Ammonium and Glutamate Released by Neurons Are Signals Regulating the Nutritive Function of a Glial Cell

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Volume 17, Number 7, Issue of April 1, 1997 pp. 2383-2390
Copyright ©1997 Society for Neuroscience

Ammonium and Glutamate Released by Neurons Are Signals Regulating the Nutritive Function of a Glial Cell

Marcos Tsacopoulos¹^,², Carol L. Poitry-Yamate¹^,²^,³, and Serge Poitry¹^,²
¹ Experimental Ophthalmology Laboratory and Departments of ² Physiology and ³ Pharmacology, University of Geneva Medical School, 1211 Geneva 4, Switzerland

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Glial cells transform glucose to a fuel substrate taken up and used by neurons. In the honeybee retina, photoreceptor neuronsconsume both alanine supplied by glial cells and exogenous proline.Ammonium (NH₄⁺) and glutamate, produced and released in a stimulus-dependentmanner by photoreceptor neurons, contribute to the biosynthesisof alanine in glia. Here we report that NH₄⁺ and glutamate are transported into glia and that a transientrise in the intraglial concentration of NH₄⁺ or of glutamate causes a net increase in the level of reducednicotinamide adenine dinucleotides [NAD(P)H]. Biochemical measurementsindicate that this is attributable to activation of glycolysisin glial cells by the direct action of NH₄⁺ and glutamate on at least two enzymatic reactions: those catalyzedby phosphofructokinase (PFK; ATP:D-fructose-6-phosphotransferase,EC2.7.1.11) and glutamate dehydrogenase (GDH; L-glutamate:NADoxidoreductase, deaminating; EC1.4.1.3). This activation leadsto an increase in the production and release of alanine by glia.This signaling, which depends on the rate of conversion of NH₄⁺ and glutamate to alanine and $alpha$ -ketoglutarate, respectively, inthe glial cells, raises the novel possibility of a tight regulationof the nutritive function of glia.
Key words: NADH; pH; fluorescence imaging; NH₄⁺ transport; glutamate transport; retina

INTRODUCTION

Growing evidence suggests that astrocytes, by their physiological interactions with neurons, are involved in mammalian brainfunction and energy metabolism (Pellerin and Magistretti, 1994).However, the complex structural interactions among astrocytes,neurons, and capillaries make functional quantitation difficultat the cellular level. Although cultured astrocytes have provideda basis for understanding brain energy metabolism, there is presentlyno clear reported case in which a molecular signal physiologicallyreleased from neurons actually exerts a fine control of glialmetabolism. Glutamate, a major excitatory neurotransmitter inthe CNS, is a case in point. Extensive electrophysiological workon acutely isolated vertebrate glia has demonstrated that glutamateis taken up electrogenically by glia (Brew and Attwell, 1987).In cultured astrocytes, this uptake activates glucose uptake andmetabolism, and it has been suggested that this activation isattributable to increased activity of a glial-specific Na⁺/K⁺ ATPase (Pellerin and Magistretti, 1994). However, alternativepossibilities can be evoked. First, because the enzyme convertingglutamate to glutamine at the expense of ammonia and ATP apparentlyis localized exclusively in glia, it is expected that an increasedglutamate uptake into astrocytes would lead to a decrease in intracellularlevels of ATP and ammonia. The question remains whether this decreaseconstitutes a primary metabolic signal and whether these levelsare restored in astrocytes by increasing oxidative metabolismand ammonia uptake. Second, glutamate uptake causes the pH inglial Müller cells to go acid, and it was suggested that thistransient pH change may be a signal to alter glial metabolism(Bouvier et al., 1992). Thus, although glutamate affects the metabolicstate of glia, whether it further constitutes a signal couplingneuron function and metabolism to those in glia only can be surmised.We approached the problem of metabolic signaling between neuronsand glia in honeybee retina because direct analysis performedin this preparation already has proven to provide an unsurpassedbasis for parallel studies in mammals (Poitry-Yamate et al., 1995).

The honeybee retina has been an appropriate model system for exploring metabolic interactions between neurons and glial cells,because light-sensitive photoreceptor neurons have almost allof the mitochondria, whereas glial cells are packed with glycogen.Moreover, although glial cells do not respond directly to light(Tsacopoulos et al., 1987; Coles, 1989), their glycogen metabolismis modified when photoreceptors are photo-stimulated (Evêquoz-Mercierand Tsacopoulos, 1991). Furthermore, glia transform glucose toalanine, which, in turn, is taken up and used by photoreceptors(Tsacopoulos et al., 1994). By analogy in mammals, evidence indicatesthat astrocytes fuel neurons with lactate (Larrabee, 1983; Poitry-Yamateet al., 1995; Tsacopoulos and Magistretti, 1996). In honeybeeretina, photoreceptors also consume proline (Tsacopoulos et al.,1994), and this consumption leads to the production and release,in a stimulus-dependent manner, of NH₄⁺ and glutamate, which, in turn, contribute to the biosynthesisof alanine in glia (Tsacopoulos et al., 1997). Here we show thatammonium (NH₄⁺) and glutamate released by photoreceptors return to glial cellsnot simply for nitrogen conservation but as information signals.

