Abstract
The brain in Alzheimer's disease (AD) shows a chronic inflammatory response characterized by activated glial cells and increased expression of cytokines and complement factors surrounding amyloid deposits. Several epidemiological studies have demonstrated a reduced risk for AD in patients using nonsteroidal anti-inflammatory drugs (NSAIDs), prompting further inquiries about how NSAIDs might influence the development of AD pathology and inflammation in the CNS. We tested the impact of chronic orally administered ibuprofen, the most commonly used NSAID, in a transgenic model of AD displaying widespread microglial activation, age-related amyloid deposits, and dystrophic neurites. These mice were created by overexpressing a variant of the amyloid precursor protein found in familial AD. Transgene-positive (Tg+) and negative (Tg−) mice began receiving chow containing 375 ppm ibuprofen at 10 months of age, when amyloid plaques first appear, and were fed continuously for 6 months. This treatment produced significant reductions in final interleukin-1β and glial fibrillary acidic protein levels, as well as a significant diminution in the ultimate number and total area of β-amyloid deposits. Reductions in amyloid deposition were supported by ELISA measurements showing significantly decreased SDS-insoluble Aβ. Ibuprofen also decreased the numbers of ubiquitin-labeled dystrophic neurites and the percentage area per plaque of anti-phosphotyrosine-labeled microglia. Thus, the anti-inflammatory drug ibuprofen, which has been associated with reduced AD risk in human epidemiological studies, can significantly delay some forms of AD pathology, including amyloid deposition, when administered early in the disease course of a transgenic mouse model of AD.
- inflammation
- cytokines
- microglia
- amyloid
- Alzheimer
- NSAID
A chronic inflammatory response characterized by activated microglia, reactive astrocytes, complement factors, and increased inflammatory cytokine expression associated with β-amyloid deposits has been described in the brains of Alzheimer's patients (Rogers et al., 1996). Evidence that this inflammation contributes to the pathogenesis of Alzheimer's disease (AD) has stemmed from 20 retrospective epidemiological studies and one prospective, longitudinal study showing up to a 50% reduction in the risk of AD associated with nonsteroidal anti-inflammatory drug (NSAID) consumption (Stewart et al., 1997; McGeer and McGeer, 1998). Ibuprofen was the most frequently used anti-inflammatory drug in these studies, taken by 39–50% of the subjects (Breitner et al., 1995; Stewart et al., 1997). These studies raise the question of how NSAIDs, particularly the nonprescription medication ibuprofen, might influence CNS inflammation and AD pathology.
To address this problem, we used a previously described transgenic mouse, Tg(HuAPP695.K670N-M671L)2576 (Tg2576), with amyloid pathology and activated microglia (Hsiao et al., 1996; Frautschy et al., 1998). These mice, which overexpress the 695 amino acid form of human amyloid precursor protein (APP) containing a double mutation found in a Swedish kindred with familial AD, display age-related hippocampal and neocortical amyloid deposits first appearing at ∼10 months of age, as well as microglial activation, reactive astrocytes with increased glial fibrillary acidic protein (GFAP), and dystrophic neurites. Plaque-associated reactive microglia in these mice also show enhanced staining for tumor necrosis factor-α (TNF-α) and interleukin-1β (IL-1β) (Benzing et al., 2000), two pro-inflammatory cytokines elevated in microglia of brains from AD patients (Dickson et al., 1993;Griffin et al., 1998). To determine whether the development of AD-related pathology is sensitive to ibuprofen treatment, we analyzed brain tissue of ibuprofen-fed Tg2576 mice for changes in levels of IL-1β, GFAP, activated microglia, dystrophic neurites, amyloid plaques, and detergent-insoluble and water-soluble amyloid β-protein (Aβ). Ten-month-old Tg2576 mice were fed chow containing no drug or ibuprofen (375 ppm) for 6 months. We found that a chronic dose of oral ibuprofen reduced changes in levels of all these parameters, indicating that ibuprofen can significantly interfere with the development of some forms of AD pathology in this transgenic mouse model of AD.
