Increased Production of Tumor Necrosis Factor-alpha  by Glial Cells Exposed to Simulated Ischemia or Elevated Hydrostatic Pressure Induces Apoptosis in Cocultured Retinal Ganglion Cells

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The Journal of Neuroscience, December 1, 2000, 20(23):8693-8700

Increased Production of Tumor Necrosis Factor- $alpha$ by Glial Cells Exposed to Simulated Ischemia or Elevated Hydrostatic Pressure Induces Apoptosis in Cocultured Retinal Ganglion Cells
Gülgün Tezel and Martin B. Wax
Department of Ophthalmology and Visual Sciences, Washington University School of Medicine, St. Louis, Missouri 63110

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Although glial cells in the optic nerve head undergo a reactivation process in glaucoma, the role of glial cells during glaucomatousneurodegeneration of retinal ganglion cells is unknown. Usinga coculture system in which retinal ganglion cells and glial cellsare grown on different layers but share the same culture medium,we studied the influences of glial cells on survival of retinalganglion cells after exposure to different stress conditions typifiedby simulated ischemia and elevated hydrostatic pressure. Afterthe exposure to these stressors, we observed that glial cellssecreted tumor necrosis factor- $alpha$ (TNF- $alpha$ ) as well as other noxiousagents such as nitric oxide into the coculture media and facilitatedthe apoptotic death of retinal ganglion cells as assessed by morphology,terminal deoxynucleotidyl transferase-mediated dUTP nick end labeling,and caspase activity. The glial origin of these noxious effectswas confirmed by passive transfer experiments. Furthermore, retinalganglion cell apoptosis was attenuated ~66% by a neutralizingantibody against TNF- $alpha$ and 50% by a selective inhibitor of induciblenitric oxide synthase (1400W). Because elevated intraocular pressureand ischemia are two prominent stress factors identified in theeyes of patients with glaucoma, these findings reveal a novelglia-initiated pathogenic mechanism for retinal ganglion celldeath in glaucoma. In addition, these findings suggest that theinhibition of TNF- $alpha$ that is released by reactivated glial cellsmay provide a novel therapeutic target for neuroprotection inthe treatment of glaucomatous opticneuropathy.

Key words: apoptosis; glaucoma; glia; nitric oxide; retinal ganglion cell; tumor necrosis factor- $alpha$

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

During development and maintenance of the nervous system there exists a complex interdependency between neurons and glialcells. The glial cells maintain normal functioning of the nervoussystem both by controlling the extracellular environment and bysupplying metabolites and growth factors. However, recent evidencechallenges the view that glial cells are purely neuroprotectiveand rather suggests that they could participate in damaging neurons.For example, after focal cerebral ischemia or during the courseof neurodegenerative diseases or trauma, reactive astrocytes aswell as microglia within the CNS produce cytokines, reactive oxygenspecies, and nitric oxide (NO), which are implicated as mediatorsof tissue injury (Hewett et al., 1994; Dugan et al., 1995; Ridetet al., 1997; Vandenberghe et al., 1998; Viviani et al., 1998;Raivich et al., 1999).

The astrocytes located at the optic nerve head undergo a reactivation process in glaucoma (Hernandez and Pena, 1997). In glaucomatousoptic neuropathy, apoptosis is implicated in the death of retinalganglion cells (Quigley et al., 1995), but the precise pathogenicmechanisms leading to apoptotic cell death are unknown. Althoughthe relationship of glial reactivation to neurodegeneration inglaucoma has not been established, increased production of someneurotoxic substances by optic nerve head astrocytes has beenidentified in glaucomatous eyes. For example, increased productionof nitric oxide synthase (NOS; Neufeld et al., 1997) and tumornecrosis factor- $alpha$ (TNF- $alpha$ ; Yan et al., 2000) has been describedin the glaucomatous optic nerve head. In addition, expressionof the inducible isoform of NOS (iNOS) and TNF- $alpha$ by chemicallyreactivated retinal glial cells has been observed in rat modelsof hereditary retinal diseases (Cotinet et al., 1997; de Kozaket al., 1997; Goureau et al., 1999). Therefore, we hypothesizethat retinal astroglial reactivation may lead to the increasedproduction of neurotoxic substances and thereby participate inneuronal damage inglaucoma.

Although neuron-glia interactions have been examined in experimental models of degenerative diseases of the CNS, there isno direct evidence suggesting that glial cells are harmful tothe survival of retinal ganglion cells. Using a coculture system,we studied the effects of glial cells on the survival of retinalganglion cells after exposure to different stress conditions.This coculture system provides a good model to study neuron-gliainteractions because it permits quantitative assessment of theeffects of different stimuli on neuronal and glial cells separately.During these experiments we used elevated hydrostatic pressureand simulated ischemia as stress conditions, because elevatedintraocular pressure and ischemia are common stress factors identifiedin glaucomatous eyes, which are thought to facilitate retinalganglion cell apoptosis (Hart et al., 1979; Quigley et al., 1980;Hayreh, 1985).

Here we present novel evidence that elevated hydrostatic pressure as well as simulated ischemia can initiate the apoptoticcell death cascade in retinal ganglion cells, mainly because ofthe reactivity of glial cells in response to these stressors.Apoptosis-promoting substances, including TNF- $alpha$ secreted by reactivatedglial cells after exposure to stress, contribute directly to neuronalcytotoxicity.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Retinal ganglion cell cultures. Primary cultures of retinal ganglion cells were derived from newborn rat retinas, using aprotocol similar to that recently described (Tezel et al., 1999).All experiments were performed in accordance with the Associationfor Research in Vision and Ophthalmology (ARVO) Statement forthe Use of Animals in Ophthalmic and Vision Research and wereapproved by The Animal Studies Committee of Washington University.Sprague Dawley rats (5-7 d old) were anesthetized, and their eyeswere enucleated. The eyes were rinsed with CO₂-independent culturemedium (Life Technologies, Grand Island, NY), and retinas weredissected mechanically under a microscope. To prepare retinalcell suspensions, we dissociated tissues in Eagle's MEM containing20 U/ml papain, 1 mM L-cysteine, 0.5 mM EDTA, and 0.005% DNase(Worthington, Lakewood, NJ) at 37°C for 40 min. Then the retinaswere rinsed in an inhibitor solution containing Eagle's MEM, 0.2%ovomucoid (US Biological, Swampscott, MA), 0.04% DNase, and 0.1%bovine serum albumin (Sigma, St. Louis, MO). At the end of thetreatment period the tissues were triturated through a 1 ml plasticpipette to yield a suspension of single cells. The retinal cellswere spun at 400 × g for 10 min, resuspended in Eagle's MEM containing0.05% bovine serum albumin, and incubated in a tissue cultureincubator until their immediate use for subsequent separationby immunomagneticselection.

