Multiple sclerosis (MS)1 is a progressive disease of the central nervous system (CNS) and characterized by multifocal areas of inflammation and demyelination (1–4). The disease is considered to be immune-mediated and directed at myelin and its cell of origin, the oligodendrocyte (OL; 4). The precise basis for this selective injury remains to be established. Depletion of OLs is a recognized feature of MS lesions, becoming more apparent as the disease evolves (5). Examples of OLs undergoing lytic (3, 4) or apoptotic (6, 7) cell death in situ in MS tissue are described, although their frequency remains to be established. OLs in situ do not appear to express MHC molecules, prerequisites for recognition by antigen-specific T cells (8). OLs in vitro are susceptible to non-MHC–restricted injury mediated either via soluble factor–dependent mechanisms (9–14) or cell–cell contact–dependent mechanisms (11, 15–19). Prolonged exposure to TNF-
or -β induces apoptotic cell death in OLs after 72–96 h (10–12). Mitogen-activated or myelin-reactive CD4+ T cells acting in a non-MHC– restricted manner can induce lysis of OLs without prior apoptosis (19).
Fas is a cell surface receptor belonging to the TNF receptor superfamily that transduces cell death signals when ligated by agonist antibodies or by fas ligand fasL (20, 21). Although fas signaling usually induces apoptotic cell death, fas ligation has been shown to trigger other cellular responses including proliferation (22). CD4+ and CD8+ T cells (21) and macrophages (23), cell types found within active MS lesions (4), all express fasL and in vitro can induce injury via engagement of fas on target cells (23–28). Although, in initial studies, fas was not detected in the uninjured brain (29, 30), recent reports suggest that fas expression can be induced in pathological conditions such as cerebral ischemia (30) and Alzheimer's disease (31). To establish the potential involvement of fas in OL cell death in MS, we have assessed fas expression on OLs in MS tissue in situ and the susceptibility of OLs to fas-mediated injury in vitro.
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Materials and Methods
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Expression of Fas and Related Molecules in Normal and MS CNS Tissue
Tissue Samples.
Early postmortem (between 4 and 8 h) CNS tissue was obtained from 10 subjects with a clinical diagnosis of chronic progressive MS (mean age of 46 yr). Two patients were assigned a pathological classification of chronic active and two a classification of chronic silent MS. A minimum of three blocks were studied from each case for a total of 10 active and 27 silent lesions. Normal CNS tissue came from three subjects (mean age of 59 yr) succumbing to nonneurological conditions (lung cancer and acute myocardial infarctions). In addition, brain tissue from five other subjects with different neurologic diseases (OND) was examined for control purposes. These included one case of tropical spastic paraparesis (inflammatory control) and one case each of Alzheimer's disease, ischemic stroke, amyotrophic lateral sclerosis, and cerebral metastases from prostate cancer. The mean postmortem delay for the OND cases was 8 h. All tissue was embedded in O.C.T. (Miles, Elkhart, IN) medium and stored at –70°C until use.
Immunohistochemistry.
Frozen sections were air-dried and then fixed in 4% paraformaldehyde for 10 min. After quenching with 0.03% hydrogen peroxide and blocking with normal serum, sections were incubated overnight with primary antibody. Monoclonal IgG1 anti-fas antibody M3 was incubated at room temperature at a dilution of 1:200, whereas monoclonal IgM antibody Leu-7 (Becton Dickinson, San Jose, CA) and two polyclonal antisera recognizing different epitopes on human fasL protein (Santa Cruz Biotechnology, Santa Cruz, CA) and CNPase were used overnight at 4°C at 1:800, 1:3200, and 1:100 dilution, respectively. Appropriate secondary biotinylated antibodies were applied for 60 min at room temperature followed by avidin-biotin-complex Elite reagent (Vector Labs, Inc., Burlingame, CA) for a further 45 min. The chromogen was 3,3'-diaminobenzidine (DAB). For doublestaining, after incubation with M3 mAb for fas antigen and visualization with DAB, sections were incubated with Leu-7 IgM mAb followed by an anti–mouse µ chain–specific secondary antibody coupled to alkaline phosphatase and nitroblue tetrazolium (NBT)/ brom-chlor-indolyl phosphate (BCIP) as substrate. Negative controls included omission of the primary antibody and the use of isotype-specific, irrelevant antibodies. In addition, preabsorption with the inhibitor peptides (1 µg per ml, Santa Cruz Biotechnology) was performed on the two fasL antisera.
Establishment of Human CNS–derived Glial Cell Cultures.
