Prostaglandin A1 Protects Striatal Neurons against Excitotoxic Injury in Rat Striatum

Assistant Professor of Medicine (Clinician-Educator)

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Vol. 297, Issue 1, 78-87, April 2001

Prostaglandin A₁ Protects Striatal Neurons against Excitotoxic Injury in Rat Striatum

Zheng-Hong Qin¹ , Yumei Wang¹ , Ren-Wu Chen, Xiaoxia Wang, Ming Ren, De-Maw Chuang and Thomas N. Chase

Experimental Therapeutics Branch, National Institute of Neurological Disorders and Stroke, National Institutes of Health, Bethesda, Maryland (Z.-H.Q., Y.W., T.N.C., X.W.); and Molecular Neurobiology Section, National Institute of Mental Health, National Institutes of Health, Bethesda, Maryland (R.-W.C., M.R., D.-M.C.)

	Abstract

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Prostaglandin A₁ (PGA₁) reportedly inhibits NF- $kappa$ B activation and induces expression of heat shock proteins. Since both theseeffects could be neuroprotective, the therapeutic potential ofPGA₁ in neurodegenerative disorders, where excitotoxicity maycontribute to pathogenesis, was evaluated in rat striatal neuronsexposed to the N-methyl-D-aspartate (NMDA) receptor agonist quinolinicacid (QA). Intrastriatal administration of PGA₁ (5-80 nmol) attenuatedQA (60 nmol)-induced internucleosomal DNA fragmentation. The inhibitoryeffects of a single dose of PGA₁ (80 nmol) on QA (60 nmol)-inducedDNA fragmentation were observed 12 to 48 h after treatment. PGA₁(80 nmol) also attenuated QA-induced DNA fragmentation when administeredup to 4 h after QA exposure. PGA₁ significantly decreased theloss of D₁ dopamine receptors and GAD₆₇ mRNA in QA-injected striatumas measured by quantitative receptor autoradiography and in situhybridization histochemistry, suggesting that it reduced the neuronalloss induced by QA. Protection of striatal neurons against QA-induceddeath by PGA₁ was further indicated by Nissl staining 10 daysafter QA administration. PGA₁ (5-80 nmol) significantly inhibitedQA-induced NF- $kappa$ B activation by blocking inhibitory $kappa$ B- $alpha$ degradationbut had no effect on activator protein-1 binding activity. PGA₁(80 nmol) treatment substantially increased 70- and 72-kDa heatshock protein levels in striatum. These results indicate thatPGA₁ blunts NMDA receptor-mediated neuronal apoptosis by a mechanismpossibly involving the up-regulation of neuroprotective heat shockproteins and inhibition of NF- $kappa$ B activation. In view of its potentneuroprotective activity, PGA₁ could prove useful in the treatmentof certain neurodegenerative disorders related toexcitotoxicity.

	Introduction

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Apoptotic mechanisms appear to contribute to excitotoxic neuronal injury in rat striatum (Portera-Cailliau et al., 1995; Qinet al., 1996). Although the role of the transcription factor nuclearfactor- $kappa$ B (NF- $kappa$ B) in apoptosis is controversial, some studiesindicate that it may participate in the excitotoxin-induced apoptoticprocess in postmitotic neurons in vivo (Clemens et al., 1997;Qin et al., 1998, 1999; Nakai et al., 1999a,b).

In cultured neurons and experimental animals, glutamate receptor stimulation activates neuronal NF- $kappa$ B by accelerating thedegradation of its cytoplasmic binding protein I $kappa$ B- $alpha$ (Guerriniet al., 1995; Qin et al., 2000). Upon its nuclear translocationin striatal neurons, NF- $kappa$ B up-regulates the proapoptotic proteinsc-Myc and p53 in response to excitotoxic insult; blockade of NF- $kappa$ Btranslocation with the recombinant peptide NF- $kappa$ B SN50 inhibitsquinolinic acid- (QA) or kainic acid-induced apoptosis (Qin etal., 1999; Nakai et al., 1999a). NF- $kappa$ B activation also occursin such human neurodegenerative disorders as Alzheimer's disease(AD) and Parkinson's disease as well as in animal models of ischemia(Clemens et al., 1997; Hunot et al., 1997; Kaltschmidt et al.,1997; Gabriel et al., 1999). NF- $kappa$ B activation could thus servea crucial postsynaptic contributor to excitotoxin-induced neuronaldestruction.

Recent pharmacological observations have begun to suggest that inhibition of the pathological activation of NF- $kappa$ B may conferprotective benefit to mature central nervous system neurons. Earlyepidemiological studies indicated that nonsteroid anti-inflammatorydrugs, such as aspirin and sodium salicylate, may have protectiveeffects in AD (Breitner, 1996). More recently, aspirin and sodiumsalicylate were found to diminish glutamate neurotoxicity throughNF- $kappa$ B inhibition (Grilli et al., 1996). Estrogen also has beenreported to diminish neuronal loss in AD (Simpkins et al., 1997)and to protect neurons against excitotoxic neuronal injury (Goodmanet al., 1996). Although its mechanisms of action remain to bedetermined, NF- $kappa$ B inhibition may be involved (Galien and Garcia,1997). Immunodepressants such as cyclosporin A protect neuronsagainst excitotoxin-, ischemia-, and oxidative stress-inducedneuronal damage (Li et al., 1997; Matsuura et al., 1997). Interestingly,cyclosporin A also inhibits NF- $kappa$ B activation (Meyer et al., 1997).In addition, the neuroprotective activity of antioxidants andmetabotropic glutamate receptor agonists against striatal injuryis also associated with an inhibitory effect on NF- $kappa$ B activation(Nakai et al., 1999b; Wang et al., 1999).

