DNA Synthesis and Neuronal Apoptosis Caused by Familial Alzheimer Disease Mutants of the Amyloid Precursor Protein Are Mediated by the p21 Activated Kinase PAK3

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The Journal of Neuroscience, July 30, 2003, 23(17):6914-6927

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DNA Synthesis and Neuronal Apoptosis Caused by Familial Alzheimer Disease Mutants of the Amyloid Precursor Protein Are Mediated by the p21 Activated Kinase PAK3
Donna L. McPhie,¹ Robert Coopersmith,⁵ Andrew Hines-Peralta,¹ Yuzhi Chen,¹ Kathryn J. Ivins,¹ Susan P. Manly,² Michael R. Kozlowski,³ Kim A. Neve,⁴ and Rachael L. Neve¹
¹Department of Psychiatry, Harvard Medical School and McLean Hospital, Belmont, Massachusetts 02478, ²Infinity Pharmaceuticals, Inc., Cambridge, Massachusetts 02139, ³Fifth Day Therapeutics, Inc., Poway, California 92064, ⁴Medical Research Service, Veterans Affairs Medical Center, Departments of Behavioral Neuroscience and Physiology and Pharmacology, Oregon Health and Science University, Portland, Oregon 97201, and ⁵Millennium Pharmaceuticals, Inc., Cambridge, Massachusetts 02139

   Abstract

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Abstract
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Materials and Methods
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Apoptotic pathways and DNA synthesis are activated in neuronsin the brains of individuals with Alzheimer disease (AD). However,the signaling mechanisms that mediate these events have notbeen defined. We show that expression of familial AD (FAD)mutants of the amyloid precursor protein (APP) in primary neuronsin culture causes apoptosis and DNA synthesis. Both the apoptosisand the DNA synthesis are mediated by the p21 activated kinasePAK3, a serine-threonine kinase that interacts with APP. Adominant-negative kinase mutant of PAK3 inhibits the neuronalapoptosis and DNA synthesis; this effect is abolished by deletionof the PAK3 APP-binding domain or by coexpression of a peptiderepresenting this binding domain. The involvement of PAK3 specificallyin FAD APP-mediated apoptosis rather than in general apoptotic pathways is suggested by the facts that a dominant-positivemutant of PAK3 does not alone cause neuronal apoptosis andthat the dominant-negative mutant of PAK3 does not inhibitchemically induced apoptosis. Pertussis toxin, which inactivatesthe heterotrimeric G-proteins G_o and G_i, inhibits the apoptosisand DNA synthesis caused by FAD APP mutants; the apoptosisand DNA synthesis are rescued by coexpression of a pertussis toxin-insensitive G_o. FAD APP-mediated DNA synthesis precedesFAD APP-mediated apoptosis in neurons, and inhibition of neuronalentry into the cell cycle inhibits the apoptosis. These datasuggest that a normal signaling pathway mediated by the interactionof APP, PAK3, and G_o is constitutively activated in neuronsby FAD mutations in APP and that this activation causes cellcycle entry and consequent apoptosis.

Key words: Alzheimer disease; apoptosis; cell cycle; amyloid precursor protein; p21 activated kinase; heterotrimeric G-proteins; APP intracellular domain