Immunomagnetic selection of the retinal ganglion cells was performed by using magnetic, 2.8 ± 0.2 µm diameter, polystyrenebeads coated with biotinylated rat monoclonal antibody againstmouse IgG₁ (Dynal, Oslo, Norway) in a two-step process. In thefirst step, after a washing with PBS solution containing 0.1%bovine serum albumin, 1 × 10⁷ beads/ml were added to the monoclonal antibody against macrophagesurface antigens (100 µg/ml; Sigma). After incubation at roomtemperature on a rotator for 30 min, the beads were washed witha specially designed magnet (Dynal). Coated beats were incubatedwith retinal cell suspension with gentle rotation for 15 min andthen removed from the cell suspension to remove the bound macrophages.As a second step, fresh magnetic beads were added to monoclonalantibody (IgG₁) specific to Thy-1.1 (Chemicon, Temecula, CA) toobtain a final concentration of 100 µg/ml. After incubation atroom temperature for 30 min and washing, the coated beads wereincubated with the macrophage-depleted retinal cell suspensionfor 15 min. Because the monoclonal antibody was attached to beadsvia streptavidin and a DNA linker, the attached cells were separatedfrom the beads by incubation with DNase-releasing buffer (50 U/µl)at 37°C for 15 min. Then the cells were seeded on extracellularmatrix-coated 24-well plates (Fisher Scientific, Pittsburgh, PA)at a density of 4 × 10⁴ cells/well and were cocultured with glial cells. Cultures wereincubated in a tissue culture incubator with a humidified atmosphereof 5% CO₂/95% air at 37°C.

A retinal glial cell line was prepared with the retinal cells that were depleted for microglial and ganglion cells by followingthe magnetic selection process described above. After the lossof residual neuronal cells by two or three cycles of replating,these cultures contained essentially glial cells as previouslydescribed, which were identified as astrocytes and Müller glialcells, as presented in Results. The retinal glial cells were seededon tissue culture inserts (Fisher Scientific) at a density of3 × 10⁴ cells/well and placed in the wells in which the retinal ganglioncells were seeded. These inserts contain polyethylene terephthalatemembrane with 0.4 µm pore size and allow for the transport ofsecreted molecules while preventing cellmigration.

The serum-free culture medium was prepared by using B27-supplemented Neurobasal (Life Technologies) as previously described(Barres et al., 1988; Brewer et al., 1993). The medium also contained(in µg/ml) 100 bovine serum albumin, 5 insulin, 16 putrescine,and 100 transferrin; 1 mM pyruvate, 1 mM glutamine; (in ng/ml)60 progesterone, 40 sodium selenite, 30 triiodo-thyronine, 50BDNF, 20 CNTF, and 10 bFGF; 5 µM forskolin, 100 µM inosine, andantibiotics (Jo et al., 1999). All supplements were purchasedfromSigma.

Retrograde labeling of retinal ganglion cells. Under general anesthesia that used a mixture of 80 mg/kg ketamine (Fort DodgeLaboratories, Fort Dodge, IA) and 12 mg/kg xylazine (Butler, Columbus,OH) given intraperitoneally and with immobilization of the ratsin a stereotaxic apparatus, bilateral microinjections of Fluoro-Gold(1.5 µl of a 5% solution of Fluoro-Gold in 0.9% sodium chloride;Fluorochrome, Englewood, CO) into the superior colliculi wereperformed according to the previously described methods (Selles-Navarroet al., 1996). One week after Fluoro-Gold application the retinaswere dissected and dissociated. After a selection of retinal ganglioncells via the immunomagnetic method, selected and unselected cellswere examined by flow cytometry after double immunolabeling ofFluoro-Gold and Thy-1.1.

Flow cytometry. Retinal cells were fixed with 2% paraformaldehyde solution for 20 min at room temperature. After centrifugeand resuspension of the cells, they were permeabilized in TritonX-100 (0.4% in PBS solution) for 30 min. Washed cells then wereincubated with a mixture of rabbit antibody against Fluoro-Gold(Fluorochrome) and mouse antibody against Thy-1.1 at a 1:100 dilutionfor 30 min. After washing, the cells were incubated with a mixtureof FITC- and Cy3-conjugated secondary antibodies (Sigma) for another30 min. Then the cells were washed, resuspended at 10⁶ cells/ml, and counted with a FACScan flow cytometer/CELLQuestsoftware system (Becton Dickinson, San Jose,CA).

Study design. The retinal ganglion cells exhibiting contact of the neuritic processes and glial cells that had been grownto approximate confluence were incubated under stress conditionsor normal conditions. For simulated ischemia the cells were exposedto reduced oxygen tensions in a medium lacking glucose. Hypoxiawas maintained by placing the cultures in a dedicated cultureincubator with a controlled flow of 95% N₂/5% CO₂. A closed pressurizedchamber equipped with a manometer was used to expose the cellsto elevated hydrostatic pressure. The pressure was elevated to50 mmHg. The chamber was placed in a regular tissue culture incubatorat 37°C. To examine the time course of cellular responses, wemaintained the simulated ischemia or elevated pressure for 6,12, 24, 48, or 72 hr. Control cells from an identical passageof cells were incubated simultaneously in a regular tissue cultureincubator at 95% air/5% CO₂ at 37°C. To examine glial sourcesof noxious insults on retinal ganglion cells, we collected conditionedmedium from glial cells that were cultured alone after their incubationin the presence or absence of stress conditions for 72 hr. Retinalganglion cells that were cultured alone then were incubated withthe conditioned medium of glial cells for 24hr.

