Upregulation of the Enzyme Chain Hydrolyzing Extracellular ATP after Transient Forebrain Ischemia in the Rat

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The Journal of Neuroscience, July 1, 1998, 18(13):4891-4900

Upregulation of the Enzyme Chain Hydrolyzing Extracellular ATP after Transient Forebrain Ischemia in the Rat
Norbert Braun¹, Yuan Zhu², Josef Krieglstein², Carsten Culmsee², and Herbert Zimmermann¹
¹ Biozentrum der J.W. Goethe-Universität, AK Neurochemie, D-60439 Frankfurt am Main, Germany, and ² Institut für Pharmakologie und Toxikologie, Phillips-Universität, D-35032 Marburg, Germany

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

A short ischemic period induced by the transient occlusion of major brain arteries induces neuronal damage in selectivelyvulnerable regions of the hippocampus. Adenosine is consideredto be one of the major neuroprotective substances produced inthe ischemic brain. It can be released from damaged cells, butit also could be generated extracellularly from released ATP viaa surface-located enzyme chain. Using the rat model of globalforebrain ischemia, we applied a short (10 min) transient interruptionof blood flow and studied the distribution of ectonucleotidaseactivities in the hippocampus. Northern hybridization of mRNAisolated from hippocampi of sham-operated and ischemic animalsrevealed an upregulation of ectoapyrase (capable of hydrolyzingnucleoside 5'-tri- and diphosphates) and ecto-5'-nucleotidase(capable of hydrolyzing nucleoside 5'-monophosphates). A histochemicalanalysis that used ATP, UTP, ADP, or AMP as substrates revealeda strong and selective increase in enzyme activity in the injuredareas of the hippocampus. Enhanced staining could be observedfirst at 2 d. Staining increased within the next days and persistedat 28 d after ischemia. The spatiotemporal development of catalyticactivities was identical for all substrates. It was most pronouncedin the CA1 subfield and also could be detected in the dentatehilus and to a marginal extent in CA3. The histochemical stainingcorresponded closely to the development of markers for reactiveglia, in particular of microglia. The upregulation of ectonucleotidaseactivities implies increased nucleotide release from the damagedtissue and could play a role in the postischemic control of nucleotide-mediatedcellular responses.

Key words: astrocyte; ectoapyrase; ecto-ATPase; ecto-5'-nucleotidase; ischemia; microglia

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Following global ischemia, neurons in specific subfields of the hippocampus reveal selective vulnerability. Neuronal deathtakes a characteristic delayed time course and becomes evidentat the light microscopic level 2-4 d after ischemia. It is accompaniedby a typical glial reaction involving both astrocytes and microglia(Kraig et al., 1995). Reactive astrocytes display hypertrophy,increased staining for the intermediate filament glial fibrillaryacidic protein (GFAP), and hyperplasia. In regions of permanentischemic injury astrocytes also express vimentin. From postischemicday 1 onward, microglia proliferate and show increased expressionof major histocompatibility complex (MHC) class I and II immunomoleculesat their surface and finally transform into intrinsic brain phagocytes,removing neuronal debris. Reactive astrocytes and microglia undergoa considerable number of additional specific functional changes,including the upregulation of many protein species and the secretionof cytokines and growth factors (Eddleston and Mucke, 1993; Gehrmannet al., 1995). Some of these may mediate tissue damage. Othersplay an important role in limiting the extent of damage or alsoa role in tissue repair.