MATERIALS AND METHODS
Materials. [U-¹⁴C]glutamate was purchased from Amersham (Zürich, Switzerland; specific activity 266 mCi/mmol, 1 Ci = 37 GBq).[U-¹⁴C]Glucose was purchased from DuPont/NEN (Boston, MA; specificactivity 298 mCi/mmol). 2,7-Biscarboxyethyl-5(6)-carboxyfluorescein-AM(BCECF-AM) was obtained from Molecular Probes (Leiden, The Netherlands).Other chemicals or enzymes have been used previously (Tsacopouloset al., 1994; Veuthey et al., 1994) and were obtained from Sigma(Buchs, Switzerland), Fluka (Buchs, Switzerland), or Calbiochem(Basel, Switzerland).

Preparation of retinal homogenates and a mitochondrial fraction from drone retinal slices. For the measurement of ammonia,retinal slices, retinal homogenates, and the mitochondrial fractionwere prepared as previously described in Tsacopoulos et al. (1987)and Veuthey et al. (1994). Briefly, nonretinal portions of a slicewere removed by microdissection with fine forceps, leaving a pureretinal slice. Batches of retinal slices then were homogenizedmanually. Parts of these homogenates were processed further bysubcellular fractionation (see Veuthey et al., 1994) for isolationof the mitochondrial fraction. NH₄⁺ was assayed with dansyl-Cl (5-dimethylamino-1-naphthalene-sulfonylchloride) derivatization in sodium borate buffer (164 mM, pH 10.0)and reverse-phase HPLC (Tsacopoulos et al., 1994). As a control,rat brain slices were homogenized and assayed with the same procedure.

Preparation of glial cells isolated from drone retina. For biochemical experiments, preparations of glial cells still attachedto the basal membrane were used. Briefly, slices of retina, preparedas previously described (Coles, 1989), were pinned onto a SYLGARDsupport and the brain matter carefully removed without mechanicallydisrupting the basal membrane. Then the tissue was exposed tocontinuously oxygenated Tris-buffered Ringer's solution (in mM):NaCl 270, KCl 10, CaCl₂ 1.6, MgCl₂ 10, and Tris(hydroxymethyl)-aminomethane10, pH 7.1, containing 5 mg/ml of Pronase (Ref 53702 from Calbiochem)for 20 min at room temperature. The cornea was removed at thisstage, and the two retinas per slice were transferred for washingto a Falcon tube that was rocked on its side for 10 min. Thenthe tissue was exposed to a 0 Ca²⁺/0 Mg²⁺-Ringer's solution containing (in mM): NaCl 200, KCl 10, EDTA1, MOPS 10, and sucrose 240, pH 6.9 [at this stage and at alllater stages, the osmolarity of Ringer's solution was raised withsucrose to match that of extracellular fluid, deduced as 630 mOsm/kgby Cardinaud et al. (1994)]. With 8-15 mg/ml of trypsin (Sigma;trypsin was dialyzed to avoid contamination by NH₄⁺) added, the contents then were vortexed at low speed for 5 min.This disrupted the glial syncytium (Tsacopoulos et al., 1987,1994; Coles, 1989), releasing and destroying the majority of photoreceptors.It left an intact preparation of glial cells still attached tothe basal membrane, and it also released some isolated glial cells(singlets or in bundles). In the preparation of glial cells attachedto the basal membrane, succinate dehydrogenase activity (succinateoxidoreductase; EC1.3.99.1) was exceedingly small; hexokinaseactivity (ATP:D-hexose-6-phosphotransferase; EC2.7.1.1) wasconserved, and cell metabolism was similar to that found in gliaof intact retinas (Evêquoz-Mercier and Tsacopoulos, 1991; Tsacopouloset al., 1994). Both preparations of glia (attached or unattachedto the basal membrane) were washed in a Ringer's solution of thefollowing composition (in mM): NaCl 200, KCl 10, CaCl₂ 2, MgCl₂4.5, MOPS 10, sucrose 200, and trehalose 40, pH 6.9; unless otherwiseindicated, this was the standard Ringer's solution used for experiments.Singlets or bundles of glial cells freed during the procedurewere used for fluorescence imaging experiments. These cells wereattached to glass coverslips coated with poly-L-lysine and leftin the standard Ringer's solution 3-12 hr at ~8°C, before fluorescenceimaging. In ~20% of the overall glial preparations used for NAD(P)Hfluorescence imaging, puffs of either glutamate or NH₄Cl had anegligible or considerably delayed effect. Despite apparent morphologicalintegrity of the preparations, these responses occurred on a givenday and so may reflect metabolic alterations of cells consequentto the dissociation procedure.