MATERIALS AND METHODS
Animals. Ten-month-old male and female Tg2576 Tg+ and Tg− mice from 12 litters were randomly split between treatment groups. Tg+ mice were fed either chow (Research Diets, New Brunswick, NJ) containing ibuprofen (Sigma, St. Louis, MO; 375 ppm; n= 9) or no drug (n = 8) for 6 months before being sacrificed. Tg littermates were fed the same chow containing no drug (n = 5) or ibuprofen (n = 9). One animal was removed from the study for failure to gain weight. At the time of sacrifice, neither the weights nor the ages of the mice were significantly different. Animals were perfused before brain dissection with 0.9% normal saline followed by HEPES buffer, pH 7.2, containing protease inhibitors. Brain regions were dissected from one hemisphere using mouse brain atlas coordinates (Franklin and Paxinos, 1997). One brain hemisphere was lined up with the interaural line at 0 mm. From the interaural line, vertical cuts were made at +3 and +0.72 mm, just posterior to the mammillary bodies. Thalamic, cortical, and hippocampal regions, as well as entorhinal cortex and piriform cortex/amygdala sections, were dissected out and snap-frozen in liquid nitrogen. Biochemical measurements were performed in the hippocampus, entorhinal cortex, piriform cortex/amygdala, and residual cortex (cortex region without frontal, entorhinal, or piriform areas). The other brain hemisphere was fixed in 4% paraformaldehyde, processed in 10–20% sucrose, frozen in liquid nitrogen, and sectioned (10 μm) for immunohistochemistry.
Tissue preparation. Tissue samples were homogenized in 10 wet weight volumes of TBS, pH 8.0, containing a cocktail of protease inhibitors (20 μg/ml each of pepstatin A, aprotinin, phosphoramidon, and leupeptin, 0.5 mm PMSF, and 1 mm EGTA). Samples were sonicated briefly (10 W, 2 × 5 sec) and centrifuged at 100,000 × g for 20 min at 4°C. The soluble fraction (supernatant) was used for IL-1β or Aβ ELISAs. To analyze insoluble Aβ, the SDS-insoluble pellet was solubilized and sonicated in 70% formic acid. The extract was neutralized with 0.25m Tris, pH 8.0, containing 30% acetonitrile and 5 m NaOH before loading onto the ELISA plate.
Sandwich ELISA for Aβ. Monoclonal 4G8 against Aβ17–24 (Senentek, Napa, CA) was used as the capture antibody at 3 μg/ml in 0.1 m carbonate buffer, pH 9.6, in a Dynex 96 well plate. Blocking was completed with 2% bovine serum albumin in TBS. Processed and neutralized samples were diluted with EC buffer (TBS containing 0.1 mm EDTA, 1% BSA, and 0.05% 3-[(3-cholamidopropyl)dimethylammonio]-1-propanesulfonic acid (CHAPS), pH 7.4, containing protease inhibitors (20 μg/ml each of pepstatin, aprotinin, phosphoramidon, and leupeptin, 0.5 mmPMSF, 1 mm EGTA, and 2 mm EDTA). Equal volumes of sample and detector antibody (biotinylated 10G4, against amino acids 5–13; 1:500) were loaded onto the wells overnight at 4°C. The reporter system was streptavidin-alkaline phosphatase using AttoPhos (JBL Scientific, San Luis Obispo, CA) as the substrate. Fluorescence of the product was monitored at an excitation wavelength of 450 nm and an emission wavelength of 580 nm.
Sandwich ELISA for IL-1β. A polyclonal antibody against mouse IL-1β (Endogen, Woburn, MA) was used as the capture antibody at 2 μg/ml in PBS in a Dynex 96 well plate. Blocking was completed with 2% bovine serum albumin in TBS. Equal amounts of sample (80 μg of brain protein extract) were loaded onto the wells overnight at 4°C. A monoclonal antibody against mouse IL1-β (Endogen; 0.5 μg/ml) was used as the detecting antibody. The development of the ELISA was performed as described above for Aβ. The minimum detectable quantity of IL-β was 0.5 pg under most conditions.
