CD45 Opposes beta -Amyloid Peptide-Induced Microglial Activation via Inhibition of p44/42 Mitogen-Activated Protein Kinase

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The Journal of Neuroscience, October 15, 2000, 20(20):7587-7594

CD45 Opposes $beta$ -Amyloid Peptide-Induced Microglial Activation via Inhibition of p44/42 Mitogen-Activated Protein Kinase
Jun Tan, Terrence Town, Takashi Mori, Yajuan Wu, Michael Saxe, Fiona Crawford, and Mike Mullan
The Roskamp Institute, Department of Psychiatry, University of South Florida, Tampa, Florida 33613

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Reactive microglia have been suggested to play a role in the Alzheimer's disease (AD) process, and previous studies have shownthat expression of CD45, a membrane-bound protein-tyrosine phosphatase(PTP), is elevated in microglia in AD brain compared with controls.To investigate the possible role of CD45 in microglial responsivenessto $beta$ -amyloid (A $beta$ ) peptides, we first co-treated primary culturedmicroglia with a tyrosine phosphatase inhibitor [potassium bisperoxo(1,10-phenanthroline) oxovanadate (phen), 5 µM] and freshly solubilizedA $beta$ peptides (1000 nM). Data show synergistic induction of microglialactivation as evidenced by tumor necrosis factor $alpha$ (TNF- $alpha$ ) productionand nitric oxide (NO) release, both of which we show to be dependenton activation of p44/42 mitogen-activated protein kinase (MAPK).Furthermore, co-treatment with phen and A $beta$ peptides results inmicroglia-induced neuronal cell injury. Stimulation of microglialCD45 by anti-CD45 antibody markedly inhibits these effects viainhibition of p44/42 MAPK, suggesting that CD45 is a negativeregulator of microglial activation. Accordingly, primary culturedmicroglia from CD45-deficient mice demonstrate hyper-responsivenessto A $beta$ , as evidenced by TNF- $alpha$ release, NO production, and neuronalinjury after stimulation with A $beta$ peptides. As a validation ofthese findings in vivo, brains from a transgenic mouse model ofAD [transgenic Swedish APP-overexpressing (Tg APP_sw) mice] deficientfor CD45 demonstrate markedly increased production of TNF- $alpha$ comparedwith Tg APP_sw mice. Taken together, these results suggest thattherapeutic agents that stimulate the CD45 PTP signaling pathwaymay be effective in suppressing microglial activation associatedwithAD.

Key words: Alzheimer's disease; $beta$ -amyloid; microlgia; neurons; mitogen-activated protein kinase; CD45; protein-tyrosine phosphatase; tyrosine phospatase inhibitor; TNF- $alpha$ ; nitric oxide

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

It has been suggested that activated microglia play a key role in the inflammatory processes of neurodegenerative diseasessuch as Alzheimer's disease (AD), because reactive microglia secretecytokines, including tumor necrosis factor $alpha$ (TNF- $alpha$ ) and interleukin-1 $beta$ ,which promote neurodegeneration (Meda et al., 1995; Rogers etal., 1996; Barger and Harmon, 1997). However, current anti-inflammatorytherapeutics directed against AD, such as nonsteroidal anti-inflammatorydrugs (NSAIDs), only partially suppress microglial activation(Mackenzie and Munoz, 1998) and, therefore, may not provide thegreatest therapeutic benefits for AD. This suggestion is supportedby clinical evidence, in which elderly persons using NSAIDs demonstrateonly an ~20% reduction in risk for AD (Beard et al., 1998), andAD patients using NSAIDs have only partial amelioration of diseasesymptoms (Rich et al., 1995). Thus, a more viable therapeuticstrategy may be combination of NSAIDs with specific inhibitorsof microglialactivation.