Fluorescence imaging of individual glial cells. Fluorescence was measured at room temperature on an inverted Axiovert 135TVepifluorescence microscope equipped with Zeiss Pan-Neofluar 63×oil immersion lens [1.25 numerical aperture (NA)] and fit witha xenon arc lamp, neutral density filters, and an electromagneticshutter. Selected cells were positioned in the middle of the opticalfield, and the focal plane was centered on the cells, the surfacesof which were attached to the coverslip. Injection pipettes (tipdiameter ~4 µm) were advanced from both sides to just above thecentral portion of the preparation and remained in place for theduration of the entire protocol. Images were captured every 2sec with a CCD (charged-coupled device) camera (Photonic Science,Robertsbridge, UK) and processed by IonVision software (ImproVision,Coventry, UK) on a Power Macintosh 8100/100AV computer. Sequencesof raw images were played as film before analysis and quantitationto exclude cell movement. For NAD(P)H fluorescence, excitationwas at 380 nm, and light emitted near 470 nm was collected. Fluorescenceintensities were expressed in arbitrary pixel units. For pH_i measurements,cells were exposed for 30 min to the fluorescent dye BCECF-AM(5 mg/ml). After washout of extracellular dye, pH_i was measuredfrom the ratio of light emitted near 550 nm on excitation at 490and 440 nm after background substraction, as described (Bouvieret al., 1992).

[U-¹⁴C]glutamate uptake, ¹⁴C-alanine production from [U-¹⁴C]glucose and [NH₄⁺]. In experiments designed to determine the sodium dependenceof glutamate uptake, freshly isolated preparations of glial cellsattached to the basal membrane were washed in either normal (i.e.,Na⁺-containing) or Na⁺-free (choline replacing Na⁺) standard Ringer's solution for 15 min before transfer to closedincubation microwells at room temperature. Four preparations perincubation were used. ¹⁴C(U)-Glutamate was used at a concentration of 50 µM for the timesindicated in sodium- or choline-containing Ringer's solution (totalbath volume, 100 µl). Afterward, the bath was pipetted and thecells washed of adhering ¹⁴C(U)-glutamate, and both were stored in liquid nitrogen beforeHPLC analysis. During the protein assay, the basal membrane wasseparated from the glial cells.

In experiments involving the production of ¹⁴C-alanine from ¹⁴C(U)-glucose, glial cells (still attached to the basal membrane)from two retinas were incubated in standard Ringer's solution(no trehalose) carrying the indicated amounts of ¹⁴C(U)-glucose for 60 min in the presence of NH₄⁺ plus glutamate (1 mM each) or NH₄⁺ alone (1 mM). In controls, no glutamate or NH₄⁺ was added. For the determination of alanine and of glutamateinside the glial cells and in the corresponding bath, the preparationindicated as "fresh" in Figure 3 was exposed to proline (150 mM)during the final wash before being frozen in liquid nitrogen.Analysis of amino acids was performed with reverse-phase chromatographycoupled to precolumn derivatization with orthophthaldehyde andfluorescence detection (HP 1090 HPLC system, Hewlett-Packard,Palo Alto, CA) (Tsacopoulos et al., 1994; Poitry-Yamate et al.,1995).
Fig. 3. NH₄⁺ alone or NH₄⁺ plus glutamate causes an increase in alanine synthesis and release in glia. a, Amounts of alanine (Ala, openbars) and glutamate (Glu, filled bars) found in glial cells (left)and in the bathing solution (right); all values are expressedrelative to cell volume. Intraglial concentrations of glutamateand alanine decrease when cells are maintained for 60 min in Ringer'ssolution. On addition of NH₄⁺ (1 mM) or of glutamate and NH₄⁺ (1 mM each), both [glutamate]_i and [alanine]_i increased after60 min. The concentration of glutamate in glial cells was muchhigher than its actual concentration in the bath (bath volume> 100 × cells volume), indicating very restricted release andprobable accumulation. Glutamate plus NH₄⁺ or NH₄⁺ alone caused a significant increase (p < 0.001 and p < 0.02,respectively) in the biosynthesis and release of alanine intothe bath relative to control conditions. b, Specific radioactivityof alanine in the cells (left) and in the bath (right) after incubationfor 60 min in Ringer's solution containing either of two [U-¹⁴C]glucose concentrations. In the cells, only NH₄⁺ alone had a significant (p < 0.02) effect on the specific radioactivityof alanine. Alanine was the only amino acid labeled from [U-¹⁴C]glucose. All controls are pooled on the same column. Data areexpressed as mean ± SEM (n = 9).
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RESULTS

