Glial Cell Inhibition of Neurons by Release of ATP

QUICK SEARCH:

[advanced]

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

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in ISI Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via ISI Web of Science (108)

Citing Articles via Google Scholar

Google Scholar

Articles by Newman, E. A.

Search for Related Content

PubMed

PubMed Citation

Articles by Newman, E. A.

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

Previous Article  |  Next Article

The Journal of Neuroscience, March 1, 2003, 23(5):1659

Glial Cell Inhibition of Neurons by Release of ATP
Eric A. Newman
Department of Neuroscience, University of Minnesota, Minneapolis, Minnesota 55455

  ABSTRACT

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

ATP is released by neurons and functions as a neurotransmitter and modulator in the CNS. Here I show that ATP released fromglial cells can also serve as a potent neuromodulator, inhibitingneurons in the retina of the rat. Activation of glial cells byfocal ejection of ATP, ATP $gamma$ S, dopamine, thrombin, or lysophosphatidicacid or by mechanical stimulation evoked hyperpolarizing responsesand outward currents in a subset of retinal ganglion cells byincreasing a Ba²⁺-sensitive K⁺ conductance in the neurons. This glia-evoked inhibition reducedthe firing rate of those neurons that displayed spontaneous spikeactivity. The inhibition was abolished by the A₁ adenosine receptorantagonist DPCPX (8-cyclopentyl-1,3-dipropylxanthine) (10 nM)and was reduced by the ecto-ATPase inhibitor ARL-67156 (6-N,N-diethyl-D- $beta$ , $gamma$ -dibromomethyleneATP)(50 µM) and by the ectonucleotidase inhibitor AOPCP [adenosine-5'-O-( $alpha$ , $beta$ -methylene)-diphosphonate](250 µM). Selective activation of retinal glial cells demonstratedthat Müller cells, but not astrocytes, mediate the inhibition.ATP release from Müller cells into the inner plexiform layerof the retina was shown using the luciferin-luciferase chemiluminescenceassay. These findings demonstrate that activated glial cells caninhibit neurons in the retina by the release of ATP, which isconverted to adenosine by ectoenzymes and subsequently activatesneuronal adenosine receptors. The results lend support to thehypothesis that glial cells play an active role in informationprocessing in theCNS.

Key words: astrocyte; Müller cell; glial cell; ganglion cell; retina; ATP; adenosine; modulation; inhibition

  Introduction

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Glial cells have traditionally been viewed as passive elements in the CNS, providing structural and metabolic support to neuronsbut playing little role in information processing. Recent studieshave demonstrated, however, that glial cells may directly modulateneuronal activity by releasing neuroactive substances. In bothglial-neuronal cocultures (Hassinger et al., 1995; Araque et al.,1998a,b) and in intact tissue preparations (Pasti et al., 1997;Newman and Zahs, 1998; Castonguay and Robitaille, 2001), activatedglial cells have been shown to depolarize neurons and to modulatetransmitter release from presynaptic terminals. In some of thesesystems, glial modulation of neuronal activity is believed tobe mediated by the release of glutamate from glial cells (Araqueet al., 2001; Haydon, 2001; Vesce et al., 2001). It has been suggested,but not yet demonstrated, that glial cells may also modulate neuronalactivity by releasing ATP (Cotrina et al., 2000; Newman, 2001b).

ATP, when released from neurons, functions as a neurotransmitter and neuromodulator. ATP is coreleased with classical neurotransmittersat neuronal synapses, where it activates purinergic receptors(Zimmermann, 1994). ATP released at synapses is also metabolizedextracellularly to adenosine, which is a potent inhibitory neuromodulator,increasing postsynaptic K⁺ conductance and decreasing presynaptic Ca²⁺ conductance (Trussell and Jackson, 1985; Gerber et al., 1989;Greene and Haas, 1991; Zimmermann, 1994; Cunha, 2001).

Neurons have traditionally been considered to be the sole source of neuromodulatory ATP and adenosine in the CNS. Recently,however, glial cells have also been shown to release ATP (Cotrinaet al., 1998; Wang et al., 2000; Newman, 2001b), raising the possibilitythat glial cells might modulate neuronal activity by activatingpurinergicreceptors.

We have demonstrated previously that activated glial cells can either excite or inhibit the light-evoked spike activity ofneurons in the mammalian retina (Newman and Zahs, 1998). HereI show that activation of glial cells in the retina leads to therelease of ATP from glial cells, the activation of neuronal adenosinereceptors, and the generation of an inhibitory response in retinalneurons. The results demonstrate that, in addition to the glutamate-releasemechanism described previously, glial cells can actively modulateneuronal activity by releasingATP.

  Materials and Methods

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Recording procedures. Recordings were made from whole-mount retinas of male Long-Evans rats (250-400 gm). Retinas were enzymaticallytreated with collagenase-dispase and DNase and the vitreous wasremoved, as described previously (Newman and Zahs, 1998). Retinaswere superfused at 2-3 ml/min in HEPES-buffered Ringer's solution.Except when otherwise noted, experiments were conducted at 24°C.The animals used in this study were treated in accordance withthe guidelines of the Institutional Animal Care and Use Committeeof the University of Minnesota (Minneapolis,MN).

Whole-cell recordings were made from neuronal somata in the ganglion cell layer of the retina, viewed with infrared differentialinterference contrast (IR-DIC) optics (BX60 microscope, 40 × 0.8numerical aperture objective; Olympus, Tokyo, Japan). Patch pipettes(see Fig. 1a) were lowered into the ganglion cell layer, and pipettesolution was expelled to blow away glial cell processes surroundinga cell soma. Suction was then applied to obtain a high-resistanceseal. Whole-cell current-clamp and voltage-clamp recordings weremade with a MultiClamp 700A amplifier (Axon Instruments, UnionCity, CA). Voltage-clamp holding potentials were set to the cellresting membrane potential. Cell voltage was corrected for thepipette junction potential (JPCalc-pClamp software; Axon Instruments),which equaled 10mV.

Neuronal morphology was characterized by filling cells with Lucifer yellow CH contained in the patch pipette. After recordingfrom a neuron, the Lucifer yellow-filled cell was viewed withconfocal microscopy using 458 nm excitation and a 500 nm long-passbarrierfilter.

The depth of the deepest dendrites of a neuron was determined from confocal fluorescence and IR-DIC observations made on thelive retina immediately after recording from the neuron. The depthsof the inner surface of the retina and the inner and outer bordersof the inner plexiform layer (IPL) were determined from IR-DICobservations. [The inner and outer borders of the IPL were distinguishedusing the adjacent somata of the ganglion cell and inner nuclearlayers as landmarks.] The depth of the deepest (outermost) dendritesof the neuron was determined from confocal observations of theLucifer yellow-filled cell. The location of the deepest dendriteswas then expressed as a percentage of the total depth of theIPL.