Most of our knowledge concerning the molecular mediators of microglial activation comes from studies involving peripherallymphocytes. For example, the CD40-CD40L signaling pathway isinvolved in both T-cell and microglial cell activation (Yang andWilson 1996; Maxwell et al., 1999; Tan et al., 1999a), yet althoughblockade of this pathway has proved an efficient means of opposingT-cell activation (Grewal et al., 1996; Stuber et al., 1996),interruption of this pathway is largely unexplored as a meansof opposing microglial activation. We have recently shown thatligation of microglial CD40 synergistically enhances activationof these cells by a low dose of freshly solubilized $beta$ -amyloid(A $beta$ ; Tan et al., 1999b), indicating that the CD40-CD40L interactionis critically involved in microglial activation induced by A $beta$ .In searching for novel cell surface molecules that may play arole in opposing microglial activation, we focused on CD45, afunctional transmembrane protein-tyrosine phosphatase (PTP), which,when cross-linked, has been shown to play a critical role in negativeregulation of T and B lymphocyte activation (Justement, 1996).CD45 is particularly interesting, because microglia express itin the frontal cortex and hippocampus of normal aging individuals,and this expression level is markedly increased in these brainregions in AD cases (Masliah et al., 1991; Licastro et al., 1998).Furthermore, in an animal model of neurodegeneration, upregulationof phosphotyrosine signal associated with activated microgliawas found in and around the degenerating brain region (Karp etal., 1994). These data led us to investigate the possible involvementof CD45 PTP signaling as a putative regulator of microglialactivation.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Materials. Monoclonal antibodies (purified rat anti-mouse CD45 and purified rat IgG_2b control antibodies and FITC-conjugatedrat anti-mouse CD45 and FITC-conjugated rat IgG_2b control antibodies)were purchased from PharMingen (San Diego, CA). To test whetherCD45 cross-linkage could result in stimulation of CD45 PTP activity,we measured free inorganic phosphate (P_i) in microglial cell lysatestreated in the presence or absence of anti-CD45 antibody and foundsignificantly higher levels of P_i in microglial cell lysates treatedwith CD45 antibody compared with untreated cells (data not shown).Antibodies for phospho-p44/42 mitogen-activated protein kinase(MAPK) (Thr-202/Tyr-204) and total p44/42 MAPK were obtained fromNew England Biolabs (Beverly, MA). A $beta$ _1-40 and A $beta$ _1-42 peptidesand control peptide (A $beta$ _40-1) were obtained from QCB (Hopkinton,MA) and were freshly solubilized in distilled H₂O immediatelybefore use. To determine the oligomeric state of A $beta$ in our assays,A $beta$ was immunoprecipitated from cell supernatants after incubationwith microglia and/or neurons, and Western blot analysis was performedat time points of 12, 24, and 48 hr. Data revealed that both A $beta$ _1-40and A $beta$ _1-42, irrespective of the time points assayed, existed asa ladder of SDS-stable oligomers, with a predominant species of~32 kDa. Human CD45 recombinant protein (specific activity, 20,000U/mg of protein) and PD98059 were obtained from Calbiochem (LaJolla, CA), as well as the phosphatase inhibitors including potassiumbisperoxo (1,10-phenanthroline) oxovanadate (phen), sodium orthovanadate,and okadaic acid. Each of these was dissolved in DMSO before addingto complete cell culture medium, and DMSO alone was used as asolvent control, which did not differ from the untreated controlspresented. Bacterial lipopolysaccharide (LPS) was purchased fromSigma (St. Louis, MO) and dissolved in complete cell culture medium.Anti-mouse HRP-conjugated IgG secondary antibody and Western blottingluminol reagent were obtained from Santa Cruz Biotechnology (SantaCruz, CA). Immun-Blot polyvinylidene difluoride (PVDF) membraneswere purchased from Bio-Rad (Hercules, CA). Anti-mouse TNF- $alpha$ polyclonalantibody was obtained from R & D systems (Minneapolis,MN).

Murine primary cell culture. Breeding pairs of BALB/c and CD45-deficient (C57BL/6OlaHsd-Ptprc) mice were purchased from TheJackson Laboratory (Bar Harbor, ME) and housed in the animal facilityat the University of South Florida Health Science Center. TransgenicSwedish APP-overexpressing (Tg APP_sw) mice are the 2576 line back-crossedto C57B6/SJL as previously described (Hsiao et al., 1995, 1996).Murine primary culture microglia were isolated from mouse cerebralcortices and were grown in RPMI 1640 medium supplemented with5% fetal calf serum, 2 mM glutamine, 100 U/ml penicillin, 0.1µg/ml streptomycin, and 0.05 mM 2-mercaptoethanol according topreviously described methods (Chao et al., 1992). Briefly, cerebralcortices from newborn mice (1-2 d old) were isolated under sterileconditions and were kept at 4°C before mechanical dissociation.Cells were plated in 75 cm² flasks, and complete medium was added. Primary cultures werekept for 14 d so that only glial cells remained, and microgliawere isolated by shaking flasks at 200 rpm in a Lab-Line incubator-shaker.More than 98% of these glial cells stained positive for Mac-1(CD11b/CD18; Boehringer Mannheim, Indianapolis, IN). Mouse primaryculture neuronal cells were prepared as previously described (Chaoet al., 1992). Briefly, cerebral cortices were isolated from BALB/cmouse embryos, between 15 and 17 d in utero, and cortices weremechanically dissociated in trypsin (0.25%) after incubation for15 min at 37°C. Cells were collected after centrifugation at 1200rpm, resuspended in DMEM (Life Technologies, Gaithersburg, MD)supplemented with 10% fetal calf serum, 10% horse serum, uridine(33.6 mg/ml; Sigma) and fluorodeoxyuridine (13.6 mg/ml; Sigma),and plated in 24-well tissue culture plates at 2.5 × 10⁵ cells per well after collagen coating the plates. Where microgliawere isolated from CD45-deficient mice, to verify CD45 deficiencystatus, fluorescence-activated cell sorter analysis was performedas previously described (Tan et al., 1999a), and CD45 was undetectablein these cells (data notshown).

TNF- $alpha$ ELISA and nitric oxide release assay. Primary cultured microglial cells were plated in 24-well tissue-culture plates(Costar, Cambridge, MA) at 5 × 10⁴ cells per well and stimulated for 12 hr with phen (5 µM), A $beta$ peptides (1000 nM), phen and A $beta$ peptides in the presence or absenceof anti-CD45 antibody (1:200) or PD98059 (5 µM) pretreatment for1 hr, or appropriate controls. Cell-free supernatants were collectedand assayed by a TNF- $alpha$ ELISA kit (Genzyme, Cambridge, MA) or anitric oxide (NO) assay kit (Calbiochem) in strict accordancewith the manufacturer's instructions. The Bio-Rad (Hercules, CA)protein assay was performed to measure total cellular proteinfrom each of the cell groups under consideration just before quantificationof cytokine release by ELISA or NO secretion by NOassay.