A loss of energy charge resulting from the interrupted blood supply results in a massive release of excitatory neurotransmitters.Glutamate is considered to play a major role in cytotoxicity byinducing an intracellular and lethal increase in neuronal Ca²⁺. Extracellular adenosine is increased as an early response toischemia and may, in turn, exert neuroprotective actions by inhibitingglutamate release via presynaptic receptors (Schubert and Kreutzberg,1993). It can be released via carrier-mediated mechanisms as aresult of the hypoxia-induced massive breakdown of intracellularnucleotides, but hypoxia may result also in the direct releaseof nucleotides such as ATP (Dubyak and El-Moatassim, 1993). Bothneurons and glia possess receptors for ATP and other nucleotides(ADP, UTP, UDP) either that function as ion channels (P2X receptors)or that are G-protein-coupled (P2Y receptors) (Boarder et al.,1995; Buell et al., 1996). P2X receptors are permeable not onlyfor Na⁺ and K⁺ but also for Ca²⁺. Their hyperactivation is, therefore, potentially cytotoxic.Extracellular ATP is inactivated by a surface-located enzyme chainthat results in the extracellular formation of adenosine (Zimmermann,1996). The chain potentially includes the recently cloned ecto-ATPdiphosphohydrolase (ectoapyrase) and ecto-ATPase as well as ecto-5'-nucleotidase(Kegel et al., 1997). Whereas ecto-ATPase has a high preferencefor ATP, ectoapyrase hydrolyzes ATP and ADP, resulting in theformation of AMP. Ecto-5'-nucleotidase catalyzes the formationof adenosine from AMP. An upregulation of these enzymes in thedamaged tissue could serve the rapid elimination of any cytotoxiceffects of ATP and in addition provide extracellular adenosinefor purine salvage or as a neuroprotective agent. We previouslyhave observed increased activity of ecto-5'-nucleotidase in thevolume bordering the infarcted tissue after permanent middle cerebralartery occlusion (MCAO) (Braun et al., 1997). In the present studywe induced transient forebrain ischemia by bilateral common carotidartery occlusion and hypertension in rats, and we probed for theexpression of the entire ectonucleotidase chain.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Transient forebrain ischemia. Forebrain ischemia was induced in 28 male Wistar rats (300-350 gm, Charles River, Sulzfeld,Germany). Rats were fasted overnight with free access to water.They were anesthetized with halothane (1.5%) in a mixture of N₂O/O₂(70%/30%). Body and skull temperatures were maintained at 37.0-37.5°Cby a temperature control feedback system (Technical and ScientificEquipment, Bad Homburg, Germany). The skull temperature was monitoredwith a thermocouple placed subcutaneously over the midline ofthe skull. Ischemia was induced for 10 min by clamping both commoncarotid arteries and lowering the mean blood pressure to 40 mmHg by trimethaphan camphor sulfonate (5 mg/kg, i.v.) and centralvenous exsanguination (Smith et al., 1984). After 10 min the clipswere removed, and the shed blood was reinjected rapidly. ArterialpH, pCO₂, pO₂, blood pressure, and plasma glucose concentrationwere measured before ischemia. Sham-operated animals were preparedas described above without clamping carotid arteries and loweringblood pressure. They were compared with untreated animals. Afterischemia, animals were kept at an environmental temperature of30°C for 2 hr and then at 20°C in their home cages. At 6 hr andat 2, 3, 7, 14, and 28 d after ischemia the rats received a lethaldose of chloral hydrate and were decapitated. Brains were removed,snap-frozen in prechilled ( $-$ 20°C) 2-methylbutane, and stored at $-$ 70°C until sectioning.

Nucleotidase histochemistry. For localization of nucleotidase activity a lead phosphate method (Braun et al., 1997) was applied.Frozen sections (12 µm) were deposited on 3-aminopropyltriethoxySilane-coated (Sigma, Deisenhofen, Germany) slides and allowedto dry for 1 hr. The dry tissue sections were stored at $-$ 80°Cuntil further processing. Sections warmed to room temperaturewere fixed with 0.05 M cacodylate-buffered 4% paraformaldehyde,pH 7.4, for 12 min at room temperature and subsequently were washedwith 0.05 M cacodylate buffer, pH 7.4, containing 0.25 M sucrose.Preincubation was performed for 30 min at room temperature ina Tris-maleate sucrose buffer (TMS; 0.25 M sucrose and 50 mM Tris-maleate,pH 7.4) containing 2 mM MgCl₂ when 5'-nucleotidase activity wasto be analyzed or 2 mM CaCl₂ for the subsequent detection of hydrolysisof ATP, UTP, or ADP. Nucleotides (ATP, UTP, ADP, and AMP) (allfrom Sigma) were added to the buffer solution at a concentrationof 1 mM. The enzyme reaction for the detection of ATPase, ADPase,or UTPase activity was performed for 2.4 hr at room temperaturein a Tris-maleate-buffered substrate solution [composition (inmM): 2 Pb(NO₃)₂, 5 MnCl₂, 2 CaCl₂, and 50 Tris-maleate, plus 0.25M sucrose, pH 7.4]. AMP was applied in the same buffer solutionexcept that CaCl₂ was omitted. After the sections were washedwith demineralized water, the lead orthophosphate that was precipitatedas a result of nucleotidase activity was visualized as a browndeposit by incubating sections in an aqueous solution of ammoniumsulfide (2% v/v). To control for nonspecific phosphatase activity,we substituted nucleotides by p-nitrophenyl phosphate (Sigma).To control for nonspecific lead precipitation, we omitted nucleotidesfrom the incubation medium. Subsequently, the sections were processedas for immunocytochemistry.

