Extracellular ATP or ADP Induce Chemotaxis of Cultured Microglia through Gi/o-Coupled P2Y Receptors

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The Journal of Neuroscience, March 15, 2001, 21(6):1975-1982

Extracellular ATP or ADP Induce Chemotaxis of Cultured Microglia through G_i/o-Coupled P2Y Receptors
Shizuyo Honda¹, Yo Sasaki¹, Keiko Ohsawa¹, Yoshinori Imai¹, Yasuko Nakamura¹, Kazuhide Inoue², and Shinichi Kohsaka¹
¹ Department of Neurochemistry, National Institute of Neuroscience, 4-1-1 Ogawa-higashi, Kodaira, Tokyo 187-8502, Japan, and ² Division of Pharmacology, National Institute of Health Sciences, 1-18-1 Kamiyoga, Setagaya, Tokyo 158-8501, Japan

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The initial microglial responses that occur after brain injury and in various neurological diseases are characterized by microglialaccumulation in the affected sites of brain that results fromthe migration and proliferation of these cells. The early-phasesignal responsible for this accumulation is likely to be transducedby rapidly diffusible factors. In this study, the possibilityof ATP released from injured neurons and nerve terminals affectingcell motility was determined in rat primary cultured microglia.Extracellular ATP and ADP induced membrane ruffling and markedlyenhanced chemokinesis in Boyden chamber assay. Further analysesusing the Dunn chemotaxis chamber assay, which allows direct observationof cell movement, revealed that both ATP and ADP induced chemotaxisof microglia. The elimination of extracellular calcium or treatmentwith pyridoxalphosphate-6-azophenyl-2',4'-disulphonic acid, suramin,or adenosine-3'-phosphate-5'-phosphosulfate did not inhibit ATP-or ADP-induced membrane ruffling, whereas AR-C69931MX or pertussistoxin treatments clearly did so. As an intracellular signalingmolecule underlying these phenomena, the small G-protein Rac wasactivated by ATP and ADP stimulation, and its activation was alsoinhibited by pretreatment with pertussis toxin. These resultsstrongly suggest that membrane ruffling and chemotaxis of microgliainduced by ATP or ADP are mediated by G_i/o-coupled P2Yreceptors.

Key words: microglia; ATP; ADP; membrane ruffling; chemotaxis; G_i/o-coupled P2Y receptors

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Accumulated evidence suggests that extracellular ATP functions in various tissues and cells (Dubyak and El-Moatassim, 1993).The roles of extracellular ATP as a neurotransmitter and neuromodulatorin the CNS have been well documented. For example, ATP inducesexcitation and increases in calcium in various neurons in thebrain (Edwards et al., 1992; Shen and North, 1993; Chen et al.,1994; Inoue et al., 1995; Nabekura et al., 1995). In additionto the role played by ATP in neurons, effects of ATP on glialcells have also been demonstrated. In astrocytes, for example,DNA synthesis, process formation, and the increase in the expressionof glial fibrillary acidic protein (Neary et al., 1994), arachidonicacid release (Chen and Chen, 1998), Erk activation (Neary et al.,1999), and calcium wave propagation (Scemes et al., 2000) werereported to be stimulated by ATP. Ca²⁺ release from internal stores by ATP stimulation was also reportedin oligodendrocytes (Kirischuk et al., 1995). This evidence suggestsdiverse roles of extracellular ATP in theCNS.