In addition, to examine the role of TNF- $alpha$ and NO on cell survival, we performed incubations under stress conditions in thepresence or absence of specific inhibitors. A neutralizing antibody(AF510NA) was used to inhibit TNF- $alpha$ activity (R&D Systems, Minneapolis,MN). The ability of this antibody to neutralize the bioactivityof recombinant rat TNF- $alpha$ in the L-929 cell line in the presenceof actinomycin D revealed that the neutralization dose₅₀ was ~0.3-0.9µg/ml in the presence of 0.025 ng/ml of recombinant rat TNF- $alpha$ .The neutralizing antibody of TNF- $alpha$ activity was neuroprotectivein in vitro or in vivo experiments (Barone et al., 1997; Lavineet al., 1998; Downen et al., 1999). In addition, [N-(3-[aminomethyl]benzyl)acetamidinedihydrochloride] (1400W; Alexis, San Diego, CA), a selective inhibitorof iNOS, was used to inhibit inducible synthesis of NO (Garveyet al., 1997). We used 10 µg/ml of the neutralizing antibody ofTNF- $alpha$ and 2.5 µM of the iNOS inhibitor 1400W, because these wereoptimum conditions to inhibit TNF- $alpha$ and iNOS, respectively, inour cocultures on the basis of concentration-response experiments(data not shown). At the end of the incubation period the cellswere subjected immediately to the experiments described below,which were repeated at least three times for eachcondition.

The viability of the cells was determined with the Live/Dead Kit (Molecular Probes, Eugene, OR), which contains calcein-AMand ethidium homodimer (Haugland and Larison, 1994). Calcein-AMis a cell-permeable fluorogenic esterase substrate. The kit relieson the intracellular esterase activity within living cells tohydrolyze calcein-AM to a green fluorescent product, calcein.In dead cells ethidium can pass easily through the compromisedplasma and nuclear membranes and attach to the DNA, yielding redfluorescence. Cells were counted in at least 10 random fieldsof each well at 200× magnification (~150 ganglion cell per well)with a fluorescence microscope (Olympus, Tokyo, Japan). The viabilityof the cells was expressed as the average ratio of esterase (+)cells to the total number of cells multiplied by100.

Morphological analysis of apoptosis. An in situ cell death detection kit (Boehringer Mannheim, Mannheim, Germany) was usedto identify the apoptotic cells by the terminal deoxynucleotidyltransferase-mediated dUTP nick end labeling (TUNEL) technique(Gavrieli et al., 1992). Briefly, after fixation, permeabilization,and blocking steps the air-dried cells were incubated with a mixtureof fluorescein-labeled nucleotides and terminal deoxynucleotidyltransferase for 1 hr. Terminal deoxynucleotidyl transferase catalyzesthe polymerization of labeled nucleotides to free 3'-OH terminalsof DNA fragments. Cells incubated with fluorescein-labeled nucleotidemixture without the presence of terminal deoxynucleotidyl transferaseserved as a negative control. Cells previously treated with DNaseI (1 mg/ml) to induce breaks in the DNA strands served as a positivecontrol. TUNEL-positive cells were counted in triplicate wellsunder a fluorescence microscope, and the percentage of apoptosiswas calculated by using the total number of cells in thesewells.

Western blotting. After the cells were washed with PBS solution, they were lysed in sample buffer (1% SDS, 100 mM dTT, 60mM Tris, pH 6.8, and 0.001% bromophenol blue). Protein concentrationswere determined via the bicinchoninic acid (BCA) method (Sigma).The samples were boiled for 5 min before they were subjected toelectrophoresis.

Samples were separated by electrophoresis in 10-15% SDS polyacrylamide gels at 160 V for 1 hr and electrophoretically transferredto polyvinylidene fluoride membranes (Millipore, Marlboro, MA)via a semi-dry transfer system (Bio-Rad, Hercules, CA). Aftertransfer the membranes were blocked in a buffer (50 mM Tris HCl,154 mM NaCl, and 0.1% Tween-20, pH 7.5) containing 5% nonfat drymilk for 1 hr and then overnight in the same buffer containinga dilution of primary antibody and sodium azide. Primary antibodieswere monoclonal antibodies to TNF- $alpha$ (R&D Systems), isotypes ofNOS (neuronal NOS and iNOS; Transduction Laboratories, Lexington,KY), caspase-8, or polyclonal antibody to caspase-3 (PharMingen,San Diego, CA); they were used at a dilution of 1:1000. Afterseveral washes and a second blocking for 20 min, the membraneswere incubated with a dilution of secondary antibodies conjugatedwith horseradish peroxidase (Fisher Scientific) at 1:2000 for1 hr. Immunoreactive bands were visualized by enhanced chemiluminescencewith the use of commercial reagents (Amersham Life Science, ArlingtonHeights,IL).

Examination of caspase activity. Caspase-3-like activity was examined in situ after staining with Phiphilux-G₆D₂ (Alexis,San Diego, CA). Phiphilux-G₆D₂ is a cell-permeable fluorogenicsubstrate that is cleaved to produce rhodamine molecules and thatcan be used to detect caspase-3-like activity in living cells(Finucane et al., 1999). For staining, the washed cells were incubatedwith a substrate solution of 10 µM for 20 min at 37°C. Rhodaminefluorescence was visualized under a fluorescencemicroscope.

In addition, caspase-3-like protease activity was measured in a fluorometric assay by measuring the extent of cleavage ofthe fluorometric peptide substrate as previously described (Chenget al., 1998; Tezel and Wax, 1999). Briefly, cell lysates wereincubated with Ac-Asp-Glu-Val-Asp-7-amino-4-trifluoro-methyl coumarin(Ac-DEVD-AMC) fluorometric substrate (50 µM). Positive controlsincluded purified recombinant caspase-3 (0.1 µg; Upstate Biotechnology,Lake Placid, NY). Fluorescence was measured at an excitation wavelengthof 360 nm and an emission wavelength of 460 nm in a fluorescentplate reader at different time points up to 180 min. The proteaseactivity was expressed as picomoles of substrate per milligramof protein per minute as calculated by using the linear rangeof theassay.