Lactate dehydrogenase release assay in neuronal and microglial co-cultures. After 5 d in vitro, neuronal cells were passedin preparation for subsequent experiments. More than 96% of thesecells stained positive for neurofilament L (using rabbit anti-humanneurofilament L antibody, 1:300; Serotec Ltd., Kidlington, Oxon,UK; data not shown), a marker of differentiated neuronal cells.Neuronal cells were seeded in 24-well tissue culture plates at1 × 10⁵ cells per well for 48 hr and used as target cells for lactatedehydrogenase (LDH) release assay. In this experimental paradigm,neuronal cells or neuronal-microglial co-cultures (microglia,5 × 10⁴ cells per well, a 2:1 ratio of neurons to microglia) were treatedwith phen (5 µM), A $beta$ _1-40 (1000 nM), A $beta$ _1-42 (1000 nM), controlpeptide (1000 nM), anti-CD45 antibody (1:200), phen and A $beta$ peptides,anti-CD45, phen, and A $beta$ peptides, or appropriate controls. AnLDH release assay (Promega, Madison, WI) was performed as described(Tan et al., 1999a) after either 36 or 48 hr of treatment in neuronalcultures, microglial cultures or neuronal-microglial co-cultures.Total LDH release represents maximal lysis of target cells with5% Triton X-100.

Immunocytochemistry in neuronal and microglial co-cultures. For morphological examination and immunocytochemistry, primarycultured neuronal cells were isolated as described above, passedonto glass coverslips in six-well tissue culture plates at 2 ×10⁵ cells per well, and then co-cultured with various groups of microgliaat 1 × 10⁵ cells per well (yielding a 2:1 ratio of neurons to microglia).Co-cultures then went untreated (control) or were treated withphen (5 µM), A $beta$ _1-42 (1000 nM), or both for 48 hr. After this treatmentperiod, morphological examination and immunocytochemistry wereperformed. Double immunocytochemical staining was performed witha combination of an indirect method (using an HRP-conjugated DABchromogen system) and the Dako (Carpinteria, CA) EnVision system(with an alkaline phosphatase-conjugated fast red chromogen system),using anti-mouse CD11b antibody (clone M1/70, 1:50 dilution; Chemicon,Temecula, CA) as a microglia marker and anti-mouse neuorfilamentL antibody (neurofilament 68 clone NR4, 1:300 dilution; Sigma)as a neuronal marker. Morphological changes in co-cultured primaryneurons and microglia were recorded by bright-field microscopicexamination.

Western immunoblotting. Murine primary culture micrgolia were plated in six-well tissue culture plates at a density of 8 ×10⁵ cells per well. These cells were incubated for 30 min with orwithout phen (5 µM) and A $beta$ peptides (1000 nM) in the presenceor absence of anti-CD45 or control antibodies (1:200 dilutionfor each) or PD98059 (5 µM) pretreatment for 1 hr, or appropriatecontrols. Immediately after culturing, microglia were washed inice-cold PBS three times, scraped into ice-cold PBS, and lysedin an ice-cold lysis buffer containing 20 mM Tris, pH 7.5, 150mM NaCl, 1 mM EDTA, 1 mM EGTA, 1% Triton X-100, 2.5 mM sodiumpyrophosphate, 1 mM $beta$ -glycerolphosphate, 1 mM Na₃VO₄, 1 µg/mlleupeptin, and 1 mM PMSF. After incubation for 30 min on ice,samples were centrifuged at high speed for 15 min, and supernatantswere collected. Total protein content was estimated using theBio-Rad protein assay. An aliquot corresponding to 50 µg of totalprotein of each sample was separated by SDS-PAGE and transferredelectrophoretically to Immun-Blot PVDF membranes. Nonspecificantibody binding was blocked with 5% nonfat dry milk for 1 hrat room temperature in Tris-buffered saline (20 mM Tris and 500mM NaCl, pH 7.5). Membranes where first hybridized with a phospho-specificp44/42 MAPK antibody, stripped with $beta$ -mercaptoethanol strippingsolution (62.5 mM Tris-HCl, pH 6.8, 2% SDS, and 100 mM $beta$ -mercaptoethanol),and then reprobed with an antibody that recognizes total p44/42MAPK. Alternatively, membranes with identical samples were probedeither with a phospho-specific p44/42 MAPK antibody or with anantibody that recognizes total p44/42 MAPK. Immunoblotting wasperformed with a primary antibody followed by an anti-mouse HRP-conjugatedIgG secondary antibody as a tracer. The luminol reagent was usedto develop the blots. Densitometric analysis was performed forall blots using the Flour-S MultiImager with Quantity One software(Bio-Rad).

For TNF- $alpha$ Western blot, brains from 6-month-old transgenic mice were isolated under sterile conditions on ice and placed inice-cold lysis buffer containing 20 mM Tris, pH 7.5, 150 mM NaCl,1 mM EDTA, 1 mM EGTA, 1% Triton X-100, 2.5 mM sodium pyrophosphate,1 mM $beta$ -glycerolphosphate, 1 mM Na₃VO₄, 1 µg/ml leupeptin, and1 mM PMSF. Brains were then sonicated on ice for ~3 min, let standfor 15 min at 4°C, and centrifuged at 15,000 rpm for 15 min. Supernatantswere then collected for protein assay and Western immunoblottingas describedabove.

