Activation of c-Jun N-Terminal Kinase and p38 in an Alzheimer's Disease Model Is Associated with Amyloid Deposition

doi:20026352

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Web of Science (91)

Citing Articles via Google Scholar

Google Scholar

Articles by Savage, M. J.

Articles by Scott, R. W.

Search for Related Content

PubMed

PubMed Citation

Articles by Savage, M. J.

Articles by Scott, R. W.

Previous Article  |  Next Article

The Journal of Neuroscience, May 1, 2002, 22(9):3376-3385

Activation of c-Jun N-Terminal Kinase and p38 in an Alzheimer's Disease Model Is Associated with Amyloid Deposition
Mary J. Savage, Yin-Guo Lin, John R. Ciallella, Dorothy G. Flood, and Richard W. Scott
Department of Neurobiology, Cephalon Inc., West Chester, Pennsylvania 19380

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The mechanisms by which neurons and synapses are lost in Alzheimer's disease (AD) are not completely understood. To characterizepotential signaling events linked to AD pathogenesis, activation-specificantibodies were used to examine mitogen-activated protein kinase(MAPK) kinase pathways at various ages in mice transgenic forhuman amyloid precursor protein-695 with the Swedish familialAD mutations (Tg2576) and homozygous for a P264L familial AD mutationintroduced by targeting of the presenilin-1 gene (PS1^P264L). Although the c-Jun N-terminal kinase (JNK) and p38 pathwayswere significantly activated in the cortex at both 7 and 12 monthsof age, there was no significant activation of the extracellularsignal-regulated kinase pathway. MAPK kinase-4, an upstream activatorof JNK, was also significantly activated at 7 and 12 months, whereasc-Jun, a downstream effector of JNK-associated apoptotic signaling,was not induced. The lack of c-Jun activation is consistent withthe absence of neuronal loss in both cortex and hippocampal CA1at 12 months. The JNK activation was localized to amyloid deposits,within neurites containing phosphorylated tau. Synaptophysin wasquantified biochemically as a measure of synaptic integrity andwas significantly reduced in an age-dependent manner in the Tg2576/PS1^P264L cortex but not in either PS1^P264L or Tg2576 cortex. Stress-responsive MAP kinase pathways wereactivated in the brain of the Tg2576/PS1^P264L AD model, and this activation was coincident with the age-dependentincrease in amyloid deposition, tau phosphorylation, and lossofsynaptophysin.

Key words: JNK; p38; ERK; tau; presenilin; synaptophysin; amyloid precursor protein

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The memory impairments in Alzheimer's disease (AD) are attributable to the loss of both neurons and synapses (West et al.,1994; DeKosky et al., 1996; Gomez-Isla et al., 1997). Toxic proteinsthat accumulate in the AD brain are thought to precipitate thisloss. Amyloid $beta$ protein (A $beta$ ) is a cleavage product of the amyloidprecursor protein (APP) and accumulates as extracellular plaque,a diagnostic lesion of the AD brain. Elevated levels of solubleA $beta$ precede disease pathology in familial forms of AD (FAD) (Scheuneret al., 1996) and in Down's syndrome (Tokuda et al., 1997).

Hyperphosphorylated tau protein accumulates as insoluble paired helical filaments (PHF) within neuronal cell bodies [neurofibrillarytangles (NFTs)] and amyloid-associated processes (dystrophic neurites).Hyperphosphorylated tau binds poorly to microtubules (Iqbal andGrundke-Iqbal, 1996; Mandelkow et al., 1996), likely reducingthe efficiency of axonal transport and contributing to neuronaldysfunction. Although tau mutations cause NFTs in frontotemporaldementia with parkinsonism (Hutton et al., 1998), tau mutationsresulting in AD have not beendemonstrated.

Accompanying increased brain levels of A $beta$ and tau are elevations in the inflammation-related proteins of the complement cascade,as well as interleukin-1 $beta$ and tumor necrosis factor- $alpha$ (Akiyamaet al., 2000). Any or all of the above mentioned proteins arepotential triggers for the neuronal death and synaptic loss; however,the mechanism(s) by which these losses occur isunknown.

Mitogen-activated protein kinase (MAPK) signaling pathways regulate many cellular processes, including gene expression, differentiation,and cell death (Chang and Karin, 2001). In AD brain, activationof three MAPK pathways has been demonstrated in neurons and dystrophicneurites: c-Jun N-terminal kinase (JNK) (Shoji et al., 2000; Zhuet al., 2001a), p38 (Hensley et al., 1999; Zhu et al., 2000),and extracellular signal-regulated protein (ERK) (Perry et al.,1999; Ferrer et al., 2001). Furthermore, ERK activation was reportedin hippocampal slices after treatment with soluble A $beta$ 1-42 (Dineleyet al., 2001), whereas JNK pathway activation occurred in bothcortical neurons treated with A $beta$ 25-35 and differentiated PC12cells after exposure to aggregated A $beta$ 1-42 (Bozyzcko-Coyne et al.,2001; Morishima et al., 2001; Troy et al., 2001). Inhibition ofthe JNK pathway significantly reduced the toxicity attributableto A $beta$ in all three studies. Increased p38 activity has been reportedafter A $beta$ treatment of microglia (McDonald et al., 1998; Pyo etal., 1998).

MAPK pathways have also been implicated in tau hyperphosphorylation. Cell-free assays have demonstrated that JNK, p38, andERK phosphorylate tau at sites found in AD (Goedert et al., 1997;Reynolds et al., 2000), yet cell-associated phosphorylation oftau by these kinases has not beenreported.

Here, MAPK activation was studied using a mouse model incorporating two FAD mutations: (1) a human APP695 transgene with theSwedish FAD mutations (Tg2576) (Hsiao et al., 1996) and (2) apresenilin 1 (PS1)-P264L FAD knock-in mutation (Flood et al.,2001). This model exhibits an aggressive rate of amyloid depositionand associated pathology, achieving 24% cortical amyloid burdenat 12 months (Flood et al., 2001). We now report JNK activationin Tg2576/PS1^P264L cortex that colocalizes with phospho-tau staining in the abnormalneurites that surround amyloid deposits. Notably, this activationis absent in neuronal cell bodies. p38 is also activated in thecortex of the AD model, whereas ERK is not. Accompanying kinaseactivation and tau phosphorylation is a reduction in synaptophysin,indicating synapticabnormalities.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Transgenic and gene-targeted mouse lines. Mice overexpressing human APP695 with the Swedish FAD mutations (SwAPP695) havebeen described previously (Tg2576; Hsiao et al., 1996). Thesetransgenic animals were crossed with mice expressing a PS1 FADknock-in mutation at P264L (Campion et al., 1995; Wasco et al.,1995). Details of PS1 cloning, targeting vector construction,homologous recombination, and chimera production have been reportedpreviously (Siman et al., 2000; Flood et al., 2001). Tg2576/PS1^P264L/+ heterozygous males were crossed with nontransgenic PS1^P264L/+ heterozygous females to generate the four genotypes used in thisstudy. The following littermate-controlled genotypes were analyzed:(1) Tg2576/PS1^P264L/P264L (Tg2576/PS1^P264L or TgPS1, Tg and homozygous for PS1 mutation), (2) PS1^P264L/P264L (PS1^P264L or PS1, homozygous for PS1 mutation and non-Tg), (3) Tg2576/PS1^+/+ (Tg2576, Tg and carrying the normal mouse PS1), and (4) non-Tg/PS1^+/+ (wild type or WT). The shortened designations of the genotypesare used hereafter. The use of animals in this study was in accordancewith Cephalon's Institutional Animal Care and Use Committee andfollowed National Institutes of Healthguidelines.

Antibodies. The following antibodies from Cell Signaling Technology (Beverly, MA) were used for either immunohistochemistry(IHC) or Western blotting (WB): phospho-JNK (9255; WB), phospho-MAPKkinase-4 (MKK4) (9151; IHC and WB), phospho-ser63-c-Jun (9261;WB), c-Jun (9162; WB), p38 (9212; WB), phospho-ERK (9106; WB),and ERK (9102; WB). Additional antibodies were received from SantaCruz Biotechnology (Santa Cruz, CA): phospho-JNK (sc6254; IHC),MKK4 (sc837; WB), tau (sc5587; WB), and actin (sc1616; WB). Thefollowing antibodies were from Innogenetics (Alpharetta, GA):phospho-tau-ser202 (AT8; IHC and WB) and phospho-tau-thr231 (AT180;IHC and WB). JNK (15691A; WB) was from PharMingen (San Diego,CA), and phospho-p38 (M8177; WB) and synaptophysin (S5768; WB)were from Sigma (St. Louis, MO). Antibody 1153, recognizing humanA $beta$ sequences 1-28, was generated as described previously (IHC;Savage et al., 1994).