Immunocytochemical procedures. For immunocytochemical labeling of microglia, the monoclonal antibody MRC OX42 (Camon, Wiesbaden,Germany) was applied (Milligan et al., 1991). This antibody recognizesthe rat complement receptor type 3 (Robinson et al., 1986). Amonoclonal antibody G-A-5 (Sigma) against the GFAP from pig spinalcord was used as an astroglial marker. Vimentin was detected byusing a monoclonal antibody (VIM 3B4, Progen Biotechnik, Heidelberg,Germany) against vimentin from bovine lens. Frozen sections wereprepared as described for enzyme histochemistry. For immunoperoxidaselabeling, frozen sections were warmed to room temperature, fixedwith absolute methanol (7 min at $-$ 20°C), and rinsed with PBS [composition(in mM): 137 NaCl, 3 KCl, and 15 Na⁺/K⁺-phosphate buffer, pH 7.4]. Nonspecific binding was suppressedwith 5% bovine serum albumin (BSA; Roth, Karlsruhe, Germany).Antibodies were diluted with PBS containing 1% BSA. Sections wereincubated for 80 min at room temperature with antibodies againstGFAP (1:100), OX42 (1:50), or vimentin (1:10). All further stepswere performed at room temperature. After being washed with PBSfor 25 min, the sections were incubated for 1 hr with a peroxidase-linkedaffinity-purified secondary antibody against mouse-IgG (Amersham,Braunschweig, Germany). After excess washing with PBS, the peroxidasereaction was performed with a diaminobenzidine (DAB) substratesolution (0.25 mg of DAB/ml, 0.03% NiCl₂, 0.01% H₂O₂, and 100mM Tris-HCl, pH 7.5). In control experiments only the secondaryantibody was applied. After dehydration in graded ethanol, thesections were mounted with Permount (Fisher Scientific, Springfield,NY). They were examined with a Zeiss Axiophot microscope (Oberkochen,Germany) and photographed on Ilford Pan F film developed in Ultrafin(Tetenal).

Northern analysis. For Northern blotting, hippocampi were excised from rat brains 7 d after vessel occlusion or sham operation.Polyadenylated RNA was isolated by using the Oligotex direct kit(Qiagen, Hilden, Germany). Polyadenylated RNA (0.5 µg), as determinedphotometrically, was separated on a 1% agarose formaldehyde gel.Subsequently, the RNA was transferred by pressure (PosiBlot, Stratagene,Germany) onto a Hybond N membrane (Amersham). Using various constructsof DIG-labeled RNA as a probe, we hybridized blots overnight at68°C in the presence of 5× SSC and 50% formamide. Filters werewashed twice at room temperature with 2× SSC containing 0.1% SDSand twice at 68°C for 15 min with 0.2× SSC containing 0.1% SDS.The hybridization signal was visualized by using an alkaline phosphatase-conjugatedanti-DIG antibody and a chemiluminescent substrate (CSPD; bothfrom Boehringer Mannheim, Mannheim, Germany) according to themanufacturer's instructions. For obtaining riboprobes, the mouseectoapyrase construct CD39-5b (Maliszewski et al., 1994) and therat ecto-ATPase construct rat9.4 (Kegel et al., 1997) were digestedwith SalI and with BamHI, respectively. The insert of the ratliver ecto-5'-nucleotidase construct $lambda$ cNT34 (Misumi et al., 1990)was subcloned into pBluescript II SK and digested with BamHI.DIG-labeled antisense RNAs (ectoapyrase, 2.3 kb; ecto-ATPase,1.6 kb; ecto-5'-nucleotidase, 1.8 kb) were transcribed by usingT3 or T7 RNA polymerase according to the manufacturer's instructions(Boehringer Mannheim). For detection of $beta$ -actin mRNA, a riboprobefrom a cDNA clone coding for mouse $beta$ -actin (Stratagene, Heidelberg,Germany) was used.

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Northern analysis

To probe for the expression of ectonucleotidases identified in molecular terms, we isolated polyadenylated RNA from hippocampi7 d after transient forebrain ischemia or 7 d after sham operation.Equal amounts (0.5 µg) of mRNA were analyzed for ecto-5'-nucleotidase,ectoapyrase, and ecto-ATPase (Fig. 1). The probe for rat ecto-5'-nucleotidasehybridized with a 3.9 kb mRNA species (Misumi et al., 1990). Correspondingto previous results (Kegel et al., 1997), the probe for ectoapyrasedetected two major bands of 4.9 and 5.4 kb, which may representthe use of different polyadenylation sites at the 3'-uncodingregion, whereas the riboprobe for ecto-ATPase yielded a prominentmRNA band at 2.2 kb. The hybridization signal for $beta$ -actin (2.2kb) was determined as a control. As compared with sham-operatedcontrols, the hybridization signals for both ecto-5'-nucleotidaseand ectoapyrase were increased distinctly 7 d after ischemia.In contrast, the hybridization signal for ecto-ATPase was notaffected by forebrain ischemia. Actin mRNA levels were evaluatedby rehybridization. They did not differ between controls and postischemichippocampi.