Glial cells were activated by ejecting agonists mixed in Ringer's solution from a pipette (1-2 µm tip diameter; 17 psi) (seeFig. 1b) onto the inner surface of the retina. The agonist concentrationsspecified are the concentrations within the pipette. Concentrationsat the retinal surface after ejection were lower because of dilution.Astrocyte somata were also stimulated mechanically, with the tipof a patch pipette moved sinusoidally at 5 Hz and 15-20 µm peak-to-peakamplitude.

Calcium imaging. Retinas were incubated in the Ca²⁺-indicator dye Fluo-4 AM (21 µg/ml) and pluronic acid (2.6 mg/ml) for 25min at room temperature, as described previously (Newman, 2001b).Dye incubation filled astrocytes and Müller cells but did notfill retinal neurons. Indicator dye fluorescence was monitoredwith 488 nm excitation, a 500 nm long-pass barrier filter, andconfocal microscopy (Odyssey scanner; Noran, Middleton, WI). GlialCa²⁺ changes and neuronal responses were recordedsimultaneously.

ATP imaging. ATP release from glial cells was detected using the luciferin-luciferase chemiluminescence assay, as describedpreviously (Newman, 2001b). When imaging ATP release from theretinal surface, retinas were bathed in Ringer's solution containingluciferin and luciferase. Glial cells at the retinal surface werestimulated mechanically, and the resulting chemiluminescence signalwas measured at thesurface.

When imaging ATP release within the inner plexiform layer (see Fig. 1c), a small volume of Ringer's solution containing luciferinand luciferase was pressure-ejected from a pipette into this retinallayer. The luciferin-luciferase solution was ejected into theretina 5 sec before mechanical stimulation of glial cells at theretinal surface. The ATP chemiluminescence signal detected afterglial stimulation always occurred near the luciferin-luciferaseejection site within the inner plexiformlayer.

For both experiments, the luciferin-luciferase solution contained 70 µl of luciferase stock solution (L-1759; Sigma, St. Louis,MO; 10 mg/ml in 0.5 M Tris buffer, pH 7.6) and 70 µl of luciferinstock solution (L-6882; Sigma; 11.1 mg/ml in H₂O) per milliliterof HEPES Ringer's solution. ATP chemiluminescence was detectedwith an intensified, cooled CCD camera (I-PentaMAX; Roper Scientific,Trenton, NJ) using an integration time of 1 sec and 2 × 2binning.

Solutions. The HEPES-buffered Ringer's solution contained (in mM): 135.5 NaCl, 3.0 KCl, 2.0 CaCl₂, 1.0 MgSO₄, 0.5 NaH₂PO₄,15.0 D-glucose, and 10 HEPES, pH 7.44, equilibrated with 100%O₂. The intracellular pipette solution contained (in mM): 5.0Na-methanesulfonate, 128.0 K-methanesulfonate, 2.0 MgCl₂, 5.0K-EGTA, 1.0 glutathione, 2.0 MgATP, 0.2 NaGTP, and 5.0 HEPES,pH 7.4. In some experiments, 0.005% Lucifer yellow CH was addedto the pipette solution to characterize neuronalmorphology.

ATP $gamma$ S was purified by HPLC using an AG MP-1 column and a gradient of trifluoroacetic acid. Reagents were purchased from Sigma,except for 2,3-dihydroxy-6-nitro-7-sulfonyl-benzo[f]quinoxaline(NBQX), DL-AP-7, bicuculline, saclofen, scopolamine, and 8-cyclopentyl-1,3-dipropylxanthine(DPCPX), which were purchased from Tocris (Ellisville,MO).

Statistics. Numerical values are given as mean ± SEM. Statistical significance was determined by the Student's t test (pairedsamples).

  Results

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Glial cell activation inhibits neurons

Glial cell modulation of neurons was studied in whole mounts of the rat retina. Astrocytes and Müller cells, the two macroglialcells of the retina (Fig. 1) (Newman, 2001a), were stimulatedby pressure-ejecting agonists onto the inner retinal surface.Glial cell responses to the ejections were monitored by measuringchanges in intracellular glial Ca²⁺ with a Ca²⁺ indicator dye and confocal microscopy. Responses of neurons toglial cell stimulation were monitored in whole-cell voltage- andcurrent-clamp recordings.

View larger version (35K):
[in this window]
[in a new window]
Figure 1. Recording configuration and cells of the inner retina. Shown are the two macroglial cells of the mammalian retina, astrocytes (restricted to the inner border of the retina), and radial Müller cells (extended throughout the depth of the retina). Also shown is the whole-cell recording pipette (a), the agonist ejection pipette (b), the level at which ATP release was monitored (c), the inner nuclear layer (INL), and the IPL. Triangles represent synapses.

Ejection of agonists onto the retinal surface often evoked Ca²⁺ increases in astrocytes and Müller cells. Glial cells displayingsuch Ca²⁺ increases are referred to as being activated. The physiologicalconsequences of activating glial cells are not completely understood,although glial release of glutamate (Araque et al., 2001; Haydon,2001; Vesce et al., 2001) and ATP (Cotrina et al., 1998; Wanget al., 2000; Newman, 2001b) is associated with glial activation.Activation of retinal glial cells does not necessarily resultin changes in glial cell membrane potential or membrane conductance(Newman and Zahs, 1997).

Ejection of a number of agonists, including ATP (100 µM), ATP $gamma$ S (a nonhydrolyzable ATP analog; 100 µM), dopamine (1 or 2 mM),thrombin (100 U/ml), and lysophosphatidic acid (LPA) (500 µM),as well as mechanical stimulation of astrocyte somata, evokedCa²⁺ increases in both astrocytes and Müller cells, as reported previously(Biedermann et al., 1995; Puro and Stuenkel, 1995; Manning andSontheimer, 1997; Newman and Zahs, 1997; Newman, 2001b). Thesestimuli also evoked hyperpolarizing responses and the generationof outward currents in a subset of neurons (Fig. 2A-C).