Immunohistochemistry. Mice were perfused with 10 ml of Ringer's solution after deep anesthesia with Avertin (1.25% 2,2,2-tribromoethanoland 2.5% 2-methyl-2-butanol). Brains were removed, post-fixedin 70% ethanol and 0.15 M NaCl for 48 hr, and then paraffin embedded.Sections were cut at 10 µm, deparaffinized, and rinsed with 0.01M PBS. For detection of phospho-JNK, sections were microwavedat 50% power for 10 min in 0.01 M citrate buffer, pH 4.5, andrinsed with water. Detection of phospho-tau, phospho-MKK4, orA $beta$ deposition required no pretreatment. Endogenous peroxidasewas quenched with 0.3% methanol/water (50:50) for 30 min, andnonspecific binding was blocked with 5% goat serum in 0.1 M PBS.After overnight incubation at 4°C with primary antibody in 2%goat serum, horseradish peroxidase (HRP) immunohistochemistrywas performed using detection kits from Biogenex (San Ramon, CA)and nickel-intensified 3, 3'-diaminobenzidine. To demonstratespecific staining, primary antibody waseliminated.

Tissue processing and Western blots. Mouse brains were removed after deep anesthesia with Avertin. Cortex was dissected andfrozen at $-$ 70°C. Tissue was homogenized in 4°C lysis buffer (10mM Tris, pH 7.6, 50 mM NaCl, 0.03 µM sodium pyrophosphate, 50mM sodium fluoride, and 1% Triton X-100) containing 1 mM phenylmethylsulfonylfluoride, 20 µg/ml aprotinin, and 1 mM sodium vanadate. Sampleswere then centrifuged at 14,000 × g for 10 min at 4°C, and supernatantwas assayed for total protein concentration using a BCA assaykit (Pierce, Rockford, IL). Samples of 3, 10, or 100 µg of proteinper well were added in NuPage sample buffer (Invitrogen, Carlsbad,CA) to visualize synaptophysin/actin, JNK, and all other proteins,respectively. Proteins were resolved using SDS-PAGE with 10% NuPagegels and morpholinopropanesulfonate buffer (both Invitrogen) andtransferred to polyvinylidene difluoride membranes. Membraneswere blocked for nonspecific binding with 5% nonfat dry milk inTris-buffered saline and 0.05% Tween 20 detergent. Primary antibodieswere used in this same blocking buffer and incubated with membranesovernight at 4°C. After incubation with HRP-linked secondary antibodies(Southern Biotechnology Associates, Birmingham, AL), proteinswere detected using ECL detection reagent (Amersham Biosciences,Piscataway, NJ). Linear ranges were determined for each protein.For quantification of both phosphorylated and nonphosphorylatedproteins, RFLPscan software (Scanalytics, Billerica, MA) was used.Phosphoprotein levels were normalized, calculating a density ratioof phosphoprotein/phospho-independent protein (or synaptophysin/actin)within the same sample and gel, first visualizing phosphoprotein(phospho-JNK) and then stripping the blot for detection of specificprotein (JNK). This ratio is termed the active fraction for thekinase pathway members. To control for inter-gel variability,the average density ratios for wild-type samples on each gel wereset to 100%. Statistical differences were determined using Kruskal-Wallisone-way ANOVA on ranks (SigmaStat software; SPSS Science, Chicago,IL) with Dunnett's method for comparison with wild-type control.Significance was indicated on each graph with an asterisk at p< 0.05.

Neuronal counting. Mice were perfused with Ringer's solution, followed by 4% paraformaldehyde in 0.1 M phosphate buffer, pH7.4. Frozen sections were cut at 30 µm in the coronal plane, slidemounted, and stained with cresyl violet to visualize neuronalnuclei. Using a 100× objective lens, all neurons with a visiblenucleolus were counted. Every 12th section was counted, yieldingan average of seven sections counted per brain for CA1 and 18sections for cortex. Neurons were counted with the CASTGrid System(Olympus Optical, Denmark, Copenhagen) using the optical dissectortechnique (West and Gundersen, 1990). Total neuronal number wasestimated by calculating the volume of the CA1 pyramidal layeror the cortex of both hemispheres (excluding piriform and entorhinalcortex) according to the method of Cavalieri. Neuronal numberwas estimated using ~100 dissectors for CA1 and 200 dissectorsfor the cortex. Dissectors were 8 µm high (in an average actualsection thickness of 13 µm, measured with an optical encoder attachedto the microscope), and the frame area was 880 µm² for the cortex and 440 µm² for CA1. The estimation of total neurons was calculated by multiplyingthe neuronal density by the volume of CA1 or cortex. A singleexaminer (M.J.S.) performed the counting and was blinded as togenotype. Coefficients of error were <5% with the parameters usedto estimate counts in bothregions.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Activation of the JNK pathway in AD model cortex

The active, phosphorylated fractions of JNK, MKK4, and c-Jun in the brains of Tg2576/PS1^P264L mice at various ages and levels of amyloid deposition were measuredby immunoblot. At 3, 7, and 12 months, amyloid deposition was~2, 12, and 24% of the cortical area, respectively (Flood et al.,2001). Wild-type controls were examined at 12 months and had nodeposited amyloid. Levels of both phospho-JNK (Fig. 1A, top) andtotal JNK (Fig. 1A, bottom) migrating at two molecular weights,p54 and p46, are demonstrated from the same samples. There wasan age-dependent increase in phosphorylation of p54 JNK, whereassteady-state levels of the protein decreased. p46 demonstrateda relatively constant steady-state phosphorylation with decreasedtotal protein. When the densities of the phospho-JNK bands werestandardized to the total JNK bands for each sample and wild-typeratios were set to 100% to control for inter-gel variability,p54 demonstrated an age-dependent increase at 2.7-fold and 5.8-foldover the wild-type ratio at 7 and 12 months, respectively (Fig.1B). There was a twofold increase in the active fraction of thep46 form at 12 months, with no significant elevation at 7 months.

View larger version (39K):
[in this window]
[in a new window]
Figure 1. JNK activation is age dependent in Tg2576/PS1^P264L cortex. A, The top demonstrates 10 µg of cortical protein per sample stained with an antibody against phospho-JNK (phospho-thr183/phospho-thr185). These sites can be phosphorylated by MKK4 and indicate the presence of activated JNK in older Tg2576/PS1^P264L cortex. The bottom demonstrates total JNK protein from the same blot after stripping of the phospho-JNK antibodies. JNK protein levels decrease in the Tg2576/PS1^P264L cortex with age. B represents the active fraction of JNK from a density ratio of phospho-JNK to total JNK for each form. Six samples per group were assayed in triplicate on immunoblot. *p $<=$ 0.05 indicates significant differences. WT 12, Wild-type mice at 12 months of age.

To confirm that JNK activation was attributable to amyloid deposition and not an effect of either APP overexpression or thePS1-P264L mutation alone, the following littermate-controlledcortical samples at 12 months were compared with wild-type cortexfor JNK activation: (1) PS1^P264L homozygous knock-in mutation, (2) Tg2576 with human SwAPP695overexpression, or (3) the combined Tg2576/PS1^P264L genotypes. Relatively constant levels of phospho-JNK were presentin all groups, except Tg2576/PS1^P264L, in which levels of phospho-JNK were increased substantially(Fig. 2A, middle). When the active fraction of JNK was again representedas a percentage of the wild-type samples on each gel, the JNKactivity continued to be significantly upregulated in the Tg2576/PS1^P264L cortex at 12 months (Fig. 2B). In this group, the p54 JNK wasincreased 5.5-fold, whereas the p46 JNK was increased ~2.5-fold.Interestingly, the level of phospho-ser202-tau, detected withthe AT8 antibody (Fig. 2A, top), mirrored the JNK activation.In Tg2576 cortex, with 0.5% amyloid burden (Flood et al., 2001),the increased JNK activity was not statistically significant comparedwith wild-type samples.