   Introduction

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Abstract
Introduction
Materials and Methods
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All individuals with Alzheimer disease (AD) experience a progressiveloss of cognitive function, resulting from selective neurodegeneration.Alzheimer disease can occur as a "sporadic" event, it can resultfrom the possession of an extra copy of chromosome 21 (Downsyndrome), or it can be caused by mutations in the amyloidprecursor protein (APP) gene on chromosome 21 or in the presenilingenes on chromosomes 1 and 14.
The mechanism by which neurons die in the disease remains tobe defined. Failure of regulation of the cell cycle has beenobserved in AD brain (for review, see Arendt, 2002). Notably,ectopic expression of cdc2, cdk4, p16, Ki-67, cyclin B1, andcyclin D has been reported in pathologically affected or vulnerableneurons in AD brain (Liu et al., 1995; Smith and Lippa, 1995;Vincent et al., 1996, 1997; Arendt et al., 1996; Vincentet al., 1996, 1997; McShea et al., 1997; Busser et al.,1998). Busser et al. (1998) found abnormal appearance of cellcycle markers in regions of AD brain where cell death is extensive,and Chow et al. (1998) found increases in expression of genesencoding cell cycle proteins in single neurons in late-stagerelative to early-stage AD brain. A number of the cell cycle regulators have been detected in vulnerable neurons before lesionformation (Kondratick and Vandre, 1996; Busser et al., 1998; Vincent et al., 1998). Patrick et al. (1999) have shown that p25, a truncated form of p35, the regulatory subunit of Cdk5,is increased in AD brain. One of the consequences of the aberrantexpression of cell cycle proteins for the neuropathology ofAD appears to be that vulnerable neurons in AD brain re-enterthe cell cycle. Yang et al. (2001) have demonstrated that a significant number of neurons in affected regions of AD brainhave undergone full or partial DNA replication, showing thatthey have completed the S phase.
Activation of cell cycle proteins in neurons can, in some cases,lead to a form of cell suicide called apoptosis (for review,see Copani et al., 2001). The notion that apoptosis contributesto the neuropathology of AD was first proposed by Su et al.(1994), when they reported evidence for DNA fragmentation inneurons in AD brain; this observation subsequently was confirmedby others. Notably, Guo et al. (1998) found that levels ofa marker of apoptosis, Par-4 (prostate apoptosis response-4)protein, are elevated in vulnerable neurons in AD brain. Inrecent years, several groups have reported the presence ofactivated caspase 3 and downstream caspases in AD brain (forreview, see Roth, 2001). These findings suggest strongly thatapoptotic pathways may be activated in AD.
Overexpression of wild-type APP in neurons causes apoptosis (Bursztajn et al., 1998; Nishimura et al., 1998; McPhie etal., 2001), and familial AD (FAD) mutants of APP cause DNAfragmentation and apoptosis in cell lines and neurons (Yamatsujiet al., 1996; Zhao et al., 1998; McPhie et al., 2001). Thesedata suggest that APP may participate in the apoptotic eventsthat have been observed in AD brain. We have used herpes simplexvirus (HSV)-mediated delivery of genes into neurons to demonstrate that FAD mutants of APP cause apoptosis in primary neurons andthat FAD APP-mediated neuronal apoptosis is more severe thanthat caused by overexpression of wild-type APP. Infection ofneurons with FAD APP viral vectors causes DNA synthesis alsoto occur in neurons. We show that both the apoptosis and theDNA synthesis are mediated by the p21 activated kinase (PAK) 3, which interacts with APP to activate these pathways. Treatmentwith pertussis toxin blocks FAD APP-mediated apoptosis andDNA synthesis, implicating G_o in the pathways as well. Sustainedexposure of neurons to a ligand mimetic for APP, the antibody22C11, causes both apoptosis and DNA synthesis. Neuronal DNAsynthesis precedes apoptosis in neurons infected with HSVFADAPP vectors; and inhibition of neuronal entry into the cellcycle inhibits the apoptosis. These data suggest the existenceof a neuronal signaling pathway involving APP, PAK3, and G_othat becomes constitutively activated and causes cell cycleentry and apoptosis after overexpression of APP or FAD mutantsof APP.

   Materials and Methods

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Abstract
Introduction
Materials and Methods
Results
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References