Reports have shown that ATP stimulates microglia, another kind of glial cell in the CNS, to release various biologically activesubstances, such as interleukin-1 $beta$ (Ferrari et al., 1996, 1997),plasminogen (Inoue et al., 1998), and tumor necrosis factor- $alpha$ (Hide et al., 2000). Microglial cell death was also demonstratedafter stimulation with high-dose ATP (Ferrari et al., 1999). Afterneuronal damage, microglia migrate to the affected sites, wherethey function to secrete a variety of cytokines and neurotrophicfactors, to express major histocompatibility complex antigen classII, and in certain cases to perform phagocytic activities (Kreutzberg,1996; Thomas, 1999). For microglia to function in the proper regionof the brain, there must be a mechanism underlying the regulationof microglial motility. In fact, in regions of the facial nucleusaffected with neuronal damage after facial nerve axotomy, forinstance, the accumulation of microglia resulting from their proliferationand migration was clearly observed (Streit et al., 1988; Graeberet al., 1998; Ito et al., 1998). The search for factors influencingmicroglial motility is an important issue in understanding thefunction of microglia in brain pathology. To date, transforminggrowth factor- $beta$ , complement 5a (C5a), epidermal growth factor,and various kinds of chemokines have been reported to enhancemicroglial motility, and these factors have been postulated aspossible chemoattractants for microglia in brain (Yao et al.,1990; Hayashi et al., 1995; Nolte et al., 1996, 1997; Cross andWoodroofe, 1999). In the present study, we demonstrated that extracellularATP and ADP induced membrane ruffling and cell migration in themanner of chemoattraction, possibly mediated by G_i/o-coupled P2Yreceptors.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Microglial culture. Rat primary cultured microglia were prepared according to the method described previously (Nakajima etal., 1992). In brief, mixed glial culture was prepared from thecerebral cortex of neonatal Wistar rats and maintained for 12-23d in DMEM (Life Technologies, Grand Island, NY) with 10% fetalbovine serum (Irvine Scientific, Santa Ana, CA). Microglia wereobtained as floating cells over the mixed glial culture. The floatingcells were collected by a gentle shake and transferred to appropriatedishes or glasses, then the microglia attached to them were usedfor variousassays.

Membrane ruffling. The thus-prepared microglia were attached to glass coverslips (Matsunami, Osaka, Japan) coated with 100µg/ml of poly-L-lysine (Sigma, St. Louis, MO). After attachmentfor 2 hr, microglia were washed with serum-free DMEM and starvedfor 4 hr in the same medium. They were then stimulated with ATP(Yamasashyoyu, Chiba, Japan), ADP (Sigma), UTP (Wako Pure ChemicalIndustries, Osaka, Japan), and adenosine (Sigma) at 50 µM, orrecombinant murine macrophage colony stimulating factor (M-CSF)(R & D Systems, Minneapolis, MN) at 100 ng/ml for 5 min at 37°C.In the control, cells were treated with PBS instead of nucleotides.The reaction was stopped by the addition of PBS containing 3.7%formaldehyde. After fixation for 5 min and washing with PBS, thecells were permeabilized with PBS containing 0.1% Triton X-100for 5 min and washed three times with PBS. To visualize membraneruffling, cells were stained with Texas Red-conjugated phalloidin(Texas Red-X Phalloidin) (Molecular Probes, Eugene, OR) and observedunder the fluorescence microscope PROVIS AX (Olympus, Tokyo, Japan).In the experiments to determine the effects of inhibitors, cellswere preincubated with suramin (Wako) (300 µM), pyridoxal-phosphate-6-azophenyl-2',4-disulphonicacid tetrasodium salt (PPADS) (Research Biochemicals International,Natick, MA) (300 µM), adenosine-3'-phosphate-5'-phosphosulfate(A3P5PS) (Sigma) (300 µM), or AR-C69931MX (AstraZeneca UK Limited,London, UK) (1 µM) for 10 min after starvation and then stimulatedwith nucleotides. The cells were also preincubated with pertussistoxin (PTx) (Sigma) (50 ng/ml) for 4hr.

To evaluate extracellular calcium dependency, attached microglia were washed with Ca²⁺-containing balanced salt solution (BSS) [(in mM): 150 NaCl, 5.0KCl, 1.2 MgCl₂, 25 HEPES, 10 D-glucose, and 1.2 CaCl₂] or Ca²⁺-free BSS [in mM: 150 NaCl, 5.0 KCl, 1.2 MgCl₂, 25 HEPES, 10 D-glucose,and 1 EGTA] (Inoue et al., 1998) and stimulated with nucleotidesin the sameBSS.

Chemokinesis assay using the Boyden chamber. Chemokinesis of microglia was assessed using the Boyden chamber (Neuroprobe,Bethesda, MD) according to the method described previously (Yokomizoet al., 1997). In brief, polycarbonate filters (5 µm pore) werecoated with 10 µg/ml fibronectin (Sigma) in PBS for 60 min. Adry coated filter was installed in the Boyden chamber, whose bottomwells were filled with serum-free DMEM containing nucleotidesat the various concentrations indicated. Freshly prepared microgliawere suspended in serum-free DMEM containing nucleotides at thesame concentration as that in each bottom well, and the cell suspensionwas placed into the top wells (2-5 × 10⁴ cells/well). The chamber was kept in a CO₂ incubator at 37°Cfor 90 min. The filter was removed and stained with 0.05% crystalviolet, 12% formaldehyde, and 10% ethanol in PBS. The cells onthe top side of the filter were wiped off, and the number of cellsthat had migrated to the bottom side was measured at 595 nm witha BioLumin 960 fluorescence/absorbance microassay reader (Pharmacia-LKB,Uppsala,Sweden).