Prostaglandin A₁ (PGA₁) is known to induce heat shock protein (HSP) synthesis and block the cell cycle and viral replication(Lacal et al., 1994; D'Onofrio et al., 1995). Recent in vitrostudies have found that PGA₁ inhibits degradation of the NF- $kappa$ Binhibitory protein I $kappa$ B- $alpha$ (Rossi et al., 1997, 2000). The inductionof HSPs is a highly conserved cellular defense mechanism againstadverse environmental conditions. More specifically, HSP inductionhas been associated with the protection of neurons against theinjurious effects of heat shock and ischemia, probably by a mechanisminvolving the inhibition of apoptosis (Lowenstein et al., 1991;Rordorf et al., 1991; Samaili and Cotter, 1996; Yenari et al.,1998). Taken together, these observations suggest that PGA₁ couldact to attenuate excitotoxic neuronal damage. To evaluate thispossibility, we studied the effects of PGA₁ on QA-induced striatalneuronal injury, NF- $kappa$ B activation, and HSP induction in an animalmodel of Huntington's disease. The results showed that PGA₁ inhibitedNF- $kappa$ B activation, induced HSP expression, and protected striatalneurons against apoptoticdeath.

	Materials and Methods

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Animals. Male Sprague-Dawley rats weighing 300 to 350 g were purchased from Taconic Farms (Germantown, NY). Rats were housed two percage in an animal room with a 12-h light/dark cycle and had freeaccess to food and water. All procedures were performed in accordancewith National Institutes of Health Guidelines for the Care andUse of LaboratoryAnimals.

Drug Administration. Intrastriatal drug administration was performed as previously described (Qin et al., 1996). Synthetic PGA₁ was purchased fromSigma (St. Louis, MO), dissolved in absolute ethanol (EtOH), andthen diluted with saline (final ethanol concentration of 40%).To study the effects of PGA₁ pretreatment on QA-induced internucleosomalDNA fragmentation, three experiments were performed. In the first,rats were pretreated with intrastriatal injection of PGA₁ (5-80nmol) or vehicle (1 µl of 40% EtOH) 10 min before QA (60 nmol)and killed 24 h later for extraction of genomic DNA. In the secondexperiment, rats were pretreated with PGA₁ (80 nmol) or vehicle10 min before QA (60 nmol) as described above and killed 12, 24,or 48 h later. In the third experiment, one group of animals waspretreated with intrastriatal injection of PGA₁ (80 nmol) 10 minbefore QA (60 nmol); other animals were first given QA and thenPGA₁ (80 nmol) was injected intrastriatally 2, 4, or 6 h later.All were killed 24 h after QA treatment. The animals were thenkilled and striatal tissues used for DNA extraction. Three ratswere used in each group. To study the effect of PGA₁ on the numberof striatal GABAergic neurons, rats were treated with intrastriatalinjection of PGA₁ (5-80 nmol) or vehicle before QA (60 nmol) asdescribed above and killed 10 days later. Brains were sectionedfor receptor autoradiography and in situ hybridization histochemistry.To confirm the neuroprotective effects of PGA₁, rats were pretreatedwith the intrastriatal injection of PGA₁ (5-80 nmol) or vehicle10 min before QA (60 nmol) and were killed 10 days later. Brainswere sectioned and processed for Nissl staining and microscopicexamination. Four rats were used in each group. To study the effectof PGA₁ on QA-induced NF- $kappa$ B and AP-1 activation, rats were pretreatedwith intrastriatally infused PGA₁ (5-80 nmol) or vehicle 10 minbefore the intrastriatal administration of QA (60 nmol). Animalswere killed 12 h later and their striata taken for nuclear proteinextraction. To study the effects of PGA₁ on QA-induced I $kappa$ B- $alpha$ degradation,or on levels of HSPs, rats were treated with intrastriatal infusionof PGA₁ (80 nmol) or vehicle 10 min before QA (60 nmol) and killed12 h later. Striatal proteins were extracted for Western blotanalysis. To study the cellular localization of induced 70-kDaheat shock protein (HSP70), rats were treated with vehicle (40%EtOH, 1 µl), QA (60 nmol) plus vehicle, or PGA₁ plus QA and werekilled 12 h later. Brains were perfused via the ascending aortawith 40 mM phosphate-buffered saline (PBS, pH 7.4) containing4% paraformaldehyde. Brains were sectioned forimmunohistochemistry.