Immunocytochemistry. Cells were washed in PBS solution and fixed with 4% paraformaldehyde solution for 30 min at room temperature.After washing, they were permeabilized with 0.1% Triton X-100in 0.1% sodium citrate solution on ice for 4 min. Then the cellswere treated with 3% bovine serum albumin for 30 min to blockthe nonspecific binding sites. Triplicate wells were incubatedwith monoclonal antibodies against TNF- $alpha$ (R&D Systems) or isotypesof NOS (neuronal NOS and iNOS; Transduction Laboratories) at 37°Cfor 2 hr. Next the samples were washed and incubated with theappropriate second antibodies conjugated with Cy3 (Sigma). Afterwashing, they were examined with a fluorescencemicroscope.

For examination of the purity of cultures the cells were double-immunolabeled with specific cell markers. For double immunofluorescencelabeling after the fixation, permeabilization, and blocking steps,the cultures were incubated with a mixture of two antibodies (onerabbit and one mouse antibody) against Thy-1.1, neurofilamentprotein, glial fibrillary acidic protein, or S-100 protein (Sigma)at 1:100 dilution for 30 min. After being washed, the cells wereincubated with a mixture of Cy3- and FITC-conjugated secondaryantibodies (Sigma) for another 30 min. Negative controls wereperformed by replacing the primary antibody with nonimmune serumor by incubating the cells with each primary antibody, followedby the inappropriate secondary antibody to determine that eachsecondary antibody was specific to the species it was made against.Then the cultures were examined with a fluorescencemicroscope.

Enzyme-linked immunosorbent assay (ELISA). We used a kit to measure TNF- $alpha$ levels in conditioned medium by quantitative sandwichELISA technique (R&D Systems). Conditioned medium was incubatedin microwells coated with monoclonal antibody specific for ratTNF- $alpha$ . After a wash, horseradish peroxidase-conjugated polyclonalantibody specific for rat TNF- $alpha$ was added to the wells. Afteranother wash, a substrate solution containing hydrogen peroxideand tetramethylbenzidine was added. The enzyme reaction was terminatedby the addition of hydrochloric acid solution, and absorbancewas measured at 450 nm. Using a standard curve prepared from sevendilutions of recombinant rat TNF- $alpha$ , we calculated the concentrationsof TNF- $alpha$ in conditioned medium. The sensitivity was <5 pg/ml.

Colorimetric assay. To measure breakdown products of NO in conditioned medium, we used a colorimetric assay kit (R&D Systems).This assay determined NO on the basis of the enzymatic conversionof nitrate to nitrite by nitrate reductase. The reaction was followedby a colorimetric detection of nitrite as an azo dye product ofthe Griess reaction. As an additional step, lactate dehydrogenaseand pyruvic acid were used before color formation to oxidize theexcess of NADPH because NADPH, an essential cofactor for the functionof NOS enzyme, interferes with the chemistry of Griess reagents.Because the relative levels of nitrate and nitrite can vary substantially,depending on the ambient conditions and redox state of the biologicalfluids, for the most accurate determination of total NO productionboth the nitrate and nitrite levels were measured. The absorbancewas read at 540 nm, and the concentrations of breakdown productsof NO were calculated by using a standard curve. The sensitivityof the nitrite assay was <0.22 µmol/l, and the sensitivity ofthe nitrate assay was <0.54 µmol/l.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cell morphology and viability

Retinal ganglion cells were identified on the basis of retrograde labeling with Fluoro-Gold, morphology, and expression ofcell markers. After retrograde labeling with Fluoro-Gold and theselection of retinal ganglion cells by an immunomagnetic separationmethod, the cells were immunolabeled by antibodies against Fluoro-Goldand Thy-1.1. Using flow cytometry, we observed that the immunolabelingby Fluoro-Gold and Thy-1.1 antibodies was colocalized in >90%of these cells; >95% of the cells were positive for Thy-1.1 (Fig.1A). Cells unselected by sorting were negative for both Fluoro-Goldand Thy-1.1 (Fig. 1B).

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Figure 1. Cultured retinal cells. After retrograde labeling by Fluoro-Gold and the selection of retinal ganglion cells by the use of an immunomagnetic separation method, the selected cells were immunolabeled with antibodies against Fluoro-Gold and Thy-1.1; they were examined with flow cytometry. A, Immunolabeling with Fluoro-Gold (FL1-H) and Thy-1.1 (FL3-H) antibodies was colocalized in >90% of these cells; >95% of these cells were positive for Thy-1.1. B, Unselected cells were negative for both Fluoro-Gold (FL1-H) and Thy-1.1 (FL3-H). Cultured retinal ganglion cells had round or oval cell bodies with a diameter of 10-20 µm, phase-bright appearance, and branched neuritis of uniform caliber and varying length. C, A retinal ganglion cell derived from newborn rat retina. D, Fluorescence microscope image of the retinal ganglion cell shown in C after labeling for neurofilament protein. E, Fluorescence microscope image of the retinal ganglion cell shown in C after labeling for Thy-1.1. F, Glial cells derived from newborn rat retina. G, Fluorescence microscope image of the retinal glial cells shown in F after labeling for glial fibrillary acidic protein. H, Fluorescence microscope image of the retinal glial cells shown in F after labeling for S-100. Scale bars: C-E, 20 µm; F-H, 60 µm.

Cultured retinal ganglion cells had round or oval cell bodies with a diameter of 10-20 µm, a phase-bright appearance, andbranched neurites of uniform caliber and varying length (Fig.1C), as previously identified (Barres et al., 1988). In addition,the purity of cultured retinal cells was examined by using immunolabelingfor specific markers. The retinal ganglion cells were homogenouslypositive for Thy-1.1 and neurofilament protein, but negative forglial markers. Glial cells were homogenously labeled for glialfibrillary acidic protein, selectively labeled for S-100, butunlabeled for neuronal markers (Fig. 1).

At the beginning of the incubation of the cocultures under stress conditions, the percentage of living retinal ganglion cellsand glial cells was 96.69 ± 1.6 and 97.84 ± 1.9%, respectively.The cell viability decreased to 69.69 ± 2.0 and 76.64 ± 1.9% inretinal ganglion cells after 72 hr of incubation in the presenceof simulated ischemia or elevated hydrostatic pressure, respectively.However, the viability of glial cells was 96.24 ± 2.1% at theend of incubation period under either simulated ischemia or elevatedhydrostaticpressure.