Plasmid construction. All plasmid constructs were made in the pHSVPr-pUC vector using standard techniques and were verifiedby sequence analysis.
Apoptosis assays. Primary cultures were plated on poly-D-lysine-coatedglass or ACLAR (Ted Pella, Inc., Redding, CA) coverslips. Fivedays after plating, neurons were infected with the appropriateviruses at a multiplicity of infection (MOI) of one per virus;16 hr later (except in the cases of HSV-C57 and HSV-C31 infections,in which the cells were processed 6 hr after infection), thecells were fixed for 20 min in freshly made 4% paraformaldehyde.Bisbenzamide assays were performed as described previously(Bursztajn et al., 1998). Ten random fields of 200-300 cellseach were analyzed for each condition. The number of cellswith condensed nuclei relative to the total number of cellsper field was calculated and expressed as a percentage. One-wayANOVA and post hoc unpaired t tests with the Bonferroni multiplecomparisons test were used for data analysis. For a number of experiments, apoptosis was also measured using the terminal deoxynucleotidyl transferase-mediated biotinylated UTP nickend labeling (TUNEL) assay, as described (Bursztajn et al.,1998). In every case, the data obtained using the TUNEL assay were identical to those obtained using bisbenzamide staining.Three replicates of each experiment were done; a representativeexperiment is shown in each figure. Cells with condensed nucleiwere deemed to be neuronal, on the basis of their morphology.
DNA synthesis assays. BrdU (Sigma, St. Louis, MO) was addedto the neuronal cultures 5 d after plating at a final concentrationof 10 µM at the time of infection with HSV vectors. Sixteenhours later (except in the cases of HSV-C57 and HSV-C31 infections,in which the cells were processed 6 hr after infection), cellswere fixed in cold 70% ethanol for 30 min and processed accordingto the protocol provided with the Zymed (San Francisco, CA)BrdU labeling kit. Ten random fields of cells were countedper condition, and the number of BrdU-positive cells was expressedas a percentage of the total number of cells. Data analysiswas performed as above. Three replicates of each experimentwere done; a representative experiment is shown in each figure.Staining of the infected cultures with an antibody to the neuron-specificantigen NeuN has shown that $~$ 20% of the cells in the culturesat the time of infection are non-neuronal and that the inductionof DNA synthesis occurs selectively in neurons (data not shown).
Antibodies and immunoblots. A goat polyclonal antibody to theN terminus of PAK3 was purchased from Santa Cruz Biotechnology(Santa Cruz, CA), and a rabbit polyclonal to mPAK3 was purchasedfrom Up-state Biotechnology (Lake Placid, NY). The polyclonalantibody 369 (Buxbaum et al., 1990) was raised against a regionfrom amino acids 645-694 of human APP-695 and was a generousgift of Dr. Sam Gandy (Farber Institute of Neuroscience, Philadelphia,PA). Antibody C8 was raised against the C terminal 20 amino acids of APP and was a generous gift of Dr. Dennis Selkoe (HarvardMedical School, Boston, MA). Anti-rab5A(S-19) and anti-rab7(C19)were from Santa Cruz. Antibody 6E10 was from Signet (Dedham,MA). Anti-rab11 was from Transduction Laboratories (Lexington,KY). The anti-myc antibody 9E10 and the anti-APP antibody 22C11were from Roche Products, Hertforshire, UK. For immunoblots demonstrating expression of transgenes from HSV vectors, infectedprimary neurons were homogenized in lysis buffer (100 mM Tris-HCl,20 mM NaCl, 10 mM EDTA, 10 mM EGTA, and 1% SDS with theseprotease inhibitors: 10 µg/ml leupeptin, 10 µg/mlaprotinin, 1 mM Na₃VO₄, 1 mM PMSF, 1 mM benzamidine, and 10mM ${beta}$ -glycerol phosphate), and proteins in the lysates were separatedby SDS-PAGE. Immunoblots were performed as described previously(McPhie et al., 1997).
Isolation of PAK3 cDNAs. ³⁵S-APP-C100 was prepared in vitroas described (Kozlowski et al., 1992), except that transcriptionand translation reagents were purchased from Ambion (Austin,TX). After the incubation, N-acetyl-D-glucosamine (Sigma, St.Louis, MO) was added to each reaction at a final concentrationof 10 mM. The ³⁵S-APP-C100 [1.2 ml lysate/50 ml binding buffer(see below)] was used as a ligand to screen a rat fetal [embryonicday 18 (E18)] brain expression cDNA library (Neve et al., 1987) in ${lambda}$ gt11. After a wash in binding buffer [in mM: 50 Tris,pH 7.7, 50 NaCl, 2 MgCl₂, and 1 dithiothreitol (DTT)], filterscontaining library proteins were incubated with ³⁵S-APP-C100at 3 n_M for 2 hr at 4°C. After three 3 min washes at 4°C,consisting of (1) binding buffer, (2) binding buffer plus 0.1%NP-40, and (3) binding buffer, filters were air-dried and exposedto X-OMAT RP film for 6-14 d. Positive plaques were isolatedand taken through six further rounds of binding and purification,yielding finally a single positive plaque-pure cDNA clone,which was used for additional screens of the cDNA library toisolate the full-length coding sequence.
Coimmunoprecipitation. Primary cortical neurons were seededat 4 x 10⁶ viable cells per dish in 60 mm poly-_D-lysine-coateddishes. Neurons were infected with the appropriate viral vectors;16 hr after infection, the cells were lysed in the followingbuffer: 50 mM Tris, pH 8.0, 100 mM NaCl, 3 mM MgCl₂, 10% glycerol,1% IGEPAL-CA630 (Sigma), and 0.5% sodium deoxycholate withthe following protease and phosphatase inhibitors: 50 mM NaF,1 mM PMSF, 10 µg/ml aprotinin, 10 µg/ml leupeptin,1 mM Na₃VO₄, 1 mM iodoacetamide, 1 mM benzamidine, and 10 mM ${beta}$ -glycerol phosphate. The lysates were homogenized in a Dounce homogenizer, 10 times on ice, and then allowed to sit on icefor 1 hr. Lysates were then centrifuged at 16,000 x g to removeinsoluble material. An aliquot from each lysate was set asidefor immunoblot analysis of protein expression. Lysates wereprecleared with protein A beads in a 1:1 slurry in lysis bufferfor 1 hr, after which antibody 369 or rabbit preimmune serumwas added, and the mixture was tumbled overnight at 4°C.Protein A was then added for 1 hr to precipitate the immunecomplexes. The immune complexes were washed three times withlysis buffer. The proteins in the samples were separated bySDS-PAGE. Immunoblots were performed as described previously(McPhie et al., 1997).