View larger version (30K):
[in this window]
[in a new window]
Figure 2. Inhibitory neuronal responses are evoked by glial cell stimulation. A, Glial cell activation by ATP $gamma$ S ejection elicits a Ca²⁺ increase in glial cells and evokes a hyperpolarization and the generation of an outward current in a neuron. The voltage and current traces were recorded in sequential trials from the same neuron. Resting membrane potential and holding potential are $-$ 72 mV. B, Activation of glial cells by ejection of 1 mM dopamine and 500 µM LPA and by mechanical (mech) stimulation all evoke Ca²⁺ increases in glial cells and the generation of an outward current in neurons. Records are from three different neurons. Holding potential, $-$ 61, $-$ 74, and $-$ 71 mV, respectively. C, Activation of glial cells by agonist ejection (100 µM ATP; 2 sec duration) and mechanical (Mech) stimulation (3 sec duration) both elicit hyperpolarization in a neuron. For each stimulus, the time course of the glial Ca²⁺ response and the neuronal hyperpolarization closely match each other. The two sets of records were recorded in consecutive trials from the same neuron. Resting membrane potential, $-$ 72 mV. D, Relationship between outward neuronal currents and glial Ca²⁺ increases recorded in consecutive trials on a single neuron. The relationship is fit by least squares (correlation coefficient, r = 0.99). Glial cells were activated by 100 µM ATP $gamma$ S ejections of varying duration (10 msec to 2 sec). Glial Ca²⁺ increases were measured from Müller cell processes in the inner plexiform layer (Fig. 1c).

Of the 138 neurons studied, 35.5% showed little or no hyperpolarization (<0.2 mV), 52.2% showed moderate hyperpolarizations(0.2-5 mV), and 12.3% showed large hyperpolarizations (>5 mV).Neuronal hyperpolarization was slow, peaking at 6.0 ± 0.2 secand lasting for 19.2 ± 0.8 sec (n = 31), when evoked by briefejection of agonist solution (0.2-2 secduration).

Regardless of the stimulus used to activate the glial cells, the time course of the neuronal response closely followed increasesin glial Ca²⁺ (Fig. 2A-C), suggesting that the response was evoked by glialcells rather than directly by the stimulus. This correlation wasparticularly clear in neurons in which two different stimuli wereused to activate the glial cells. In the experiment illustratedin Figure 2C, for instance, the glial Ca²⁺ increase elicited by mechanical stimulation peaked later andwas more prolonged than was the Ca²⁺ increase elicited by ATP ejection. The time course of the resultinghyperpolarizations in the neuron followed these glial Ca²⁺ increasesclosely.

There was a close correlation between the amplitude of glial Ca²⁺ responses and neuronal inhibitory responses as well. The amplitudeof the outward current evoked in a given neuron increased linearlyas the amplitude of the glial Ca²⁺ response increased (Fig. 2D). Inhibitory responses were not evokedwhen agonist ejection failed to elicit a glial Ca²⁺ response. The correlation between glial Ca²⁺ increases and neuronal current was best when glial Ca²⁺ responses were measured in Müller cells within the inner plexiformlayer (Fig. 1c). The correlation coefficient of the glial Ca²⁺-neuronal current relationship, r, equaled 0.92 ± 0.04 (n =4).

Most experiments were conducted at 24°C, because higher temperatures caused retinal preparations to deteriorate quickly andresulted in rapid fading of Fluo-4 labeling in glial cells. However,a series of experiments were conducted at 35°C to determine whetherthe inhibitory neuronal responses observed at 24°C were also evokedat a temperature close to that present in vivo. Raising the temperaturefrom 24 to 35°C resulted in glial-evoked outward currents in neuronsthat were larger in amplitude and had a faster time course (Fig.3A). Mean current amplitude increased 72 ± 18% (n = 8; p < 0.001),and latency to the peak of the current decreased from 7.2 to 5.2sec (n = 8; p < 0.001) when the temperature was increased from24 to 35°C.

View larger version (20K):
[in this window]
[in a new window]
Figure 3. Properties of the inhibitory neuronal response. A, Raising the temperature of the retina from 24 to 35°C resulted in a glial-evoked outward current that was larger in amplitude and had a faster time course. The two responses were recorded in consecutive trials on the same neuron. Holding potential, $-$ 76 mV. B, The spontaneous spike activity of a neuron was inhibited when glial cells were activated by agonist ejection. The glial-evoked hyperpolarization in the neuron was 1.7 mV. The action potentials (vertical lines in the neuron voltage record) have been truncated. Resting membrane potential, $-$ 63 mV. C, The outward current generated in a neuron in response to glial cell activation was not reduced when synaptic transmission was blocked with Cd²⁺. Holding potential, $-$ 76 mV.

Neuronal hyperpolarizations evoked by activating glial cells resulted in a reduction in the frequency of action potentialgeneration in those neurons that displayed spontaneous spike activity.Even small glial-evoked hyperpolarizations (1-2 mV) decreasedneuronal spike frequency (Fig. 3B).

The glial-evoked inhibitory neuronal responses described above could be mediated by a direct inhibitory action of glial cellson the neurons or indirectly by glial cell excitation of amacrinecells, which inhibit ganglion cells in the retina. To distinguishbetween these two possibilities, synaptic signaling between neuronswas blocked by addition of Cd²⁺, which blocks synaptic transmission onto ganglion cells in theretina (Chen and Diamond, 2002). Addition of 200 µM Cd²⁺ to the superfusate did not reduce the outward current generatedin the neurons (122 ± 10% of control; n = 10) (Fig. 3C), demonstratingthat activation of inhibitory interneurons was not responsiblefor glial cell-mediated neuronalinhibition.

Morphological characterization of neurons

The morphology of the neurons studied was characterized by filling cells with Lucifer yellow. Within the ganglion cell layer,all filled neurons with somata >10 µm in diameter had axons (Fig.4A), demonstrating that they were ganglion cells rather than displacedamacrine cells, which are present in the ganglion cell layer ofthe rat retina (Perry and Walker, 1980). All neurons characterizedin this study were ganglion cells.

View larger version (69K):
[in this window]
[in a new window]
Figure 4. Relationship between neuronal inhibition and dendritic depth. A, B, Confocal micrographs of a Lucifer yellow-filled neuron. A, Eight micrometers below the retinal surface, at the level of the cell soma. Arrowheads indicate the axon of the neuron. The recording pipette is shown to the right. B, Eighteen micrometers below the retinal surface. The deepest dendrites of the neuron in A, as well as the out-of-focus soma are shown. Scale bar, 25 µm. C, Relationship between glial-evoked neuronal hyperpolarization and the depth of the deepest dendrites of neurons. Each filled circle represents a single neuron. The absolute depths of the inner and outer borders of the IPL differed for each cell studied. Mean depths corresponding to 0 and 100% of the IPL equaled 18 and 49 µm, measured from the inner surface of the retina.