Induction of apoptosis in retinal ganglion cells in cocultures exposed to simulated ischemia or elevated hydrostatic pressure

Apoptosis was induced in retinal ganglion cells after the incubation of the cocultures in the presence of simulated ischemiaor elevated hydrostatic pressure for as long as 72 hr. Specificmorphological changes of apoptotic cell death included cell bodyshrinkage and compaction of the nucleus (Fig. 2A-C). In addition,apoptotic cell death was examined via the TUNEL technique. Theapoptotic retinal ganglion cells exhibited bright labeling offragmented nuclear DNA by TUNEL (Fig. 2D-F). However, there wasno evidence of apoptosis in glial cells in the cocultures thatwere incubated under stress conditions by either morphologicalexamination or TUNEL technique (Fig. 2G-L).

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Figure 2. Morphological analysis of apoptotic cell death in cocultures of retinal ganglion cells and glial cells. A-C, Phase-contrast microscope images of retinal ganglion cells that were incubated under different conditions for 72 hr. A, Normal conditions. B, Simulated ischemia. C, Elevated hydrostatic pressure. Fluorescence microscope images of TUNEL in D-F correspond to retinal ganglion cells seen in A-C, respectively. G-I, Phase-contrast microscope images of glial cells that were incubated under different conditions for 72 hr. G, Normal conditions. H, Simulated ischemia. I, Elevated hydrostatic pressure. Fluorescence microscope images of TUNEL in J-L correspond to glial cells seen in G-I, respectively. After the incubation of cocultures under stress conditions, apoptosis was induced in retinal ganglion cells, although there was no evidence of apoptosis in glial cells.

Quantitative examination of apoptotic cell death after incubation under stress conditions revealed that the percentage ofpositive TUNEL was approximately three times greater in retinalganglion cells cocultured with glial cells as compared with retinalganglion cells cultured alone. After incubation under stress conditionsfor 72 hr, >20% of the retinal ganglion exhibited positive TUNEL;in the retinal ganglion cells that were cultured alone the rateof positive TUNEL was <7% (Mann-Whitney U test; p = 0.006 andp = 0.04 for simulated ischemia and elevated hydrostatic pressure,respectively; Fig. 3A). In addition, after incubation under stressconditions apoptosis was induced in retinal ganglion cells incocultures in a time-dependent manner (Fig. 3A). Although therate of positive TUNEL was 24.10 ± 6.0 and 19.90 ± 5.4% in retinalganglion cells in cocultures that were exposed to simulated ischemiaor elevated hydrostatic pressure for 72 hr, respectively, retinalganglion cells in control cultures that were incubated under normalconditions exhibited apoptosis in <2% of the cell population (Mann-WhitneyU test, p = 0.017, p = 0.023, respectively). However, the percentageof positive TUNEL was virtually absent in glial cells that wereincubated in the absence or presence of stress conditions (0.94± 0.6 and 1.12 ± 1.0%, respectively; p > 0.05 for both conditions).

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Figure 3. A, Quantitative analysis of positive TUNEL in retinal ganglion cells that were incubated under simulated ischemia or elevated hydrostatic pressure. After incubation in the presence of simulated ischemia or elevated hydrostatic pressure for 72 hr, the rate of positive TUNEL was higher in retinal ganglion cells in cocultures compared with that in retinal ganglion cells that were cultured alone (RGCs; p = 0.006 and p = 0.04, respectively). In addition, the rate of positive TUNEL was higher in retinal ganglion cells in cocultures exposed to simulated ischemia or elevated hydrostatic pressure for 72 hr, respectively, compared with that in retinal ganglion cells in cocultures incubated under normal conditions (Mann-Whitney U test; p = 0.017 and p = 0.023, respectively). B, Quantitative analysis of positive TUNEL in retinal ganglion cells after passive transfer experiments. Conditioned medium of glial cells that were cultured alone was collected after their incubation in the presence or absence of simulated ischemia or elevated hydrostatic pressure for 72 hr. Then retinal ganglion cells that were cultured alone were incubated with the glial-conditioned medium for 24 hr. The rate of positive TUNEL was higher in retinal ganglion cells that were incubated with the conditioned medium of stressed glial cells as compared with that in retinal ganglion cells that were incubated with the conditioned medium of control glial cells (p = 0.04 and p = 0.02 for simulated ischemia and elevated hydrostatic pressure, respectively).

In addition, we performed passive transfer experiments to examine the glial source of noxious insults on retinal ganglioncells. For this purpose, the conditioned medium of glial cellsthat were cultured alone was collected after their incubationin the presence or absence of simulated ischemia or elevated hydrostaticpressure for 72 hr. Retinal ganglion cells that were culturedalone then were incubated with the glial conditioned medium for24 hr. The TUNEL was positive in ~17% of retinal ganglion cellsthat were incubated with the conditioned medium of stressed glialcells, whereas <2% of retinal ganglion cells exhibited positiveTUNEL in cultures that were incubated with the conditioned mediumof glial cells incubated under normal conditions (Mann-WhitneyU test; p = 0.04 and p = 0.02 for simulated ischemia and elevatedhydrostatic pressure, respectively; Fig. 3B).

Caspase activation accompanying retinal ganglion cell apoptosis

To examine caspase activation, we used lysates of retinal cells in Western blotting. Western blot analysis demonstrated cleavageof caspase-8 and caspase-3 in retinal ganglion cells after exposureof the cocultures to simulated ischemia or elevated hydrostaticpressure. Western blots that used the lysates of retinal ganglioncells incubated under stress conditions revealed a 55 kDa immunoreactiveband corresponding to caspase-8 and ~30 and 20 kDa cleaved products.The presence of caspase-3 activation was assessed by the observationof 17 kDa subunit that was derived from the cleavage of the 32kDa pro-enzyme caspase-3. No cleavage of caspase-8 or caspase-3was detected by using the lysates of glial cells that were incubatedunder stress conditions (Fig. 4A,B).