Immunoblot of GFAP. Brain homogenates (50 μg) were electrophoresed on a 10% acrylamide gel under reducing conditions. Proteins were transferred to a polyvinylidene difluoride membrane (400 mA for 2 hr) before blocking in 10% nonfat dry milk and 0.1% gelatin in PBS for 1.5 hr. Blots were incubated with monoclonal antibodies against GFAP (Sigma) overnight at 4°C. After three rinses, blots were incubated in HRP-conjugated goat anti-mouse (1:10,000) for 45 min before development with SuperSignal (Pierce, Rockford, IL). Bands were analyzed using densitometric software (Molecular Analyst II).
Immunostaining and image analysis. Ten micrometer hemibrain cryostat sections were cut from the posterior pole to the anterior margin of the hippocampus. Anti-phosphotyrosine (anti-PT) staining was performed on cryostat sections from middle hippocampus as previously described (Frautschy et al., 1998). To identify neuritic plaques, sections were incubated overnight at 4°C (1:100) in “DAE” polyclonal antibody (anti-Aβ1–13) made against synthetic peptides Aβ1–13 and named after the first three amino acids of the Aβ peptide, Asp-Ala-Glu. Vascular amyloid was labeled overnight at 4°C with a polyclonal antibody anti-Aβ34–40 (Mak et al., 1994). Dystrophic neurites were labeled overnight at 4°C with a polyclonal antibody against ubiquitin (1:500; Dako, Carpinteria, CA). Slides were incubated in biotinylated goat anti-rabbit antibodies (1:1000) followed by ABC reagent, each for 30 min at 37°C. Sections were developed using peroxidase/DAB (Pierce). If sections were double-labeled for DAE, immunostaining was developed with alkaline phosphatase substrate kit III (Vector Laboratories, Burlingame, CA).
For image analysis of DAE and ubiquitin staining, we examined immunolabeling from three coronal sections taken from anterior (bregma, −1.22 mm), middle (bregma, −1.70 mm), and posterior hippocampus (bregma, −2.80 mm) of Tg+ animals treated or untreated with ibuprofen. Specifically, residual cortex areas were defined as the cortical region dorsal to the rhinal fissure, whereas entorhinal and piriform/amygdala regions were defined as areas ventral to the rhinal fissure on coronal sections. All images were acquired from an Olympus Vanox-T (AHBT) microscope with an Optronix Engineering LX-450A CCD video system. The video signal was routed into a Macintosh computer via a Scion Corporation AG-5 averaging frame grabber, and these digitized images were analyzed with NIH Image public domain software. Custom Pascal macro subroutines were written to calculate various parameters of DAE and ubiquitin immunostaining. DAE parameters included number of plaques, mean diameter, mean area, mean percentage area, and total area of plaques. Ubiquitin parameters consisted of the number of small particles (ranging from 3 to 25 μm), mean area and total area of small ubiquitin particles, and percentage area of positively stained particles per subregion. Analysis of anti-PT immunostaining was performed using a quantitative ring analysis as previously described (Frautschy et al., 1998).
Statistical analyses. A two-factor ANOVA (diet × region or transgene × region) was performed to analyze differences in IL-1β and GFAP levels, Aβ levels, and image analysis data. Post hoc comparisons between regions were performed using Fisher's protected least significant difference. Bartlett's test for homogeneity of variances was also performed to determine whether variances were equal. Some analyses required logarithmic or square root transformations to establish homogeneity.P values < 0.05 were considered significant.
RESULTS
Ibuprofen decreases IL-1β and GFAP levels in brains of transgenic animals
IL-1β levels were quantified in brain supernatant extracted from dissected brain regions in three groups of mice: Tg+ mice fed control diet, Tg− mice fed control diet, and Tg+ mice fed ibuprofen diet. Dissected brain regions included hippocampus, entorhinal cortex, piriform cortex/amygdala, and residual cortex. Results analyzed by ANOVA revealed a significant transgene-dependent increase in IL-1β in hippocampal and residual cortical regions (F(1,21) = 19.934; p = 0.0002) (Fig. 1A), but not in entorhinal and piriform/amygdala areas (F(1,20) = 2.696; p = 0.11). Hippocampus and residual cortex data were grouped together because their variances were more similar to each other than entorhinal and piriform cortex regions. Levels of IL-1β were elevated 2.4-fold in hippocampus and 6.7-fold in residual cortex. ANOVA analyses showed an overall treatment effect in all regions (F(1,50) = 13.689; p = 0.0005) (Fig. 1B). There was also a significant treatment–region interaction, indicating that reductions in IL-1β levels were dependent on region. Levels were decreased 75% in hippocampus and 68% in residual cortex.