Chemotaxis assay using the Dunn chemotaxis chamber. Chemotaxis was assessed by the Dunn chemotaxis chamber (Weber ScientificInternational Ltd., Teddington, UK), which allows direct observationof cell movement. The assay was performed according to the methoddescribed in the previous report (Webb et al., 1996). In brief,microglia were attached to square coverslips for 2 hr, washedthree times with serum-free DMEM, and kept for 4-16 hr until thechemotaxis assay was performed. After starvation, the coverslipwas placed over the chamber, whose outer and inner wells werefilled with DMEM. The coverslip was sealed with a 1:1 mixtureof molten paraffin wax and Vaseline around three edges to leavea slit for exchange of the medium in the outer well. To observethe chemically directed cell migration, the medium in the outerwell was exchanged through the slit for DMEM containing 50 µMATP or ADP. Then the last edge of the coverslip was sealed immediately,and the chamber was set on the stage of a microscope (ECLIPSETE300; Nikon, Tokyo, Japan), which was maintained at 37°C. Controlexperiments were performed under the condition in which both outerand inner wells were filled withDMEM.

A region of the bridge was viewed via a CCD video camera (Hamamatsu Photonics, Hamamatsu, Japan), and the phase-contrast imageswere recorded every 5 min during 1 hr of observation using imagingsoftware (fishPPC; Hamamatsu Photonics). The straight distancebetween the starting point and the point of a cell reached after1 hr was measured by plotting the point of the microglial nucleuson a computer display using drawing software. The distance anddirection were shown as x,y coordinates on scatter diagrams whosex-axis was positioned parallel to the outer edge of thebridge.

Rac translocation. To determine the translocation of Rac to the region of membrane ruffling, double staining was performedafter stimulating the cells with ATP or ADP. After fixation, thecells were incubated with mouse anti-human Rac antibody (UpstateBiotechnology, Lake Placid, NY) and fluorescein isothiocyanate(FITC)-conjugated anti-mouse IgG (BioSource, Sunnyvale, CA). F-actinwas stained with Texas Red-conjugated phalloidin. Images wereobtained with a confocal laser-scanning microscope CLSM2010 (Pharmacia-LKB).

Pull-down assay of Rac. Activated Rac was measured by the method described previously (Manser et al., 1998; Ohsawa et al.,2000). In brief, the microglia attached to dishes for 2 hr werewashed with serum-free DMEM and starved for 4 hr with or withoutpertussis toxin (50 ng/ml). The starved microglia were stimulatedwith 50 µM ATP or ADP for 1 min, and lysed in lysis buffer A (25mM HEPES, pH 7.3, 0.15 M NaCl, 5 mM MgCl₂, 0.5 mM EGTA, 20 mM $beta$ -glycerophosphate, 0.5% Triton X-100, 4% glycerol, 10 mM NaF,2 mM sodium orthovanadate, 5 mM dithiothreitol, 0.5 mM phenylmethylsulfonylfluoride, 10 µM leupeptin, and 10 µM pepstatin). The lysates werecentrifuged at 12,000 × g to remove debris. Part of the supernatantwas mixed with SDS sample buffer, and the remainder was incubatedfor 30 min at 4°C with glutathione S-transferase (GST)-fused p21-activatedkinase (PAK) that was coupled to Glutathione Sepharose 4B beads(Pharmacia Biotech). After incubation, the samples were centrifugedat 500 × g and washed twice with lysis buffer A. The precipitatedbeads were boiled with SDS sample buffer. The total cell lysatesand pull-down samples were subjected to SDS-PAGE using 10-20%gradient gel (Daiichi Pure Chemicals, Tokyo, Japan), immunoblottedwith anti-Rac antibody and horseradish peroxidase (HRP)-conjugatedanti-mouse antibody (Pharmacia), and visualized with ECL Westernblotting detection reagents(Pharmacia).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