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Figure 4. Examination of caspase activity in cocultures incubated under simulated ischemia or elevated hydrostatic pressure. A, Western blot analysis of caspase-8 expression in cocultures. B, Western blot analysis of caspase-3 expression cocultures. Column 1, Control retinal ganglion cells; column 2, retinal ganglion cells incubated under simulated ischemia for 72 hr; column 3, retinal ganglion cells incubated under elevated hydrostatic pressure for 72 hr; column 4, control glial cells; column 5, glial cells incubated under simulated ischemia for 72 hr; column 6, glial cells incubated under elevated hydrostatic pressure for 72 hr. Western blots revealed that the 55 kDa immunoreactive band corresponding to caspase-8 cleaved to 30 and 20 kDa products in retinal ganglion cells that were incubated under stress conditions. In addition, 32 kDa pro-enzyme caspase-3 cleaved to a 17 kDa active subunit in retinal ganglion cells. No cleavage of caspase-8 or caspase-3 was detected with the use of the extracts of glial cells. Caspase activation also was examined, in situ, using Phiphilux-G₆D₂ in retinal ganglion cells that were incubated under different conditions for 72 hr. C, Normal conditions. D, Simulated ischemia. E, Elevated hydrostatic pressure. Fluorescence microscope images seen in F-H correspond to phase-contrast images of the retinal ganglion cells seen in C-E, respectively. Rhodamine fluorescence (red) indicates caspase-3-like activity in retinal ganglion cells that were incubated under stress conditions. I, The amount of DEVD-AMC cleaving activity with the use of fluorometric analysis was higher in retinal ganglion cells in cocultures that were incubated under simulated ischemia or elevated hydrostatic pressure for 72 hr as compared with cocultures that were incubated under normal conditions (Mann-Whitney U test; p = 0.006 and p = 0.04, respectively).

In addition, we examined caspase-3-like protease activity in cocultures. In situ examination that used the fluorogenic substratePhiphilux-G6D2 demonstrated caspase-3-like activity in livingretinal ganglion cells exposed to simulated ischemia or elevatedhydrostatic pressure for 72 hr (Fig. 4C-H). We also performedfluorometric analysis that used lysates of retinal ganglion cellsto measure the cleavage of Ac-DEVD-AMC, which reflects caspase-3-likeactivity. The amount of DEVD-AMC cleaving activity was ~10 timeshigher in retinal ganglion cells in cocultures that were incubatedunder simulated ischemia or elevated hydrostatic pressure for72 hr (38.67 ± 7.4 and 31.00 ± 6.2 pmol/mg protein/min, respectively)compared with control cultures that were incubated under normalconditions (3.50 ± 1.1 pmol/mg protein/min; Mann-Whitney U test;p = 0.006 and p = 0.04, respectively; Fig. 4I).

Increased production of TNF- $alpha$ and NO by glial cells in response to stressors

We examined the possibility that the production of TNF- $alpha$ and NOS by glial cells in cocultures exposed to stress conditionswas involved directly in facilitating retinal ganglion cell apoptosis.Western blot analysis that used cell lysates revealed that theexpression of TNF- $alpha$ and iNOS was undetectable in retinal ganglioncells incubated under either normal or stress conditions. However,the expression of TNF- $alpha$ and iNOS increased in glial cells in coculturesexposed to simulated ischemia or elevated hydrostatic pressure(Fig. 5A,B). Immunocytochemistry similarly demonstrated the increasedexpression of TNF- $alpha$ and iNOS in glial cells in cocultures thatwere incubated under stress conditions (Fig. 5C-H).

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Figure 5. Examination of TNF- $alpha$ and iNOS expression in cocultures that were incubated under simulated ischemia or elevated hydrostatic pressure. Both Western blot analysis (A, B) and immunocytochemistry (C-H) revealed increased expression of TNF- $alpha$ and iNOS in glial cells, but not in retinal ganglion cells, in cocultures that were incubated under stress conditions. A, Western blot analysis of TNF- $alpha$ expression. B, Western blot analysis of iNOS expression. Column 1, Control retinal ganglion cells; column 2, retinal ganglion cells that were incubated under simulated ischemia for 72 hr; column 3, retinal ganglion cells that were incubated under elevated hydrostatic pressure for 72 hr; column 4, control glial cells; column 5, glial cells that were incubated under simulated ischemia for 72 hr; column 6, glial cells that were incubated under elevated hydrostatic pressure for 72 hr. C-E, TNF- $alpha$ expression in glial cells that were incubated under different conditions for 72 hr. C, Normal conditions. D, Simulated ischemia. E, Elevated hydrostatic pressure. F-H, iNOS expression in glial cells that were incubated under different conditions for 72 hr. F, Normal conditions. G, Simulated ischemia. H, Elevated hydrostatic pressure.

We measured the levels of TNF- $alpha$ and the end products of NO in conditioned medium of the cocultures. TNF- $alpha$ levels in the conditionedmedium measured by ELISA were approximately eight times higherin cocultures that were exposed to simulated ischemia or elevatedhydrostatic pressure as compared with cocultures that were incubatedunder normal conditions (Mann-Whitney U test, p = 0.003; Fig.6A). As measured by a colorimetric assay, breakdown products ofNO in conditioned medium increased approximately sevenfold incocultures that were exposed to stress conditions compared withcocultures that were incubated under normal conditions (p = 0.003;Fig. 6B).

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Figure 6. Measurement of TNF- $alpha$ and end products of NO in conditioned medium of cocultures that were incubated under stress conditions. A, Titers of TNF- $alpha$ in conditioned medium as measured by ELISA. B, Titers of end products of NO in conditioned medium as measured by a colorimetric assay. Levels of both TNF- $alpha$ and NO end products were higher in the conditioned medium of cocultures that were exposed to simulated ischemia or elevated hydrostatic pressure as compared with cocultures that were incubated under normal conditions (Mann-Whitney U test; p = 0.003 and p = 0.003, respectively).