Immunocytochemistry and confocal microscopy. HSV-infected cells were fixed for 45 min in freshly made 4% paraformaldehyde, rinsedwith PBS, blocked for 30 min at room temperature in PBS with0.1% Triton X-100 and 5% normal goat serum, and incubated for2 hr at room temperature with primary antibody in PBS with5% normal goat serum. Cells were rinsed with PBS and incubatedfor 90 min at room temperature with secondary antibody (Cappel, Cochranville, PA) in PBS with 5% normal goat serum. After afinal rinse in PBS, cells on coverslips were mounted onto glassmicroscope slides using Gel/Mount (Biomeda, Hayward, CA). Omissionof the primary antibodies resulted in only nonpunctate backgroundfluorescence. Confocal images were generated using a Leica(Nussloch, Germany) TCS-NT laser confocal microscope. In double- and triple-labeling immunofluorescence experiments, bleed-throughwas controlled for by observing the absence of fluorescenceof a given fluorochrome-labeled secondary antibody when itwas illuminated using the alternative fluorochrome excitationwavelength.
Fractionation of endosomes. The fractionation of endosomes was based on the method of Seemann et al. (1997). Briefly, 10 15cm plates of primary neurons were rinsed twice with ice-coldPBS. The cells in each dish were scraped up in 1 ml of PBS,after which the cells from the 10 dishes were combined andpelleted at 1300 x g for 10 min. The pellet was resuspendedin 1.5 ml of homogenization buffer (HB) plus protease inhibitors(250 mM sucrose, 3 mM imidazole, pH 7.4, 1 mM EDTA plus 1 mMPMSF, 1 mM sodium orthovanadate, 10 µg/ml aprotinin,10 µg/ml leupeptin, 1 mM benzamidine, and 10 mM ${beta}$ -glycerolphosphate).The pellet was then homogenized 10 strokes in a Dounce homogenizerand passed three times through a 25 gauge needle. After a 1300x g spin, the postnuclear supernatant (PNS) was adjusted to40.6% sucrose, 3 mM imidazole, pH 7.4, with 62% sucrose andplaced at the bottom of a Beckman Instruments (Fullerton, CA)SW41 tube. This was overlaid successively with 4 ml 35% sucrose,3 mM imidazole, pH 7.4, 3 ml of 25% sucrose, 3 mM imidazole,pH 7.4, and 2 ml of HB. All sucrose solutions contained thesame protease inhibitor mixture as the HB. The step gradientwas centrifuged at 160,000 x g for 90 min. Bands were pulledat the following interfaces: 25%-HB (membranes enriched inlate endosomes, endosome carrier vesicles), 25-35% (membranesenriched in early endosomes), and 35-40.6% (heavy membranes).Twenty micrograms of each sample were loaded onto 10-20% Tris-glycineSDS-PAGE gels. After transfer to polyvinylidene difluoride membranes, replicate blots of the three fractions were probedwith the antibodies C-8 (1:6000), anti-mPAK3 (1:1000), anti-rab5(1:1000), and anti-rab11 (1:1000), and the blots were visualizedwith enhanced chemiluminescence as described in McPhie et al. (1997).
RNA blot analysis and in situ hybridization histochemistry.Methods for doing RNA blots have been described previously(Neve et al., 1987). For in situ hybridization histochemistry,tissues were fresh-frozen and cut in 12-µm-thick sectionson a cryostat. Sections were fixed in buffered 4% paraformaldehydefor 10 min at room temperature, rapidly air-dried, and storeddesiccated at -70°C. At the time of use, sections wereblocked with 0.1 M glycine, rinsed, and acetylated with 0.25%acetic anhydride in 0.1 M triethanolamine, pH 8.0. Sectionswere washed in 2x SSC and delipidated by treatment with ethanol and chloroform. Sections were then partially rehydrated andincubated overnight at 60°C with 10,000 cpm/µl ³⁵S-labeledriboprobes (synthesized using a template representing bp 24-230of the PAK3 cDNA) in a solution containing 50% form-amide,10% dextran sulfate, 20x Denhardt's solution, 300 µg/mlsheared salmon sperm DNA, 150 µg/ml tRNA, 2x SSC, and20 mM ${beta}$ -mercaptoethanol. After hybridization, sections weretreated with RNase A and were washed with increasing stringency(final stringency: 0.1x SSC at 60°C). Sections were dried,dipped in a 1:1 dilution of Eastman Kodak (Rochester, NY) NTB2 emulsion with water, and developed after 5 weeks. Some of thesections were exposed to Amersham Biosciences (Arlington Heights,IL) ${beta}$ Max Hyperfilm. At least four independent sets of hybridizationswere performed. Controls (not shown) included hybridizationswith sense probes.
Chemically induced apoptosis. The staurosporine and etoposide experiments were performed as described by Bursztajn et al. (1998).
Protein kinase assays. PAK kinase assays were performed as described by Joneson et al. (1998) with the following modifications.Briefly, 16 hr after infection, neurons were lysed in lysis buffer (10 mM HEPES, pH 7.5, 150 mM NaCl, 10% glycerol, 0.6%Triton X-100 plus the following protease and phosphatase inhibitors:1 mM Na₃VO₄, 50 mM NaF, 1 mM benzamidine, 1 mM PMSF, 10 µg/mlaprotinin, and 10 µg/ml leupeptin). After the lysateswere precleared with protein G (Pierce, Rockford, IL), anti-mycantibody 9E10 was added to precipitate the myc-PAKs, and thelysates were incubated overnight at 4°C with tumbling. ProteinG was then added to precipitate the immune complexes, and themixture was tumbled for 1 hr. The beads were washed four timeswith lysis buffer and once with kinase buffer (20 mM HEPES,pH 7.6, 20 mM MgCl₂, 20 mM ${beta}$ -glycerol phosphate, 0.1 mM Na₃VO₄,and 2 mM DTT). Forty microliters of final kinase mixture (20µM ATP, 10 µCi ³³P-ATP, and 3 µg of histoneH4 in kinase buffer) was added to each tube. After a 30 minincubation at 37°C, the reactions were terminated by theaddition of Laemmli Sample Buffer and were boiled for 5 min before electrophoresis on 10-20% Tris-HCl gels (Bio-Rad, Hercules,CA). The gels were fixed, dried, and exposed to film to visualizeincorporated radioactivity.
Pertussis toxin treatment. Pertussis toxin (RBI, Natick, MA)was added to the cultures at a final concentration of 100 ng/ml2 hr before infection with HSV recombinants. The constructionof a pertussis toxin-insensitive mutant of G ${alpha}$ _o (G ${alpha}$ _o^*) cDNA inwhich a serine replaces a cysteine four residues from the Cterminus has been described previously (Taussig et al., 1992).This G ${alpha}$ _o^* cDNA was generously provided by Dr. Ronald Taussig(University of Michigan, Ann Arbor, MI).
Mimosine, deferoxamine, and pan-caspase inhibitor treatment. Mimosine and deferoxamine (Sigma) were added at a final concentrationof 400 µM and 1 mM, respectively, at the time of HSV infection. BOC-Asp(OMe)-fluoromethyl ketone (Boc-D-FMK; Calbiochem,La Jolla, CA) was added at a final concentration of 50 µMat the time of infection.