Electrophoresis Mobility Shift Assay. Striatal nuclear proteins were prepared as previously described (Qin et al., 1998). Briefly, striatal tissues were gentlyhomogenized and nuclear proteins were obtained with high saltextraction. Protein concentrations were determined with a bicinchoninicacid kit (Pierce, Rockford, IL). Double-stranded DNA oligonucleotidescontaining consensus sequences for NF- $kappa$ B and AP-1 (Promega, Madison,WI) were labeled with [³²P]ATP by T4 polynucleotide kinase (Promega). Nuclear proteins(8-12 µg) were incubated with radiolabeled DNA probes (approximately40,000 cpm) for 15 min at room temperature in the binding buffer(Promega). Nonspecific binding was assessed by adding 60-foldnonradioactive NF- $kappa$ B probes to the reaction mixture. The samplewas then electrophoresed on 4.5% nondenaturing polyacrylamidegel with 0.5× Tris borate-EDTA buffer. Autoradiograms were developedby exposing the vacuum-dried gels to X-ray film at $-$ 80°C withintensifying screens for 24 to 48 h. Results were quantitativelyanalyzed with an image analyzer (NIH Image 1.60). The specificbinding of NF- $kappa$ B or AP-1 was obtained by subtracting nonspecificbinding (with cold competitors) from total binding (without coldcompetitors).

Western Blot Analysis. Western blotting was performed as previously described (Qin et al., 1999). Striatal tissues were homogenized and protein concentrationsdetermined using a bicinchoninic acid protein assay kit (Pierce).Samples were mixed with loading buffer and boiled for 5 min. Analiquot of 30 µg of protein from each sample was separated on12% SDS-polyacrylamide gel electrophoresis gel using constantcurrent. Proteins were subsequently transferred to Immobilon-Pmembranes (Millipore, Bedford, MA) with a semidry blotting system.After blocking for 1 h in 0.1 M PBS (pH 7.5) with 0.1% Tween 20(PBST) and 5% nonfat dry milk, membranes were incubated for 3h with primary antibodies in PBST containing 3% nonfat dry milk.Membranes were then washed and incubated with a horseradish peroxidase-conjugatedsecondary antibody in PBST containing 3% nonfat dry milk for 1h. Immunoreactivity was detected by enhanced chemiluminescentautoradiography (ECL kit; Amersham Life Science, Arlington Heights,IL) in accordance with the manufacturer's instructions. A mousemonoclonal antibody against 72-kDa HSP (RPN 1197) was purchasedfrom Amersham Life Science (Arlington Heights, IL). Antibodiesagainst HSP70 and 70-kDa heat shock cognate protein (HSC70) weremouse monoclonal antibodies W27 and B-6. The antibody against $kappa$ B- $alpha$ [I $kappa$ B- $alpha$ (FL)] was a goat polyclonal antibody. All were purchasedfrom Santa Cruz Biotechnology (Santa Cruz,CA).

Genomic DNA Preparation and Electrophoresis. Striatal genomic DNA was prepared as previously described (Qin et al., 1996). Briefly, striatal tissues were homogenized ina buffer containing 100 mM NaCl, 25 mM EDTA-Na₂, 10 mM Tris-HCl(pH 8.0), 0.5% SDS, and 0.5 mg/ml RNase. Homogenates were incubatedat 55°C for 2 h; 0.6 mg of protease K was added and the incubationcontinued overnight. The homogenates were then extracted withphenol/chloroform/isoamyl alcohol (25:24:1) three times and DNAwas precipitated with 1 volume of isopropanol and 1/10 volumeof 5 M ammonium acetate and centrifuged at 14,000 rpm for 20 min.DNA pellets were washed once with precooled 80% alcohol, vacuum-dried,and resuspended in 50 mM Tris-EDTA (TE) buffer. DNA fragmentswere separated on 2% agarose gel (NuSieve 3:1) and detected withan UV transilluminator after staining with ethidiumbromide.

Receptor Autoradiography and in Situ Hybridization Histochemistry. To determine D₁ dopamine (DA) receptors, brain sections were rinsed twice in precooled 50 mM Tris-HCl buffer (pH 7.4) containing120 mM NaCl, 5 mM KCl, 2 mM CaCl₂, and 1 mM MgCl₂. Sections werethen incubated in 50 mM Tris-HCl buffer with 2 nM [³H]SCH-23390 and 80 nM ketanserin for 1 h at room temperature.Nonspecific binding was determined by incubating adjacent sectionsin the presence of 2 µM SCH-23390 added to the above-describedsolution. Sections were exposed to X-ray film with tritium standards(Amersham Life Science) for 10 days. Autoradiograms were quantitativelyanalyzed with an image analyzer (NIH Image 1.60). Antisense oligodeoxynucleotideprobes complimentary to 67-kDa glutamic acid decarboxylase (GAD₆₇)mRNA were labeled with [³³P]dATP using terminal deoxynucleotidyl transferase and purifiedby filtration chromatography (Chroma Spin-10; Clontech, Palo Alto,CA). To determine GAD₆₇ mRNA, brain sections were fixed in 0.1M PBS (pH 7.4) containing 4% paraformaldehyde for 10 min and rinsedin PBS. Sections were then incubated in tetraethylammonium-acetatebuffer containing 0.9% NaCl, 0.25% acetate anhydride, and 0.2M triethanolamine for 10 min, rinsed in PBS, and dehydrated. Sectionswere next hybridized with radioactively labeled oligodeoxynucleotideprobes in a buffer containing 50% formamide, 4× standard salinecitrate, 0.1% Denhardt's solution, 10% dextran sulfate, 0.25 mg/mlyeast transfer RNA, 0.5 mg/ml salmon sperm DNA, 10 mM dithiothreitol,and 5 × 10⁶ cpm ³³P-labeled oligodeoxynucleotide probes for 18 h at 40°C with coverslips.After hybridization, sections were washed in standard saline citratesolution with increasing stringency. The final wash was carriedout at 58°C for 40 min. Autoradiograms were developed by exposingthe sections to X-ray films (Hyperfilm $beta$ -max; Amersham Life Science)for 10 days and quantitatively analyzed with an image analyzer(NIH Image 1.60). Determination of D₁ DA receptor density madeuse of a standard curve constructed using coexposed ³H Microscales (Amersham Life Science). Optical density of theGAD₆₇ mRNA autoradiograms resulting from in situ hybridizationhistochemistry made use of a standard curve constructed from aKodak photographic table No 3 (Kodak, Rochester, NY). Both D₁DA receptors and GAD₆₇ mRNA were measured in three brain sectionsfrom each animal (bregma 1.7-0.2). These three individual measurementswere pooled to generate a mean density of D₁ DA receptors or opticaldensity of GAD₆₇ mRNA, and the data were converted to percentageof control (contralateral striatum) after ANOVA analysis for presentationas bargraphs.