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Figure 1. Northern blot analysis of ectonucleotidases. Equal amounts (0.5 µg) of polyadenylated RNA isolated from hippocampi 7 d after sham operation (a) or 7 d after 10 min of global ischemia (b) were subjected to electrophoresis, blotted, and hybridized with rat ecto-5'-nucleotidase (e-5'-nucl.), ectoapyrase (e-apyrase), and ecto-ATPase (e-ATPase) antisense riboprobes. A significant postischemic enhancement of the hybridization signals is detectable for ecto-5'-nucleotidase and ectoapyrase. The riboprobe for ectoapyrase hybridizes with two major bands at 4.9 and 5.4 kb. A riboprobe for mouse $beta$ -actin was used as an internal control.

Increase in the activity of ATPase, UTPase, and ADPase in lesioned regions

The postischemic reaction was investigated at the septodorsal level of the hippocampus. Brain sections were analyzed at 6hr and at 2, 3, 7, 14, and 28 d after ischemia. The extent ofneuronal degeneration was visualized by Nissl staining (Figs.2A, 3A, 4A). In the pyramidal cell layer of CA1, damaged neuronsfirst became apparent at 2 d after ischemia. At 3 d the cell deathof pyramidal cells was increased (Fig. 3A), and from day 7 onwardmost neurons of CA1 were disintegrated (Fig. 4A). No neuronaldamage was detected in hippocampal sections of sham-operated animals(see Fig. 2A).

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Figure 2. Corresponding hippocampal sections 7 d after sham operation. Comparison of Nissl staining (A), immunocytochemistry (B-D), and nucleotidase histochemistry (E-H). A, Nissl staining revealed no neuronal damage in the hippocampus. B, OX42 immunostaining is significant only in fiber tracts, as for example in the corpus callosum. C, Vimentin is detectable in capillaries. D, GFAP immunoreaction is strongest in the stratum lacunosum moleculare. E-G, ATPase (E), UTPase (F), and ADPase (G) reaction product in the hippocampus is restricted mainly to capillaries. Staining is enhanced slightly in the stratum lacunosum. H, 5'-Nucleotidase activity is highest in CA1 and in the stratum lacunosum moleculare of CA1 and CA3. The pyramidal cell layers and the dentate granule cell layer are free of reaction product. CA1, CA3, Subfields of the hippocampus; cc, corpus callosum; gr, granular cell layer of the dentate gyrus; H, hilus of the dentate gyrus; lm, stratum lacunosum moleculare; pyr, stratum pyramidale; PC, plexus choroideus; M, meninx. Scale bar, 1 µm.

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Figure 3. Corresponding hippocampal sections 3 d after global ischemia. Comparison of Nissl staining (A), immunocytochemistry (B-D), and nucleotidase histochemistry (E-H). A, Reduced Nissl staining in CA1 (arrowheads) indicates damaged pyramidal neurons. Immunostaining for OX42 (B), vimentin (C), and GFAP (D) is upregulated most significantly in CA1 and the dentate hilus. E-H, ATPase (E), UTPase (F), ADPase (G), and 5'-nucleotidase activity (H) is enhanced in the pyramidal cell layer of CA1 (arrows). Abbreviations as in Figure 2. Scale bar, 1 µm.

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Figure 4. Corresponding hippocampal sections 7 d after global ischemia. Comparison of Nissl staining (A), immunocytochemistry (B-D), and nucleotidase histochemistry (E-H). A, Reduced Nissl staining in the CA1 subfield (arrowheads) indicates damaged pyramidal cells. Immunolabeling for OX42 (B), vimentin (C), and GFAP (D) is strongly enhanced in CA1 and the dentate hilus. In contrast to GFAP immunoreactivity, OX42 and vimentin immunostaining is very distinct in the layer of damaged pyramidal cells. E-H, Strong upregulation of ATPase (E), UTPase (F), ADPase (G), and 5'-nucleotidase (H) activity in all layers of CA1 and the dentate hilus. The reaction product is most intense in the layer of damaged pyramidal cells and the stratum lacunosum moleculare. Abbreviations as in Figure 2. Scale bar, 1 µm.