There was a correlation between the amplitude of the inhibitory responses of the neurons characterized and the depth to whichtheir dendrites extended (Fig. 4B). The largest inhibitory responseswere recorded from neurons whose dendrites extended deep intothe outer portion of the inner plexiform layer. This relationshipis revealed in a plot of neuronal hyperpolarization evoked byglial cell activation, graphed as a function of the depth of thedeepest dendrites of the neuron (Fig. 4C). This relationship showsthat the deeper the dendrites of a neuron extend into the IPL,the greater the inhibitory response of the neuron can be. Theplot also demonstrates, however, that many neurons show littleor no inhibition, even when their dendrites extend deep into theouterIPL.

Müller glial cells inhibit neurons

The stimuli used to activate glial cells produced Ca²⁺ increases in both astrocytes and Müller cells, and either of these glialcells could be responsible for generating inhibitory responsesin the neurons. Astrocytes and Müller cells were selectivelyactivated to determine which was responsible for inhibiting theneurons. I have demonstrated previously that Ca²⁺ waves do not propagate between astrocytes and Müller cells bydiffusion of an intracellular messenger but rather by the releaseof ATP, and that selective activation of either type of glialcell can be achieved by limiting the strength of the stimulus(Newman, 2001b).

UTP ejection onto the retinal surface was effective in activating astrocytes but much less effective in activating Müllercells. When 100 µM UTP was ejected and failed to evoke Ca²⁺ increases in Müller cells, indicating that Müller cells werenot activated, outward currents were not observed in neurons (n= 6) (Fig. 5A, UTP). When ATP $gamma$ S was ejected at the same site,activating both Müller cells and astrocytes, outward currentswere recorded from the same neurons (n = 6) (Fig. 5A, ATP $gamma$ S).

View larger version (75K):
[in this window]
[in a new window]
Figure 5. Müller glial cells evoke neuronal inhibition. Shown for each trial are two pseudocolor Ca²⁺ ratio images and a record of neuronal current. The image on the left shows Ca²⁺ changes at the retinal surface, reflecting Ca²⁺ in both astrocytes (outlined by black lines) and Müller cells (outside these black lines). The image in the middle indicates Ca²⁺ changes in the inner plexiform layer (Fig. 1c), reflecting Ca²⁺ changes in Müller cells. A, ATP $gamma$ S (100 µM) ejected onto the retinal surface activates both astrocytes and Müller cells and evokes an outward current in a neuron. UTP (100 µM) ejection activates astrocytes but not Müller cells and fails to evoke a current. The Ca²⁺ images and current records were acquired in four consecutive trials on the same neuron. The neuron currents and the corresponding inner plexiform layer Ca²⁺ images were acquired simultaneously. Holding potential, $-$ 76 mV. B, ATP $gamma$ S (100 µM) ejection into the inner nuclear layer activates Müller cells but not astrocytes and evokes an outward current in a neuron in a different preparation from A. The neuron current and inner plexiform layer Ca²⁺ image were acquired simultaneously. Holding potential, $-$ 73 mV. The pseudocolor scale at the bottom left indicates Ca²⁺ ratio values. Scale bar , 25 µm.

In complementary experiments, when ATP $gamma$ S was ejected into the inner nuclear layer, activating Müller cells but not astrocytes,outward currents were observed in neurons (n = 6) (Fig. 5B). Theseresults demonstrate that activation of Müller cells, but notastrocytes, is both necessary and sufficient to evoke neuronalinhibitoryresponses.

Neuronal adenosine receptor activation

The nature of the glial transmitter evoking neuronal inhibition was investigated in pharmacological experiments. Antagoniststo AMPA (10 µM NBQX), NMDA (100 µM DL-AP-7), GABA_A (5 µM bicuculline),GABA_B (200 µM saclofen), glycine (1 µM strychnine), and muscarinic(10 µM scopolamine) receptors, when added to the superfusate,did not substantially reduce glia-evoked outward currents in neurons.In contrast, the A₁ adenosine receptor antagonist DPCPX (Cunhaet al., 1998; Huang et al., 1999), when added to the superfusate,completely blocked outward currents at low concentrations (Fig.6A). When glial cells were activated by ATP $gamma$ S or ATP, outwardcurrent amplitude was reduced to 1.1 ± 0.8% of control (n = 13;p < 0.005) by 10 nM DPCPX. Similarly, when glial cells were activatedby 2 mM dopamine, outward currents were reduced to 1.0 ± 1.0%of control (n = 7; p < 0.005) by 10 nM DPCPX. These results indicatethat glial cells inhibit neurons by stimulating neuronal adenosinereceptors.

View larger version (32K):
[in this window]
[in a new window]
Figure 6. A₁ adenosine receptor activation evokes neuronal inhibition. A, The A₁ adenosine receptor antagonist DPCPX abolishes the outward neuronal current evoked by glial cell activation. Holding potential, $-$ 71 mV. B, Adenosine ejection evokes a larger, shorter-latency neuronal current than does ATP $gamma$ S ejection at the same retinal location and with the same neuron. Holding potential, $-$ 76 mV. C, The ectonucleotidase inhibitor AOPCP reduces and slows the time course of the neuronal current. The effect is largely reversible. Recovery time, 11 min. Holding potential, $-$ 75 mV.

I hypothesized that the source of the inhibitory adenosine was ATP released from Müller cells and hydrolyzed to adenosinein extracellular space. Release of ATP from glial cells has beendemonstrated in a number of in vitro and in situ systems (Cotrinaet al., 1998; Wang et al., 2000; Newman, 2001b). Released ATPwould be rapidly metabolized to adenosine by ecto-ATPases andectonucleotidases, leading to the activation of neuronal adenosinereceptors, which are present on ganglion cells (Braas et al.,1987; Kvanta et al., 1997; Zhang and Schmidt, 1999).

This hypothesis was supported by a number of findings. Direct activation of neuronal adenosine receptors by ejection of adenosineevoked outward currents in ganglion cells. The adenosine-evokedcurrents, although not statistically different in amplitude (132± 23%; n = 8; p > 0.05), had shorter latencies (0.61 ± 0.18 secvs 1.51 ± 0.18 sec; n = 8; p < 0.005) than the currents evokedby ATP $gamma$ S ejection (Fig. 6B). The outward currents evoked by adenosineejection were not significantly reduced by 200 µM Cd²⁺ (85 ± 6% of control; n = 4; p > 0.05), demonstrating that thecurrents resulted from direct stimulation of ganglion cells ratherthan from stimulation ofinterneurons.