ATP- and ADP-induced membrane ruffling in microglia

We first examined extracellular ATP in terms of morphology and ruffle formation in microglia after 5 min of stimulation witheither 50 µM ATP, ADP, UTP or adenosine by staining with TexasRed-conjugated phalloidin. Freshly prepared microglia showed theramified morphology after 4 hr of incubation in serum-free medium.After the addition of PBS (control), there was no change in morphology(Fig. 1A). However, as shown in Figure 1B, the cells were spreadand showed amoeboid-like morphology at 5 min after ATP stimulation.The structure of membrane ruffling was clearly observed by stainingwith phalloidin. The prominent morphological change that occurredwith ruffle formation was also detected with extracellular ADP(Fig. 1C). Although UTP induced obvious morphological change,ruffle formation was not significant (Fig. 1D). The morphologicalchanges of microglia induced by ATP, ADP, and UTP were observedin almost all of the stimulated cells. By contrast, adenosineinduced neither morphological change nor ruffle formation (datanot shown).

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Figure 1. Nucleotide-induced membrane ruffling in microglia. The cells were stimulated with PBS (A) or 50 µM ATP (B), ADP (C), or UTP (D) for 5 min. After fixation, the cells were stained with Texas Red-conjugated phalloidin. ATP and ADP clearly induced membrane ruffling (indicated by arrows). Scale bar, 20 µm.

ATP- and ADP-enhanced chemokinesis of microglia in the Boyden chamber

Membrane ruffles are structures that are found primarily at the front edges of migrating cells (Lauffenburger and Horwitz,1996). To investigate whether the nucleotides that induce membraneruffling act as a chemoattractant for microglia, a chemotaxisassay using the Boyden chemotaxis chamber was initially performed.In assessing chemotaxis in the Boyden chamber, we usually observecell migration under two assay conditions, one in which the ligandis in only the bottom compartment and the other in which it isin both the bottom and top compartments. We preliminarily comparedthe two kinds of microglial migration stimulated by ATP and foundthat cell migration was enhanced in both cases (data not shown).This preliminary result indicated that ATP-induced cell migrationdetected in the Boyden chamber is chemokinesis (enhanced migrationwithout chemical gradient). Although we could not evaluate ATP-inducedchemotaxis in this assay system, we collected data on the chemokinesisinduced by nucleotides. As shown in Figure 2, ATP clearly promotedthe chemokinesis of microglia in a dose-dependent manner. ADPexerted a more marked effect than ATP on the chemokinesis of microglia,whereas UTP had no effect (Fig. 2). Unlike nucleotide-inducedcell migration, we were able to assess the chemotaxis of microgliain the Boyden chamber by stimulation with C5a. C5a-induced cellmigration could be detected only when the ligand was in the bottomcompartment. Under this condition, almost the same extent of cellmigration was observed between ATP (50 µM)- and C5a (1 µM)-inducedchemotaxis at 90 min of incubation (data not shown).

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Figure 2. Nucleotide-induced chemokinesis of microglia in the Boyden chamber. The cells were exposed to ATP (circle), ADP (square), or UTP (triangle) for 90 min. Nucleotides were added to both top and bottom wells at the concentrations indicated. The absorbance of the stained cells on the bottom side of the filter was measured with a plate reader. Each point and vertical line represent the mean and SD for three wells. We confirmed that the three independent experiments showed the same tendency.

ATP- and ADP-induced chemotaxis of microglia in the Dunn chemotaxis chamber

To evaluate whether the nucleotides induced chemotaxis of microglia, we performed another cell migration assay using the Dunnchemotaxis chamber, which allows direct observation of cell movement.The displacements of cells after 1 hr of incubation were plottedas x,y coordinates on scatter diagrams (Fig. 3A). As shown inFigure 3Aa, microglia have weak motility in the absence of ligands.Compared with that, the great majority of cells that were incubatedin the gradient of ATP or ADP migrated toward the source of ligands(Fig. 3Ab,Ac), whereas UTP did not induce migration (Fig. 3Ad).Two-tailed Student's t tests showed that none of the mean valuesof x components that were measured for the cells stimulated withATP (4.07 µm), ADP (7.68 µm), or UTP ( $-$ 1.76 µm) was significantlydifferent from that of control cells without stimulation (1.58µm) (p > 0.05). By contrast, the mean value of the y componentthat was measured for cells stimulated with UTP (1.29 µm) wasnot significantly different from that without nucleotides ( $-$ 0.91µm), whereas each of the mean y components that was measured forthe cells stimulated with ATP (53.04 µm) or ADP (51.30 µm) wassignificantly different from the control (p < 0.0001). Representativeimages obtained 5 min and 30 min after setting the coverslip inthe chamber are presented in Figure 3B. The cells produced membraneruffles at 5 min, as indicated by arrowheads, and migrated tothe ATP gradient (vertically upward) at 30 min. These resultsindicated that extracellular ATP and ADP promote microglial motilityin the manner of chemoattraction, which may have been mediatedby P2 receptors.