Because suitable antibodies for the immunodetection of ectonucleotidases were not available, we analyzed the hippocampi byenzyme cytochemistry. The histochemical staining pattern in thehippocampal formation was practically identical for the hydrolysisof ATP, UTP, and ADP and demonstrated a parallel and strong postischemicincrease in staining intensity. UTP was included in the analysisto probe for the presence of ectoapyrase that hydrolyzes bothATP and UTP. The enzyme reaction in hippocampal sections of sham-operatedanimals (see Fig. 2E-G) was very low and identical to the stainingpattern obtained for untreated rats. There was a faint stainingof the entire tissue section, except for fiber tracts, the pyramidalcell layer, and the granule cell layer of the dentate gyrus. Theseneuronal layers became apparent as a light and unstained band.Reaction product was enhanced slightly in the stratum lacunosummoleculare. Intense lead staining was restricted to the endotheliumof brain capillaries, the meninges covering the hippocampal formation,and the choroid plexus. These observations suggest that the histochemicalstaining performed at alkaline pH does not represent the activityof intracellular nucleoside 5'-triphosphate or 5'-diphosphate-hydrolyzingenzymes that are present at high activity in every cell.

At 2 d after global ischemia the unstained band corresponding to the pyramidal cell layer of CA1 had disappeared. It now revealedthe same faint staining as the stratum oriens and stratum pyramidale.At 3 d the histochemical reaction for all three substrates clearlywas enhanced in the stratum pyramidale of CA1 (see Fig. 3E-G).There was also a small increase in staining intensity in the dentatehilus. The postischemic enzyme reaction was developed stronglyat 7 d (see Fig. 4E-G). All layers of CA1 exhibited a distinctupregulation of ATP, UTP, and ADP hydrolysis. The pyramidal celllayer revealed the strongest enhancement. Staining was increasedin the stratum lacunosum moleculare and in the dentate hilus.There were small variations in overall staining intensity betweenindividual experiments and also between individual days of experimentation.This did not affect, however, the qualitative staining pattern.The intense staining in CA1 persisted 14 and 28 d after globalischemia. The reaction in the dentate hilus was still presentat 14 d but had disappeared at 28 d. No reaction product was obtainedin the control experiments in which nucleotides were replacedby p-nitrophenyl phosphate or when nucleotides were omitted fromthe incubation medium.

Lesion-induced increase in 5'-nucleotidase activity

When AMP was used as a substrate, the staining pattern differed clearly from that obtained with the other nucleotides, butthe time course of the postischemic increase was comparable. 5'-Nucleotidaseactivity was high in all layers of CA1 of sham-operated (see Fig.2H) or untreated animals. Also, the stratum lacunosum moleculareof CA3 displayed a distinct reaction. The other layers of CA3and the hilus and the molecular layer of the dentate gyrus werestained only faintly. The pyramidal cell layer and the dentategranule cell layer were unlabeled. Fiber tracts were labeled intensely(for example, fimbria, alveus, and corpus callosum). This alsoapplied to the choroid plexus. As for the other nucleotides, thepreviously unstained pyramidal cell layer in CA1 had disappearedby 2 d. At 3 d a slight enhancement of 5'-nucleotidase activitybecame apparent in the CA1 pyramidal cell layer and in the dentatehilus (see Fig. 3H). At 7 d the upregulation of enzyme activitywas apparent in all layers of CA1, whereby the pyramidal celllayer and the stratum lacunosum moleculare displayed the strongeststaining. A clear enhancement of the enzyme reaction also wasobserved in the dentate hilus. The enhanced staining of the dentatehilus had disappeared at 28 d, but the increase in CA1 persisted.No reaction product was obtained when 5'-AMP was replaced by p-nitrophenylphosphate as a substrate or when 5'-AMP was omitted from the incubationmedium.

Comparison with the distribution of astrocytes and microglia

To identify cell types that could be responsible for the increase in nucleotidase activities, we compared $---$ within correspondingsections $---$ the pattern obtained by enzyme histochemistry with thatfor immunostaining for GFAP (astrocytes), vimentin (endothelialcells, reactive astrocytes, and activated microglia) (Graeberet al., 1988; Schmidt-Kastner et al., 1990), and complement receptor3 (OX42, microglia). In the hippocampal formation of sham-operated(see Fig. 2B,C) and untreated animals the immunostaining for vimentinand OX42 was very low. The immunoreaction for vimentin was confinedto capillaries (Fig. 5D). GFAP-labeled astrocytes were frequentthroughout the entire hippocampus of sham-operated (see Fig. 2D)or control animals. GFAP staining was strongest in the stratumlacunosum moleculare. The pyramidal cell layer (see Figs. 2D,5G) and the granule cell layer of the dentate gyrus (see Fig.2D) were mainly free of GFAP positive astrocytes. GFAP-positiveastroglial cells displayed a normal morphology, with small cellbodies and fine branched processes (see Figs. 2D, 5G).