Western analysis was used to determine the effect of ibuprofen treatment on GFAP levels in Tg2576 mice. GFAP is a marker of astrocytosis that is elevated with age in mammals and is increased in amyloid-forming APP transgenic mice (Laping et al., 1994; Irizarry et al., 1997). ANOVA analyses demonstrated an overall transgene-dependent increase in GFAP levels (F(1,38) = 37.997; p = 0.001) (Fig. 1C), that was region-dependent (F(3,38) = 7.693;p = 0.004). GFAP levels were significantly lower in the ibuprofen-treated group (F(1,48) = 4.891; p = 0.03), with no significant treatment–region interaction (Fig. 1D). Regionally, the largest transgene-associated increase in GFAP was observed in entorhinal cortex (7.1-fold), whereas GFAP levels were reduced 76% with ibuprofen treatment. Smaller (1.25- to 2-fold) transgene-dependent elevations in GFAP were observed in other regions, whereas relatively lesser 15–25% reductions were observed with ibuprofen treatment.
Microglial activation is significantly decreased in ibuprofen-treated mice
Quantitative morphometric image analysis of anti-PT-labeled microglia was previously used to demonstrate evidence of activated microglia clustered within and around plaques in aging Tg2576 mice (Frautschy et al., 1998). This ring analysis, which quantifies PT-labeled microglia within four plaque-centered rings one to four plaque radii from the center of Aβ-labeled deposits, was performed on cryostat sections stained for Aβ (DAE, blue) and microglia (PT, brown). Results of double-blind ring analysis of plaques in parietal and temporal cortex and hippocampus showed that the percentage of area occupied by PT-labeled microglia was significantly decreased in the ibuprofen group (Fig.2A). Within four plaque radii from plaque center, there was a 29% reduction (F(1,1472) = 56.208; p< 0.0001) in the area covered by activated microglia in the ibuprofen group. Two-factor ANOVA analysis showed a significant treatment–ring interaction, indicating that the ibuprofen-associated reductions of microglial activation were dependent on distance from the Aβ deposits. Microglial activation decreased significantly within and immediately adjacent to Aβ-labeled plaques (rings 1 and 2;p < 0.0001), but not significantly in outlying rings 3 and 4 (Fig. 2B).
The effect of ibuprofen on microglial staining was more dramatic outside the plaques (ring 2) than within the plaques (ring 1). This effect is illustrated in Figure 3, in which sections of piriform cortex/amygdala regions from Tg+ mice fed control diet (D) and Tg+ fed ibuprofen (E) were double-labeled for Aβ (Vector,blue) and phosphotyrosine (diaminobenzidine,brown). In brains of Tg+ mice fed control diet in which PT labeling was upregulated, Aβ deposits (purple) are surrounded by activated microglia (brown), which are more numerous when close to (arrowheads) than when distal to deposits (arrows). Compared to microglia surrounding plaques in Tg+ mice fed control diet (F), fewer microglia cluster around plaques in the Tg+ mice fed ibuprofen (E).