We also performed experiments in which cocultures were incubated under stress conditions in the presence of specific inhibitorsof TNF- $alpha$ or iNOS. Our experiments revealed that inhibitors ofTNF- $alpha$ or iNOS were able to diminish apoptotic cell death in retinalganglion cells induced by simulated ischemia or elevated hydrostaticpressure. Inhibition of the bioactivity of TNF- $alpha$ by a specificneutralizing antibody (AF510NA; 10 µg/ml) resulted in a decreasedrate of positive TUNEL from 24 to 8% (67%) in cocultures thatwere incubated under simulated ischemia and from 20 to 5% (75%)in cocultures that were incubated under elevated hydrostatic pressure(Mann-Whitney U test; p = 0.0002). Treatment of cocultures with2.5 µM of the selective inhibitor of iNOS, 1400W, decreased therate of positive TUNEL ~50% in cocultures that were incubatedunder simulated ischemia and ~35% in cocultures that were incubatedunder elevated hydrostatic pressure (p = 0.003; Fig. 7). Inhibitionof apoptosis by a neutralizing antibody against TNF- $alpha$ was moreprominent than that by 1400W (p = 0.008).

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Figure 7. Inhibition of apoptosis in retinal ganglion cells in cocultures that were incubated under stress conditions in the presence of specific inhibitors of TNF- $alpha$ or iNOS. Treatment of cocultures with a specific antibody neutralizing the activity of TNF- $alpha$ (10 µg/ml) or with a selective inhibitor of iNOS, 1400W (2.5 µM), decreased the rate of positive TUNEL after incubation under stress conditions (Mann-Whitney U test; p = 0.0002 and p = 0.003, respectively). Inhibition of apoptosis by a neutralizing antibody against TNF- $alpha$ was more prominent than that by 1400W (p = 0.008).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Both elevated intraocular pressure and ischemia are common stress factors identified in glaucomatous eyes that are thoughtto affect retinal ganglion cell survival adversely (Hart et al.,1979; Quigley et al., 1980; Hayreh, 1985). However, the pathophysiologicalmechanisms by which elevated intraocular pressure leads to neuronaldamage in glaucoma are unknown. The blockade of axoplasmic flowat the lamina cribrosa in the optic nerve head and thereby theblockage of neurotrophin transport to the retinal ganglion cells(Anderson and Hendrickson, 1974; Minckler et al., 1976; Quigleyand Addicks, 1980; Pease et al., 2000) as well as ischemia secondaryto elevated intraocular pressure (Hayreh, 1985; Flammer, 1994;Chung et al., 1999) have been suggested to be two mechanisms contributingto retinal ganglion cell death inglaucoma.

Although some evidence indicates that apoptotic cell death can be triggered by elevated hydrostatic pressure itself, as shownin human lymphoblasts (Takano et al., 1997), studies on the directeffect of elevated pressure on neuronal survival are limited [AgarA, Hill M, Coroneo MT (1999). Abstract. Invest Ophthalmol VisSci. 40:A265]. Our experiments provide evidence that environmentalstress created by elevated hydrostatic pressure as well as simulatedischemia could affect neuronal survival. These findings are inaccordance with previous observations that different cells exposedto biomechanical forces, including elevated hydrostatic pressure,exhibit functional as well as morphological changes. For example,hydrostatic pressure induces cytokine expression in a chondrocyte-likecell line, which includes TNF- $alpha$ (Takahashi et al., 1998). In theeye, human lamina cribrosa astrocytes have been shown to reactto pressure changes in their environment by modulating the productionand secretion of extracellular matrix macromolecules (Hernandezand Pena, 1997). In addition, recent evidence suggests that celllines derived from several intraocular tissues, including retinalcells and optic nerve head astrocytes, respond to acute and sustainedlevels of elevated hydrostatic pressure by changing their cellmorphology as well as by increasing basal adenylyl cyclase activity(Wax et al., 2000).

In the current study, cell survival was examined in primary cocultures of retinal ganglion cells and glial cells that hadbeen exposed to elevated hydrostatic pressure for a longer period(up to 72 hr), and it was demonstrated that the elevated hydrostaticpressure decreased neuronal survival. Increased production ofapoptosis-promoting substances by retinal glial cells after exposureto elevated hydrostatic pressure or simulated ischemia accounts,in part, for the increased rate of cell death in cocultured retinalganglion cells. Passive transfer experiments confirmed that thesource of noxious insults on retinal ganglion cells was retinalglial cells that had been exposed to stress conditions. We thereforepropose that alterations in the cellular functions of glial cellsin the presence of environmental stress created during the courseof glaucomatous optic neuropathy in vivo may lead to retinal ganglioncell death in these eyes. Reactivated glial cells in the outerretina have been implicated similarly in the ensuing death ofphotoreceptor cells (Cotinet et al., 1997; de Kozak et al., 1997;Goureau et al., 1999). Here, we focused on TNF- $alpha$ and NO amongseveral soluble factors secreted by stressed glial cells on thebasis of findings obtained from glaucomatous eyes (Neufeld etal., 1997; Yan et al., 2000).

Tumor necrosis factor- $alpha$ is known as a potent immunomediator and proinflammatory cytokine that is upregulated rapidly in thebrain after injury (Liu et al., 1994; Barone et al., 1997). TNF- $alpha$ is produced by reactivated macrophages, astrocytes, microglia,and retinal glial cells (Lieberman et al., 1989; Semenzato, 1990;Brenner et al., 1993; de Kozak et al., Meda et al., 1995; Cotinetet al., 1997). The dramatic increase in TNF- $alpha$ production afterischemic and excitotoxic brain injury suggests an important rolefor this cytokine in modifying the neurodegenerative process.TNF- $alpha$ also is known to be a potent activator of neurotoxic substancessuch as NO and excitotoxins (McGeer et al., 1993; Rothwell andHopkins, 1995; Martin-Villalba et al., 1999). Its excessive synthesisafter trauma has been correlated with poor outcome (Ertel et al.,1995), and its inhibition is accompanied by reduced brain damage(Shohami et al., 1996). In addition, a new concept in neurodegenerationexclaims that picogram concentrations of TNF- $alpha$ , which is knownto be noncytotoxic, induces cell death via the "silencing of survivalsignals" (Venters et al., 2000). Regarding optic nerve, TNF- $alpha$ has been thought to account for axonal degeneration and glialchanges that have been observed in the optic nerves of patientswith AIDS (Lin et al., 1997). Furthermore, intravitreal injectionsof TNF- $alpha$ into rabbit eyes produced axonal degeneration in theiroptic nerves (Madigan et al., 1996). Because our cultures weredepleted of microglia, astrocytes and retinal Müller glial cellsappeared to be the likely sources of TNF- $alpha$ secreted into the conditionedmedium. TNF- $alpha$ released by chemically reactivated glial cells hasbeen implicated similarly in the increased rate of apoptosis incocultured neurons (Viviani et al., 1998; Downen et al., 1999).