Immune complex kinase assay. Primary culture microgial cells were seeded in six-well tissue culture plates at 8 × 10⁵ per well. Thirty minutes after co-treatment with phen and A $beta$ peptides in the presence or absence of anti-CD45 antibody or appropriatecontrols, microglial cells were lysed in ice-cold lysis buffer(as described above). Total cellular protein was quantified withthe Bio-Rad protein assay, and an aliquot of 100 µg of proteinfor each treatment condition was separated by SDS-PAGE. p44/42MAPK activity was determined using the p44/42 MAP Kinase assaykit (New England Biolabs) in strict accordance with the manufacturer'sinstructions. The phosphorylated form of the Elk1 p44/42 MAPKfusion protein was visualized by Western immunoblotting (as describedabove) using a specific antibody for phosphorylated Elk1 suppliedwith thekit.

Statistical analysis. Data were analyzed using ANOVA followed by post hoc comparisons of means by Bonferroni's or Dunnett'sT3 method, for which Levene's test for homogeneity of varianceswas used to determine the appropriate method of post hoc comparison.In instances of single-mean comparisons, t test for independentsamples was used to assess significance. $alpha$ levels were set at0.05 for each analysis. All analyses were performed using SPSSfor Windows release 9.0.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Co-treatment with phen and A $beta$ peptides results in synergistic microglial acitvation

It has been shown that a tyrosine phosphorylation cascade plays an important role in A $beta$ -induced microglial activation (McDonaldet al., 1998; Combs et al., 1999). To test whether promotion oftyrosine phosphorylation could affect A $beta$ -induced microglial activation,we co-incubated primary cultured microglial cells with phen, aspecific tyrosine phosphatase inhibitor, and A $beta$ peptides for 12hr. Microglial activation was measured by TNF- $alpha$ and NO productionand neuronal cell injury in co-culture experiments. Data showedthat phen synergistically enhanced A $beta$ -stimulated microglial activation(Fig. 1). To further confirm that phen and A $beta$ activated microgliathrough inhibiting the PTP signaling pathway, we co-cultured microgliawith A $beta$ and either sodium orthovanadate (50 µM, another PTP inhibitor)or okadaic acid (50 nM, a protein phosphatase 2A inhibitor) andmeasured NO and TNF- $alpha$ release. Although sodium orthovanadate treatmentin conjunction with A $beta$ produced results similar to those of phenand A $beta$ peptide co-treatment (data not shown), NO and TNF- $alpha$ werenot detectable in the media of okadaic acid- and A $beta$ -co-treatedmicroglia (data not shown). This result led us to focus on stimulatingmicroglial PTP activity to oppose A $beta$ -induced activation of thesecells.

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Figure 1. Co-treatment with phen and A $beta$ peptides synergistically affects microglial activation. Microglial cells were treated as indicated for 12 hr or co-cultured with primary neuronal cells (microglia/neurons, 1:2) under the indicated treatment conditions for 48 hr. Control peptide is A $beta$ _40-1. Microgial activation was measured by TNF- $alpha$ production (mean ± 1 SEM, picograms per milligram of total protein) in cultured media by TNF- $alpha$ ELISA (a), NO release (mean ± 1 SEM, micromolar concentration per milligram of total protein) in cultured media by NO assay (b), neuronal cell injury by immunocytochemistry and microscopic examination (c), and neuronal cell injury by LDH assay [mean LDH (percent) release ± 1 SEM] (d). Data shown in a and b are representative of five independent experiments, and data in c and d are representative of two independent experiments. For c, co-cultures of microglia and neurons are shown before (top panel) and after (bottom panel) co-treatment with phen and A $beta$ _1-42. CD11b-positive cells (brown) are microglia, whereas neurofilament L-staining cells (red) are neurons. Scale bar, 50 µm (calculated for each panel). Neuronal, but not microglial, degeneration is apparent only after co-treatment and is not detectable after treatment with A $beta$ _1-42 or phen alone. For a, b, and the neuronal-microglial co-culture conditions in d, ANOVA revealed significant main effects of A $beta$ _1-40 (p < 0.001), A $beta$ _1-42 (p < 0.001), and phen (p < 0.001). There were also significant interactions between A $beta$ _1-40 or A $beta$ _1-42 and phen (p < 0.001). One-way ANOVA revealed significant between-group differences (p < 0.001), and post hoc testing revealed significant differences between phen/A $beta$ _1-40 or phen/A $beta$ _1-42 when compared with phen/control peptide (p < 0.001).