ATP, when released into extracellular space, is metabolized rapidly (~200 msec) from ATP to ADP to AMP to adenosine (Zimmermann,1994; Dunwiddle et al., 1997; Cunha et al., 1998). If glial inhibitionof neurons results from the release of ATP, then interfering withthis metabolic cascade should block the inhibition. Addition of50 µM 6-N,N-diethyl-D- $beta$ , $gamma$ -dibromomethyleneATP (ARL-67156) to thesuperfusate, an ecto-ATPase inhibitor that prevents conversionof ATP to ADP (Westfall et al., 1996), resulted in a reductionof neuronal outward current to 47 ± 7% of control (n = 5; p <0.05). Similarly, addition of 250 µM adenosine-5'-O-( $alpha$ , $beta$ -methylene)-diphosphonate(AOPCP), an ectonucleotidase inhibitor that prevents conversionof AMP to adenosine (Kreutzberg et al., 1978; Kreutzberg and Hussain,1982; Cunha et al., 1998), reduced outward currents to 35 ± 3%of control (n = 6; p < 0.001) (Fig. 6C). Both inhibitors slowedthe time course of the outward currents and were partially reversible.The results support the hypothesis that glial cells inhibit neuronsby releasing ATP that is subsequently metabolized toadenosine.

ATP release from Müller cells

I have shown previously using the luciferin-luciferase chemiluminescence assay that glial cell stimulation results in therelease of ATP from the surface of the retina (Newman, 2001b).In that study, glial cells were the likely source of the releasedATP. However, ATP release from neurons could not be ruled out.I have now repeated this experiment in the presence of 100 µMCd²⁺, which blocks Ca²⁺-dependent release of ATP from neurons. With Cd²⁺ added to the superfusate, mechanical stimulation of glial cellsevoked a chemiluminescence signal that spread outward from thepoint of stimulation (Fig. 7A). The presence of the ATP-inducedchemiluminescence signal after addition of Cd²⁺ strengthens the conclusion that ATP release in these experimentscomes from glial cells rather than from neurons.

View larger version (19K):
[in this window]
[in a new window]
Figure 7. Release of ATP from glial cells. A, Mechanical stimulation of glial cells at the retinal surface evokes ATP release at the surface, detected by the luciferin-luciferase chemiluminescence assay. The five line-scans show the spatial pattern of chemiluminescence in a line passing through the stimulation site at the indicated times after stimulation. B, ATP release into the inner plexiform layer. A small volume of luciferin-luciferase solution was ejected from a pipette into the IPL, 5 sec before mechanical stimulation of glial cells at the retinal surface. The traces show the chemiluminescence signal recorded near the ejection pipette tip in the IPL (Fig. 1c) and are averages of five trials. Addition of the ecto-ATPase inhibitor ARL-67156 increases the chemiluminescence signal. A 100 µM concentration of Cd²⁺ was present in the superfusate in both A and B to block Ca²⁺-dependent transmitter release from neurons.

The experiment described above indicates that activated glial cells release ATP at the surface of the retina. The luciferin-luciferaseassay was also used to demonstrate that Müller glial cells releaseATP directly into the inner plexiform layer. Instead of bathingthe entire retina in luciferin-luciferase solution, as was doneto demonstrate ATP release at the retinal surface, a small volumeof luciferin-luciferase Ringer's solution was ejected directlyinto the IPL. Using this protocol, only ATP release into the IPLwould result in a chemiluminescence signal. Experiments were conductedin the presence of 100 µM Cd²⁺ to block Ca²⁺-dependent release of ATP fromneurons.

When glial cells at the surface of the retina were stimulated mechanically, a chemiluminescence signal was observed near thetip of the luciferin-luciferase ejection pipette (Fig. 7B). Additionof the ecto-ATPase inhibitor ARL-67156 (50 µM) to the superfusatesubstantially increased the chemiluminescence signal by preventingthe rapid hydrolysis of ATP. In control experiments, ejectionof the luciferin-luciferase solution without glial cell stimulationdid not produce a chemiluminescence signal. The results confirmthat activation of glial cells results in the release of ATP intotheIPL.

Neuronal K⁺ conductance increase

The mechanism by which adenosine receptor activation results in the generation of inhibitory neuronal responses was also studied.Neuronal hyperpolarization evoked by glial cell activation wasaccompanied by a decrease in cell input resistance (Fig. 8A),indicating that inhibition is mediated by an opening of ion channels.The reversal potential of the outward current generating the hyperpolarizationwas $-$ 93 ± 2 mV (n = 4) (Fig. 8B). This value is close to the calculatedK⁺ equilibrium potential of $-$ 97 mV, suggesting that K⁺ channels open during inhibition. Addition of the K⁺ channel blocker Ba²⁺ (100 µM) to the superfusate reduced the inhibition (outward currentor hyperpolarization) to 28 ± 12% (n = 10; p < 0.05) of controlamplitude (Fig. 8C). The Ba²⁺ effect was largely reversible.

View larger version (22K):
[in this window]
[in a new window]
Figure 8. Glial-evoked neuronal inhibition is generated by the opening of Ba²⁺-sensitive K⁺ channels. A, Neuronal hyperpolarization is accompanied by a decrease in cell input resistance. Responses to $-$ 32 pA current pulses injected into a neuron are reduced during the hyperpolarization. Resting potential, $-$ 83 mV. B, Reversal potential of the current generating the hyperpolarization is $-$ 98 mV in this neuron, near the K⁺ equilibrium potential. Holding potentials are given to the right. C, The K⁺ channel blocker Ba²⁺ reduces the neuronal current evoked by glial cell activation. The effect is largely reversible. Recovery time, 6 min. Holding potential, $-$ 72 mV.

In contrast, the outward current was unaffected by changes in the Cl gradient across neurons. Substitution of methanesulfonate forCl in the superfusate solution did not reduce neuronal hyperpolarization(111 ± 19% of control; n = 6), demonstrating that Cl-permeable channels do not mediate theinhibition.

The results demonstrate that ganglion cell inhibition is generated by the opening of Ba²⁺-sensitive K⁺ channels. A₁ receptor activation leads to a similar K⁺ conductance increase in many types of neurons by stimulatingG_i/G_o proteins and opening Ba²⁺-sensitive, G-protein-coupled inwardly rectifying K⁺ channels (Trussell and Jackson, 1985, 1987; Gerber et al., 1989;Greene and Haas, 1991; Zimmermann, 1994; Mark and Herlitze, 2000;Cunha, 2001). The glial-evoked inhibition of retinal ganglioncells observed in this study is most likely mediated by G-protein-coupledinwardly rectifying K⁺ channels aswell.