Tumor necrosis factor- $alpha$ is an inducer of apoptotic cell death via TNF- $alpha$ receptor-1 occupancy in a caspase-mediated pathway,which includes the activation of caspase-8 (Hsu et al., 1995).Our observation of caspase-8 activation suggests the involvementof TNF- $alpha$ as a mediator of the apoptosis of retinal ganglion cells.Furthermore, it has been demonstrated recently that the expressionof TNF- $alpha$ and its receptor are increased in glaucomatous opticnerve head. Although the TNF- $alpha$ is expressed mostly in astroglialcells, the expression of TNF- $alpha$ receptor-1 is more prominent innerve bundles located in the anterior region of the glaucomatousoptic nerve head (Yan et al., 2000). These observations supportour current findings that retinal neuronal tissue is an importanttarget for the effects of TNF- $alpha$ that are produced by glialcells.

In addition to TNF- $alpha$ , we found that increased production of NO in retinal glial cells that have been exposed to differentstress conditions induced cell death in cocultured retinal ganglioncells. Previous studies suggested that glial expression of iNOScaused delayed neurotoxicity in mixed cultures of cortical neuronaland glial cells (Dawson et al., 1994). Similar to TNF- $alpha$ , NO, whichis formed from L-arginine by NOS, has been implicated in severalneurodegenerative diseases. Although two isoforms, neuronal NOSand endothelial NOS, are expressed constitutively, iNOS is inducedafter infection and trauma (Bredt and Snyder, 1994). Inductionof NOS in brain tissue results in neuronal cell death (Iadecolaet al., 1995) in which astrocytes and microglia are major sourcesof the iNOS production (Liu et al., 1996). Inducible NOS producedby glial cells also is thought to cause retinal neuronal celldeath in different retinal diseases and after optic nerve axotomy(Cotinet et al., 1997; de Kozak et al., 1997; Koeberle and Ball,1999). In addition, intravitreal injection of the NO donor hasbeen shown to cause retinal ganglion cell and photoreceptor loss,whereas reduction of NO levels by systemic inhibition of NOS reducesretinal ganglion cell loss in a rat model of retinal ischemia(Lam and Tso, 1996). Nitric oxide also has been suggested to playa role in the neurodegeneration process in glaucoma (Neufeld etal., 1997, 1999).

Our experiments that used inhibitors of TNF- $alpha$ or iNOS revealed an inhibition of apoptotic cell death in retinal ganglion cellsin cocultures that had been exposed to simulated ischemia or elevatedhydrostatic pressure. Although iNOS inhibition provided partialprotection against apoptotic cell death in cocultures, a moreprominent inhibition of apoptosis was observed after the inhibitionof TNF- $alpha$ . These results indicate a crucial role for endogenousTNF- $alpha$ in mediating neurotoxicity in cultured retinal ganglioncells. Because TNF- $alpha$ induces NO secretion (Goureau et al., 1997;Shafer and Murphy, 1997; Heneka et al., 1998), inhibition of itsactivity indirectly could decrease the harmful effect createdby NO as well. Similar to our observations, neutralizing anti-TNF- $alpha$ antiserum, rather than a NOS inhibitor, inhibited neurotoxicityof cytokine-induced production of iNOS and TNF- $alpha$ in neuron-astrocytecultures that were derived from human fetal cerebrum (Downen etal., 1999). Furthermore, the inhibition of TNF- $alpha$ has been shownto reduce iNOS expression and NOS activity (Perkins et al., 1998).In addition, in vivo observations support the idea that neutralizationof systemic TNF- $alpha$ ameliorates target organ damage in brain ischemiaor in experimental autoimmune uveoretinitis (Dick et al., 1996;Sartani et al., 1996; Barone et al., 1997; Lavine et al., 1998).However, selective inhibition of iNOS does not prevent the organinjury/dysfunction that is caused by endotoxin (Wray et al., 1998).These findings emphasize the importance of further research todetermine the potential neuroprotective role of TNF- $alpha$ or iNOSinhibition in stressed retinal ganglion cells under in vivo conditions,as occurs in glaucoma, and to identify strategies that are feasiblefor patienttreatment.

In conclusion, our findings provide evidence that the functional state of glial cells determined by environmental factorsmay be important for determining the ultimate role of glial cellsas either neuroprotective or neurotoxic. The retinal glial cellsexposed to stress conditions similar to that created in vivo duringthe process of glaucoma, such as elevated hydrostatic pressureor simulated ischemia, have a neurotoxic influence on retinalganglion cells. Because of increased production of death-promotingsubstances, including TNF- $alpha$ , alterations in the functional stateof glial cells in response to these stressors lead to retinalganglion cell death. These findings reveal a novel pathogenicmechanism for retinal ganglion cell death in glaucoma and providea novel therapeutic target for neuroprotection in the treatmentof glaucomatous opticneuropathy.

  FOOTNOTES

Received June 19, 2000; revised Aug. 14, 2000; accepted Sept. 11, 2000.

This study was supported in part by The Glaucoma Foundation (New York, NY; to G.T.), National Eye Institute Grant EY12314(Bethesda, MD), Glaucoma Research Foundation (San Francisco, CA;to M.B.W.), and an unrestricted grant to Washington UniversitySchool of Medicine, Department of Ophthalmology and Visual Sciences,from Research to Prevent Blindness (New York,NY).
Correspondence should be addressed to Dr. Martin B. Wax, Department of Ophthalmology and Visual Sciences, Washington UniversitySchool of Medicine, Box 8096, 660 South Euclid Avenue, St. Louis,MO 63110. E-mail: Wax{at}vision.wustl.edu.

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Increased Production of Tumor Necrosis Factor- by Glial Cells Exposed to Simulated Ischemia or Elevated Hydrostatic Pressure Induces Apoptosis in Cocultured Retinal Ganglion Cells

Increased Production of Tumor Necrosis Factor- $alpha$ by Glial Cells Exposed to Simulated Ischemia or Elevated Hydrostatic Pressure Induces Apoptosis in Cocultured Retinal Ganglion Cells