Human brain tissue was obtained from patients undergoing temporal lobe resection or callosotomy as part of a surgical therapeutic treatment for intractable epilepsy. The glial cell isolation procedure has previously been described (32). Briefly, the brain tissue was subjected to enzymatic dissociation by using trypsin (0.25%; GIBCO BRL, Burlington, Ontario, Canada) and DNase I (25 µg/ml; Boehringer Mannheim, Laval, Quebec) for 30 min at 37°C and mechanical dissociation by passage through a 132-µm nylon mesh (Industrial Fabrics Corporation, Minneapolis, MN). Mixed glial cells, consisting of 
70% OLs, 25% microglia, and 5% astrocytes (assessed by 2':3'-cyclic nucleotide phosphodiesterase [CNPase], LeuM5, and glial fibrillary acidic protein [GFAP] immunoreactivity, respectively) were obtained by separation on a 30% Percoll (Pharmacia LKB, Montreal, Quebec) gradient (15,000 rpm at 4°C for 30 min). To enrich for OLs, freshly isolated mixed glial cells were left overnight in Falcon tissue culture flasks (VWR, Montreal, Québec), and the less adherent OLs were removed by gentle shaking. The differential adhesion protocol was repeated 24 h later on this semi-enriched OL culture. This population of OLs was identified using rabbit anti–3':5'-CNPase polyclonal antibody, a marker for mature OLs (1 h at 1:40 dilution; gift from Dr. Peter Braun, McGill University, Montreal, Canada), followed by goat anti–rabbit IgG conjugated with Texas red (1 h at 1:100 dilution; Jackson ImmunoResearch Labs, Inc., West Grove, PA) and was found to contain >90% OLs. The derived OLs were plated onto poly-L-lysine–coated (10 µg/ml; Sigma, St. Louis, MO) Aclar 9-mm diameter coverslips or into 96-well Nuntron plates (Becton Dickinson, Mountain View, CA) at a density of 5 x 104 cells per coverslip or microwell; coverslips were placed in Nuntron petri dishes. Microwells or petri dishes were filled with minimum essential culture medium supplemented with 5% FCS, 2.5 U/ml penicillin, 2.5 µg/ml streptomycin, and 0.1% glucose (all from GIBCO BRL). The OLs were allowed to extend processes and were used in functional assays 2–4 wk from the time of isolation. At this time, the OL preparations lacked endothelial and fibroblast cell contamination (32). The remaining adherent populations containing astrocytes and microglia were trypsinized and plated as described for the OLs to give mixed astrocyte-microglia cultures (
30% astrocytes); pure microglia cultures (>95% enriched) were obtained by shaking the less adherent astrocytes off (5 h on a rotary shaker in a humidified incubator maintained at 37°C and 5% CO2) and trypinizing and plating the cells as described for the OLs. Astrocytes were identified using polyclonal rabbit antiGFAP (1 h at 1:100 dilution; Boehringer Mannheim), followed by goat anti–rabbit Ig conjugated with Texas red (1 h at 1:100 dilution), and microglia were identified using an anti-LeuM5 (1 h, neat; Becton Dickinson), followed by Texas red–conjugated goat anti–mouse IgG2b Ab (Jackson ImmunoResearch Labs Inc.).
Expression of Fas on Human Adult Glial Cells In Vitro.
To determine whether target cells expressed fas, live unfixed target cells on coverslips were incubated with either M3 or M33, activating and nonactivating anti-fas IgG1 monoclonal antibodies, respectively (1 h at 5 µg/ml; Immunex Corp., Seattle, WA), followed by biotinylated goat anti–mouse IgG (1 h at 1:100 dilution; Boehringer Mannheim), followed by FITC-conjugated Streptavidin (1 h at 1:20 dilution) (Boehringer Mannheim). The cells were then fixed in acid/alcohol (5% glacial acetic acid/95% absolute ethanol). OLs were identified by anti-CNPase immunostaining; astrocytes were identified by anti-GFAP immunostaining, and microglia, after blocking with mouse serum for 30 min, were identified by anti-LeuM5 immunostaining, as described above. Glial cell fas immunoreactivity (IR) was compared with fas IR on a panel of fas-expressing (U251 glioma cells, Jurkat T cells, U937 monocytic cells) and fas-nonexpressing (L929 fibroblast cells) cell lines; the cell lines used in this study were single-stained for fas IR, as described above. Immunocytochemical analysis was performed using either a Reichert Polyvar 2 Leica immunofluorescence microscope or, for the OLs, a confocal laser scanning microscope (Leica Lasertechnik, Heidelberg, Germany). Negative controls included omission of the primary antibody and the use of isotypespecific, irrelevant antibody. Samples were scanned with a 40 x 1.3 NA oil immersion objective with a band pass filter peaking at 535 ± 7 nm for FITC specificity and a 580-nm-high pass filter for Texas red.