Ammonia transport and signaling
Ammonia essentially is produced in the mitochondria of photoreceptors (Fig. 1, left) and subsequently is released into theextracellular space (Tsacopoulos and Poitry, 1995; Coles et al.,1996a; Tsacopoulos et al., 1997). Previously, we showed that lightstimulation of honeybee retinal slices or exposure to dinitrophenol(both induce an increase in the O₂ consumption of photoreceptors;Tsacopoulos et al., 1987) causes an increased release of NH₄⁺ into the extracellular space. Recent measurements with NH₄⁺- and pH-sensitive microelectrodes showed that photoreceptors,within seconds of an increase in their oxidative metabolism, releasean increased amount of NH₄⁺/NH₃, which, in turn, induces an increase of pH in the interstitialcleft and NH₄⁺/NH₃ entry into presumably glial cells (Coles et al., 1996a).In keeping with these results, we observed that the intraglialpool of NH₄⁺ varies with the level of NH₄⁺ in the extracellular space (Fig. 1a, right). In addition, whenglial cells 3-8 hr after isolation were puffed with NH₄Cl, pH_ibecame acid (Fig. 1e), indicating that either NH₄⁺, rather than NH₃, entered the cells (Kikeri et al., 1989; Coleset al., 1996a) or that glycolysis was activated. This acidificationwas smaller than that measured under similar conditions aftera longer (2 min) exposure of the cells to 2 mM NH₄⁺ (Coles et al., 1996b). As shown in Figure 1b,c, puffs of NH₄Clat the glial surface caused up to a 100% increase in the fluorescenceof reduced nicotinamide adenine dinucleotides [i.e., NADH and/orNADPH, abbreviated in this text as NAD(P)H]. Exposure to 8 mMBaCl₂ from the bath reversibly suppressed this effect (Fig. 1c).Suppression also was observed on cell exposure to Na⁺-free (Fig. 2b) or to Cl-free solution (Fig. 1d), consistent with a strong decrease ofthe NH₄⁺-induced transient acidosis (Fig. 1e). Thus, NH₄⁺ entry into these glial cells shares properties with that in kidneycells (Kinne et al., 1986; Kikeri et al., 1989; Amlal et al.,1994), suggesting that it also may be mediated by a Na⁺/K⁺/2 Cl cotransporter and a barium-sensitive K⁺/H⁺ exchanger. This uptake system allows the entry of NH₄⁺ into glia, but not its exit. Thus, the slow recovery of [NH₄⁺] after a transient accumulation (Fig. 1a) probably reflects itschemical fixation in the process of alanine biosynthesis (seebelow). The extreme scarcity of mitochondria in drone glia (Tsacopouloset al., 1987; Coles, 1989), as well as the relative homogeneityof the basal fluorescence along the cells (Fig. 1b, right), favorsthe idea that the measured fluorescence was cytosolic. It is,however, difficult to determine whether it was attributable toNADH or to NADPH, because the spectral properties of these compoundsare almost identical. We suggest that the rapid rise of fluorescencein response to puffing NH₄Cl reflected an increase in the NADHlevel consecutive to an activation of glycolysis by NH₄⁺ ions. We do not exclude that NADH in excess then was convertedto NADPH, but this would require the presence of a transhydrogenase,which was not determined here. When the kinetics of intraglial $Delta$ NAD(P)H and $Delta$ pH in response to puffs of NH₄Cl were compared,no clear differences were revealed in their rising phases. However,citrate caused a larger and longer-lasting acidification thanNH₄⁺ but a correspondingly smaller change in NAD(P)H fluorescence(Fig. 1d,e). Hence, we suggest that transient increases in NAD(P)Hlevels are elicited by a direct, pH-independent action of NH₄⁺ on a glycolytic enzyme. Phosphofructokinase (PFK; ATP:D-fructose-6-phosphotransferase,EC2.7.1.11) is a possible target because it has been shown inmammalian brain extracts that NH₄⁺ acts on it as an allosteric activator (Lowry and Passonneau,1966). In agreement, activation of glycolysis in rat brains wasreported when NH₄⁺ concentration in the blood was raised from 0.01 to 1.74 mM (Hawkinset al., 1973).
Fig. 1. NH₄⁺ produced by oxidative metabolism in photoreceptors is taken up by glial cells, where it decreases pH_i and increases NAD(P)H.a, Left panel, [NH₄⁺] in whole retinal slices and in subcellular compartments. A,Fresh slice, immediately frozen; B, retinal homogenate; C, mitochondrialfraction of retinal homogenate. Right panel, Dependence of [NH₄⁺] in freshly isolated glial cells on incubating conditions. D,After 1 hr in 0-NH₄⁺, Ringer's solution; E, after 1 hr in 400 µM NH₄⁺; F, 1/2 hr after returning to 0-NH₄⁺; G, at 18 hr after returning to 0-NH₄⁺. Values are mean ± SEM (n = 10). b, Left panel, Increase of NAD(P)Hfluorescence in glial cells in response to puffing NH₄Cl; theincrease was larger and faster near the puffer tip (traces 2 and3). Puff duration, 20 sec. Arrows indicate times of capture offluorescence images shown on right panel. Numbers 1-3 correspondto analyzed cell regions (right panel, top). Right panel, Bundleof five isolated glial cells (top) and image of their basal (middle)and peak (bottom) NAD(P)H fluorescence captured after NH₄Cl puff.Pseudocolor scale of NAD(P)H fluorescence levels, with increasestoward red. Asterisk overlies NH₄Cl puffer. c, Exposure of glialcells to BaCl₂ (8 mM) reversibly suppressed NH₄Cl-induced $Delta$ NAD(P)Hresponse. d, NH₄⁺ at indicated concentrations, but not citrate, leads to significantNAD(P)H increases. Cl-free Ringer's solution suppresses the effect of NH₄⁺. e, pH_i changes elicited by same substances as in d. Resultsin d and e are means of n (superimposed on bars) measurements± SEM.
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Fig. 2. Glutamate induces in glial cells an increase of NAD(P)H fluorescence and a decrease of pH_i. a, A 20 sec puff of 0.5 mM glutamate(Glu), but not of 0.5 mM aspartate (Asp), induces NAD(P)H fluorescenceincrease. Puffing glutamate after aspartate (recovery) led toa slower rise in NAD(P)H fluorescence. b, Effect of glutamate(1 mM) on NAD(P)H fluorescence was reversibly suppressed whenNa⁺ in the bath was replaced by equimolar amounts of choline. Duringcholine exposure, puffing NH₄Cl in choline-Ringer's solution (secondtime bar) had no effect on fluorescence. Response to glutamatepartially recovered, 5 min after return to normal Na⁺ (recovery). Lower panel, Bundle of four glial cells and tipsof two puffers. c, Puffing 1 mM NH₄Cl after 1 mM glutamate inducesa further increase in NAD(P)H fluorescence. Puff duration in a-cwas 20 sec. d, Glutamate at three concentrations, but not aspartate,leads to significant NAD(P)H increases. e, Both glutamate andaspartate induce a significant, transient, intracellular acidosisin glial cells. Results in d and e are means of n (superimposedon bars) measurements ± SEM. f, Transport of radiolabeled [U-¹⁴C]glutamate into glia is Na⁺-dependent. Cells were exposed to 50 µM [U-¹⁴C]glutamate for the times indicated, in either Na⁺ or choline containing Ringer's solution. Each time point representsfour separate experiments (4 × 4 retinas) ± SEM.
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Glutamate transport and signaling
There is strong evidence that glutamate production and its nonvesicular release in the synapse-free honeybee retina (Coles,1989; Tsacopoulos et al., 1994) are predominantly neuronal. First,analysis of the retinal interstitial fluid in living honeybeesshowed that the concentration of glutamate there is 10 times higherthan in the hemolymph (Cardinaud et al., 1994), indicating retinalproduction and release. Second, when the intact retina is exposedto [¹⁵N]proline, which is consumed in the mitochondria of photoreceptors(Tsacopoulos et al., 1994), ¹⁵N-glutamate is produced and rapidly released into the extracellularspace (Tsacopoulos et al., 1997). Third, freshly isolated gliado not produce and release extracellularly measurable amountsof glutamate (Fig. 3a, right), and [glu]_i in isolated glial cellsis ~20-fold lower (Fig. 3a, left) than that measured in retinalslices (Tsacopoulos et al., 1994). Fourth, using an enzyme-basedglutamate-sensitive microelectrode (Innocent, 1995) positionednear the surface of freshly isolated honeybee photoreceptors (Tsacopouloset al., 1994), we measured a glutamate concentration of 2-4 µM(3 cells), whereas it was virtually zero in the surrounding bath.These findings suggest that glial cells take up glutamate releasedby photoreceptors. Because the production of alanine from glucoseis coupled to the recycling of NAD(P)⁺ via the activity of glutamate dehydrogenase (GDH; L-glutamate:NADoxidoreductase, deaminating; EC1.4.1.3) in glial cells (Tsacopouloset al., 1994; Veuthey et al., 1994) and because NH₄⁺/NH₃ feeds into this reaction consuming NAD(P)H (Fahien et al.,1971), we tested whether glutamate enters glial cells and modulatesNAD(P)H. Puffing glutamate (0.25-1 mM) onto individual glial cellscaused a net increase in NAD(P)H fluorescence (Fig. 2a-d), aswould be expected if glycolysis were activated and GDH activitywere decreased via product inhibition. Consistent with this hypothesis,when NH₄⁺ was puffed 20 s after glutamate, NAD(P)H fluorescence increasedfurther (Fig. 2c). The effect of glutamate on NAD(P)H was reversiblysuppressed when Na⁺ in the bathing solution was replaced by choline (Fig. 2b), indicatingthat glutamate enters glial cells through a high-affinity Na⁺-dependent glutamate transport system similar to that alreadydescribed for vertebrate glial cells (Brew and Attwell, 1987).Furthermore, cell exposure for ~40 min to 1 mM $beta$ -methyl-aspartate,an inhibitor of glutamate transporter (Kanai and Hediger, 1992),irreversibly suppressed the glutamate-induced $Delta$ NAD(P)H withoutsignificantly changing basal NAD(P)H fluorescence. To assess whetherglutamate is deaminated oxidatively to $alpha$ -ketoglutarate as a consequenceof product inhibition and Na⁺-dependent entry, we incubated bundles of glial cells with radiolabeledglutamate and followed its uptake and transformation over time(Fig. 2f). There was a rapid uptake of [U-¹⁴C]glutamate, and within 20 min the amount of [U-¹⁴C]glutamate that had accumulated in the cells approached a plateau(Fig. 2f), in part because there was in parallel a productionof ¹⁴C- $alpha$ -ketoglutarate (0.68 ± 0.17 mmol/l of glia/min; n = 16 cellbatches), which was released mainly in the bath. (Remarkably,there was no ¹⁴C-glutamine synthesized in these experiments, indicating thatglutamine synthetase is not active in these glial cells.) Thisis consistent with a sustained uptake and metabolism of glutamateby glia. The accumulation of [U-¹⁴C]glutamate was strongly Na⁺-dependent in accordance with the Na⁺ dependence of the NAD(P)H response (Fig. 2b,f).