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Figure 3. Nucleotide-induced chemotaxis of microglia in the Dunn chemotaxis chamber. A, Vector diagrams of cell displacement at 60 min after setting up the chamber. The cells were incubated in the absence of nucleotides (a) or in the presence of 50 µM ATP (b), ADP (c), or UTP (d) in the outer well. The position of the outer well of the chamber is vertically upward. All diagrams were obtained from a representative experiment using the same lot of microglial culture. We confirmed that the three independent experiments showed the same tendency. B, Displacement and morphological change at 5 and 30 min after setting up the chamber. The cells were incubated in the presence of 50 µM ATP in the outer well. The images of the same area are presented such that the position of the outer well of the chamber is vertically upward. Arrowheads indicate membrane ruffles.

Determination of subtype of P2 receptors

P2 receptors have been divided into two types, ionotropic P2X and G-protein-coupled P2Y receptors (Barnard et al., 1997).P2X receptors act as ligand-gated, nonselective cation channels.We have previously demonstrated that ATP-induced plasminogen releasefrom microglia depends on extracellular-Ca²⁺ influx via P2X₇ receptors (Inoue et al., 1998). To identify thetypes of P2 receptors involved in ATP- and ADP-induced membraneruffling, we examined the effect of extracellular calcium deprivation.Unlike the plasminogen release (Inoue et al., 1998), ATP and ADPinduced membrane ruffling in Ca²⁺-free BSS as well as in Ca²⁺-containing BSS (Fig. 4). These results suggest that the membraneruffling induced by ATP and ADP is not dependent on extracellularCa²⁺ influx via ionotropic P2X receptors, but is mediated by P2Y receptors.

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Figure 4. Effect of extracellular calcium deprivation on membrane ruffling induced by ATP or ADP. Cells were stimulated with PBS (A, D), 50 µM ATP (B, E), or 50 µM ADP (C, F) in BSS with (A-C) or without (D-F) calcium. After stimulation, the cells were fixed and stained with Texas Red-conjugated phalloidin. Arrowheads indicate membrane ruffles. Scale bar, 20 µm.

In our experiments, ATP and ADP acted as potent agonists, whereas UTP exerted only a slight effect on membrane ruffling. Somereports have shown that human P2Y₁, among various P2Y receptors,is activated by ADP and that mouse P2Y₂ is equally activated byATP and UTP (Lustig et al., 1993; Léon et al., 1997). Althoughsome discrepancy exists regarding the potency of UTP, we speculatedthat P2Y₁ or P2Y₂ might be a possible receptor for ADP- or ATP-inducedmembrane ruffling and cell migration. We examined this possibilityusing three kinds of selective antagonists, suramin, PPADS, andA3P5PS. Charlton et al. (1996) reported that suramin caused antagonisticeffects on turkey P2Y₁ and human P2Y₂ expressed in human astrocytomacell line 1321N1, whereas PPADS antagonized the effects via P2Y₁and not P2Y₂. A3P5PS was reported as a selective antagonist ofthe P2Y₁ receptor (Boyer et al., 1996). By contrast, pretreatmentwith a rather high dose (300 µM) of PPADS, suramin, or A3P5PSdid not inhibit the ATP- and ADP-induced membrane ruffling inmicroglia, as shown in Figure 5. These data suggest that neitherP2Y₁ nor P2Y₂ plays a main role in the ADP- and ATP-evoked responsesin microglia.

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Figure 5. Effects of PPADS, suramin, and A3P5PS on nucleotide-induced membrane ruffling. Microglia were stimulated with 50 µM ATP (B, E, H, K) or ADP (C, F, I, L) for 5 min after 10 min of pretreatment with PBS (A-C), 300 µM suramin (D-F), 300 µM PPADS (G-I), or 300 µM A3P5PS (J-L). After fixation, the cells were stained with Texas Red-conjugated phalloidin. Arrowheads indicate membrane ruffles. Scale bar, 20 µm.