Immunohistochemistry and Nissl Staining. Sections were washed in 0.1 M Tris-buffered saline (pH 7.4) and then incubated in Avidin/Biotin Blocking solution (VectorLaboratories, Burlingame, CA) for 15 min at room temperature.After washing in 10 mM PBS (pH 7.4), sections were incubated freefloating in 10 mM PBS containing primary antibodies (HSP70, W27),0.3% Triton X-100, and 1% normal serum at 4°C for 72 h. Sectionswere finally washed and incubated with secondary antibodies usinga Vectastain Elite kit (Vector Laboratories) according to themanufacturer's protocol. Some sections were also counterstainedwith thionin. The specificity of the antibodies was characterizedby the manufacturer and tested in our studies by omitting theprimary or the secondary antibodies. For Nissl staining, animalswere perfused with 4% paraformaldehyde in PBS (pH 7.4) and thenpostfixed in the same perfusate for an additional 6 h. Brainswere then frozen andsectioned.

	Results

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Effect of PGA₁ on QA-Induced Internucleosomal DNA Fragmentation. The effects of PGA₁ on QA-induced DNA fragmentation were first analyzed individually in each animal with agarose gels. Equalamount of DNA was then taken from three animals and pooled torun the gels again (Figs. 1 and 2). These studies showed thatthe intrastriatal administration of QA (60 nmol) produced intenseinternucleosomal DNA fragmentation. Pretreatment with PGA₁ (5-80nmol) inhibited the QA-induced DNA fragmentation in a dose-dependentmanner. Vehicle treatment appeared to slightly reduce the intensityof DNA fragmentation. PGA₁ alone did not produce appreciable DNAfragmentation (Fig. 1). Inhibition of QA-induced DNA fragmentationby a single dose of PGA₁ (80 nmol) was observed from 12 to 48h after QA treatment (Fig. 2A). To determine whether PGA₁ canrescue striatal neurons shortly after excitotoxin exposure, PGA₁(80 nmol) was administered 2, 4, or 6 h after the intrastriatalinfusion of QA. Under these conditions, PGA₁ diminished QA-inducedDNA fragmentation when administered up to 4 h after QA, but toa lesser degree than when given as a pretreatment (Fig. 2B).

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Fig. 1. Dose-dependence of effects of PGA₁ on QA-induced internucleosomal DNA fragmentation. Rats were treated intrastriatally with PGA₁ (5-80 nmol) or vehicle (40% EtOH, 1 µl) 10 min before intrastriatal administration of QA (60 nmol) and killed 24 h later. Genomic DNA was extracted from each animal (three animals in each group) and was first analyzed individually with agarose gels. Then an equal amount of pooled DNA was loaded onto each lane of the agarose gel for the presentation in Fig. 1. Lane 1, 100-bp DNA marker; 2, QA (60 nmol); 3, QA + EtOH (40%, 1 µl); 4, QA + PGA₁ (5 nmol); 5, QA + PGA₁ (20 nmol); 6, QA + PGA₁ (80 nmol); 7, PGA₁ (5 nmol); 8, PGA₁ (20 nmol); 9, PGA₁ (80 nmol).

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Fig. 2. Time course of effects of PGA₁ on QA-induced internucleosomal DNA fragmentation. A, rats were treated intrastriatally with PGA₁ (80 nmol) or vehicle (40% EtOH, 1 µl) 10 min before intrastriatal administration of QA (60 nmol) and killed 12, 24, or 48 h later. Genomic DNA was extracted from each animal (three animals in each group) and was first analyzed individually with 2% agarose gels. Then an equal amount of pooled DNA was loaded onto each lane of the agarose gel for the presentation in Fig. 2A. Lane 1, 100-bp DNA marker; 2, QA + Veh 12 h; 3, QA + PGA₁ 12 h; 4, QA + Veh 24 h; 5, QA + PGA₁ 24 h; 6, QA + Veh 48 h; 7, QA + PGA₁ 48 h. B, rats were treated intrastriatally with PGA₁ (80 nmol) or vehicle (40% EtOH, 1 µl) 10 min before or 2, 4, and 6 h after intrastriatal administration of QA (60 nmol) and killed 24 h later. Genomic DNA was extracted from each animal (three animals in each group) and was first analyzed individually with 2% agarose gels. Then an equal amount of pooled DNA was loaded onto each lane of the agarose gel for the presentation in Fig. 2B. Lane 1, 100-bp DNA marker; 2, QA + Veh; 3, pretreatment with PGA₁ 15 min before QA; 4, post-treatment with PGA₁ 2 h after QA; 5, post-treatment with PGA₁ 4 h after QA; 6, post-treatment with PGA₁ 6 h after QA.