View larger version (44K):
[in this window]
[in a new window]
Figure 2. JNK activation is genotype dependent. A, The middle demonstrates cortical samples at 12 months stained as in Figure 1 for detection of activated JNK. Increased phosphorylation of p54 JNK in the Tg2576/PS1^P264L cortex compared with wild-type, Tg2576, or PS1^P264L cortex. The bottom depicts total JNK as in Figure 1. The top shows the same samples stained for a third time for phosphorylated tau at ser202. Note the increase in phospho-tau in the Tg2576/PS1 cortex with the greatest amyloid burden and an intermediate degree of phospho-tau in Tg2576. B depicts a significant increase at p $<=$ 0.05 (asterisks) in the active fraction of both p54 and p46 JNK in the Tg2576/PS1^P264L cortex compared with wild type. Three samples per group were assayed in triplicate on immunoblot.

In addition to the presence of active JNK, the upstream kinase MKK4 was activated in Tg2576/PS1^P264L cortex. Brains were examined for phospho-MKK4 on Western blotsand normalized to MKK4 protein within the same samples. Therewas a significant eightfold and sixfold increase in the ratioof activated MKK4 to total MKK4 protein at 7 and 12 months, respectively(Fig. 3B). The increase in phosphorylated MKK4 (Fig. 3A, top)occurred with a subtle decrease in total protein (Fig. 3A, bottom).When brains of Tg2576/PS1^P264L mice at 12 months were immunostained for phospho-MKK4, the staininglocalized to neuronal cell bodies and axons, as seen for totalMKK4 in rat brain (Flood et al., 1998). Both amyloid depositsand the surrounding neurites were free of stain. At 12 months,there was no obvious change in staining intensity or locationwhen comparing wild-type and Tg2576/PS1^P264L animals.

View larger version (26K):
[in this window]
[in a new window]
Figure 3. MKK4 is activated in Tg2576/PS1^P264L cortex. A, The top demonstrates 100 µg of cortical protein per sample stained with an antibody against phosphorylated MKK4 (phospho-thr261). This site is phosphorylated by MAPKK kinases and indicates the presence of more activated MKK4 in 7 and 12 month cortical samples compared with 12-month-old wild-type littermates (WT 12). The bottom demonstrates total MKK4 using the same blot. B represents the active fraction of MKK4 from a density ratio of phospho-MKK4 to total MKK4. Six samples per group, each assayed in triplicate by immunoblot. *p $<=$ 0.05 indicates significant differences.

Unlike JNK and MKK4, there was no demonstrable increase in phospho-c-Jun in the Tg2576/PS1^P264L cortex. Compared with the 12-month-old wild-type animals thathad barely detectable phospho-c-Jun, this activity was reducedin the Tg2576/PS1^P264L cortex at all ages (Fig. 4, top). This phosphorylated specieswas defined by reaction with a phospho-ser63-c-Jun antibody, molecularweight, and colocalization with total c-Jun after stripping andreprobing with an antibody against c-Jun protein. Like JNK, c-Junlevels were decreased in the cortex of the older Tg2576/PS1^P264L animals (Fig. 4, bottom).

View larger version (48K):
[in this window]
[in a new window]
Figure 4. c-Jun phosphorylation is not increased with age in cortex of Tg2576/PS1^P264L mice. Top blot demonstrates cortical protein at 100 µg per well, stained with an antibody against phosphorylated c-Jun (phospho-ser63). This site can be phosphorylated by JNK and induces c-Jun transcription factor activity. Bottom blot demonstrates a reduction in levels of total c-Jun with age in the Tg2576/PS1^P264L cortex using the same blot. WT 12, Wild-type mice at 12 months of age.

Active JNK is found within abnormal neurites

The brains of Tg2576/PS1^P264L animals at 2, 4, 6, 9, and 12 months were examined histologically for the location of phospho-JNKimmunoreactivity. Serial sections were stained with antibody 1153(recognizing A $beta$ sequences 1-28) and antibodies specific for phospho-JNKand phospho-tau. Phospho-JNK immunoreactivity (Fig. 5B,E) colocalizeswith that of deposited amyloid (Fig. 5A,D). On top of a backgroundof light JNK neuropil staining and within the mass of depositedamyloid, there were defined profiles detected with the phospho-JNKantibody (Fig. 5E). Phospho-JNK immunoreactivity, detected asearly as 4 months, was located around amyloid deposits at allages, with increased staining corresponding to increased amyloidburden. This degree of induction at ages <4 months may be belowthe sensitivity of the Western blot method because there was nodetectable increase at 3 months (Fig. 1) on the Western blot.When the serial phospho-JNK (Fig. 6B,E) and phospho-tau (Fig.6, pthr231, A, D; pser202, C, F) sections are compared, profilesof the same size and shape colocalize, although they are not completelysuperimposable because of the small diameter of the neurites (~3µm) and the thickness of the sections (10 µm). No detectable phospho-JNKlocalized to neuronal cell bodies in the brains of the Tg2576/PS1^P264L mice, which appear unstained (Fig. 5E) compared with the surroundingneuropil.

View larger version (124K):
[in this window]
[in a new window]
Figure 5. Activated JNK is localized to amyloid deposits. Tg2576/PS1^P264L cortex at 12 months, stained with anti- A $beta$ 1-28, recognizing deposited amyloid (A, D) or phosphorylated JNK (B, E). pJNK immunoreactivity is localized to defined profiles within the amyloid deposits. C, Twelve-month-old control without amyloid deposits treated with the phospho-JNK antibody. F, No primary antibody control on Tg2576/PS1^P264L cortex, as in B. Arrows indicate amyloid deposits and phospho-JNK staining that colocalize on adjacent sections. Scale bars: (in C) A-C, F, 100 µm; (in D) D, E, 30 µm.

View larger version (116K):
[in this window]
[in a new window]
Figure 6. Activated JNK within amyloid deposits is localized to neurites containing phospho-tau. Tg2576/PS1^P264L cortex at 12 months, stained with an antibody to phospho-thr231 tau (A, D) phospho-JNK (B, E), or phospho-ser202 tau (C, F). A-C and D-F constitute serial sections through two separate amyloid deposits. Arrows indicate some of the neurites that overlap between two serial sections; arrowheads indicate neurites that overlap between all three sections. Scale bars: (in A) A-C, 15 µm; (in D) D-F, 12 µm.

Activation of p38 in AD model cortex

p38 activation was examined by immunoblot in the Tg2576/PS1^P264L mouse cortex at 7 and 12 months using a phospho-specific, activity-dependentantibody. Again, wild-type cortex was compared at 12 months. p38phosphorylation (Fig. 7A, top) was increased significantly ina progressive manner, whereas total p38 protein was constant withage (Fig. 7A, bottom). The active fractions of phospho-p38/totalp38 were increased threefold and eightfold, respectively, at 7and 12 months in Tg2576/PS1^P264L in cortex (Fig. 7B). Specific phospho-p38 staining was not detectedimmunohistochemically in the animal brain with available reagents.

View larger version (34K):
[in this window]
[in a new window]
Figure 7. Age-dependent activation of p38 in the Tg2576/PS1^P264L cortex. A, The top demonstrates 100 µg of cortical protein, stained with an antibody selective for activated p38 phosphorylated by an upstream kinase such as MKK3/6. The bottom depicts total p38 protein, which is relatively constant with age. B depicts the active fraction of p38 that increases with age and amyloid burden. Six samples per group were each assayed in triplicate on immunoblot. *p $<=$ 0.05 indicates significant differences.

ERK is not activated in AD model cortex

Whereas the stress-related pathways JNK and p38 demonstrated increased activity consistent with a role in the response ofthe brain to deposited amyloid, the trophic arm of the MAPK pathwayswas not induced with age and amyloid deposition. The two molecularweight forms of phospho-ERK, p42 and p44 (Fig. 8A, top), werenot elevated when normalized to the corresponding total ERK protein(Fig. 8A, bottom). In fact, the active fraction of the highermolecular weight form, p44 ERK, was significantly decreased at12 months in Tg2576/PS1^P264L cortex attributable to relatively constant levels of phospho-p44ERK and increased levels of p44 ERK (Fig. 8B). Although therewas a subtle increase in p42 activity at 7 months with a decreaseat 12 months, these effects were not statistically significant.

View larger version (33K):
[in this window]
[in a new window]
Figure 8. ERK pathway is not activated in the Tg2576/PS1^P264L cortex. A, The top demonstrates 100 µg of cortical protein, stained with anti-phospho-ERK. A very small increase in p44-ERK phosphorylation was present in cortical samples from Tg2576/PS1^P264L mice compared with the increase in total ERK from the same blot (A, bottom). The active fraction of p44 is reduced in an age-dependent manner (B). The active fraction of p42 is not changed significantly. Six samples per group were each assayed by immunoblot in triplicate. *p $<=$ 0.05 indicates significant differences. WT 12, Wild-type mice at 12 months of age.