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Figure 5. Immunocytochemical detection of the postischemic glial reaction in CA1. A-C, OX42 immunoreactivity 7 d after sham operation (A) and 3 d (B) and 7 d (C) after ischemia. Arrows depict activated microglial cells that are apparent at 3 and 7 d. At 7 d the accumulation of the OX42 immunoreaction is strongest in the pyramidal cell layer. D-F, Vimentin immunoreactivity 7 d after sham operation (D) and 3 d (E) and 7 d (F) after ischemia. Capillaries are strongly labeled for vimentin (arrowheads). Vimentin-expressing cells with radiate ramifications (arrows) presumably represent reactive astrocytes, whereas rod-shaped cells presumably represent microglia. G-I, GFAP immunoreactivity 7 d after sham operation (G) and 3 d (H) and 7 d (I) after ischemia. Reactive and swollen astrocytes are clearly detectable at 3 and 7 d. Note that astrocytes do not accumulate in the pyramidal cell layer after the disappearance of neurons. ori, Stratum oriens; pyr, pyramidal cell layer; rad, stratum radiatum. Scale bar, 100 µm.

The postischemic microglial activation was detectable first at 2 d as a faint enhancement in OX42 staining of the pyramidallayer. At 3 d a distinct microglial activation appeared in thelayer of damaged pyramidal cells within CA1 and in the dentatehilus (see Fig. 3B). At higher magnification, activated microgliaalso could be detected in the stratum oriens and the stratum radiatumof CA1 (see Fig. 5B). At 7 d immunostaining for OX42 was strongestin the pyramidal cell layer and the stratum lacunosum moleculare(see Fig. 4B). Rod-shaped microglial cells were frequent in thestratum radiatum (see Fig. 5C). This general staining patternpersisted up to 28 d, with the exception of the dentate hilus,where the microglial reaction was reduced.

Ischemia-induced immunostaining for vimentin appeared first at 2 d in sparsely distributed astroglia-like processes of CA1.At 3 d vimentin expression was clearly detectable in cells withradiating processes that could represent activated astrocytesand also in smaller elongated cells that presumably representmicroglia (see Figs. 3C, 5E). Staining for vimentin was enhancedsignificantly at 7 d in CA1 and the dentate hilus (see Fig. 4C).The pyramidal cell layer containing damaged neurons expressedstrong vimentin immunoreactivity (see Fig. 5F). At 28 d afterischemia the reaction clearly was reduced in the dentate hilus.

GFAP staining of the hippocampus was enhanced at 2 d, and at 3 d positive astrocytes displayed the swollen morphology typicalfor reactive astrocytes (see Figs. 3D, 5H). The staining for GFAPwas enhanced further at 7 d, particularly in CA1, dentate hilus,and CA3 (see Fig. 4D). There was a significant difference in thepostischemic expression within the pyramidal cell layer of CA1between GFAP on the one hand and OX42 and vimentin on the otherhand. The band corresponding to the dead pyramidal cells displayeda very strong immunoreactivity for OX42 and vimentin (see Figs.5C,F). GFAP-reactive astrocytes invaded this layer with increasingtime but did not accumulate there (see Fig. 5I). This patternpersisted at 28 d. In control experiments no immunoreaction wasobtained when only the secondary antibody was applied.

Spatial distribution and the time course of the increased immunoreactivity for OX42 and vimentin within the layer of damagedpyramidal cells of CA1 correspond closely to the increase in postischemicnucleotidase activity. This suggests that the expression of nucleotidasesin this region is mainly by activated microglia. Considering thelack of cellular resolution for the nucleotidase histochemistry,we also cannot, however, exclude an expression of these enzymesby reactive astrocytes. Nucleotidase activity also is upregulateddistinctly in the stratum oriens, stratum radiatum, and the dentatehilus. This increase in enzyme activity is not paralleled by acomparable increase in immunoreactivity of OX42 and, rather, correspondsto the distribution of GFAP immunoreactivity (see Figs. 4D, 5I).

  DISCUSSION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Neural death and upregulation of glial markers after transient two-vessel occlusion

The two-vessel or the four-vessel occlusion models are used when transient interruption of blood flow and reperfusion arerequired. The two models yield similar neuronal injury in thehippocampus, including the CA1 and CA4 pyramidal cells and thesubiculum (Ginsberg and Busto, 1989). Our results obtained forthe markers GFAP, vimentin, and OX42 correspond closely to thosepreviously described by others, using the four-vessel occlusionmodel and similar occlusion times. The immunoreactivity for themicroglial marker OX42 develops progressively during the postischemictime period. It is restricted mainly to the band of injured pyramidalcell bodies and to a lesser extent to the stratum lacunosum moleculareand the dentate gyrus (Morioka et al., 1992; Jørgensen et al.,1993; Kato et al., 1995). The hippocampal distribution of vimentinis very similar to that of OX42 immunoreactivity. Several studieson transient cerebral ischemia have demonstrated an increase inimmunoreactivity for vimentin in the lesioned neuronal layersand have interpreted it as an astrocytic reaction. In contrastto vimentin, the immunoreactivity for the astrocytic marker GFAPalso is prominent throughout the hippocampus in unlesioned animals.Ischemia causes a time-dependent increase in GFAP immunoreactivitywithin the entire hippocampus, particularly in CA1 and dentatehilus (Petito et al., 1990; Schmidt-Kastner et al., 1990; Jørgensenet al., 1993). Prolonged postischemic survival time results inthe immigration of GFAP-positive astrocytes into the damaged pyramidalcell layer of CA1, but the immunoreactivity never becomes as intenseas that for OX42 and vimentin.