Amyloid pathology is reduced by ibuprofen
To evaluate the effect of ibuprofen on amyloid and plaque pathology, cryostat sections from anterior to posterior hippocampus were immunostained for Aβ using a rabbit polyclonal antibody made to synthetic Aβ1–13 peptide (“DAE”). This antibody labeled plaques similarly to the commercially available mouse monoclonal antibody, 4G8 (Senentek) (data not shown), and more robustly than anti-Aβ34–40 (Fig. 3A), but exhibited lower levels of endogenous IgG artifacts associated with using mouse antibodies on mouse tissue. An example of anti-Aβ DAE immunostaining of piriform cortex/amygdala of Tg+ mice fed control diet is shown in Figure 3B. Using NIH Image public domain software, sections were analyzed for total plaque counts, plaque size, and total area of plaques. The ibuprofen diet group had significantly fewer (53%) overall plaque numbers compared to the control diet group analyzed across all regions (F(1,28) = 5.78; p = 0.02) (Table 1). The treatment group also showed a reduction in the overall percentage and total area staining for Aβ by 53% (F(1,28) = 3.603;p = 0.07) and 56% (F(1,28) = 5.515; p = 0.01), respectively, compared with the control diet group. A 57% reduction in percentage area stained was observed in residual cortex of ibuprofen-treated animals. Ibuprofen treatment did not affect plaque size (mean area) (F(1,28) = 0.032;p = 0.85). None of the treatment effects on amyloid deposits showed a significant dependence on region.
In addition to analysis of Aβ immunohistochemically, the effect of ibuprofen on Aβ levels in the opposite hemisphere was also analyzed biochemically in dissected brain regions by an ELISA that detects total Aβ. “Soluble” Aβ was first extracted with TBS and then in 2% SDS, and the remaining SDS “insoluble” Aβ was pelleted at 100,000 × g and extracted with 70% formic acid. Insoluble Aβ levels were significantly decreased overall by 39% in the ibuprofen-treated mice (F(1,50) = 4.709; p = 0.03) (Fig.4A). There was no significant treatment–region interaction, indicating that the reduction of insoluble Aβ was fairly uniform across regions. Analysis of individual regions showed the greatest reduction of 40% in the residual cortex (54.7 ng of control diet vs 32.7 ng of ibuprofen diet), with a consistent trend for reductions of 20–35% in every other region. Two-factor ANOVA for soluble Aβ similarly demonstrated that levels were decreased overall by 34% in the ibuprofen-treated group (Fig. 4B) (F(1,41) = 3.683; p = 0.06), with no significant treatment–region interaction. Regionally, strong trends toward ibuprofen-associated reductions in soluble Aβ were found in all regions varying from 21 to 62%.
Ubiquitin-positive structures are significantly decreased in number with ibuprofen
The effect of ibuprofen on the numbers and size of small ubiquitin-positive profiles (neurites) was measured using image analysis of cryostat sections immunolabeled with anti-ubiquitin from mice fed either ibuprofen or control diet. A representative example of this labeling is seen in Figure 3C. Anti-ubiquitin labeled no neurites in Tg- mice. Double labeling in Tg+ mice with anti-Aβ or synaptic markers revealed most ubiquitin staining in plaque-associated dystrophic neurites (data not shown). Image analysis (NIH Image) revealed that the numbers of small ubiquitin-labeled dystrophic neurites (ranging from 3 to 20 μm in diameter) were decreased by 48% in the ibuprofen group (F(1,30) = 4.903; p = 0.03) (Table2). Whereas the average size of small particles was increased by 31%, the mean percentage of area occupied by ubiquitin-positive small particles was significantly smaller with ibuprofen (67%) than in the control group (F(1,30) = 9.299; p = 0.005). Furthermore, the total area of ubiquitin-positive staining was decreased by 51% in ibuprofen-treated animals (F(1,30) = 7.058; p = 0.01), indicating that ibuprofen affected dystrophic neurite pathology. None of these treatment effects were region-dependent.
DISCUSSION
In this study we found that ibuprofen, a commonly used nonprescription NSAID associated with reduced AD risk in epidemiological studies, decreased inflammation, dystrophic neurite formation, and amyloid deposition in aging transgenic mice expressing a familial AD gene. This is the first report to demonstrate significant effects of NSAID treatment on AD pathology in a transgenic Alzheimer's model.