Effect of PGA₁ on Striatal Cell Death. Receptor autoradiography for D₁ DA receptors and in situ hybridization histochemistry for GAD₆₇ mRNA revealed that PGA₁ markedlyreduced the loss of striatal neurons induced by QA. Quantitativeanalysis of these results showed that QA reduced the density ofD₁ DA receptors in the ipsilateral striatum to 39 ± 7.3% of control(contralateral side) (p < 0.05, n = 6). PGA₁ (5-80 nmol) decreasedthe QA-induced loss of D₁ DA receptors in a dose-dependent manner:D₁ DA receptors increased from 39 ± 7.3% of control in the QA-treatedgroup to up to 82 ± 2.7% of control in the QA plus PGA₁-treated(80 nmol) group (p < 0.05, n = 6, Fig. 3). Similarly, QA diminishedstriatal GAD₆₇ mRNA levels to 37 ± 6.7% of control (contralateralside) (p < 0.05, n = 6). Pretreatment with PGA₁ (5-80 nmol) alsoreduced the QA-induced decrease in GAD₆₇ mRNA levels: GAD₆₇ mRNAincreased from 37 ± 6.7% of control in the QA-treated group toup to 91 ± 2.8% of control in the QA plus PGA₁-treated (80 nmol)group (p < 0.05, n = 6, Fig. 4). Pretreatment with vehicle alsotended to reduce the QA-induced decrease in D₁ DA receptors (increasedfrom 39 ± 7.3% of control in the QA-treated group to 50 ± 6.5%of control in the QA plus vehicle-treated group, n = 6) and inGAD ₆₇ mRNA levels (increased from 37 ± 6.7% of control in theQA-treated group to 49 ± 6.8% of control in the QA plus vehicle-treatedgroup, n = 6), although these changes failed to attain statisticalsignificance.

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Fig. 3. Effects of PGA₁ on QA-induced loss of striatal D₁ DA receptors. Rats were treated intrastriatally with PGA₁ (5-80 nmol) or vehicle (40% EtOH, 1 µl) 10 min before intrastriatal administration of QA (60 nmol) and killed 10 days later. Brain sections were processed for D₁ DA receptor autoradiography. Results from six animals in each group were quantitatively analyzed with an image analyzer and expressed as percentage of control (contralateral striatum, mean ± S.E.M.). Statistical comparisons of QA + Veh or QA + PGA₁ with QA-treated group were performed using ANOVA followed by a Dunnett's t test. *p < 0.05.

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Fig. 4. Effects of PGA₁ on QA-induced loss of striatal GAD₆₇ mRNA. Rats were treated as described in the legend to Fig. 3. Brain sections were processed for in situ hybridization histochemistry for GAD₆₇ mRNA. Results from six animals in each group were quantitatively analyzed with an image analyzer and expressed as percentage of control (contralateral striatum, mean ± S.E.M.). Statistical comparisons of QA + Veh or QA + PGA₁ with QA-treated group were performed using ANOVA followed by a Dunnett's t test. *p < 0.05.

Consistent with changes in levels of D₁ DA receptors and GAD₆₇ mRNA in the QA-injected striatum, Nissl staining revealed thatQA induced a substantial loss of striatal neurons and gliosis.Pretreatment of rats with PGA₁ (80 nmol) markedly attenuated thisQA-induced loss (Fig. 5). Reduction in QA-induced neuronal losswas also observed when smaller doses of PGA₁ were administered(5 and 20 nmol, data not shown). Pretreatment with vehicle hadno apparent effect on the QA-induced reduction in striatal neurons.Injection of PGA₁ alone (80 nmol) caused relatively little neuronalloss except along the needle track (data not shown).

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Fig. 5. Effects of PGA₁ on the QA-induced loss of striatal neurons. Rats were treated intrastriatally with PGA₁ (5-80 nmol) or vehicle (40% EtOH, 1 µl) 10 min before intrastriatal administration of QA (60 nmol) and killed 10 days later. Brains were fixed with 4% paraformaldehyde and sectioned for Nissl staining. A and B, normal striatum. C and D, QA (60 nmol) treated. E and F, QA + PGA₁ (80 nmol) treated. Note: arrows in B and F indicate Nissl-stained striatal neurons. Asterisks in A, C, and E indicate regions where high-power photographs (B, D, and F) were taken. Arrowheads in C and E indicate needle tracks. In the QA-injected striatum (B and C), the number of Nissl-stained neurons was greatly reduced but Nissl-stained glial nuclei increased. In the QA + PGA₁ (80 nmol)-treated striatum (E and F), the loss of Nissl-stained neurons was reduced. Scale bar, 50 µm.