CD45 cross-linking significantly inhibits microglial activation induced by phen and A $beta$ peptides

It has been reported that CD45, a protein-tyrosine phosphatase that is constitutively expressed on microglia (Karp et al.,1994), is markedly increased on microglia from AD frontal cortices(Masliah et al., 1991; Licastro et al., 1998). To examine theputative role of CD45 in microglial activation, we treated primarycultured microglial cells with monoclonal anti-CD45 antibody beforestimulation with phen and A $beta$ peptides. Microglial activation,as evidenced by TNF- $alpha$ and NO release after co-treatment of microgliawith phen and A $beta$ peptides, was significantly inhibited by cross-linkingCD45 (Fig. 2a,b). Hyperstimulation of microglia commonly resultsin bystander cell injury, and we went on to evaluate whether cross-linkingof CD45 might protect neuronal cells against injury from activatedmicroglia (resulting from phen and A $beta$ peptide co-treatment). Whenactivated microglia were co-cultured with primary cultured neuronalcells in the presence of anti-CD45 antibody, we observed thatneuronal cells were significantly protected against injury inducedby reactive microglia (Fig. 2c). In addition, to determine whetherdirectly increasing CD45 activity could block microglial activationresulting from co-treatment with phen and A $beta$ , we added CD45 recombinantprotein (20 U/ml) to activated microglia and measured NO and TNF- $alpha$ release. Results showed that release of NO and TNF- $alpha$ were markedlydecreased after addition of CD45 recombinant protein comparedwith the appropriate control (denatured CD45 protein; data notshown), further substantiating the role of CD45 in negative regulationof microglial activation.

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Figure 2. CD45 cross-linking markedly inhibits phen and A $beta$ peptide-induced microglial activation. Microglial cells were treated as indicated for 12 hr or co-cultured with primary cultured neuronal cells (microglia/neurons, 1:2) under the same treatment conditions for 48 hr. Control antibody is rat IgG_2b. Microglial activation was determined by TNF- $alpha$ production (mean ± 1 SEM, picograms per milligram of total protein) in cultured media (a), NO release (mean ± 1 SEM, micromolar concentration per milligram of total protein) in cultured media (b), and neuronal cell injury [mean LDH (percent) release ± 1 SEM] in co-culture experiments (c). Data shown in a and b are representative of five independent experiments, and data in c are representative of two independent experiments. For a and b, one-way ANOVA revealed significant between-group differences (p < 0.001), and post hoc testing revealed significant differences between phen/A $beta$ _1-40/anti-CD45 and phen/A $beta$ _1-40/control antibody (p < 0.01) or phen/A $beta$ _1-42/anti CD45 and phen/A $beta$ _1-42/control antibody (p < 0.02). For the neuronal-microglial co-culture conditions in c, one-way ANOVA revealed significant between-group differences (p < 0.001), and post hoc testing revealed a significant difference between phen/A $beta$ _1-42/anti-CD45 and phen/A $beta$ _1-42/control antibody (p < 0.02).

Cross-linking of CD45 suppresses microglial activation through a p44/42 MAPK-dependent pathway

Previous studies have shown that activation of mitogen-activated protein kinase kinase (MEK1/2) and downstream p44/42 MAPKis involved in TNF- $alpha$ production in macrophages, monocytes, andmicroglia after activation of these cells with a variety of stimuli,including LPS and CD40 ligand (Hambleton et al., 1995; Suttleset al., 1999; Tan et al., 1999c). These data led us to ask whetherthe observed effect of CD45 cross-linking on opposing microglialactivation might be mediated via activation of the MAPK module.Thus, we analyzed p44/42 MAPK phosphorylation status and activityin microglial cell lysates after co-treatment with phen and A $beta$ peptides or appropriate control conditions. Results showed thatp44/42 MAPK phosphorylation and activity were both synergisticallyinduced within 30 min after co-treatment with phen and A $beta$ _1-40or A $beta$ _1-42 peptides (Fig. 3a,b). Furthermore, we observed thattreatment of microglia with PD98059, a selective inhibitor ofMEK1/2, results in significant reduction of phen- and A $beta$ -mediatedphosphorylation and activity of p44/42 MAPK (Fig. 3c,d). To determinewhether activation of p44/42 MAPK was responsible for TNF- $alpha$ andNO production after co-treatment of microglia with phen and A $beta$ peptides, we treated microglia with PD98059 before stimulationwith phen and A $beta$ peptides. Production of TNF- $alpha$ and NO were markedlydecreased compared with appropriate controls within 12 hr aftertreatment with PD98059 and phen and A $beta$ peptides (Fig. 3e,f). Thesedata suggest that activation of p44/42 MAPK is crucial for microglialTNF- $alpha$ and NO production after co-treatment of microglia with phenand A $beta$ peptides.