Increased tau phosphorylation in AD model cortex

Tau phosphorylation increases with amyloid deposition in a number of AD models (Moechars et al., 1999; Sturchler-Pierrat andStaufenbiel, 2000; Masliah et al., 2001; Tomidokoro et al., 2001).Similar to the AD brain, phospho-tau was localized to amyloid-associatedneurites (Fig. 6) in the brain of Tg2576/PS1^P264L animals at 12 months. Elevated phospho-tau staining was not detectedin neuronal cell bodies compared with wild-type cortex. Increasedtau phosphorylation was evident on Western blots with AT8, recognizingphosphorylated serine 202 (Fig. 2A, top). Confirming the phosphorylationat this site, steady-state levels of the tau-1 epitope (dephosphorylatedserine 202) were reduced (data not shown). There was also increasedphosphorylation at threonine 231 (Fig. 9, top), whereas totaltau protein levels were relatively constant (Fig. 9, bottom).As expected after increased phosphorylation, the form of totaltau comigrating with the phosphorylated forms (Fig. 9, bottom,thinner top band) was increased in the depositing animals. Althoughthe increase in the higher molecular weight species of phospho-tauis apparent at 7 months, there is no corresponding increase inthe specific thr231 phospho-tau epitope at this age, suggestingthat another site(s) contributes primarily to the shift in molecularweight.

View larger version (49K):
[in this window]
[in a new window]
Figure 9. Increased phosphorylation of tau occurs with age in Tg2576/PS1^P264L cortex. Whereas concentrations of total tau are relatively constant with increasing amyloid burden (bottom blot), phosphorylated tau at thr231 increases in intensity (top blot), as does the higher molecular weight species stained with the antibody to total tau in Tg2576/PS1^P264L mice (bottom, arrow). This higher molecular weight tau species comigrates with phosphorylated tau stained with both phospho-tau antibodies used in this study. The phosphorylated tau epitope ser202 increases as well in 12-month-old Tg2576/PS1^P264L cortex, as seen in Figure 2. WT 12, Wild-type mice at 12 months of age.

Progressive neuronal loss is not present in the cortex or CA1

Neuronal cell counts were performed in the cortex (excluding piriform and entorhinal) at 12 months in both wild-type and Tg2576/PS1^P264L littermates. There were no differences in numbers of corticalneurons between these groups (WT, 1.35 × 10⁷; n = 5; Tg2576/PS1^P264L, 1.45 × 10⁷, n = 3). Neuronal counts were also performed in hippocampal CA1at 12 months in wild-type, PS1^P264L, and Tg2576/PS1^P264L littermate brains and at 2 months in wild-type and Tg2576/PS1^P264L littermates. Although there were no significant differences,there was a small reduction of 17% in neuronal number at 12 monthsin Tg2576/PS1^P264L compared with wild-type mice (Fig. 10). A similar magnitude ofreduction was present at 2 months when amyloid deposition wasvirtually undetectable in the Tg2576/PS1^P264L brains. In addition, animals with the PS1-P264L mutation alonehad an equivalent reduction at 12 months of age compared withwild type. Therefore, the small reduction in CA1 neuronal numberin this model was independent of age or amyloid deposition andmost likely attributable to a developmental reduction driven byeither the PS1-P264L mutation or the reduction in PS1 endoproteolyticcleavage products in this model (Flood et al., 2001).

View larger version (19K):
[in this window]
[in a new window]
Figure 10. Neuronal cell bodies were not lost in the hippocampal CA1 subfield at 12 months in Tg2576/PS1^P264L. Cell counts were performed in littermate brains after cresyl violet staining of Tg2576/PS1^P264L, PS1^P264L, or wild-type frozen sections. Animals were either 2 or 12 months of age. A 17% reduction in CA1 neuronal number present at 12 months in Tg2576/PS1^P264L CA1 was also present at 12 months in PS1^P264L mice and at 2 months in Tg2576/PS1^P264L mice. These data indicate that any reduction is not attributable to age/amyloid burden but may be developmental and attributable to the PS1^P264L mutation. Five subjects in each group, except for the PS1^P264L group with three subjects.

Synaptophysin is reduced with age and amyloid deposition

Synaptophysin was measured in the four littermate-controlled genotypes at 12 months as an indicator of synaptic loss or dysfunction.Synaptophysin levels were significantly reduced by 50% in theTg2576/PS1^P264L cortex at 12 months compared with wild type, whereas the PS1^P264L and Tg2576 groups demonstrated no significant reduction at thisage (Fig, 11A, top blot, B). The actin blot demonstrates comparableprotein loads per lane (Fig. 11A, bottom blot). When the same measurementswere performed in Tg2576/PS1^P264L animals at increasing ages and levels of amyloid deposition,there is a progressive loss of synaptophysin (Fig. 11C). Althoughthere is a nonsignificant reduction of 22% at 3 months, corticalsynaptophysin is significantly reduced at both 7 and 12 monthsto 60 and 40% of wild-type values, respectively.

View larger version (23K):
[in this window]
[in a new window]
Figure 11. Cortical synaptophysin is significantly reduced in aged Tg2576/PS1^P264L mice, and the reduction is genotype dependent. A, The top demonstrates 3 µg of cortical protein per sample stained with an antibody recognizing synaptophysin (Syn). At 12 months, a reduction was seen only in the Tg2576/PS1^P264L cortex compared with wild type. The bottom demonstrates approximately equivalent actin (Act) protein per well on the same blot, as a control. Graphs depict the density ratios of synaptophysin/actin. B, A 50% reduction is found in the Tg2576/PS1^P264L cortex compared with the wild-type controls at 12 months. Three subjects per group with seven immunoblot assay replicates. C, Progressive reductions in the synaptophysin/actin ratio exist at 7 and 12 months in the Tg2576/PS1^P264L mice compared with wild-type controls. Six samples per group with duplicate assays. *p $<=$ 0.05 indicates significant differences. WT 12, Wild-type mice at 12 months of age.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In this report, activation of both JNK and p38 is demonstrated in the cortex of the Tg2576/PS1^P264L mouse model of AD. A third MAP kinase family member, ERK, wasnotactivated.

JNK activation was age dependent and was associated with both amyloid deposition and tau phosphorylation. Increased phospho-JNKimmunoreactivity was detected both on Western blot and in tissuesections, despite decreased levels of total JNK. Thus, the JNKactivation was likely to be mediated by activation of an upstreamkinase. This was confirmed by an increase in the active fractionof MKK4 in the Tg2576/PS1^P264L cortex. MKK4 and MKK7 are both JNK-activating MAPK kinases, whichcan be activated by a number of MAPKK kinases, such as mixed-lineagekinase, apoptosis signal-regulating kinase-1, MAPK kinase kinase-1,and transforming growth factor- $beta$ -activated kinase-1 (Kyriakisand Avruch, 2001). MKK4 activity was increased eightfold and sixfoldat 7 and 12 months, respectively. Because the phospho-MKK4 immunostainingdid not colocalize with phospho-JNK in the neurites (data notshown) and demonstrated greater activation at 7 months comparedwith 12 months, unlike that of JNK, the direct role of MKK4 inthe neuritic JNK activation is unclear. The localization of phospho-MKK4in AD brain has not beenreported.

The species of JNK activated in this model was not determined because activation-specific reagents do not distinguish betweenJNK isoforms. Twelve isoforms result from the alternative splicingof three JNK genes, JNK1-JNK3 (Kyriakis and Avruch, 2001). Twomolecular weight forms, p54 and p46, were detected with the JNKantibodies used here. Both forms were activated in the Tg2576/PS1^P264L cortex at 12 months, although p54 exhibited 5.8-fold activationcompared with twofold for p46. JNK activation was not attributableto either the PS1-P264L mutation or the overexpression of SwAPP695alone, because cortical samples at 12 months from the individualgenotypes did not demonstrate significant activation on the blotcompared with wild-typelittermates.