Glial upregulation of ectonucleotidases

Northern analysis demonstrates an ischemia-induced upregulation of ectoapyrase and ecto-5'-nucleotidase. Together, the twoenzymes can account for the entire hydrolysis chain from ATP toadenosine. Ecto-5'-nucleotidase is bound to the membrane via aglycosyl phosphatidylinositol (GPI) anchor. Ectoapyrase representsa transmembrane protein with two hydrophobic domains at the N-and C-terminal ends and the catalytic site facing the extracellularspace. Both enzymes have a very broad substrate specificity towardnucleoside 5'-di- and tri- and monophosphates, respectively (Zimmermann,1996). ATP, UTP, and ADP thus could be hydrolyzed by a singleenzyme (ectoapyrase). These results suggest that the histochemicalstaining pattern observed in the injured regions is attributableto the activity of two defined enzymes, ectoapyrase and ecto-5'-nucleotidase.

Hydrolysis of nucleoside 5'-tri- and diphosphates was very low in the hippocampal subfield of unlesioned animals. Stainingfor 5'-nucleotidase activity was strong in CA1 and within fibertracts. This corresponded to earlier histochemical analyses of5'-nucleotidase in the rat hippocampus (Lee et al., 1986; Fastbomet al., 1987). With all substrate nucleotides, ischemia inducedan increase in staining intensity in select hippocampal regions.Its temporal development corresponded to that of markers for activatedglia. There was a strong and continued increase in the entireCA1 subfield, with particular emphasis on the layer of damagedpyramidal cell bodies and the stratum lacunosum moleculare. Enzymeactivity also was upregulated within the dentate hilus and toa small extent in CA3. CA1 neurons, along with some hilar neurons,are considered to represent the most vulnerable neurons of thehippocampus. The strong focus of histochemical reaction productin the pyramidal layer and the stratum lacunosum moleculare suggeststhat enzyme activity there is attributable mainly to activatedmicroglia. The more diffuse upregulation in the other areas couldresult from both activated microglia and astrocytes. In our previousstudy applying permanent MCAO, staining for 5'-nucleotidase atthe immediate rim of the infarcted tissue corresponded to thedistribution of binding sites for OX42, whereas the more distantand less intensive staining corresponded to the distribution ofGFAP (Braun et al., 1997).

Hydrolysis of inosine 5'-diphosphate (IDP) previously has been allocated to the surface of microglia and subsequently hasbeen used as a microglial marker. The ischemia-induced increasein staining for IDP as a substrate (Finsen et al., 1993) is similarto that observed for ATP, UTP, and ADP as substrates. This wouldbe expected if all substrates were hydrolyzed by the same enzyme(ectoapyrase). The presence of the extracellular hydrolysis chainfrom ATP to adenosine previously has been demonstrated in astrocyticcultures (Lai and Wong, 1991) and hippocampal slices (Wieraszkoet al., 1989; Cunha et al., 1996; Dunwiddie et al., 1997). Theactivity of ectonucleotidases also is associated with isolatedsynaptosomes (Nagy et al., 1986) and cultured neural cells (Stefanovicet al., 1976). We have no indication for an upregulation of ectoapyraseand ecto-5'-nucleotidase on neural cells or their processes.

Upregulation of ectonucleotidases and nucleotide release

The upregulation of ectonucleotidases implies increased nucleotide release. ATP can be released from a large variety of cellsand mechanisms of membrane passage other than exocytosis may beinvolved (Cantiello, 1997). Tissue injury or hypoxia alone canrelease ATP and other adenine nucleotides from a variety of tissues,including the brain (Dubyak and El-Moatassim, 1993; Lutz and Kabler,1997). Transient global ischemia resulting in the alteration ofboth composition and flow rate of the blood may induce osmoticstress with changes in cell volume (van der Toorn et al., 1996).Increases in cell volume can lead, in turn, to the cellular effluxof ATP. ATP is released from HTC rat hepatoma cells by hypotonicexposure and subsequently is required for recovery from swelling(Wang et al., 1996). Because this effect is attenuated by enzymeshydrolyzing ATP, an increase in ectonucleotidase activity wouldbe damaging rather than protective. The increase in ectonucleotidaseactivity may be induced directly by neural cell damage or indirectlyby general homeostatic shifts. Because the increase is not globalbut is restricted to sites of intense neural damage, it appearsto be correlated directly with neural cell death. Its onset coincideswith that of significant neural cell death, which becomes apparentat the microscopic level after 2 d (Sweeney et al., 1995).