The mechanism by which NSAIDs reduce the risk of Alzheimer's disease is unknown. Two possibilities are: (1) NSAIDs decrease the inflammatory reaction engendered by amyloid deposits, leading to diminished neurotoxicity; and (2) NSAIDs attenuate the production of inflammatory cytokines, such as IL-1β and transforming growth factor-β (TGF-β), and products of reactive glia, such as apolipoprotein E (ApoE), which have been implicated in amyloid deposition (Mrak et al., 1995; Wyss-Coray et al., 1997; Harris-White et al., 1998). The results of our study strongly support the latter hypothesis, because amyloid deposition was dramatically suppressed with ibuprofen treatment. Support for the former hypothesis was less obvious and more difficult to assess, because traditional measures of neurotoxicity such as neuron loss and a reduction in synaptic markers are not evident in 16-month-old Tg 2576 mice (Irizarry et al., 1997). However, the percentage of plaque area occupied by microglia was smaller in treated animals, suggesting a decreased inflammatory reaction per plaque. One measure of neurotoxicity, the area occupied by ubiquitin-labeled dystrophic neurites, was diminished 48% in ibuprofen-treated mice, but this reduction in dystrophic neurites could be directly related to the reduction in amyloid deposition because final plaque number and total plaque area decreased 52–56% with ibuprofen treatment.
Ibuprofen also reduced both water-soluble and SDS-insoluble Aβ by 34 and 40%, respectively, effects that were less pronounced that the >50% decrease in amyloid plaque deposition. The inclusion of vascular Aβ in the ELISA, but not in the image analyses of amyloid deposits, may have limited the size of the ibuprofen effect in the biochemical measurements of Aβ relative to the immunohistochemical measurements. Because Aβ40 comprises >50% of the total Aβ in Tg2576 mice (Hsiao et al., 1996) and is the major component of vascular amyloid, we stained vascular amyloid with anti-Aβ34–40 in Tg+ mice and found ibuprofen had no significant effect on the amount of vascular Aβ40 immunoreactivity in meningeal and plexus vessels (data not shown).
The observed reduction in soluble Aβ by ibuprofen treatment at an early stage might contribute to a decrease in amyloid seeds and subsequent plaque numbers. This could occur through its influence on microglia, which have been proposed to affect the formation or clearance of small, diffusible Aβ oligomers or multimers (Ard et al., 1996), or through an effect on ApoE, TGFβs, or other cytokine circuits with diffusible effectors (Griffin et al., 1998). In AD brain, soluble Aβ is sixfold higher than in control brains and contains both monomers and oligomers (10 to >100 kDa), hypothesized to be seeds or precursors to insoluble, filamentous amyloid (Kuo et al., 1996). Soluble Aβ levels in residual cortex of 16-month-old untreated Tg2576 mice averaged 174.6 pmol/gm tissue but were less than 60 pmol/gm tissue in 3- to 4-month-old Tg2576 mice (data not shown). The attenuation of this rise by ibuprofen in Tg2576 mice supports the possibility that small Aβ aggregates or oligomers were reduced by this treatment. In humans a greater impact of NSAID treatment at an earlier stage of AD has been suggested by two epidemiological studies, which found a greater risk reduction when NSAID use was begun more than 2 years before diagnosis (Stewart et al., 1997; In't Veld et al., 1998). Conversely, the lack of effect of NSAIDs on plaque numbers in the mesial temporal cortex of clinically normal elderly control and arthritic patients (Mackenzie and Munoz, 1998) might be explained by the fact that plaques stop accumulating rapidly with age in this brain area (Mackenzie et al., 1995), obscuring any potential effect on plaque initiation that NSAID consumption could produce.