  Discussion

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Glial inhibition of neurons in the retina

The results demonstrate that activated glial cells can evoke inhibitory responses in retinal neurons by the release of ATPand the subsequent activation of neuronal adenosine receptors.Several lines of evidence support this conclusion. Stimulationof glial cells by a number of agonists results in the inhibitionof retinal ganglion cells. Ganglion cell inhibition is also evokedwhen a distant astrocyte is stimulated mechanically. Neuronalinhibition is blocked by the A₁ adenosine receptor antagonistDPCPX. Inhibition is also reduced by the ecto-ATPase inhibitorARL-67156 and the ectonucleotidase inhibitor AOPCP, demonstratingthat the source of the inhibitory adenosine is the hydrolysisof ATP released into extracellular space. In addition, ATP imagingusing the luciferin-luciferase chemiluminescence assay demonstratesthat stimulation of glial cells results in the release of ATPinto the inner plexiformlayer.

The source of the ATP that mediates neuronal inhibition is almost certainly glial rather than neuronal, as demonstrated bythe following findings: (1) Glial-induced inhibition of neuronsis not reduced by addition of Cd²⁺, which blocks Ca²⁺-dependent release of ATP from neurons. ATP release from glialcells, in contrast, is believed to be Ca²⁺ independent (Wang et al., 2000) (E. A. Newman, unpublished observations)and, as demonstrated here, is not blocked by Cd²⁺. (2) A number of different stimuli (ATP, ATP $gamma$ S, dopamine, thrombin,LPA, mechanical stimulation) all activate glial cells and areall effective in evoking neuronal inhibition. It is unlikely thatall of these stimuli also evoke a prolonged release of ATP (lastingmany seconds) from neurons. [ATP, used as a stimulus to activateglial cells in the present experiments, could directly inhibitneurons after its conversion to adenosine. The primary effectof ejected ATP is to activate glial cells rather than to directlyinhibit neurons, however, because the time courses of neuronalinhibition in response to ejected ATP and ejected ATP $gamma$ S are similar.Presumably, little of the ATP that is ejected onto the retinalsurface is converted to adenosine, and of this adenosine, littlediffuses into the inner plexiform layer before being removed byuptake systems (Cunha et al., 1998).] (3) The time course of neuronalinhibitory responses closely follows the time course of Ca²⁺ increases in glial cells, suggesting a direct relationship betweenglial cell activation and neuronal inhibition. [The precise timingbetween a glial Ca²⁺ response and a neuronal inhibitory response is influenced bya number of factors. ATP release from glial cells is believedto be Ca²⁺ independent (Wang et al., 2000) and may actually precede theglial Ca²⁺ increase (Newman, 2001b). This will have the effect of advancingthe neuronal response with respect to the glial response. On theother hand, the delay introduced by the conversion of ATP to adenosineand the delay inherent in second messenger system activation ofneuronal K⁺ channels will retard the neuronal response with respect to theglial response.] (4) The amplitude of neuronal inhibitory responsesis closely correlated to the magnitude of glial Ca²⁺ increases, also suggesting a direct relationship between glialcell activation and neuronalinhibition.

The results demonstrate that, of the two types of macroglial cells in the retina, Müller cells, rather than astrocytes, evokeinhibitory neuronal responses. Selective activation of each typeof glial cell reveals that activation of Müller cells is bothnecessary and sufficient to evoke neuronal inhibition. This isnot surprising, because neuronal inhibition occurs in the innerplexiform layer (the synaptic layer of retinal ganglion cells).Müller cells, but not astrocytes, are present in this retinallayer.

Morphological analysis demonstrates that neurons whose dendrites extend deep into the inner plexiform layer display largerinhibitory responses than do cells with more superficial dendrites.Thus, OFF ganglion cells, whose dendrites ramify in the outerhalf of the IPL, are more likely to be inhibited by glial cellsthan are ON ganglion cells. Localization of glial inhibition ofneurons to the outer portion of the IPL could arise for severalreasons, including the following: (1) Müller cells may releaseATP selectively into this region, (2) the activity of the ectoenzymesthat convert ATP to adenosine may be higher in this region, or(3) A₁ adenosine receptors or the K⁺ channels that generate the inhibition may be present at higherdensities on the dendrites of ganglion cells in the outer portionof the inner plexiformlayer.

Of the neurons characterized, 35% showed little or no inhibition by glial cells, whereas 12% showed large hyperpolarizations(>5 mV). This indicates that glial inhibition of neurons in theretina is not a global, indiscriminant phenomenon, but ratherrepresents a selective interaction between glial cells and a subsetof neurons. As discussed above, ganglion cells responding to theOFF of light are more likely to be inhibited by glial cells thanare ON ganglioncells.

Glial cell inhibition of neurons can be substantial. In our preparation, 12% of the neurons studied showed hyperpolarizationsof >5 mV and lasting tens of seconds. These hyperpolarizationscan have a large inhibitory effect on the spike activity of ganglioncells. As demonstrated by recordings from neurons displaying spontaneousspike activity, even small glial-evoked hyperpolarizations (1-2mV) can substantially inhibit the firing rate of neurons. Experimentsperformed at 35°C indicate that glial-evoked inhibitory responsesin neurons will be even larger at body temperature than at 24°C,the temperature at which most experiments wereconducted.

We have shown previously that activation of glial cells can inhibit light-evoked spike activity in retinal ganglion cells(Newman and Zahs, 1998). In these previous experiments, inhibitionof spike activity was blocked by antagonists to glutamate, GABA,and glycine receptors. In the present work, in contrast, theseantagonists were ineffective in blocking glial inhibition of neurons.It is likely, therefore, that the mechanism of glial inhibitionof neurons described here, the release of ATP and activation ofneuronal adenosine receptors, is not responsible for the inhibitionof light-evoked spike activity observed previously. This suggeststhat a second mechanism of glial inhibition of neurons, perhapsinhibiting the release of neurotransmitters from presynaptic terminals,may also be present in the retina. Presynaptic inhibition couldbe mediated by the release of either ATP (Cunha, 2001) or glutamate(Araque et al., 1998a) from Müller cells. The existence of aglial-evoked presynaptic inhibition is supported by preliminaryobservations that indicate that spontaneous and evoked EPSCs recordedin ganglion cells are reduced when glial cells are activated.Glial inhibition of transmitter release from presynaptic terminalshas been observed previously in glial-neuronal cocultures (Araqueet al., 1998a). The experiments conducted in the present studywould not have detected glial-mediated presynapticinhibition.

It remains to be established to what degree glial cells inhibit neuronal activity in the retina in vivo and what role thisinhibition plays in the processing of visual information. It isnot known, for instance, whether light-evoked neuronal activityactivates glial cells in the retina. Preliminary experiments indicatethat spontaneous Ca²⁺ oscillations occur in retinal Müller cells (Newman, 2002). TheseCa²⁺ increases may be associated with ATP release and could resultin neuronal inhibition in vivo.