Significance of increased ectonucleotidase activity

A major factor for neuron survival is the efficient replenishment of the depleted ATP stores. An effective extracellular hydrolysisof released ATP to adenosine would provide the nucleoside forpurine salvage via carrier-mediated cellular uptake. There isa wealth of literature in support of a neuroprotective functionof extracellular adenosine in attenuating the release of cytotoxicamino acids or as a vasodilating agent (Rudolphi et al., 1992;Sweeney, 1997). ATP, on the other hand, may be cytotoxic. A roleof ATP as a fast neurotransmitter as well as a neuromodulatorhas been demonstrated for several central and peripheral synapses(Gibb and Halliday, 1996). When released in large amounts andfor an extended period of time, it may cause a P2X receptor-mediatedbuildup of intracellular calcium that would be equally damagingas that induced by excess glutamate (Edwards, 1996). Studies onhippocampal neurons suggest that glutamate itself may stimulatethe release of ATP, which in turn can act as a transmitter andinduce an increase in [Ca]_i via P2 receptors. This increase alsocan be elicited in the presence of high Mg²⁺ concentrations and thus can evoke membrane depolarization thatremoves Mg²⁺ blocking of the NMDA receptor. ATP therefore even could potentiatethe cytotoxic effects of glutamate (Inoue et al., 1995). Upregulatedectonucleotidases would counteract this effect.

Ectonucleotidase activity also could be relevant for glial cells. The reactive glial cells may have a demand for increasedenergy supply and thus may reinforce the extracellular purinesalvage pathway. In addition, nucleotides can affect glial cellsdirectly. Cultured astrocytes and microglia express metabotropicas well as ionotropic receptors for nucleotides (Walz et al.,1994; Nörenberg et al., 1997). ATP or also UTP mediates an increasein intracellular Ca²⁺ concentrations in cultured astrocytes in vitro (Czubayko andReiser, 1996; Centemeri et al., 1997). In vitro ischemia has beenfound to promote Ca²⁺ influx and intracellular Ca²⁺ release in hippocampal astrocytes (Duffy and MacVicar, 1996).ATP or adenosine can stimulate the proliferation of astrocytes(Abbracchio, 1996). ATP induces astrogliosis in vitro, includingan increase in expression of GFAP, promotion of astrocytic hypertrophy,and elongation of cellular processes (Bolego et al., 1997). ExtracellularGTP increases the synthesis and release of NGF from cultured astrocytes(Middlemiss et al., 1995).

Microglial cells are endangered by ATP. They express the cytolytic P_2z (P2X₇) subtype of ATP receptors as do peripheral macrophages(Collo et al., 1997; Ferrari et al., 1997a). Activation of thisreceptor mediates a reversible permeabilization of the plasmamembrane that causes the opening of a pore associated with ionfluxes and the leakage of small metabolites such as nucleotides.Sustained exposure to ATP would be a potent cytolytic stimulus.Microglial cell lines release mediators of inflammation, includinginterleukin-1 $beta$ , when stimulated with bacterial endotoxins, andthis release can be inhibited by the blockade of P2X₇ receptors(Ferrari et al., 1997b). The upregulation of ectoapyrase on activatedmicroglia may be a protective reaction.

In summary, our data suggest that transient forebrain ischemia results in an upregulation of the enzyme chain for the completehydrolysis of extracellular ATP and other nucleoside 5'-triphosphatesin the damaged hippocampal areas. Enzyme activity appears to beassociated mainly with reactive glia. The increase in ectonucleotidaseactivity implies increased nucleotide release and could play arole in the postischemic control of nucleotide-mediated cellularresponses.

  FOOTNOTES

Received Feb. 12, 1998; revised April 7, 1998; accepted April 17, 1998.

This study was supported by Grants from the Deutsche Forschungsgemeinschaft (SFB 269, A4), the European Community (BMH4-CT96-0676),and the Fonds der Chemischen Industrie. We are grateful to KlausHammer for expert technical support. Rat ecto-5'-nucleotidasecDNA was kindly provided by Dr. Y. Ikehara, Fukuoka University,Japan.
Correspondence should be addressed to Dr. Norbert Braun, Biozentrum der J.W. Goethe-Universität, AK Neurochemie, ZoologischesInstitut, Marie-Curie-Strasse 9, D-60439 Frankfurt am Main, Germany.

  REFERENCES

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

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