The metabolic effect of glutamate in glia is not directly pH-dependent
In vertebrate retinal glial cells, exposure to glutamate causes a transient acidosis, probably because the glutamate uptakecarrier countertransports pH-changing anions (OH or HCO₃) (Bouvier et al., 1992). Because both mitochondria and carbonicanhydrase are absent in honeybee glial cells (Tsacopoulos et al.,1987; Walz, 1988), this countertransport is expected to be limitedto OH when these cells are isolated. We show that the glutamate-inducedacidosis was mild (Fig. 2e), in comparison with that recordedin vertebrate cells (Bouvier et al., 1992). Aspartate, which usesthe same transport carrier as glutamate (Christensen, 1990; Bouvieret al., 1992), caused a mild, transient acidosis of similar amplitudeto that induced by glutamate (Fig. 2e) but smaller than that causedby the weak acid citrate (Fig. 1e). In sharp contrast to glutamate,however, aspartate (Fig. 2a,d) and citrate (Fig. 1d) did not inducesignificant NAD(P)H fluorescence increases. It seems, therefore,that the glutamate-induced increase in NAD(P)H is attributableto a direct effect on a specific intracellular enzymatic target,probably cytosolic GDH (Veuthey et al., 1994), and not throughintracellular pH changes as suggested before (Bouvier et al.,1992).