Glial inhibition of neurons in the brain

The ATP-release mechanism of neuronal inhibition described here may operate throughout the CNS. Application of neurotransmitters(Finkbeiner, 1993), as well as electrical stimulation of neurons(Jahromi et al., 1992; Porter and McCarthy, 1996; Pasti et al.,1997; Grosche et al., 1999; Araque et al., 2002), results in theactivation of astrocytes, the principal glial cells of the brain.Astrocyte activation, in turn, results in ATP release (Cotrinaet al., 1998; Wang et al., 2000; Newman, 2001b). The subsequentbreakdown of glial-released ATP to adenosine could have widespreadmodulatory effects on neuronal activity, because adenosine isa potent inhibitory neuromodulator in the brain (Trussell andJackson, 1985; Gerber et al., 1989; Greene and Haas, 1991; Zimmermann,1994; Cunha, 2001).

Indeed, the results of a previous report (Cunha et al., 1998) suggest that glial cells may inhibit neurons in the hippocampus.Application of ATP $gamma$ S and other nonhydrolyzable ATP analogs inthis preparation inhibited neurons through activation of A₁ receptors.This inhibition was attributed to residual hydrolysis of thesenonhydrolyzable analogs to adenosine. It is more likely, however,that the ATP analogs stimulated hippocampal glial cells, which,in turn, released ATP that was then hydrolyzed to adenosine. Thus,the mechanism of glial inhibition of neurons described in thepresent study may also be responsible for neuronal inhibitionin thehippocampus.

Glial cells have been shown previously to modulate neuronal activity through the release of glutamate (Kang et al., 1998;Araque et al., 2001; Haydon, 2001; Vesce et al., 2001). Our resultsnow demonstrate that glial cells can modulate neuronal activitythrough a second, independent mechanism, the release of ATP. Together,these findings lend support to the hypothesis that glial cellsplay an active role in information processing in the brain. Inaddition, adenosine has been shown to modulate several forms ofsynaptic plasticity, including long-term potentiation (Huang etal., 1999) and depression (de Mendonca and Ribeiro, 1997), raisingthe possibility that glial cells, through the release of ATP,may participate in the regulation of learning andmemory.

  FOOTNOTES

Received Oct. 17, 2002; revised Dec. 6, 2002; accepted Dec. 9, 2002.

This work was supported by National Institutes of Health Grant EY04077. I thank H. C. Lee for purification of ATP $gamma$ S, P. Ceelenfor technical assistance, and J. I. Gepner, K. R. Zahs, and R.F. Miller for helpfuldiscussions.

Correspondence should be addressed to Dr. Eric A. Newman, Department of Neuroscience, University of Minnesota, 6-145 JacksonHall, 321 Church Street Southeast, Minneapolis, MN 55455. E-mail:ean{at}umn.edu.