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Figure 3. Co-treatment of microglia with phen and A $beta$ peptides activates p44/42 MAPK, resulting in microglial activation. Microglial treatment conditions are indicated and are further described in Materials and Methods. Control peptide is A $beta$ _40-1. Cell lysates were analyzed by Western immunoblotting using specific antibodies that recognize phosphorylated or total p44/42 MAPK. a, b, Phosphorylation and activity of p44/42 MAPK after co-treatment with phen and A $beta$ peptides. c, d, Inhibition of this effect by PD98059 (a specific MEK1/2 inhibitor). Histograms below the immunoblots represent the mean band density ratio ± 1 SEM (phospho-p44/42 MAPK/total p44/42 MAPK) and band density in optical density units (phospho-Elk1), respectively (n = 3 for each condition presented). Microglial activation is evidenced by mean TNF- $alpha$ release ± 1 SEM (picograms per milligram of total protein) (e) and mean NO release ± 1 SEM (micromolar concentration per milligrams of total protein) (f) in cultured media by ELISA or by NO release assay, respectively (n = 3 for each condition presented). For a and b, ANOVA revealed significant main effects of phen, A $beta$ _1-40, and A $beta$ _1-42 (p < 0.001), and there were significant interactive terms between phen and either A $beta$ _1-40 or A $beta$ _1-42 (p < 0.001). One-way ANOVA revealed significant between-group differences (p < 0.001), and post hoc testing showed significant differences between A $beta$ _1-40 and phen/A $beta$ _1-40 (p < 0.001) and between A $beta$ _1-42 and phen/A $beta$ _1-42 (p < 0.001)_. For c-f, one-way ANOVA revealed significant between-group differences (p < 0.001), and post hoc testing showed significant differences between phen/A $beta$ _1-40 and phen/A $beta$ _1-40/PD98059 (p < 0.01) and between phen/A $beta$ _1-42 and phen/A $beta$ _1-42/PD98059 (p < 0.01).

Having shown that cross-linking of CD45 opposed microglial activation, we wished to determine whether reduced p44/42 MAPKactivity could be responsible for this effect. To investigatethis possibility, microglial cells were co-incubated with anti-CD45antibody, phen, and A $beta$ peptides. Cell lysates were then analyzedfor phosphorylated forms of p44/42 MAPK by Western immunoblotting.Results showed that cross-linking of CD45 significantly inhibitedphosphorylation of p44/42 MAPK induced by phen and A $beta$ peptideco-treatment compared with controls (Fig. 4a). To determine whetherthis effect could result in decreased MAPK activity, an immunecomplex kinase assay was performed. Results showed that cross-linkingof CD45 markedly reduced p44/42 MAPK activity in phen- and A $beta$ peptide-co-treated cells (Fig. 4b), demonstrating the functionalityof CD45 cross-linking on p44/42 MAPK activity.

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Figure 4. Cross-linking of microglial CD45 markedly suppresses p44/42 MAPK activation resulting from phen and A $beta$ peptide co-treatment. Microglial treatment conditions are indicated and are further described in Materials and Methods. Cell lysates were analyzed by Western immunoblotting using specific antibodies that recognize phosphorylated or total p44/42 MAPK (a) or the p44/42 MAPK fusion protein Elk-1 (b) by immune complex kinase assay. Histograms below immunoblots represent the mean band density ratio ± 1 SEM (phospho-p44/42 MAPK/total p44/42 MAPK) (a) or the mean band density ± 1 SEM in optical density units (b), with n = 3 for each condition presented. For a and b, ANOVA revealed significant main effects of A $beta$ _1-40 and A $beta$ _1-42 (p < 0.001), and there was statistical interaction between either A $beta$ _1-40 or A $beta$ _1-42 and phen (p < 0.001). One-way ANOVA revealed significant between-group differences (p < 0.001), and post hoc testing showed significant differences between phen/A $beta$ _1-40 and phen/A $beta$ _1-40/anti-CD45 (p < 0.001) and between phen/A $beta$ _1-42 and phen/A $beta$ _1-42/anti-CD45 (p < 0.001).

Stimulation of CD45-deficient microglia with A $beta$ peptides directly results in microglial activation

To further substantiate the role of CD45 in A $beta$ -mediated microglial activation, microglia were obtained from CD45-deficientor wild-type mice and treated with either A $beta$ or control peptidefor 12 hr. Data showed that A $beta$ treatment greatly resulted in microglialactivation, which was quantified by TNF- $alpha$ and NO release. Resultsshown in Figure 5, a and b, indicate marked activation of CD45-deficientmicroglia compared with wild-type microglia after stimulationwith A $beta$ peptides. Because we have consistently shown that microglialactivation resulting from phen and A $beta$ peptide treatment firstresulted in p44/42 MAPK phosphorylation and activation followedby TNF- $alpha$ release and NO production, we assessed whether treatmentof CD45-deficient microglia with A $beta$ peptides could result in increasedp44/42 MAPK phosphorylation and activation at the 30 min timepoint. Results showed that A $beta$ treatment of CD45-deficient microgliagreatly increased p44/42 MAPK phosphorylation and activation comparedwith CD45 wild-type microglia (data not shown). Furthermore, todetermine whether CD45-deficient microglia in this scenario couldcause neuronal cell injury, primary cultured cortical neuronsand microglia were co-cultured, and morphological examination(data not shown) and LDH assay were performed. Data showed thatcortical neurons were markedly injured by A $beta$ -treated, CD45-deficientmicroglia compared with wild-type cells (Fig. 5c). When takentogether, these data show that CD45 is a negative regulator ofA $beta$ -induced microglial activation.