Cell Death Assays
Membrane Injury: Lactate Dehydrogenase Release Assay and Trypan Blue Uptake.
As previously described (11), cell-free supernate was collected from OL cultures exposed to fas ligation. Sample tubes containing 0.5 ml of 2 mg/ml NADH, 0.5 ml of 1.5 mmol/l pyruvate substrate, and 100 µl of test sample were incubated for 30 min at 37°C. Pyruvate calibration curve tubes were set up. 1 ml of color reagent was added to each tube to stop the reaction. Absorbency was read at 460 nm. Test sample lactate dehydrogenase (LDH) was calculated by comparison with a curve generated using the pyruvate standards.
To assess trypan blue uptake, trypan blue (Sigma) was added at a 1:1 dilution to cell cultures previously exposed to fas ligation. Cells staining blue, indicating membrane disruption, were counted and expressed as a percentage of the total number of cells counted.
Nuclear Injury: Propidium Iodide and TUNEL Labeling
Nuclear fragmentation was assessed morphologically (nuclear fragmentation and chromatin condensation) by propidium iodide (PI) staining (10 µg/ml for 20 min on coverslips fixed with acetone/methanol 1:1 for 10 min at –20°C), as previously described (11). DNA fragmentation was assessed using the terminal transferase (TdT)– mediated (d-uridine triphosphate [UTP])-biotin nick-end-labeling (TUNEL) technique, as previously described (11). For adherent target cells (OL, astrocytes, microglia, U251 glioma cells, and L929 cells), coverslips were fixed in acetone/methanol (1:1) for 10 min at –20°C; nonadherent target cells were cytospun onto gelatin-coated slides and then fixed in acetone/methanol as described above. After rehydration for 30 min in PBS, cells were incubated for 1 h at 37°C with 50 µl of nick-end-labeling solution containing TdT (0.3 U/ml) and biotinylated dUTP (0.01 nmol/ ml) in TdT buffer (Promega, Madison, WI). The reaction was terminated by incubation in Tris buffer (10 mM Tris-HCl, pH 6.8, for 15 min). After blocking with 2% BSA for 15 min, the cells were incubated with streptavidin-FITC (1:20 dilution, 30 min at 37°C; Boehringer Mannheim). Hoechst dye 33258 (10 µg/ml, 20 min; Sigma) was used to identify target cell nuclei.
For each experiment (n), 200–400 cells were counted per coverslip, and counting was done by an observer blinded to the treatment received by the cells. Each test condition was assessed in triplicate per experiment.
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Results
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Expression of Fas and Related Molecules in Normal and MS CNS Tissue In Situ.
In normal CNS white matter, faint fas immunoreactivity was detected on scattered glial cells by immunohistochemistry using the M3 mAb. This occurred on cells with small, round nuclei, a thin rim of cytoplasm, and one or two tenous processes (Fig. 1 a). Such elements were identified as OLs by their morphologic phenotype and positive staining for Leu-7 and CNPase in serial sections. Fas was also constitutively expressed on endothelial cells of small blood vessels. Other glial cells and neurons were invariably fas-negative. Immunostaining for fasL on normal CNS tissue revealed low-level constitutive reactivity on microglial cells (Fig. 1 b). The specificity of the fasL reactivity was confirmed by peptide preabsorption, the latter resulting in a lack of fasL immunoreactivity. In tissue from all cases of MS, fas reactivity was prominent on OLs along the margin of lesions and in adjacent white matter (Fig. 1, c and d). These same cells also stained positively for CNPase and Leu-7 in serial sections (Fig. 1 e), although the pattern of staining was different with Leu-7 and CNPase staining the cell body and M3, the cell membrane, and its fine processes. Definitive identification of these cells as faspositive oligodendrocytes was confirmed by double-staining with M3 and Leu-7 antibodies (Fig. 1 f ). Fas IR on OLs in MS lesions was confirmed using another anti-fas mAb, UB2 (Immunotech Inc., Westbrook, ME), and similar results were obtained (data not shown). Apart from endothelial cells and infiltrating lymphocytes (Fig. 1 g), no other cell type showed fas reactivity. Staining for fas ligand in MS lesions (Fig. 1 h) revealed intense positivity on microglia and scattered infiltrating lymphocytes but not on OLs or astrocytes. In sections from OND cases, immunostaining for fas and fasL was comparable to the normal controls.
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