Inhibition of membrane ruffling by AR-C69931MX and pertussis toxin

P2T_AC receptors, which are highly sensitive to ADP but distinct from P2Y₁, have recently been predicted to be present in platelets(Daniel et al., 1998), although they have not yet been cloned.Therefore, we examined the effect of AR-C69931MX, a potent andselective antagonist against P2T_AC receptors (Ingall et al., 1999;Ishii-Watabe et al., 2000), on ATP- and ADP-induced membrane ruffling.Pretreatment with 1 µM AR-C69931MX completely inhibited ATP- andADP-induced membrane ruffling in microglia, whereas the same treatmentdid not inhibit M-CSF-induced membrane ruffling (Fig. 6). Theantagonistic effect of AR-C69931MX was further confirmed againstthe poorly hydrolyzable analog ATP $gamma$ S (50 µM) (data not shown).These receptors were also reported to be PTx-sensitive (Danielet al., 1998). To verify the possibility of this type of P2 receptorbeing involved, we further examined the effects of PTx on ATP-and ADP-induced membrane ruffling and chemokinesis. The 4 hr pretreatmentwith PTx at 50 ng/ml completely inhibited membrane ruffling inducedby ATP and ADP (Fig. 7), whereas M-CSF-induced membrane ruffling,which is well known to be mediated by a tyrosine kinase receptor,Fms, was not affected by PTx. Furthermore, the pretreatment withPTx also inhibited ATP-induced chemokinesis in the Boyden chamberassay (Fig. 8). These results strongly suggest that G_i/o-coupledP2Y receptors, most likely P2T_AC receptors, are involved in themembrane ruffling and chemotaxis of microglia induced by ATP orADP, although precise identification of the specific receptorremains unclear.

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Figure 6. Effect of AR-C69931MX on nucleotide-induced membrane ruffling. Microglia were stimulated with 50 µM ATP (B, F) or ADP (C, G) or 100 ng/ml M-CSF (D, H) for 5 min after 10 min of pretreatment with PBS (A-D) or 1 µM AR-C69931MX (E-H). After fixation, the cells were stained with Texas Red-conjugated phalloidin. Arrowheads indicate membrane ruffling. Scale bar, 20 µM.

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Figure 7. Effects of PTx on nucleotide-induced membrane ruffling. Microglia were stimulated with PBS (A, E), 50 µM ATP (B, F), 50 µM ADP (C, G), or 100 ng/ml M-CSF (D, H) for 5 min after 4 hr of pretreatment with PBS (A-D) or 50 ng/ml pertussis toxin (E-H). After fixation, the cells were stained with Texas Red-conjugated phalloidin. Arrowheads indicate membrane ruffles. Scale bar, 20 µm.

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Figure 8. Effect of PTx on ATP-induced chemokinesis in the Boyden chamber. The chemokinesis assay was performed in the presence of 50 µM ATP with (white column) or without (black column) pertussis toxin treatment. Cells were pretreated with 50 ng/ml PTx for 4 hr.

ATP- and ADP-induced Rac activation in microglia

Finally, to determine whether ATP- and ADP-induced membrane ruffling and chemotaxis of microglia are mediated by G_i/o-coupledP2Y receptors, intracellular signaling was investigated. It hasbeen well established that the Rho family of small G-proteinsare key molecules in the reorganization of actin cytoskeleton(Hall, 1998). Among the Rho family, Rac is known to be activatedwhen cells form membrane ruffles and lamellipodia (Ridley et al.,1992; Ohsawa et al., 2000). Activated Rac was found to be translocatedto the membrane after stimulation (Ridley et al., 1992; Bokochet al., 1994). Thus, we performed double staining to examine thetranslocation of Rac after ATP or ADP stimulation by using TexasRed-conjugated phalloidin (red) and anti-Rac antibody visualizedwith FITC-conjugated secondary antibody (green) (Fig. 9A). Wecould detect the translocation of Rac to the ruffling region colocalizedwith phalloidin staining 5 min after stimulation.

