the glial Ca²⁺ increase was similarly related. Finally, attenuation of glialCa²⁺ increases by thapsigargin resulted in a significant decreasein the magnitude of neuronal modulation. All of these findingssupport the hypothesis that increases in glial [Ca²⁺]_i, or some other response associated with the propagation ofCa²⁺ waves through glial cells, results in the modulation of neuronalfiring.

Alternative explanations of neuronal modulation

It is conceivable that a mechanism other than direct glial-neuronal communication was responsible for the observed modulation.The mechanical stimulus used to initiate glial Ca²⁺ waves could stimulate, in theory, the neurons being monitoredand alter their firing rate. This is highly unlikely, however.Identical mechanical stimuli applied to the same retinal locationhad different effects on neuronal firing, depending on whetherthe stimulated Ca²⁺ wave reached the cell. In addition, direct mechanical stimulationof a neuron would have a latency of milliseconds rather than theseveral seconds observed.

It is possible that neuronal modulation was mediated by a signal propagated within a network of neurons. The mechanical stimulusused to initiate glial Ca²⁺ waves might also initiate intercellular Ca²⁺ waves within neurons, for instance. Such Ca²⁺ waves, propagated through ganglion cells and amacrine cells,have been observed in the neonatal ferret retina (Wong et al.,1995; Feller et al., 1996). This mechanism seems unlikely, however.First, it is not known whether these waves can be initiated mechanically;they occur spontaneously in the ferret retina (Wong et al., 1995).Furthermore, the mechanical stimulus used to initiate glial Ca²⁺ waves in our study was small in amplitude (15 µm) and was directedat individual glial cells. The stimulus would presumably be lesseffective in initiating Ca²⁺ waves in neurons lying beneath the surface. In addition, neuronalCa²⁺ waves, if they were initiated, would have to mimic the glialCa²⁺ waves in many respects, including their extent of travel, magnitude,and timing, to account for the observed results. The chance ofthis occurring in many of the trials is highly unlikely.

Identity of neurons that are modulated

The neurons recorded in this study lay just beneath the surface of the retina in the ganglion cell layer and thus were presumablyganglion cells. Their responses to light resembled those reportedpreviously for ganglion cells in the rat (Brown and Rojas, 1965).It is possible, however, that some of these cells were displacedamacrine cells, which are prevalent in the ganglion cell layerof the rat (Perry and Walker, 1980) and generate spike responsessimilar to those of ganglion cells (Bloomfield, 1996).

Mechanism of modulation of neuronal activity

The following model of the inhibition of neuronal activity by glial cells is suggested by our experiments. The arrival ofa Ca²⁺ wave in a glial cell leads to the release of glutamate from thecell and to the excitation of inhibitory interneurons. The interneurons,in turn, release GABA and glycine onto ganglion cells, leadingto a decrease in their firing rate. Amacrine cells, which arestimulated by glutamate and release both GABA and glycine (Miller,1994), are likely to be the interneurons that mediate the inhibitionof ganglion cell activity.

This model is supported by our transmitter antagonist experiments as well as by the known pharmacology of retinal neurons.GABA and glycine antagonists each reduced the inhibition of neuronalactivity, as they would if they interrupted the inhibitory linkbetween amacrine cells and ganglion cells. Glutamate antagonistsalso reduced inhibition of ganglion cell activity, as they shouldif the major effect of glutamate release from glial cells is toexcite amacrine cells rather than ganglion cells. (If glutamatereleased by glia primarily excited ganglion cells, then glutamateantagonists would increase rather than decrease the inhibitionof ganglion cell activity.) It has been shown previously thatamacrine cells possess both AMPA and NMDA receptors and that ganglioncells possess both GABA_A and glycine receptors (Miller, 1994).