Griffin et al. (1998) and Sheng et al. (1996, 1998) argue that plaque-associated IL-1 elevations in Down's syndrome and AD brains play an important role in cytokine circuits promoting GFAP and S100β overexpression, APP synthesis, astrocyte activation, dystrophic neurite formation, and neuritic plaque pathogenesis. In particular, dystrophic neurites, the hallmark of neuritic plaques, appear closely correlated with activated microglia and are hypothesized to be induced by cytokines from activated microglia. Increased expression of IL-1β has also been implicated in memory deficits and reduced long-term potentiation in aging rat hippocampus (Lynch, 1998). Our results show that chronic administration of ibuprofen prevents transgene- and age-related increases in brain levels of the inflammatory cytokine IL-1β in Tg2576 mice. This treatment also diminished the proliferation of activated microglia associated with amyloid plaques and decreased the number of ubiquitin-positive dystrophic neurites in plaque-forming regions of these mice. A significant reduction in overall dystrophic neurite formation may have resulted from a decrease in amyloid plaque number and a weakened microglial response surrounding plaques. Neuritic plaques are an important endpoint because increased density of neocortical neuritic plaques is associated with even very mild dementia (Haroutunian et al., 1998) and correlates with cognitive deficits (Nagy et al., 1995).
Interestingly, ring analyses of the microglial response to ibuprofen within and around plaques showed a more marked attenuation in ring 2 just outside plaques than in ring 1 located within plaques of 40 and 25%, respectively. This positional effect is consistent with a report showing NSAIDs markedly reducing microglia numbers outside and surrounding plaques in elderly, nondemented controls and arthritic patients, but producing a smaller effect on microglia in “close physical association with the plaque” (Mackenzie and Munoz, 1998).
The ibuprofen dose our mice received was estimated to be ∼56 mg/kg of ibuprofen per day, a dose considered high enough to both inhibit cyclooxygenase (COX) and stimulate peroxisome proliferator-activated receptors-γ (PPAR-γs), the two main pharmacological targets of ibuprofen and other NSAIDs (Lehmann et al., 1997; Combs et al., 2000). Because both COX and PPARγ expression are increased in Alzheimer brains (Kitamura et al., 1999), it is likely that at least some effects of ibuprofen on AD pathology are mediated through changes in the activities of these enzymes. COX inhibitors decrease production of prostaglandins, a major extracellular signal that can induce neuronal degeneration (Prasad et al., 1998). PPAR-γ agonists inhibit inflammatory cytokine synthesis by monocytic lineage cells, including IL-1, and block Aβ-stimulated expression of IL-1 and TNF-α by microglia, and thus may be important in controlling Aβ-mediated microglial inflammatory responses (Combs et al., 2000). Whether lower, safer doses of ibuprofen, such as 5–20 mg/kg (400–1000 mg/d in humans), are effective in delaying AD pathogenesis remains to be tested. If COX inhibition is the critical step, doses in this range, which are known to diminish centrally mediated nociceptive activity (Ferrari et al., 1990; Lotsch et al., 1997) and decrease prostaglandin levels in the mouse brain (Fitzpatrick and Wynalda, 1976), but are less effective in ameliorating peripheral inflammation in arthritis (Garcia Rodriguez, 1997), may nevertheless be beneficial in AD.
Our results show that a widely used NSAID, ibuprofen, can significantly delay both CNS inflammation and Alzheimer plaque deposition in the Tg2576 mouse model for AD. An effect at an early stage of plaque formation is proposed and is consistent with the reduced AD risk associated with chronic NSAID consumption in epidemiological studies. Studies in this and other mouse models will better define the choice of NSAIDs, appropriate target stages of disease, and doses for AD prevention or treatment in humans.
Footnotes
- Received April 1, 2000.
- Accepted May 5, 2000.
This work was supported by National Institute on Aging Grants AG13471 (G.M.C.) and AG15453 (K.H.A.), Veterans Affairs Merit, the Alzheimer Association, the Elizabeth and Thomas Plott Family Foundation, and the Katherine and Benjamin Kagan Alzheimer's Treatment Program. We thank Boris Oks, Robert McBean, and Ulises Garcia for their excellent work genotyping the transgenic mice. We also thank Mychica Simmons for assistance with the amyloid and ubiquitin image analysis. We are grateful to Dr. Judith Harker for her help with the statistical analyses.
Correspondence should be addressed to Dr. Greg M. Cole, Sepulveda VAMC GRECC 11E, University of California Los Angeles, Department of Medicine and Neurology (SFVP), 16111 Plummer Street, Sepulveda, CA 91343. E-mail: gmcole{at}ucla.edu.
- Copyright © 2000 Society for Neuroscience