JNK pathway activation in AD brain was demonstrated previously, in which levels of both phospho-JNK (Shoji et al., 2000; Zhuet al., 2001a) and c-Jun (Anderson et al., 1994, 1996) were measured.In AD, JNK activation was localized to both neuronal cell bodiesand neurites around amyloid deposits. In the Tg2576/PS1^P264L brain, JNK activation was also localized to reactive neuritescontaining phospho-tau, consistent with a role for amyloid ininducing this activation. The neuritic activation of JNK colocalizedwith increased tau phosphorylation at thr231 and ser202 in serialsections. In a cell-free system, JNK can phosphorylate tau atthese sites that are hyperphosphorylated in AD tau (Reynolds etal., 2000). In the brains of mice exposed to starvation-inducedstress, increased phospho-tau (phospho-ser202) also correlatedwith JNK activation (Planel et al., 2001). Chemical agents thatdisrupt microtubule structure can also activate JNK (Wang et al.,1998), suggesting, perhaps, that tau phosphorylation could leadto JNK activation. Interestingly, stress-activated protein kinasepathway activation colocalizes with tau pathology in a numberof neurodegenerative diseases (Atzori et al., 2001).

Consistent with JNK activation in vivo in both AD and animal model brains, treatment of primary rat cortical neurons withA $beta$ 25-35 or treatment of neuronal-like PC12 cells with A $beta$ 1-42 activatedthe JNK pathway (Bozyzcko-Coyne et al., 2001; Morishima et al.,2001; Troy et al., 2001). In addition, MKK4 activation was demonstratedboth in cell culture after treatment with toxic A $beta$ species (Bozyzcko-Coyneet al., 2001) and here in the Tg2576/PS1^P264L cortex with increased amyloid burden. Compared with the AD brainand the cell culture systems, however, there is no loss of neuronsor nuclear activation of either JNK or c-Jun in the Tg2576/PS1^P264L cortex. This lack of c-Jun activation is consistent with theabsence of neuronalloss.

c-Jun induction need not follow JNK activation. In a recent paper examining the distribution of active JNK in cerebellar granuleneurons (CbG) (Coffey et al., 2000), most of the activity wasnot involved in stress-activated gene transcription. The cytoplasmicJNK was instead developmentally upregulated during neurite outgrowthin parallel with increased MKK4/7 activity in the absence of c-Junactivation; similar biochemical changes are reported here. Also,JNK inhibition led to an increase in neurite outgrowth in theCbG. In another report using dorsal root ganglia, JNK inhibitionalso promoted the extension of neurites (Borasio et al., 1998),although JNK inhibition in NGF-induced PC12 cells was associatedwith a delay in neurite outgrowth (Maroney et al., 1999). Long-lastingJNK activation has also been reported after axotomy in the CNS(Herdegen et al., 1998) or peripheral nervous system (PNS) (Kenneyand Kocsis, 1998). JNK activation persisted for days after axotomyin both studies and was downregulated after reestablishment oftarget contact in the PNS. In both studies, despite persistentlyincreased induction of both JNK and c-Jun, there was no neuronaldeath. JNK activation may function to modulate regenerative neuriteoutgrowth after axotomy, during development, and in the neuriticresponse to amyloiddeposition.

p38 is part of a proinflammatory signal transduction pathway activated in response to a number of cytokines (Foltz et al.,1997). p38 activation increased with age and amyloid burden inthe Tg2576/PS1^P264L cortex. Like the JNK pathway, activated p38 was detected usingantibodies to phospho-specific epitopes that result from upstreamactivation by MAPK kinases, in this case, MKK3/6. The increasein phospho-p38 did not result from an increase in p38 protein,which remained stable with age. By 12 months, p38 was activatedby eightfold in the Tg2576/PS1^P264L cortex compared with wild type. The localization of phospho-p38was not determined here; however, activation of both p38 and MKK6has been localized in the AD brain to neuronal cell bodies andabnormal neurites surrounding amyloid deposits (Hensley et al.,1999; Zhu et al., 2000, 2001b). Like JNK, p38 can phosphorylatetau in a cell-free system (Reynolds et al., 2000) and was coimmunoprecipitatedwith PHF-1 tau (Zhu et al., 2000) from AD brain. In addition,cell culture experiments demonstrated p38 activation after A $beta$ treatment of primary rat microglia (McDonald et al., 1998; Pyoet al., 1998). JNK was not activated in this microglial model(McDonald et al., 1998).

There was no significant ERK activation in the Tg2576/PS1^P264L cortex. In fact, there was a significant, age-dependent reductionin the active fraction of p44 to 30% of wild-type levels by 12months. p42 was not significantly affected; however, there wasa slight increase in the active fraction at 7 months and a decreaseat 12 months. This is similar to the findings of Dineley et al.(2001) in the CA1 of Tg2576 hippocampus. They reported a subtleyet significant increase in phospho-ERK2 (p42) at 13 months inCA1 accompanied by a comparable increase in total ERK2. By 20months, levels of both total and phospho-ERK were significantlyreduced. Tg2576 animals at 20 months have a cortical amyloid burdencomparable with the Tg2576/PS1^P264L at 12 months (24%) (Flood et al., 2001). These results togethersuggest that chronic exposure to high levels of amyloid downregulateERK signaling in AD animal models. This could lead to memory deficitsbecause ERK is required for some aspects of long-term potentiation(English and Sweatt, 1997; Impey et al., 1998). ERK was activatedin the AD brain (Perry et al., 1999; Ferrer et al., 2001) andtransiently in the dentate gyrus of Tg2576 (Dineley et al., 2001).Whether this activation is present before end-stage AD isunknown.

Although neurons were not lost as a result of increased amyloid burden in our model, synaptophysin levels were reduced inan age- and genotype-dependent manner. The loss of synapses inother mouse models of A $beta$ deposition has been demonstrated previously(Hsia et al., 1999; Wong et al., 1999; Mucke et al., 2000), andthe loss of neurons was reported in two models (Calhoun et al.,1998; Hsia et al., 1999). In two studies (Hsia et al., 1999; Muckeet al., 2000), the reported reductions in synapse number likelyresulted from increased soluble A $beta$ rather than insoluble amyloidbecause the reductions were present earlier than the depositsand there was little progressive loss with increasing plaque burden.Increased soluble A $beta$ may also play a role in reducing the synaptophysin/actinratio in the Tg2576/PS1^P264L cortex; however, the loss did progress with age to 50-60% ofwild-type levels with increasing plaque burden. The role of JNKor p38 in this loss is unknown; however, the progressive lossin synaptophysin is associated with the concomitant increase inJNK and p38 activity. The behavioral and electrophysiologicalconsequences of this reduction in synaptophysin are presentlyunknown in thismodel.

The intersection of MAP kinase pathways with APP and tau biology has been suggested by the reports already mentioned and bya number of additional reports: (1) presenilin activity inhibitsJNK (Kim et al., 2001); (2) JNK phosphorylates APP (Standen etal., 2001); (3) JNK binding-inhibitory protein binds APP (Matsudaet al., 2001); and (4) Dishevelled increases APP secretion viaJNK (Mudher et al., 2001). Regarding the role of JNK and p38 inAD pathology, one possibility is that a stressor(s) activatesJNK/p38, leading to changes in APP metabolism, tau phosphorylation,synaptic/neuritic dystrophy, or glial activation. Alternatively,A $beta$ , phospho-tau, or cytokines may be the stressors that activateJNK/p38. Positive feedback loops may be present in the AD brainwhereby the initial stressor is amplified via MAP kinase pathwayactivation.

In addition to reproducing amyloid deposits and tau hyperphosphorylation in common with AD brain, the Tg2576/PS1^P264L mouse also incorporates brain activation of the JNK and p38 pathways.This reinforces the likely importance of stress-activated proteinkinase pathways in AD because pathway activation has now beendemonstrated after A $beta$ toxicity in vitro, in an AD animal model,and in the AD brain. The Tg2576/PS1^P264L mouse model of AD will allow for the testing of JNK and p38 pathwayinhibitors to determine their role in ADpathology.

  FOOTNOTES

Received Oct. 18, 2001; revised Jan. 24, 2002; accepted Feb. 5, 2002.

We thank Drs. Donna Bozyczko-Coyne and Craig Dionne for helpful comments on this manuscript, Renee Simmons and Edwin McCabefor excellent care of the animals, and James Knabb for excellenttechnicalassistance.