In cell culture, the release of glutamate from glial cells is thought to be mediated by an increase in [Ca²⁺]_i (Parpura et al., 1994, 1995). Such a Ca²⁺-dependent release of glutamate may occur in the retina as well.Not only is modulation of neuronal activity associated with [Ca²⁺]_i increases within glial cells in our experiments, but neuronalmodulation is reduced when these Ca²⁺ increases are diminished by thapsigargin. [The thapsigargin-induceddecrease in neuronal modulation (48%) was less than the observeddecrease in Ca²⁺ wave magnitude (86%), suggesting that a Ca²⁺-dependent mechanism may not fully account for the results.]

The excitation of neuronal activity observed in a few of the ON cells in our experiments could arise in several ways. Theseneurons may be ganglion cells which receive an unusually largeglutamatergic input from glial cells. Alternately, the neuronsmay be amacrine cells, which by our model receive excitatory glutamatergicinput from glial cells.

An important feature of our model that must be explained is why glutamate released from glial cells primarily stimulates amacrinecells rather than ganglion cells. Glutamate may be released preferentiallyfrom those regions of astrocytes or Müller cells that directlycontact amacrine cells, but a morphological correlate to accountfor this specialization is not known.

Glial Ca²⁺ waves in the retina travel through both astrocytes and Müller cells (Newman and Zahs, 1997). It remains to be determinedwhich of these two types of glial cells (or both) mediated themodulation of neuronal firing.

Glial modulation of neuronal activity in vivo

Our work indicates that glial cells, when stimulated mechanically, modulate the firing rate of neurons in the retina. Butdo glial cells modulate neuronal activity in vivo? This remainsan open question, because it is not known whether glial Ca²⁺ waves, or other Ca²⁺ signals, are generated in vivo. Glial Ca²⁺ increases are stimulated by neuronal activity in a number ofin situ preparations, however. In organotypic hippocampal slices,electrical stimulation of neuronal fiber tracts results in theinitiation of intercellular Ca²⁺ waves in astrocytes (Dani et al., 1992). In acutely isolatedhippocampal slices, electrical stimulation (Porter and McCarthy,1996), as well as the addition of glutamatergic (Porter and McCarthy,1995b) and purinergic (Porter and McCarthy, 1995a) agonists, leadsto increases in astrocytic [Ca²⁺]_i. Finally, in preliminary experiments on the eyecup preparationin our own laboratory, light flashes trigger transient Ca²⁺ increases within Müller cells. These increases are as largeas those observed during propagated Ca²⁺ waves (E. Newman, unpublished observations).

Significance of glial modulation of neuronal activity

There is growing evidence that glial cells can influence neuronal activity in a number of ways. Glial cells control neuronalexcitability by regulating K⁺ levels (Newman, 1995) and pH (Chesler, 1990) in the extracellularspace. Glial cells regulate synaptic efficacy by their activeuptake of neurotransmitters (Martin, 1995) and may promote thedevelopment of functional synaptic connections between neurons(Pfrieger and Barres, 1997).

Our work provides evidence for an additional mechanism of glial control of neuronal excitability. As the studies cited aboveindicate, neuronal activity may stimulate Ca²⁺ increases within glial cells, leading to the glial release ofglutamate. The resulting neuronal-glial-neuronal feedback loopcould provide either a positive or negative input onto neuronsand serve to reinforce or dampen neuronal activity, dependingon the prominence of inhibitory interneurons in the feedback circuit.Our results, along with those of others, provide evidence thatglial cells modulate neuronal activity and, as such, may directlyparticipate in information processing in the brain.

  FOOTNOTES

Received Jan. 12, 1998; revised March 12, 1998; accepted March 13, 1998.

This work was supported by National Institutes of Health Grants EY04077 and EY10383. We thank P. Ceelen for technical assistance,J. Gottesman for suggestions concerning data analysis, and D.A. Burkhardt and J. I. Gepner for helpful comments on this manuscript.
Correspondence should be addressed to Eric A. Newman, Department of Physiology, 6-255 Millard Hall, 435 Delaware Street SE,Minneapolis, MN 55455.

  REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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