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Figure 5. Stimulation of CD45-deficient microglia with A $beta$ peptides results in microglial activation. Primary cultured wild-type or CD45-deficient microglial cells were treated as indicated for 12 hr or co-cultured with primary cultured neuronal cells under the same treatment conditions for 36 hr. Control peptide is A $beta$ _40-1. Microglial activation is evidenced by TNF- $alpha$ production (mean ± 1 SEM; n = 3 for each condition presented) (a), NO assay (mean ± 1 SEM; n = 3 for each treatment condition) (b), and neuronal cell injury in co-culture experiments [mean LDH (percent) release ± 1 SEM; n = 3 for each condition presented] (c). For CD45-deficient microglia in a and b, one-way ANOVA revealed significant between-group differences (p < 0.001), and post hoc testing showed significant differences between control peptide and either A $beta$ _1-40 (p < 0.001) or A $beta$ _1-42 (p $<=$ 0.001). For neuronal-CD45 $-$ / $-$ microglial co-culture experiments, one-way ANOVA revealed significant between-group differences (p < 0.001), and post hoc testing showed significant differences between control peptide and either A $beta$ _1-40 (p < 0.001) or A $beta$ _1-42 (p < 0.001).

Tg APP_sw mice deficient for CD45 demonstrate marked TNF- $alpha$ induction

To evaluate the possibility that CD45 might be a negative regulator of A $beta$ -mediated microglial activation in vivo, we crossedTg APP_sw mice with mice deficient for CD45 and measured TNF- $alpha$ production in the brains of these animals. Results showed a markedincrease in TNF- $alpha$ protein in brain homogenates from these micecompared with Tg APP_sw mice (Fig. 6). We were only able to detectCD45 on microglia in Tg APP_sw and control mice (data not shown),and CD45 has not been reported to be expressed by other CNS cells.Thus, these data suggest that microglial CD45 negatively regulatesA $beta$ -induced microglial activation as evidenced by TNF- $alpha$ productionin vivo.

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Figure 6. TNF- $alpha$ production in vivo is markedly increased in Tg APP_sw mice deficient for CD45. Brains from 6-month-old transgenic mice were isolated and prepared for TNF- $alpha$ Western immunoblotting as described in Materials and Methods. TNF- $alpha$ protein immunoblots (top panel) and mean band density ratios to actin ± 1 SEM (bottom panel; n = 3 for each condition) are shown. ANOVA revealed significant main effects of CD45 deficiency (CD45 def.; p < 0.001) and Tg APP_sw status (p < 0.001), as well as a significant interactive term between them (p < 0.01). One-way ANOVA revealed significant between-group differences (p < 0.001), and post hoc testing showed significant differences between control and Tg APP_sw (p < 0.01) or CD45 def. (p < 0.05) and between either Tg APP_sw or CD45 def. and the crossed mice (p < 0.001).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Microglial activation has been implicated as pathogenic in a variety of neurodegenerative diseases such as multiple sclerosis,AIDS dementia, and AD, raising the possibility that therapeuticstrategies aimed at opposing microglial activation may be beneficialin treating such diseases. However, current attempts at reducingneuroinflammation mediated via microglial activation have onlybeen partially efficacious (Rich et al., 1995), possibly becauseof the fact that such strategies are more general inhibitors ofinflammation than specific inhibitors of microglial-associatedneuroinflammation. For example, Mackenzie and Munoz (1998) examinedpostmortem brain tissue from AD patients who underwent NSAID treatmentand control individuals who did not use NSAIDs (Mackenzie et al.,1998). These authors found that, although there were no significantdifferences in the mean numbers of senile plaques, senile plaquesubtypes (diffuse or neuritic), or neurofibrillary pathology betweencases and controls, the numbers of activated microglia were significantlydecreased in NSAID-treated AD patients compared with controls.These data suggest that NSAIDs are prophylactic for AD partlyby virtue of their opposition of microglial activation. Followingfrom this idea, pharmacotherapeutics specifically aimed at blockingmicroglial activation may well be more efficient at amelioratingmicroglial-associated neuropathology inAD.

In this study, we focused on identifying a specific cell surface receptor target, which, when activated, could inhibit microglialactivation far upstream of intracellular proinflammatory mediatorssuch as the MAPK pathway. Our rationale for such investigationwas that, if we could inhibit microglial activation very earlyon, the amplification of the inflammatory response associatedwith activation of proinflammatory intracellular signal transductioncascades could be abated. Our data show that microglia can beactivated after treatment with A $beta$ peptides and the PTP inhibitorphen. This result led us to investigate stimulation of the membrane-boundPTP CD45 as a putative negative regulator of microglial activation.Data showed that cross-linking CD45 markedly reduced microglialactivation resulting from A $beta$ and phen co-treatment. Furthermore,we observed decreased activation of p44/42 MAPK under these conditions,suggesting that CD45 cross-linking stimulates the CD45-associatedPTP pathway, and that stimulation of this pathway negatively controlsp44/42 MAPK activation. In accordance with this, co-treatmentof A $beta$ - and phen-activated microglia with PD98059, an inhibitorof MEK1/2 (the upstream activator of p44/42 MAPK), resulted instatistically interactive blockade of microglial activation. Wefound that microglia deficient for CD45 could be directly activatedby A $beta$ peptides in vitro, and brains from Tg APP_sw mice deficientfor CD45 demonstrated markedly increased TNF- $alpha$ levels comparedwith Tg APP_sw or CD45-deficient mouse brains. These results suggestthat stimulation of CD45 is a viable approach for downregulatingA $beta$ -induced microglialactivation.