  References

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Araque A, Parpura V, Sanzgiri RP, Haydon PG (1998a) Glutamate-dependent astrocyte modulation of synaptic transmission between cultured hippocampal neurons. Eur J Neurosci 10:2129-2142[ISI][Medline].
Araque A, Sanzgiri RP, Parpura V, Haydon PG (1998b) Calcium elevation in astrocytes causes an NMDA receptor-dependent increase in the frequency of miniature synaptic currents in cultured hippocampal neurons. J Neurosci 18:6822-6829[Abstract/Free Full Text].
Araque A, Carmignoto G, Haydon PG (2001) Dynamic signaling between astrocytes and neurons. Annu Rev Physiol 63:795-813[ISI][Medline].
Araque A, Martin ED, Perea G, Arellano JI, Buno W (2002) Synaptically released acetylcholine evokes Ca²⁺ elevations in astrocytes in hippocampal slices. J Neurosci 22:2443-2450[Abstract/Free Full Text].
Biedermann B, Frohlich E, Grosche J, Wagner H-J, Reichenbach A (1995) Mammalian Müller (glial) cells express functional D₂ dopamine receptors. NeuroReport 6:609-612[Medline].
Braas KM, Zarbin MA, Snyder SH (1987) Endogenous adenosine and adenosine receptors localizes to ganglion cells of the retina. Proc Natl Acad Sci USA 84:3906-3910[Abstract/Free Full Text].
Castonguay A, Robitaille R (2001) Differential regulation of transmitter release by presynaptic and glial Ca²⁺ internal stores at the neuromuscular synapse. J Neurosci 21:1911-1922[Abstract/Free Full Text].
Chen S, Diamond JS (2002) Synaptically released glutamate activates extrasynaptic NMDA receptors on cells in the ganglion cell layer of rat retina. J Neurosci 22:2165-2173[Abstract/Free Full Text].
Cotrina ML, Lin JHC, Alves-Rodriques A, Liu S, Li J, Azmi-Ghadimi H, Kang J, Naus CCG, Nedergaard M (1998) Connexins regulate calcium signaling by controlling ATP release. Proc Natl Acad Sci USA 95:15735-15740[Abstract/Free Full Text].
Cotrina ML, Lin JH-C, Lopez-Garcia JC, Naus CCG, Nedergaard M (2000) ATP-mediated glia signaling. J Neurosci 20:2835-2844[Abstract/Free Full Text].
Cunha RA (2001) Adenosine as a neuromodulator and as a homeostatic regulator in the nervous system: different roles, different sources and different receptors. Neurochem Int 38:107-125[ISI][Medline].
Cunha RA, Sebastiao AM, Ribeiro JA (1998) Inhibition by ATP of hippocampal synaptic transmission requires localized extracellular catabolism by ecto-nucleotidases into adenosine and channeling to adenosine A1 receptors. J Neurosci 18:1987-1995[Abstract/Free Full Text].
de Mendonca A, Ribeiro JA (1997) Adenosine and neuronal plasticity. Life Sci 60:245-251[ISI][Medline].
Dunwiddle TV, Diao L, Proctor WR (1997) Adenine nucleotides undergo rapid, quantitative conversation to adenosine in the extracellular space in rat hippocampus. J Neurosci 17:7673-7682[Abstract/Free Full Text].
Finkbeiner SM (1993) Glial calcium. Glia 9:83-104[ISI][Medline].
Gerber U, Greene RW, Haas HL, Stevens DR (1989) Characterization of inhibition mediated by adenosine in the hippocampus of the rat in vitro. J Physiol (Lond) 417:567-578[Abstract/Free Full Text].
Greene RW, Haas HL (1991) The electrophysiology of adenosine in the mammalian central nervous system. Prog Neurobiol 36:329-341[ISI][Medline].
Grosche J, Matyash V, Moller T, Verkhratsky A, Reichenbach A, Kettenmann H (1999) Microdomains for neuron-glia interaction: parallel fiber signaling to Bergmann glial cells. Nat Neurosci 2:139-143[ISI][Medline].
Hassinger TD, Atkinson PB, Strecker GJ, Whalen LR, Dudek FE, Kossel AH, Kater SB (1995) Evidence for glutamate-mediated activation of hippocampal neurons by glial calcium waves. J Neurobiol 28:159-170[ISI][Medline].
Haydon PG (2001) Glia: listening and talking to the synapse. Nat Neurosci 2:185-193[ISI][Medline].
Huang C-C, Liang Y-C, Hsu K-S (1999) A role for extracellular adenosine in time-dependent reversal of long-term potentiation by low-frequency stimulation at hippocampal CA1 synapses. J Neurosci 19:9728-9738[Abstract/Free Full Text].
Jahromi BS, Robitaille R, Charlton MP (1992) Transmitter release increases intracellular calcium in perisynaptic Schwann cells in situ. Neuron 8:1069-1077[ISI][Medline].
Kang J, Goldman SA, Nedergaard M (1998) Astrocyte-mediated potentiation of inhibitory synaptic transmission. Nat Neurosci 1:683-692[ISI][Medline].
Kreutzberg GW, Hussain ST (1982) Cytochemical heterogeneity of the glial plasma membrane: 5'-nucleotidase in retinal Müller cells. J Neurocytol 11:53-64[ISI][Medline].
Kreutzberg GW, Barron KD, Schubert P (1978) Cytochemical localization of 5'-nucleotidase in glial plasma membranes. Brain Res 158:247-257[ISI][Medline].
Kvanta A, Seregard S, Sejersen S, Kull B, Fredholm BB (1997) Location of adenosine receptor messenger RNAs in the rat eye. Exp Eye Res 65:595-602[ISI][Medline].
Manning Jr TJ, Sontheimer H (1997) Bovine serum albumin and lysophosphatidic acid stimulate calcium mobilization and reversal of cAMP-induced stellation in rat spinal cord astrocytes. Glia 20:163-172[ISI][Medline].
Mark MD, Herlitze S (2000) G-protein mediated gating of inward-rectifier K⁺ channels. Eur J Biochem 267:5830-5836[ISI][Medline].
Newman EA (2001a) Glia of the retina. In: Retina (Ryan SJ, ed), pp 89-103. St. Louis: Mosby.
Newman EA (2001b) Propagation of intercellular calcium waves in retinal astrocytes and Müller cells. J Neurosci 21:2215-2223[Abstract/Free Full Text].
Newman EA (2002) Calcium signaling in retinal glial cells and its effect on neuronal activity. Prog Brain Res 132:241-254.
Newman EA, Zahs KR (1997) Calcium waves in retinal glial cells. Science 275:844-847[Abstract/Free Full Text].
Newman EA, Zahs KR (1998) Modulation of neuronal activity by glial cells in the retina. J Neurosci 18:4022-4028[Abstract/Free Full Text].
Pasti L, Volterra A, Pozzan T, Carmignoto G (1997) Intracellular calcium oscillations in astrocytes: a highly plastic, bidirectional form of communication between neurons and astrocytes in situ. J Neurosci 17:7817-7830[Abstract/Free Full Text].
Perry VH, Walker M (1980) Amacrine cells, displaced amacrine cells and interplexiform cells in the retina of the rat. Proc R Soc Lond B Biol Sci 208:415-431[Medline].
Porter JT, McCarthy KD (1996) Hippocampal astrocytes in situ respond to glutamate released from synaptic terminals. J Neurosci 16:5073-5081[Abstract/Free Full Text].
Puro DG, Stuenkel EL (1995) Thrombin-induced inhibition of potassium currents in human retinal glial (Müller) cells. J Physiol (Lond) 485:337-348[ISI][Medline].
Trussell LO, Jackson MB (1985) Adenosine-activated potassium conductance in cultured striatal neurons. Proc Natl Acad Sci USA 82:4857-4861[Abstract/Free Full Text].
Trussell LO, Jackson MB (1987) Dependence of an adenosine-activated potassium current on a GTP-binding protein in mammalian central neurons. J Neurosci 7:3306-3316[Abstract].
Vesce S, Bezzi P, Volterra A (2001) Synaptic transmission with the glia. News Physiol Sci 16:178-184[Abstract/Free Full Text].
Wang Z, Haydon PG, Yeung ES (2000) Direct observation of calcium-independent intercellular ATP signaling in astrocytes. Anal Chem 72:2001-2007[Medline].
Westfall TD, Kennedy C, Sneddon P (1996) Enhancement of sympathetic purinergic neurotransmission in the guinea-pig isolated vas deferens by the novel ecto-ATPase inhibitor ARL 67156. Br J Pharmacol 117:867-872[ISI][Medline].
Zhang C, Schmidt JT (1999) Adenosine A1 and class II metabotropic glutamate receptors mediate shared presynaptic inhibition of retinotectal transmission. J Neurophysiol 82:2947-2955[Abstract/Free Full Text].
Zimmermann H (1994) Signaling via ATP in the nervous system. Trends Neurosci 17:420-426[ISI][Medline].

Copyright © 2003 Society for Neuroscience 0270-6474/03/2351659-08$05.00/0

This article has been cited by other articles:

R. C. Reyes and V. Parpura
Mitochondria Modulate Ca2+-Dependent Glutamate Release from Rat Cortical Astrocytes
J. Neurosci., September 24, 2008; 28(39): 9682 - 9691.
[Abstract] [Full Text] [PDF]

B. Mehta, G. Begum, N. B. Joshi, and P. G. Joshi
Nitric Oxide-mediated Modulation of Synaptic Activity by Astrocytic P2Y Receptors
J. Gen. Physiol., August 25, 2008; 132(3): 339 - 349.
[Abstract] [Full Text] [PDF]

D. T. Theodosis, D. A. Poulain, and S. H. R. Oliet
Activity-Dependent Structural and Functional Plasticity of Astrocyte-Neuron Interactions
Physiol Rev, July 1, 2008; 88(3): 983 - 1008.
[Abstract] [Full Text] [PDF]

E. Shigetomi, D. N. Bowser, M. V. Sofroniew, and B. S. Khakh
Two Forms of Astrocyte Calcium Excitability Have Distinct Effects on NMDA Receptor-Mediated Slow Inward Currents in Pyramidal Neurons
J. Neurosci., June 25, 2008; 28(26): 6659 - 6663.
[Abstract] [Full Text] [PDF]