Biochemical evidence of the metabolic effects of NH₄⁺ and glutamate in glia
In honeybee glial cells, where pyruvate is not reduced to lactate (Tsacopoulos et al., 1987), GDH works in tandem with alanineaminotransferase (ALAT; L-alanine:2-oxoglutarate aminotransferase;EC2.6.1.2) to produce alanine and NAD(P)⁺ (Fahien et al., 1971; Tsacopoulos et al., 1994; Veuthey et al.,1994; Tsacopoulos and Magistretti, 1996). The concentration ofpyruvate in these cells is low (below 0.2 mM). Consequently, therate of alanine synthesis should be controlled by the rate ofglycolytic production of pyruvate and the supply from the extracellularspace of glutamate at noninhibitory levels for GDH (Fahien etal., 1971). We provide biochemical support to this hypothesis:exposing glial cells to a mixture of 1 mM NH₄⁺ and 1 mM glutamate induced a large increase in the biosynthesisof alanine (Fig. 3a). Most significantly, the amount of alaninereleased into the bath under these conditions increased fivefoldas compared with controls, i.e., with no glutamate and no NH₄⁺ added to the bath (Fig. 3a, right). The effect of NH₄⁺ alone was significant but was less important than when combinedwith glutamate (Fig. 3a). We further asked whether alanine isalso produced from glycogen stores. Radiolabeled [U-¹⁴C]glucose therefore was added to the glial bath and thereby competedwith glycogen pools as the substrate for alanine formation (Fig.3b). The specific activity calculated for intracellular alaninewas very small at two different concentrations of [U-¹⁴C]glucose, consistent with the idea that the substrate for itsformation is mostly glycogen. The specific activity of alaninein the bath, however, was >10-fold higher than inside the cells(Fig. 3b, bottom panels), indicating that alanine is producedfrom both exogenous [U-¹⁴C]glucose and glycogen but that alanine produced from exogenousglucose is released more rapidly into the bath (Poitry-Yamateet al., 1995). The addition of 1 mM NH₄⁺ and 1 mM glutamate caused as much as a fivefold decrease in thespecific activity of alanine in the bath, whereas that insidethe cells increased further (Fig. 3b, bottom panels). This isprobably the consequence of a massive hydrolysis of glycogen causedby the pulling effect of increased glycolysis (Evêquoz-Mercierand Tsacopoulos, 1991). This mechanism is similar to that operatingin mammalian astrocytes, both fresh and cultured, with respectto glutamate signaling and lactate formation and release (Parpuraet al., 1994; Pellerin and Magistretti, 1994; Poitry-Yamate etal., 1995; Tsacopoulos and Magistretti, 1996).