Effect of PGA₁ on QA-Induced Activation of NF- $kappa$ B. Under basal conditions, NF- $kappa$ B binding activity was relatively low. QA (60 nmol) induced a marked increase in NF- $kappa$ B (to 455± 54% of control, p < 0.05, n = 6) and AP-1 (to 270 ± 62% of control,p < 0.05, n = 6) binding activities in striatal nuclear extracts.Pretreatment with PGA₁ (5-80 nmol) diminished the QA-induced NF- $kappa$ Bincrement in a dose-dependent manner. The increased NF- $kappa$ B bindingactivity in nuclear extracts was reduced by about 50% at the highestdose of PGA₁ (80 nmol, p < 0.05, n = 6, Fig. 6A). In contrast,PGA₁ had no significant effect on QA-induced increases in AP-1binding activity (Fig. 6B). QA treatment caused a robust reductionin I $kappa$ B- $alpha$ protein levels (to 19 ± 5.2% of control, p < 0.05, n= 5). Pretreatment with PGA₁ (80 nmol) reversed the QA-induceddecline in I $kappa$ B- $alpha$ protein levels (increased from 19 ± 5.2% of controlin the QA-treated group to 86 ± 11.6% of control in the QA plusPGA₁ group, p < 0.05, n = 5, Fig. 7).

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Fig. 6. Effects of PGA₁ on QA-induced activation of NF- $kappa$ B and AP-1. Rats were treated intrastriatally with PGA₁ (5-80 nmol), vehicle (40% EtOH, 1 µl), or surgical procedures 10 min before intrastriatal administration of QA (60 nmol) and killed 12 h later. Striatal nuclear proteins were extracted for electrophoresis mobility shift assay. Results from six animals in each group were quantitatively analyzed with an image analyzer. Statistical comparisons of QA + Veh or QA + PGA₁ with control (animals received surgical procedures only) as well as QA + PGA₁ or QA + Veh with QA-treated group were performed using ANOVA followed by a Dunnett's t test. Data were then converted to percentage of control (animals received surgical procedures only, mean ± S.E.M.) for presentation in the bar figures. *p < 0.05 (comparisons of QA + PGA₁ with QA-treated group). A, NF- $kappa$ B; B, AP-1.

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Fig. 7. Effects of PGA₁ on QA-induced degradation of I $kappa$ B- $alpha$ . Rats were treated intrastriatally with PGA₁ (80 nmol), vehicle (40% EtOH, 1 µl) or surgical procedures 10 min before intrastriatal administration of QA (60 nmol) and killed 12 h later. Striatal total proteins were extracted for Western blot analysis. Results from five animals in each group were quantitatively analyzed with an image analyzer. Statistical comparisons of QA, QA + Veh, or QA + PGA₁ with control group (animals received surgical procedures only) as well as QA + PGA₁ or QA + Veh with QA-treated group were performed using ANOVA followed by a Dunnett's t test. The data were then converted to percentage of control (animals received surgical procedures only, mean ± S.E.M.) for presentation in the bar figures. *p < 0.05 (comparisons of QA, QA + PGA₁, or QA + Veh with control group); ^#p < 0.05 (comparisons of QA + PGA₁ with QA-treated group).

Effect of PGA₁ on Heat Shock Proteins. Basal striatal levels of HSP72 were undetectable. Striatally infused QA (60 nmol) produced only a modest rise in HSP72 expression.A more than 10-fold increase in HSP72 levels (to 1072 ± 110% ofcontrol, p < 0.05, n = 5, Fig. 8A) was observed in animals treatedwith PGA₁ (80 nmol) before QA administration. Basal levels of70-kDa HSP were also very low. QA produced an additional bandhaving a lower molecular mass (here named HSP70b as indicatedin Fig. 8B). Animals given PGA₁ before QA injection had no statisticallysignificant change in 70-kDa HSP (HSP70a). On the other hand,PGA₁ pretreatment markedly elevated HSP70b (to 1363 ± 219% ofcontrol, p < 0.05, n = 5, Fig. 8B). PGA₁ pretreatment had no significanteffect on levels of 70-kDa HSC (HSC70, Fig. 8C). HSP70 immunoreactivity(HSP70-i) was very low in normal control animals (Fig. 9A). Afew HSP70-i-positive cells near the injection site were observedin animals that received only vehicle treatment (Fig. 9B). Similarly,in QA plus vehicle-injected animals only scatter cells were intenselystained with HSP70 antibody (Fig. 9C). An increase in the numberof cells expressing HSP70-i and in the intensity of HSP70-i instriatal neurons were observed near the injection site in QA plusPGA₁ injected striatum (Fig. 9D, filled arrows). High intensityof HSP70-i was also observed in the nerve fiber bundles (Fig.9D, open arrow). The HSP70-i was totally eliminated by the omissionof the primary or secondary antibody (data not shown).