Correspondence should be addressed to Dr. Mary Savage, Cephalon Inc., 145 Brandywine Parkway, West Chester, PA 19380. E-mail:msavage{at}cephalon.com.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Akiyama H, Barger S, Barnum S, Bradt B, Bauer J, Cole GM, Cooper NR, Eikelenboom P, Emmerling M, Fiebich BL, Finch CE, Frautschy S, Griffin WS, Hampel H, Hull M, Landreth G, Lue L, Mrak R, Mackenzie IR, McGeer PL (2000) Inflammation and Alzheimer's disease. Neurobiol Aging 21:383-421[Web of Science][Medline].
Anderson AJ, Cummings BJ, Cotman CW (1994) Increased immunoreactivity for Jun- and Fos-related proteins in Alzheimer's disease. Exp Neurol 125:286-295[Web of Science][Medline].
Anderson AJ, Su JH, Cotman CW (1996) DNA damage and apoptosis in Alzheimer's disease: colocalization with c-Jun immunoreactivity, relationship to brain area, and effect of postmortem delay. J Neurosci 16:1710-1719[Abstract/Free Full Text].
Atzori C, Ghetti B, Piva R, Srinivasan AN, Zolo P, Delisle MB, Mirra SS, Migheli A (2001) Activation of the JNK/p38 pathway occurs in diseases characterized by tau protein pathology and is related to tau phosphorylation but not to apoptosis. J Neuropath Exp Neurol 60:1190-1197[Web of Science][Medline].
Borasio GD, Horstmann S, Anneser JMH, Neff NT, Glicksman MA (1998) CEP-1347/KT7515 a JNK pathway inhibitor, supports the in vitro survival of chick embryonic neurons. NeuroReport 9:1435-1439[Web of Science][Medline].
Bozyzcko-Coyne D, O'Kane TM, Wu ZL, Dobrzanski P, Murthy S, Vaught JL, Scott RW (2001) CEP-1347/KT-7515, an inhibitor of SAPK/JNK pathway activation, promotes survival and blocks multiple events associated with A $beta$ -induced cortical neuron apoptosis. J Neurochem 77:849-863[Web of Science][Medline].
Calhoun ME, Wiederhold KH, Abramowski D, Phinney AL, Probst A, Sturchler-Pierrat C, Staufenbiel M, Sommer B, Jucker M (1998) Neuron loss in APP transgenic mice. Nature 395:755-756[Medline].
Campion D, Flaman JM, Brice A, Hannequin D, Dubois B, Margin C, Moreau V, Charbonnier F, Didierjean O, Tardieu S, Penet C, Puel M, Pawquier F, Le Doze F, Bellis G, Calenda A, Heilig R, Martinez M, Mallet J, Bellis M (1995) Mutations of the presenilin I gene in families with early-onset Alzheimer's disease. Hum Mol Genet 4:2373-2377[Abstract/Free Full Text].
Chang L, Karin M (2001) Mammalian MAP kinase signaling cascades. Nature 410:37-40[Medline].
Coffey ET, Hongisto V, Dickens M, Davis RJ, Courtney MJ (2000) Dual roles for c-Jun N-terminal kinase in developmental and stress responses in cerebellar granule neurons. J Neurosci 20:7602-7613[Abstract/Free Full Text].
DeKosky ST, Scheff SW, Styren SD (1996) Structural correlates of cognition in dementia: quantification and assessment of synapse change. Neurodegeneration 19965:417-421.
Dineley KT, Westerman M, Bui D, Bell K, Ashe KH, Sweatt JD (2001) $beta$ -Amyloid activates the mitogen-activated protein kinase cascade via hippocampal $alpha$ 7 nicotinic acetylcholine receptors: in vitro and in vivo mechanisms related to Alzheimer's disease. J Neurosci 21:4125-4133[Abstract/Free Full Text].
English JD, Sweatt JD (1997) A requirement for the mitogen-activated protein kinase cascade in hippocampal long-term potentiation. J Biol Chem 272:19103-19106[Abstract/Free Full Text].
Ferrer I, Blanco R, Carmona M, Ribera R, Goutan E, Puig B, Rey MJ, Cardozo A, Vinals F, Ribalta T (2001) Phosphorylated map kinase (ERK1, ERK2) expression is associated with early tau deposition in neurons and glial cells, but not with increased nuclear DNA vulnerability and cell death, in Alzheimer's disease, Pick's disease, progressive supranuclear palsy, and corticobasal degeneration. Brain Pathol 11:144-158[Medline].
Flood DG, Finn JP, Walton KM, Dionne CA, Contreras PC, Miller MS, Bhat RV (1998) Immunolocalization of the mitogen-activated protein kinases p42^MAPK and JNK1, and their regulatory kinases MEK1 and MEK4, in adult rat central nervous system. J Comp Neurol 398:373-392[Web of Science][Medline].
Flood DG, Reaume AG, Dorfman KS, Lin YG, Lang DM, Trusko SP, Savage MJ, Annaert WG, De Strooper B, Siman R, Scott RW (2001) FAD mutant PS-1 gene-targeted mice: increased A $beta$ 42 and A $beta$ deposition without APP overexpression. Neurobiol Aging 23:335-348.
Foltz IN, Lee JC, Young PR, Schrader JW (1997) Hemopoietic growth factors with the exception of interleukin-4 activate the p38 mitogen-activated protein kinase pathway. J Biol Chem 272:3296-3301[Abstract/Free Full Text].
Goedert M, Hasegawa M, Jakes R, Lawler S, Cuenda A, Cohen P (1997) Phosphorylation of microtubule-associated protein tau by stress-activated protein kinases. FEBS Lett 409:57-62[Web of Science][Medline].
Gomez-Isla T, Hollister R, West H, Mui S, Growdon JH, Petersen RC, Parisi JE, Hyman BT (1997) Neuronal loss correlates with but exceeds neurofibrillary tangles in Alzheimer's disease. Ann Neurol 41:17-24[Web of Science][Medline].
Hensley K, Floyd RA, Zheng NY, Nael R, Robinson KA, Nguyen X, Pye QN, Stewart CA, Geddes J, Markesberry WR, Patel E, Johnson GVW, Bing G (1999) p38 kinase is activated in Alzheimer's disease brain. J Neurochem 72:2053-2058[Web of Science][Medline].
Herdegen T, Claret FX, Kallunki T, Martin-Villalba A, Winter C, Hunter T, Karin M (1998) Lasting N-terminal phosphorylation of c-Jun and activation of c-Jun N-terminal kinases after neuronal injury. J Neurosci 18:5124-5135[Abstract/Free Full Text].
Hsia AY, Masliah E, McConlogue L, Yu GQ, Tatsuno G, Hu K, Kholodenko D, Malenka RC, Nicoll RA, Mucke L (1999) Plaque-independent disruption of neural circuits in Alzheimer's disease mouse models. Proc Natl Acad Sci USA 96:3228-3233[Abstract/Free Full Text].
Hsiao K, Chapman P, Nilsen S, Eckman C, Harigaya Y, Younkin S, Yang F, Cole G (1996) Correlative memory deficits, A $beta$ elevation, and amyloid plaques in transgenic mice. Science 274:99-102[Abstract/Free Full Text].
Hutton M, Lendon CL, Rizzu P, Baker M, Froelich S, Houlden H, Pickering-Brown S, Chakraverty S, Isaacs A, Grover A, Hackett J, Adamson J, Lincoln S, Dickson D, Davies P, Petersen RC, Stevens M, De Graaff E, Wauters E, Van Baren J (1998) Association of missense and 5'-splice-site mutations in tau with the inherited dementia FTDP-17. Nature 393:702-705[Medline].
Impey S, Obrietan K, Wong ST, Poser S, Yano S, Wayman G, Deloulme JC, Chan G, Storm DR (1998) Crosstalk between ERK and PKA is required for Ca⁺² stimulation of CREB-dependent transcription and ERK nuclear translocation. Neuron 21:869-883[Web of Science][Medline].
Iqbal K, Grundke-Iqbal I (1996) Molecular mechanism of Alzheimer's neurofibrillary degeneration and therapeutic intervention. Ann NY Acad Sci 777:132-138[Medline].
Kenney AM, Kocsis JD (1998) Peripheral axotomy induced long-term c-Jun amino-terminal kinase-1 activation and activator protein-1 binding activity by c-Jun and JunD in adult rat dorsal root ganglia in vivo. J Neurosci 18:1318-1328[Abstract/Free Full Text].
Kim JW, Chang TS, Lee JE, Huh SH, Yeon SW, Yang WS, Joe CO, Mook-Jung I, Tanzi RE, Kim TW, Choi EJ (2001) Negative regulation of the SAPK/JNK signaling pathway by presenilin 1. J Cell Biol 153:457-463[Abstract/Free Full Text].
Kyriakis JM, Avruch J (2001) Mammalian mitogen-activated protein kinase signal transduction pathways activated by stress and inflammation. Physiol Rev 81:807-869[Abstract/Free Full Text].
Mandelkow EM, Schweers O, Drewes G, Biernat J, Gustke N, Trinczek B, Mandelkow E (1996) Structure, microtubule interactions, and phosphorylation of tau protein. Ann NY Acad Sci 777:96-106[Web of Science][Medline].