DISCUSSION
We have explored the signal(s) by which neurons communicate to glia their need for energy substrate and at what level thesignals exert their metabolic effect in glia. The experimentalevidence presented in this paper shows that ammonium and glutamatereleased physiologically by neurons inform glial cells to increasetheir production and release of energy substrate.

Baseline levels of ammonia in honeybee retinal slices or homogenates are higher than in mammalian brain (Cooper and Plum,1987). However, as we have shown, the major part of ammonia isfound in the mitochondria, and this may be related to the consumptionof proline in this tissue. Although it is difficult to estimatethe cytosolic and extracellular levels of ammonia in the intactretina, it is quite likely that they are much less than the valuesreported in Figure 1a.

The model diagram based on our findings (Fig. 4) describes a novel way by which this arises. Ammonium and glutamate exerttheir signaling effect intracellularly and synchronously on threeenzymatic reactions in the glia: during activation, NH₄⁺ and glutamate operating at two sites (PFK and ALAT) acceleratethe production of alanine from pyruvate and of $alpha$ -ketoglutaratefrom glutamate. Alanine and $alpha$ -ketoglutarate are taken up by neuronsand contribute there to the homeostasis of the mitochondrial redoxpotential (Tsacopoulos et al., 1994). At the same time NH₄⁺ and glutamate have antagonistic effects at a third site (GDH).Thus, the overall effect of NH₄⁺ on glial metabolism is to increase the production of alanine,and that of glutamate is to adjust this production to the metabolicneeds of photoreceptors. In intact tissue, the operation of thisfine control during neuronal activity probably would result insmaller and faster $Delta$ NAD(P)H than those recorded in isolated cells,and the flux through GDH in glia might be expected to rise andfall with shifts of internal concentrations of glutamate and/orNH₄⁺. This signaling depends on functional plasma membrane transportsystems for NH₄⁺ and glutamate in glial cells and leads to the transformationof these molecules intracellularly. In metabolically active glialcells containing enough glycogen or in the presence of extracellularglucose, NH₄⁺ and glutamate taken up from the extracellular space do not accumulateintracellularly in excess, because they are transformed continuouslyto alanine and $alpha$ -ketoglutarate, respectively. It is conceivable,however, that in some pathological condition the metabolism ofglial cells is impaired, leading to the accumulation of NH₄⁺ and glutamate and therefore to swelling in glia (Albrecht etal., 1994). This would lead to a deficient fuelling of neuronsand possibly contribute to neuronal death.
Fig. 4. Model diagram of nitrogen and carbon metabolism in the honeybee retina showing the biochemical pathways involved in the traffickingof metabolites between glial cells and photoreceptors and showinghow NH₃/NH₄⁺ and glutamate may regulate glial metabolism. Glucose is metabolizedby glial cells to alanine, which is, in turn, transferred to photoreceptorsto fuel oxidative metabolism; the amino group carried by alanineleaves the photoreceptors as NH₃ and returns to glial cells asNH₄⁺, which enters the cells through a transport system similar tothat found in kidney cells. Proline, the second substrate foroxidative metabolism of photoreceptors, enters mitochondria, whereit is converted to glutamate and to glutamine. Both are releasedby photoreceptors; glutamate enters glial cells via a Na⁺-dependent carrier. For the return loop to photoreceptors, theglutamate carbon then leaves the glia as $alpha$ -ketoglutarate and glutamateN as alanine, as discussed by Yudkoff et al. (1986) for mammalianCNS. Nitrogen in excess can leave the retina either as NH₃/NH₄⁺ or glutamine. $alpha$ -KG, $alpha$ -Ketoglutarate; Ala, alanine; ALAT, alanineaminotransferase; GDH, glutamate dehydrogenase; Glu, glutamate;Gln, glutamine; Pro, proline; pyr, pyruvate.
[View Larger Version of this Image (62K GIF file)]