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Figure 9. Rac activation induced by ATP and ADP. A, Translocation of Rac. The cells were stimulated with PBS (a-c), 50 µM ATP (d-f), or 50 µM ADP (g-i) for 5 min and stained with Rac antibody and FITC-conjugated anti-mouse IgG (a, d, g) and Texas Red-conjugated phalloidin (b, e, h). Merged photographs show the colocalization of Rac and F-actin in the ruffling region (f, i), as indicated by arrows. Scale bar, 10 µm. B, Pull-down assay of activated Rac. Cells were stimulated with PBS (control), 50 µM ATP, or 50 µM ADP for 1 min, and pull-down assay was performed as described in Materials and Methods. Although the total amount of Rac in the cell lysate was the same for each stimulation, activated Rac was increased in the pull-down samples from ATP- and ADP-stimulated cells.

To confirm Rac activation, activated Rac was biochemically measured. Because activated Rac is known to bind to PAK kinase(Manser et al., 1998), a pull-down assay was performed using GST-fusedPAK to detect the GTP-bound form of Rac. In samples from cellsthat were stimulated with ATP or ADP for 1 min, more of the activeform of Rac was pulled down as compared with that in control cells(Fig. 9B). At the same time, we confirmed that the total amountof Rac in the cell lysates in controls was the same as that inthe nucleotide-treated cells (Fig. 9B). Moreover, pretreatmentof the cells with PTx completely blocked the activation of Racinduced by ATP or ADP (Fig. 10). These results further supportthe idea that ATP- and ADP-induced membrane ruffling and chemotaxisare mediated by G_i/o-coupled P2Y receptors.

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Figure 10. Effect of PTx on the nucleotide-induced activation of Rac. Pull-down assay was performed, as described in Materials and Methods. Microglia were stimulated with PBS (control), 50 µM ADP, 50 µM ATP, or 100 ng/ml M-CSF for 1 min after 4 hr of treatment with (+) or without ( $-$ ) PTx at 50 ng/ml.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In the present study, we demonstrated that extracellular ATP and ADP strongly enhanced the formation of membrane ruffles andchemotaxis of microglia. Nucleotide-induced chemotaxis has beenreported in rat mast cells (McCloskey et al., 1999) and humanneutrophils (Verghese et al., 1996) by using the Boyden chamberassay. We found that ATP and ADP enhanced chemokinesis in theBoyden chamber assay. Although we could not determine whethernucleotides played a role as chemoattractants on microglia bythe Boyden chamber assay, the Dunn chemotaxis chamber, which allowsthe direct observation of cell migration, revealed that the nucleotideshad the potency to induce chemotaxis of microglia. The reasonwe were unable to detect the chemotactic activity of nucleotidesin the Boyden chamber assay seems to be partly that the low molecularweight nucleotides easily diffuse from the bottom to the top compartmentof the Boyden chamber. Considering the strong effect of ADP, itis highly probable that the effects of ATP actually depend onthe metabolite ADP, which may be easily produced during incubation.However, the possibility is very slight because ATP $gamma$ S (10 µM)had the same effect as ATP (data notshown).

Considering the physiological effect of nucleotides on microglia, it is important to identify P2 receptor subtypes. P2 receptorshave been divided into two types, ionotropic P2X, and G-protein-coupledP2Y receptors (Barnard et al., 1997). Although no study has clarifiedthe profile of P2-receptor subtype expression in microglia, theexistence of several kinds of P2Y and P2X receptors has been suggestedfrom electrophysiological studies (Nörenberg et al., 1997; Visentinet al., 1999). The biological effects of ATP on microglia havebeen suggested to be mediated mainly by P2X₇ receptors (Ferrariet al., 1996, 1997, 1999; Inoue et al., 1998; Hide et al., 2000).The present study, however, suggests the involvement of P2Y receptorsin nucleotide-induced ruffle formation and cell migration, basedon the experiments of extracellular-calcium elimination and AR-C69931MXor PTxtreatment.

To date, seven G-protein-coupled P2Y receptors have been cloned in mammalian species, some of which have not been fully characterizedin nature (Alexander et al., 1999). Suramin, PPADS, and A3P5PSare commonly used for the pharmacological classification of thesubtypes of P2Y receptors. Suramin is an antagonist for both P2Y₁and P2Y₂, whereas PPADS antagonizes P2Y₁ but not P2Y₂ (Charltonet al., 1996). A3P5PS is a potent and selective antagonist ofP2Y₁ (Boyer et al., 1996). Although we examined the effects ofthese antagonists on ATP- and ADP-induced membrane ruffling inmicroglia, we did not observe any inhibitory effect. Based onthe previous reports described above, neither P2Y₁ nor P2Y₂ wouldbe involved in nucleotide-induced membrane ruffling ofmicroglia.