Maroney AC, Finn JP, Bozyczko-Coyne D, O'Kane TM, Neff NT, Tolkovsky AM, Park DS, Yan CYI, Tron CM, Green LA (1999) CEP-1347 (KT7515), an inhibitor of JNK activation, rescues sympathetic neurons and neuronally differentiated PC12 cells from death evoked by three distinct insults. J Neurochem 73:1901-1912[Web of Science][Medline].
Masliah E, Sisk A, Mallory M, Games D (2001) Neurofibrillary pathology in transgenic mice overexpressing V171F beta-amyloid precursor protein. J Neuropathol Exp Neurol 60:357-368[Web of Science][Medline].
Matsuda S, Yasukawa T, Homma Y, Ito Y, Niikura T, Hiraki T, Hirai S, Ohno S, Kita Y, Kawasumi M, Kouyama K, Yamamoto T, Kyriakis JM, Nishimoto I (2001) c-Jun N-terminal kinase (JNK)-interacting protein-1b/islet-brain 1 scaffolds Alzheimer's amyloid precursor protein with JNK. J Neurosci 21:6597-6607[Abstract/Free Full Text].
McDonald DR, Bamberger ME, Combs CK, Landreth GE (1998) $beta$ -Amyloid fibrils activate parallel mitogen-activated protein kinase pathways in microglia and THP1 monocytes. J Neurosci 18:4451-4460[Abstract/Free Full Text].
Moechars D, Dewachter I, Lorent K, Reverse D, Baekelandt V, Naidu A, Tesseur I, Spittaels K, Haute CV, Checler F, Godaux E, Cordell B, Van Leuven F (1999) Early phenotypic changes in transgenic mice that overexpress different mutants of amyloid precursor protein in brain. J Biol Chem 274:6483-6492[Abstract/Free Full Text].
Morishima Y, Gotoh Y, Zieg J, Barrett T, Takano H, Flavell R, Davis RJ, Shirasaki Y, Greenberg ME (2001) $beta$ -Amyloid induced neuronal apoptosis via a mechanism that involves the c-Jun N-terminal kinase pathway and the induction of fas ligand. J Neurosci 21:7551-7560[Abstract/Free Full Text].
Mucke L, Masliah E, Yu GQ, Mallory M, Rockenstein EM, Tatsuno G, Hu K, Kholodenko D, Johnson-Wood K, McConlogue L (2000) High-level neuronal expression of A $beta$ _1-42 in wild-type human amyloid protein precursor transgenic mice: synaptotoxicity without plaque formation. J Neurosci 20:4050-4058[Abstract/Free Full Text].
Mudher A, Chapman S, Richardson J, Asuni A, Gibb G, Pollard C, Killick R, Iqbal T, Raymond L, Varndell I, Sheppard P, Makoff A, Gower E, Soden PE, Lewis P, Murphy M, Golde TE, Rupniak HT, Anderton BH, Lovestone S (2001) Dishevelled regulates the metabolism of amyloid precursor protein via protein kinase C/mitogen-activated protein kinase and c-Jun terminal kinase. J Neurosci 21:4987-4995[Abstract/Free Full Text].
Perry G, Roder H, Nunomura A, Takeda A, Friedlich AL, Zhu X, Raina AK, Holbrook N, Siedlak SL, Harris PLR, Smith MA (1999) Activation of neuronal extracellular receptor kinase (ERK) in Alzheimer's disease links oxidative stress to abnormal phosphorylation. NeuroReport 10:2411-2415[Web of Science][Medline].
Planel E, Yasutake K, Fujita SC, Ishiguro K (2001) Inhibition of protein phosphatase 2A overrides tau protein kinase I/glycogen synthase kinase 3 $beta$ and cyclin-dependent kinase 5 inhibition and results in tau hyperphosphorylation in the hippocampus of starved mouse. J Biol Chem 276:34298-34306[Abstract/Free Full Text].
Pyo H, Jou I, Jung S, Hong S, Joe EH (1998) Mitogen-activated protein kinases activated by lipopolysaccharide and beta-amyloid in cultured rat microglia. NeuroReport 9:871-874[Web of Science][Medline].
Reynolds CH, Betts JC, Blackstock WP, Nebreda AR, Anderton BH (2000) Phosphorylation sites on tau identified by nanoelectrospray mass spectroscopy: differences in vitro between the mitogen-activated protein kinases ERK2, c-Jun N-terminal kinase and P38, and glycogen synthase kinase 3 $beta$ . J Neurochem 74:1587-1595[Web of Science][Medline].
Savage MJ, Iqbal M, Loh T, Trusko SP, Scott R, Siman R (1994) Cathepsin G: localization in human cerebral cortex and generation of amyloidogenic fragments from the $beta$ -amyloid precursor protein. Neuroscience 60:607-619[Web of Science][Medline].
Scheuner D, Eckman C, Jensen M, Song X, Citron M, Suzuki N, Bird TD, Hardy J, Hutton M, Kukull W, Larson E, Levy-Lehad E, Viitanen M, Peskind E, Poorkaj P, Schellenberg G, Tanzi R, Wasco W, Lannfelt L, Selkoe D, Younkin S (1996) Secreted amyloid $beta$ protein similar to that in the senile plaques of Alzheimer's disease is increased in vivo by the presenilin 1 and 2 and APP mutations linked to familial Alzheimer's disease. Nat Med 2:864-870[Web of Science][Medline].
Shoji M, Iwakami N, Takeuchi S, Waragai M, Suzuki M, Kanazawa I, Lippa CF, Ono S, Okazawa H (2000) JNK activation is associated with intracellular $beta$ -amyloid accumulation. Brain Res Mol Brain Res 85:221-233[Medline].
Siman R, Reaume AG, Savage MJ, Trusko S, Lin YG, Scott RW, Flood DG (2000) Presenilin-1 P264L knock-in mutation: differential effects on abeta production, amyloid deposition, and neuronal vulnerability. J Neurosci 20:8717-8726[Abstract/Free Full Text].
Standen CL, Brownlees J, Grierson AJ, Kesavapany S, Lau KF, McLoughlin DM, Miller CC (2001) Phosphorylation of thr(668) in the cytoplasmic domain of the Alzheimer's disease amyloid precursor protein by stress-activated protein kinase 1b (Jun N-terminal kinase-3). J Neurochem 76:316-320[Web of Science][Medline].
Sturchler-Pierrat C, Staufenbiel M (2000) Pathogenic mechanisms of Alzheimer's disease analyzed in the APP23 transgenic mouse model. Ann NY Acad Sci 920:134-139[Web of Science][Medline].
Tokuda T, Fukushima T, Ikeda S, Sekijima Y, Shoji S, Yanagisawa N, Tamaoka A (1997) Plasma levels of amyloid beta proteins Abeta1-40 and Abeta1-42(43) are elevated in Down's syndrome. Ann Neurol 4:271-273.
Tomidokoro Y, Harigaya Y, Matsubara E, Ikeda M, Kawarabayashi T, Shirao T, Ishiguro K, Okamoto K, Younkin SG, Shoji M (2001) Brain Abeta amyloidosis in APPsw mice induces accumulation of presenilin-1 and tau. J Pathol 194:500-506[Medline].
Troy CM, Rabacchi SA, Xu Z, Maroney AC, Connors TJ, Shelanski ML, Greene LA (2001) beta-Amyloid-induced neuronal apoptosis requires c-Jun N-terminal kinase activation. J Neurochem 77:157-164[Web of Science][Medline].
Wang TH, Wang HS, Ichijo H, Giannakakou P, Foster JS, Fojo T, Wimalasena J (1998) Microtubule-interfering agents activate c-Jun N-terminal kinase/stress-activated protein kinase through both Ras and apoptosis signal-regulating kinase pathways. J Biol Chem 273:4928-4936[Abstract/Free Full Text].
Wasco W, Pettingell WP, Jondro PD, Schmidt SD, Gurubhagavatula S, Rodes L, DiBlasi T, Romano DM, Guenette SY, Kovacs DM, Growdon JH, Tanzi RE (1995) Familial Alzheimer's chromosome 14 mutations. Nat Med 1:848[Web of Science][Medline].
West MJ, Gundersen HJ (1990) Unbiased stereological estimation of the number of neurons in the human hippocampus. J Comp Neurol 296:1-22[Web of Science][Medline].
West MJ, Coleman PD, Flood DG, Troncoso JC (1994) Differences in the pattern of hippocampal neuronal loss in normal ageing and Alzheimer's disease. Lancet 344:769-772[Web of Science][Medline].
Wong TP, Debeir T, Duff K, Cuello AC (1999) Reorganization of cholinergic terminals in the cerebral cortex and hippocampus in transgenic mice carrying mutated presenilin-1 and amyloid precursor protein transgenes. J Neurosci 19:2706-2716[Abstract/Free Full Text].
Zhu X, Rottkamp CA, Boux H, Takeda A, Perry G, Smith MA (2000) Activation of p38 kinase links tau phosphorylation, oxidative stress, and cell cycle-related events in Alzheimer disease. J Neuropathol Exp Neurol 59:880-888[Web of Science][Medline].
Zhu X, Raina AK, Rottkamp CA, Aliev G, Perry G, Boux H, Smith MA (2001a) Activation and redistribution of c-Jun N-terminal kinase/stress activated protein kinase in degenerating neurons in Alzheimer's disease. J Neurochem 76:435-441[Web of Science][Medline].
Zhu X, Rottkamp CA, Hartzler A, Sun Z, Takeda A, Boux H, Shimohama S, Perry G, Smith MA (2001b) Activation of MKK6, an upstream activator of p38, in Alzheimer's disease. J Neurochem 79:311-318[Web of Science][Medline].