This tight regulation of metabolic coupling between neurons and glial cells by means of chemical signals turns the nourishingof neurons by glia into a function, instead of a passive process,as it is widely considered (see Pfrieger and Barres, 1995). Itis tempting to extrapolate some elements of the model presentedin Figure 4 to the vertebrate nervous system, even if differencesseem to exist. The Na⁺ dependence of glutamate uptake in glial cells, notably studiedin salamander Müller glial cells, shares similar properties tothat in the honeybee glial cells. The glutamate-induced increasein NAD(P)H fluorescence described here also was found in salamanderMüller cells, initially under somewhat artificial conditionsof voltage clamp (Barbour et al., 1993) and more recently in intact,acutely isolated Müller cells. Fluorescence image analysis revealedthat this increase occurs in all parts of the cell, includingthe mitochondria-free end feet (Uga and Smelser, 1973), thus suggestinga glutamate-induced increase in glycolytic NADH (Tsacopoulos andMacLeish, 1996).

Astroglial energy metabolism is stimulated by increased Na⁺ entry, probably via a specific activation of the Na⁺ pump (Takahashi et al., 1995). Because glutamate in astrogliais cotransported with Na⁺, this would lead to an increased [Na⁺]_i and stimulation of glucose metabolism. Recent results of Pellerinand Magistretti (1994) are in accordance with this prediction.The activation of the pump is, however, an unlikely explanationfor the metabolic effect of glutamate described in acutely isolatedretinal glial cells, because aspartate uses the same transporteras glutamate (Christensen, 1990) but, in contrast to glutamate,does not induce an increase in NAD(P)H either in honeybee glialcells (see Results) or in salamander Müller cells (Bouvier etal., 1992). Honeybee glial cells play a crucial role in the positioningof sodium pumps on the plasma membrane of the photoreceptor andin retaining the pumps at the contact sites. They have, however,very few pumping sites on their own membranes (Baumann and Takeyasu,1993). Indeed, pumping Na⁺ is not a crucial mechanism for spatial buffering of K⁺ by glia during neuronal stimulation in both the insect and vertebrateretina (Coles, 1989).

Apparently, the fixation of ammonia occurs differently in honeybee glial cells and astrocytes. In vertebrate nervous tissue,glutamine synthetase is localized predominantly within astrocytes(Norenberg and Martinez-Hernandez, 1979) and in Müller glialcells (Riepe and Norenberg, 1977), suggesting a predominant formationof glutamine there. Recently, Waniewski (1992) found that ammoniumat near-physiological concentrations (~100 µM) more than doublesthe rate of glutamate to glutamine transformation in astrocytecultures. This was evidence that the metabolism of glutamate toglutamine in astrocytes depends on extracellular ammonia. However,so that ammonia might be established as a metabolic signal inastrocytes, it is necessary to demonstrate that neuronal activityinduces an increase of NH₄⁺ production that does not lead to saturation of the glutamatesynthetase reaction occurring in astrocytes (K_m for NH₄⁺ is ~0.18 mM; Palmiljans et al., 1962). Contrary to astrocytes,the acutely isolated honeybee glial cells do not synthesize glutaminebut, instead, aminate pyruvate to alanine. Glutamine found inthis retina probably is formed in the mitochondria of photoreceptors,a compartment in which the availability of ATP is likely to behigher than in the mitochondria-poor glial cells. This assumptionis compatible with the finding in superfused slices of intacthoneybee retina that ¹⁵N-glutamine is formed from ¹⁵N-proline, a substrate known to be consumed predominantly in themitochondria of photoreceptors (Tsacopoulos et al., 1994, 1997).In any case, if there is a glutamate-glutamine cycle (see discussionby Yudkoff et al., 1992), nitrogen fixed on glutamine ultimatelymust return to astrocytes so that synthesis of amino acids cancontinue. Cultured astrocytes exposed to NH₄Cl for 4 d swell (Norenberget al., 1991), possibly indicating the existence of some unidirectionalNH₄⁺ transport system similar to the one we found in the honeybeeglial cells.

Glutamate signaling between cortical astrocytes and neurons was shown recently to occur in mammalian cell culture (Parpuraet al., 1994). However, the signaling that we have described inthe present paper goes further, confirming the function of glialcells in nourishing and maintaining nervous tissue.

FOOTNOTES

Received Sept. 24, 1996; revised Dec. 17, 1996; accepted Jan. 17, 1997.

This work was supported by Swiss National Science Foundation Grants 31-39426.93 and 31-37587.93 and the Georges Kernen Foundation.We thank Drs. D. Attwell, J. A. Coles, and L. Pizurki for criticalcomments and Mr. P. Perrottet for expert technical assistance.

Correspondence should be addressed to Dr. C. L. Poitry-Yamate, Experimental Ophthalmology Laboratory, University of GenevaMedical School, 1 Rue Michel-Servet, 1211 Geneva 4, Switzerland.

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