It has previously been shown that CD45 and the TNF receptor superfamily member CD40 can antagonize each another, because stimulationof CD45 opposes CD40-induced Ig class switching of human B cellsto the IgE isotype (Loh et al., 1995). The mechanism underlyingCD45-CD40 antagonism involves dephosphorylation and phosphorylationof tyrosine residues on their respective target signaling proteins,because CD45 is a PTP, and ligation of CD40 results in protein-tyrosinephosphorylation (Lazaar et al., 1998; Friedman and Greene, 1999).We have recently shown that ligation of CD40 leads to activationof microglia, as evidenced by TNF- $alpha$ release and bystander-inducedneurotoxicity (Tan et al., 1999a). We presently show that inhibitionof microglial CD45 leads to activation of these cells, whereasstimulation of microglial CD45 opposes this effect. In the presenceof low doses of freshly solubilized A $beta$ , synergistic enhancementof microglial activation is observed in either the CD40 ligation(Tan et al., 1999b) or the CD45 inhibition paradigm. When takentogether, these observations suggest that, in microglia, CD40and CD45 may have antagonistic effects on activation of thesecells, whereby CD40 promotes and CD45 opposes it. Additionally,the possibility arises that A $beta$ is able to positively affect microglialactivation via disruption of CD45-CD40homeostasis.

We initially showed that co-treatment with the PTP inhibitor phen and A $beta$ peptides resulted in microglial activation as evidencedby increased NO and TNF- $alpha$ release (Fig. 1a,b). However, the questionarose of whether this effect was dependent on PTP inhibition asopposed to inhibition of other phosphatases. Thus, we co-treatedwild-type primary culture microglia with A $beta$ and either sodiumorthovanadate, another PTP inhibitor, or okadaic acid, an inhibitorof protein phosphatase 2A, and measured NO and TNF- $alpha$ release.We observed that sodium orthovanadate treatment in conjunctionwith A $beta$ produced results similar to those of phen and A $beta$ peptideco-treatment. However, NO and TNF- $alpha$ were not detectable in themedia of okadaic acid- and A $beta$ -co-treated microglia. These datasuggest that treatment of microglia with specific inhibitors ofPTPs, as opposed to general phosphatase inhibitors, along withA $beta$ triggers microglial activation, further substantiating thespecific effect of PTP stimulation via CD45 in opposing microglialactivation induced by phen and A $beta$ peptides.

Past studies have shown that, in general, phosphatase activity decreases with aging and even more so in AD across variouscell types (Gong et al., 1995; Pei et al., 1998). Specifically,it has been shown that peripheral T lymphocytes isolated fromAD patients demonstrate decreased amounts of the CD45R isoformcompared with age-matched nondemented control subjects (Ikedaet al., 1991). To examine whether increasing CD45 activity couldblock microglial activation resulting from co-treatment with phenand A $beta$ , we activated wild-type microglia with phen and A $beta$ , addedCD45 recombinant protein (20 U/ml) to these cells, and measuredNO and TNF- $alpha$ release. We observed marked reduction of NO and TNF- $alpha$ after addition of CD45 recombinant protein to activated microgliacompared with appropriate controls. Interestingly, treatment ofactivated microglia with CD45 recombinant protein resulted inblockade of NO and TNF- $alpha$ release to an extent similar to thatresulting from cross-linking CD45, further substantiating thatCD45 cross-linking stimulates the CD45 PTPpathway.

Our data thus far had focused on CD45-mediated downregulation of microglial activation induced by co-treatment with phen andA $beta$ . These data raised the question of whether CD45 may reducemicroglial activation induced by other stimuli, such as LPS. Toaddress this possibility, we incubated microglia with LPS (1 ng/ml)and anti-CD45 antibody. Data showed that CD45 cross-linking markedlyattenuated microglial activation as evidenced by NO and TNF- $alpha$ release (Fig. 7). These data raise the possibility that stimulationof the CD45 pathway negatively controls microglial activationinduced by various proinflammatory stimuli and suggest that pharmacotherapeuticstargeting stimulation of CD45 may be beneficial in suppressingmicroglial activation, which is a pathogenic component of a varietyof neurodegenerative diseases.

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Figure 7. CD45 cross-linking markedly inhibits production of TNF- $alpha$ and NO in LPS-treated microglia. Microglial cells were treated as indicated for 12 hr. TNF- $alpha$ production (mean ± 1 SEM, picograms per milligram of total protein) and NO release (mean ± 1 SEM, micromolar concentration per milligram of total protein) were determined by TNF- $alpha$ ELISA and nitric oxide assay, respectively. Data shown are representative of six independent experiments. One-way ANOVA revealed significant between-group differences (p < 0.001), and post hoc testing revealed a significant difference between LPS and LPS/anti-CD45 antibody (p < 0.001).

  FOOTNOTES

Received May 31, 2000; revised July 25, 2000; accepted July 27, 2000.

We are grateful to Diane and Robert Roskamp for their generous support, which helped make this work possible. We thank JodiKroeger for assistance in flow cytometric acquisition and analysisand Kiyoko Yokota for assistance in maintaining CD45-deficientmice.
Correspondence should be addressed to Dr. Jun Tan, Roskamp Institute, University of South Florida, 3515 East Fletcher Avenue,Tampa, FL 33613. E-mail: jtan{at}coml.med.usf.edu.

  REFERENCES

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MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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CD45 Opposes -Amyloid Peptide-Induced Microglial Activation via Inhibition of p44/42 Mitogen-Activated Protein Kinase

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