Recently, G_i/o-coupled P2Y receptors, designated P2TAC receptors, which are highly sensitive to ADP, were predicted in platelets(Daniel et al., 1998), although they have not yet been cloned.Based on the results showing that the effects of nucleotides onmicroglial motility were completely blocked by either AR-C69931MXor PTx pretreatment, this type of G_i/o-coupled receptor is postulatedas a candidate for the P2Y receptors involved in membrane rufflingand chemotaxis. However, there are a few reports suggesting thatP2Y₂ is partially sensitive to PTx in the stable expression systemof 1321N1 astrocytoma cells (Parr et al., 1994) and in human erythroleukemiacells (Baltensperger and Porzig, 1997). P2Y₁ was also suggestedto be PTx-sensitive in astrocytes (Chen et al., 1998), whereasSchachter et al. (1997) clarified the uncoupling of P2Y₁ to G_i/oby using the system of expression in 1321N1 cells. Under thesecircumstances, in which contradictory reports have been issued,the specific G_i/o-coupled subtype of P2Y receptors involved inthe present effects cannot be defined. Further characterizationof P2Y receptors, including cloning of the P2TAC receptor isneeded.

With regard to the intracellular signaling downstream of the G_i/o-coupled P2Y receptors, we were able to detect Rac activationin microglia when the cells formed membrane ruffles after ATPor ADP stimulation. Furthermore, PTx-induced inhibition of Racactivation indicates a signal cascade from G_i/o-coupled-P2Y receptorsto Rac activation. Rac is a member of the Rho family of smallG-proteins, and Rac activation is known to induce lamellipodiaand membrane ruffles in various kinds of cells (Ridley et al.,1992; Hall, 1998). There has been cumulative evidence suggestingof the activation of Rac via heterotrimeric G-proteins. Ma etal. (1998) suggested that cytoskeletal reorganization by fMLP(N-formyl-Met-Leu-Phe) is dependent on Rac, Vav, a guanosine exchangefactor of Rac, and phosphoinositide 3-kinase $gamma$ (PI3K $gamma$ ), in Cos-7SHcells. Although Rac activation still occurred in neutrophils obtainedfrom PI3K $gamma$ and PLC $beta$ 2/3 knock-out mice, chemokine-mediated chemotaxiswas impaired in PI3K $gamma$ knock-out mice (Li et al., 2000). Such signalingmolecules may be involved in microglia. The possibility of thepresent findings having been physiologically involved with thefunction of microglia in the pathological states of the brainmay beconsidered.

In brain with damaged neurons and astrocytes, large amounts of nucleotides are released from these cells (Dubyak and El-Moatassim,1993; Neary et al., 1996). The extracellular nucleotides, whichare easily diffused and rapidly catalyzed by ATPases, may playa role in modulating the microglial function of the brain in theearly phase of pathology. We presented a novel effect of nucleotideson microglia, that is, the induction of chemotaxis via G_i/o-coupledP2Y receptors. Considering former studies that have revealed thebiological effects of nucleotides on microglia such as the releaseof IL-1 $beta$ , plasminogen, and TNF- $alpha$ via P2X₇ (Ferrari et al., 1996,1997, 1999; Inoue et al., 1998; Hide et al., 2000), our resultssuggest that two distinct P2X and P2Y receptor subtypes are involvedin the diverse functions of microglia, such as scavenging andneuroprotective actions, in pathologicalstates.

  FOOTNOTES

Received Aug. 10, 2000; revised Dec. 29, 2000; accepted Jan. 2, 2001.

This work was supported by a grant from the Organization for Pharmaceutical Safety and Research and by a Grant-in-Aid forthe Scientific Research on Priority Areas from the Ministry ofEducation, Science, Sports, and Culture of Japan. AR-C69931MXwas kindly supplied from AstraZeneca UK Limited (London,UK).
Correspondence should be addressed to Shinichi Kohsaka, Department of Neurochemistry, National Institute of Neuroscience,4-1-1 Ogawa-higashi, Kodaira, Tokyo 187-8502, Japan. E-mail: kohsaka{at}ncnp.go.jp.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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