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Fig. 8. Effects of PGA₁ on QA-induced alterations in HSPs. Rats were treated as described in the legend to Fig. 6. Striatal total proteins were extracted for Western blot analysis. The results from five animals in each group were quantitatively analyzed with an image analyzer. Statistical comparisons of QA, QA + Veh, or QA + PGA₁ with control group (untreated animals) as well as QA + PGA₁ or QA + Veh with QA-treated group were performed using ANOVA followed by a Dunnett's t test. Data were then converted to percentage of control (untreated animals, mean ± S.E.M.) for presentation in the bar figures. *p < 0.05 (comparisons of QA + PGA₁ with control group); ^#p < 0.05 (comparisons of QA + PGA₁ with QA-treated group). A, HSP72; B, HSP70; C, HSC70.

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Fig. 9. Immunohistochemical study of induction of HSP70 by PGA₁ in striatal neurons. Rats were treated with intrastriatal injection of vehicle (40% EtOH, 1 µl), QA (60 nmol) + vehicle, or QA + PGA₁ (80 nmol) and killed 12 h later. Brains were fixed and sectioned as described under Materials and Methods. Sections were processed for immunohistochemistry. A, normal control; B, vehicle; C, QA + vehicle; D, QA + PGA₁. Filled arrows indicate striatal neurons with high intensity of HSP70-i after QA. Open arrow indicates nerve bundles with intense HSP70-i after QA. Scale bar, 50 µm.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

Prostaglandins are a class of cyclic 20-carbon fatty acids synthesized from polyunsaturated fatty acid precursors derivedfrom cell membranes. The type A and J prostaglandins are characterizedby the presence of an $alpha$ , $beta$ -unsaturated carbonyl group in the cyclopentanering of the molecule. PGA₁ has been reported to inhibit viralreplication, cause cell cycle arrest, increase HSP synthesis,and block NF- $kappa$ B activation (Lacal et al., 1994; D'Onofrio et al.,1995; Rossi et al., 1997, 2000). Based on the results of thisstudy, it now appears that PGA₁ is also capable of attenuatingthe internucleosomal DNA fragmentation and neuronal loss inducedby QA in rat striatum. The results suggest that PGA₁ exerts itsneuroprotective effects by inhibiting apoptosis. Conceivably,this action might lead to a heightened degree of necrotic celldeath. But this does not appear to have occurred, since therewas no increased smearing on the agarose gels to indicate a risein the random degradation of genomic DNA. Moreover, the decreasein internucleosomal DNA fragmentation was accompanied by a reductionin the loss of D₁ DA receptors and GAD₆₇ mRNA. Since there areno known direct effects of PGA₁ on striatal spiny GABAergic neuronmarkers, the reduced loss of these markers suggests neuroprotectionby PGA₁. Furthermore, the protective effect of PGA₁ was confirmedby the reduced loss of striatal neurons revealed by Nissl staining.Taken together, the present results suggest that PGA₁ has theability to protect striatal medium spiny neurons against NMDAreceptor-mediated toxicity by inhibiting their apoptoticdemise.

Since neuroprotection by PGA₁ has not been previously reported, the foregoing observations prompted an evaluation of its effectson an apoptotic cascade linked to the excitotoxin-induced deathof striatal neurons. In earlier investigations, we observed thathyperstimulation of NMDA or kainic acid receptors induces NF- $kappa$ Bactivation through the selective degradation of I $kappa$ B- $alpha$ (Nakai etal., 1999a; Qin et al., 2000). The present results indicate thatthe in vivo administration of PGA₁ selectively inhibits QA-inducedNF- $kappa$ B activation by blocking I $kappa$ B- $alpha$ degradation. The findings arein agreement with those deriving from in vitro studies (Rossiet al., 1997, 2000). PGA₁ had no effect on QA-induced AP-1, suggestingthat the neuroprotective action of PGA₁ is not mediated by NMDAreceptor blockade. PGA₁'s neuroprotective action also does notappear to involve cAMP, since QA and PGA₁ had no effect on cAMPlevels in rat striatum (data not shown). PGA₁ also had no effecton Bcl-2 and Bax levels in rat striatum after QA injection (datanot shown). The foregoing observations support the possibilitythat the neuroprotective effects of PGA₁ against excitotoxicityare mediated, at least in part, by NF- $kappa$ B inhibition and HSP induction.Nevertheless, it should be noted that PGA₁ has multiple pharmacologicalactions, including blood vessel dilation and inflammatory responseinhibition, and whether any of these effects influence acute excitotoxicinjury under the conditions of the present study is not known.Although several prostanoid receptors have been characterized,whether the neuroprotective action of PGA₁ is mediated throughits receptors remains to be determined (Coleman et al., 1994).

Earlier studies have found that aspirin and sodium salicylate inhibit glutamate toxicity in cultured neurons through a processinvolving NF- $kappa$ B inhibition (Grilli et al., 1996; Ko et al., 1998).Since PGA₁ reduced both the severity of internucleosomal DNA fragmentationand the size of the lesion induced by QA in rat striatum, thepresent results are consistent with the possibility that the inhibitionof glutamate receptor-stimulated NF- $kappa$ B activation protects againstexcitotoxin-induced neuronal injury (Qin et al., 1998).