Copyright © 2002 Society for Neuroscience 0270-6474/02/2293376-10$05.00/0

This article has been cited by other articles:

Q.-L. Ma, F. Yang, E. R. Rosario, O. J. Ubeda, W. Beech, D. J. Gant, P. P. Chen, B. Hudspeth, C. Chen, Y. Zhao, et al.
{beta}-Amyloid Oligomers Induce Phosphorylation of Tau and Inactivation of Insulin Receptor Substrate via c-Jun N-Terminal Kinase Signaling: Suppression by Omega-3 Fatty Acids and Curcumin
J. Neurosci., July 15, 2009; 29(28): 9078 - 9089.
[Abstract] [Full Text] [PDF]

G. Tang, Z. Xu, and J. E. Goldman
Synergistic Effects of the SAPK/JNK and the Proteasome Pathway on Glial Fibrillary Acidic Protein (GFAP) Accumulation in Alexander Disease
J. Biol. Chem., December 15, 2006; 281(50): 38634 - 38643.
[Abstract] [Full Text] [PDF]

M. Stagi, P. Gorlovoy, S. Larionov, K. Takahashi, and H. Neumann
Unloading kinesin transported cargoes from the tubulin track via the inflammatory c-Jun N-terminal kinase pathway
FASEB J, December 1, 2006; 20(14): 2573 - 2575.
[Abstract] [Full Text] [PDF]

M. Kitazawa, K. N. Green, A. Caccamo, and F. M. LaFerla
Genetically Augmenting A{beta}42 Levels in Skeletal Muscle Exacerbates Inclusion Body Myositis-Like Pathology and Motor Deficits in Transgenic Mice
Am. J. Pathol., June 1, 2006; 168(6): 1986 - 1997.
[Abstract] [Full Text] [PDF]

M. Kitazawa, S. Oddo, T. R. Yamasaki, K. N. Green, and F. M. LaFerla
Lipopolysaccharide-Induced Inflammation Exacerbates Tau Pathology by a Cyclin-Dependent Kinase 5-Mediated Pathway in a Transgenic Model of Alzheimer's Disease
J. Neurosci., September 28, 2005; 25(39): 8843 - 8853.
[Abstract] [Full Text] [PDF]

B. L. Kelly, R. Vassar, and A. Ferreira
{beta}-Amyloid-induced Dynamin 1 Depletion in Hippocampal Neurons: A POTENTIAL MECHANISM FOR EARLY COGNITIVE DECLINE IN ALZHEIMER DISEASE
J. Biol. Chem., September 9, 2005; 280(36): 31746 - 31753.
[Abstract] [Full Text] [PDF]

N. L. Malinin, S. Wright, P. Seubert, D. Schenk, and I. Griswold-Prenner
Amyloid-{beta} neurotoxicity is mediated by FISH adapter protein and ADAM12 metalloprotease activity
PNAS, February 22, 2005; 102(8): 3058 - 3063.
[Abstract] [Full Text] [PDF]

R. R. Nixon
Prion-associated Increases in Src-family Kinases
J. Biol. Chem., January 28, 2005; 280(4): 2455 - 2462.
[Abstract] [Full Text] [PDF]

Y.-F. Liao, B.-J. Wang, H.-T. Cheng, L.-H. Kuo, and M. S. Wolfe
Tumor Necrosis Factor-{alpha}, Interleukin-1{beta}, and Interferon-{gamma} Stimulate {gamma}-Secretase-mediated Cleavage of Amyloid Precursor Protein through a JNK-dependent MAPK Pathway
J. Biol. Chem., November 19, 2004; 279(47): 49523 - 49532.
[Abstract] [Full Text] [PDF]

S. L. Chan, W. Fu, P. Zhang, A. Cheng, J. Lee, K. Kokame, and M. P. Mattson
Herp Stabilizes Neuronal Ca2+ Homeostasis and Mitochondrial Function during Endoplasmic Reticulum Stress
J. Biol. Chem., July 2, 2004; 279(27): 28733 - 28743.
[Abstract] [Full Text] [PDF]

H. Taru and T. Suzuki
Facilitation of Stress-induced Phosphorylation of {beta}-Amyloid Precursor Protein Family Members by X11-like/Mint2 Protein
J. Biol. Chem., May 14, 2004; 279(20): 21628 - 21636.
[Abstract] [Full Text] [PDF]

Q. Wang, D. M. Walsh, M. J. Rowan, D. J. Selkoe, and R. Anwyl
Block of Long-Term Potentiation by Naturally Secreted and Synthetic Amyloid {beta}-Peptide in Hippocampal Slices Is Mediated via Activation of the Kinases c-Jun N-Terminal Kinase, Cyclin-Dependent Kinase 5, and p38 Mitogen-Activated Protein Kinase as well as Metabotropic Glutamate Receptor Type 5
J. Neurosci., March 31, 2004; 24(13): 3370 - 3378.
[Abstract] [Full Text] [PDF]

S. A. Barber, J. L. Uhrlaub, J. B. DeWitt, P. M. Tarwater, and M. C. Zink
Dysregulation of Mitogen-Activated Protein Kinase Signaling Pathways in Simian Immunodeficiency Virus Encephalitis
Am. J. Pathol., February 1, 2004; 164(2): 355 - 362.
[Abstract] [Full Text] [PDF]

S. Kins, P. Kurosinski, R. M. Nitsch, and J. Gotz
Activation of the ERK and JNK Signaling Pathways Caused by Neuron-Specific Inhibition of PP2A in Transgenic Mice
Am. J. Pathol., September 1, 2003; 163(3): 833 - 843.
[Abstract] [Full Text] [PDF]

A. M. Minogue, A. W. Schmid, M. P. Fogarty, A. C. Moore, V. A. Campbell, C. E. Herron, and M. A. Lynch
Activation of the c-Jun N-terminal Kinase Signaling Cascade Mediates the Effect of Amyloid-{beta} on Long Term Potentiation and Cell Death in Hippocampus: A ROLE FOR INTERLEUKIN-1{beta}?
J. Biol. Chem., July 18, 2003; 278(30): 27971 - 27980.
[Abstract] [Full Text] [PDF]

C. A. Marques, U. Keil, A. Bonert, B. Steiner, C. Haass, W. E. Muller, and A. Eckert
Neurotoxic Mechanisms Caused by the Alzheimer's Disease-linked Swedish Amyloid Precursor Protein Mutation: OXIDATIVE STRESS, CASPASES, AND THE JNK PATHWAY
J. Biol. Chem., July 18, 2003; 278(30): 28294 - 28302.
[Abstract] [Full Text] [PDF]

V. Waetzig and T. Herdegen
A Single c-Jun N-terminal Kinase Isoform (JNK3-p54) Is an Effector in Both Neuronal Differentiation and Cell Death
J. Biol. Chem., January 3, 2003; 278(1): 567 - 572.
[Abstract] [Full Text] [PDF]

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Web of Science (91)

Citing Articles via Google Scholar

Google Scholar

Articles by Savage, M. J.

Articles by Scott, R. W.

Search for Related Content

PubMed

PubMed Citation

Articles by Savage, M. J.

Articles by Scott, R. W.