The role of NF- $kappa$ B in the regulation of apoptosis is complicated. In certain circumstances, including tumor necrosis factor-inducedapoptosis in dividing somatic cells, NF- $kappa$ B signaling is associatedwith cell survival (Antwerp et al., 1996; Beg and Baltimore, 1996;Mattson et al., 1997). But under different conditions, such asthe excitotoxic destruction of postmitotic neurons, NF- $kappa$ B activationpromotes apoptosis (Qin et al., 1998; Nakai et al., 1999a; Schneideret al., 1999). Whether these opposite actions reflect differencesin the type or maturity of the cells being studied, in the apoptotictriggers being used, or whether the studies were conducted invitro or in vivo remains to be determined. Interestingly, a recentinvestigation has found that NF- $kappa$ B can play an antiapoptotic orproapoptotic role within the same type of cells (T-cell hybridomas)in response to different apoptotic stimuli (Lin et al., 1999).NF- $kappa$ B-regulated cell cycle entry may be another critical factorin determining its differing effects on apoptosis in proliferatingcells and postmitotic neurons. NF- $kappa$ B positively regulates cyclinD1 expression and stimulates G₀/G₁-to-S phase transition (Hinzet al., 1999). It now appears that cell cycle mediators contributeto the induction of neuronal apoptosis in response to ischemia,excitotoxins, oxidative stress, or nerve growth factor withdrawal(Freeman et al., 1994; Kranenburg et al., 1996; Park et al., 1998).Moreover, cell cycle inhibitors or cyclin-dependent kinase inhibitorsattenuate apoptosis triggered by nerve growth factor withdrawalin cultured neurons (Freeman et al., 1994; Park et al., 1997).In other studies, we found that cyclin D1 is induced by the NMDAreceptor agonist QA, and cyclin D1 induction can be reduced bythe NF- $kappa$ B inhibitors, including PGA₁ (Z.-H. Qin, R.-W. Chen, Y.Wang, X. Wang, D.-M. Chuang, and T. N. Chase, in preparation).The inhibition of NF- $kappa$ B activation in the present study supportsearlier reports showing PGA₁ causes cell cycle arrest (Goubinet al., 1986; Hughes-Fulford, 1994), which could serve as oneof the mechanisms underlying neuroprotection by PGA₁.

HSPs may contribute to the protective effects of PGA₁. PGA₁ has been reported to increase protein levels of HSPs (D'Onofrioet al., 1994; Lacal et al., 1994). Here we found that PGA₁ markedlyincreased levels of 70 and 72 HSPs in rat striatum. HSPs are ahighly conserved, finely regulated, cellular defense mechanismknown to be induced in various pathological states (Sloviter andLowenstein, 1992). Indeed, 70- and 72-kDa HSPs can have neuroprotectiveeffects against various insults, including glutamate toxicity(Lowenstein et al., 1991; Rordorf et al., 1991). Overexpressionof 72-kDa HSP in vivo with viral vectors protects striatal andhippocampal neurons from ischemia- and kainic acid-induced damage(Yenari et al., 1998). HSP induction could thus serve as an importantmediator of the ability of PGA₁ to protect striatal neurons againstexcitotoxin-induced apoptosis (Mailhos et al., 1993). HSPs areknown to have multiple influences on cellular function, includingprotein folding and trafficking as well as intracellular signaltransduction, and exactly how they might counteract QA-inducedneuronal apoptotic cascades remains to beelucidated.

Excitotoxicity has been proposed to contribute the pathogenesis of a number of neurodegenerative disorders, including stroke,Huntington's disease, Parkinson's disease, AD, and amyotrophiclateral sclerosis. If correct, inhibiting the effects of glutamatereceptor hyperstimulation could act to retard the degenerativeprocess. Given the prominent role of NF- $kappa$ B and heat shock proteinsin neuronal survival as well as the present finding that pretreatmentor post-treatment with PGA₁ inhibits the QA-induced apoptoticdeath of these neurons, it is tempting to speculate that drugscapable of inhibiting NF- $kappa$ B cascade and inducing heat shock proteinsmay be useful in the treatment of neurodegenerative disorderswhere excitotoxic mechanisms contribute topathogenesis.

	Footnotes

Accepted for publication January 2, 2001.

Received for publication June 20, 2000.

¹ Current address: Laboratory of Cellular Neurobiology, Massachusetts General Hospital and Harvard Medical School, Charlestown,MA02129.

Send reprint requests to: Thomas N. Chase, M.D., Chief, Experimental Therapeutics Branch, National Institute of Neurodegenerative Disorders and Stroke, Bldg. 10, Room 5C103, 10 Center Dr. MSC 1406, Bethesda, MD 20892-1406. E-mail: chase{at}helix.nih.gov

	Abbreviations

NF- $kappa$ B, nuclear factor- $kappa$ B; I $kappa$ B, inhibitory $kappa$ B; QA, quinolinic acid; AD, Alzheimer's disease; PGA₁, prostaglandin A₁; HSP, heat shock protein; EtOH, ethanol; AP-1, activator protein-1; HSP72, 72-kDa heat shock protein; PBS, phosphate-buffered saline; Veh, vehicle; PBST, phosphate-buffered saline Tween 20; HSC70, heat shock cognate 70; DA, dopamine; GAD₆₇ mRNA, 67-kDa glutamic acid decarboxylase messenger RNA; HSP70-i, heat shock protein 70 immunoreactivity; NMDA, N-methyl-D-aspartate; bp, base pair; GABA, $gamma$ -aminobutyric acid.

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