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HSV-mediated expression of FAD mutants of APP causes neuronal apoptosis and DNA synthesis
We prepared replication-defective HSV vectors expressing APP-695and -751, the Swedish mutant of APP-695 (HSV-SWE695), and theV642I mutant of APP-751 (HSV-V642I-751) as described (McPhieet al., 1997). Primary E18 rat cortical cultures at 5d in vitro were infected with the viruses at an MOI of 1 per virus.Sixteen hours later, the infected cells were harvested, andtheir proteins were analyzed by immunoblot analysis to confirmequal expression of the transgenes (Fig. 1A, inset). HSV expressingEscherichia coli ${beta}$ -galactosidase (HSV-Lac) was used as a control.

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Figure 1. HSV-mediated expression of FAD mutants of APP causes neuronal apoptosis and DNA synthesis; these effects are independent of expression level. A, Quantitative analysis of APP-mediated apoptosis in neurons demonstrates that FAD APP-mediated apoptosis is significantly more severe than that mediated by wild-type APP. Data are expressed as percentages (mean ± SEM). Significant between-group differences were confirmed by a single-factor ANOVA (F_(5,53) = 32.9; p < 0.0001). Post hoc t tests were done using Bonferroni multiple comparisons test. Significant differences were seen between the following groups: 695 versus lac or mock, 695 versus SWE 695, 751 versus lac or mock, 751 versus V642I-751 (p < 0.01 for all). All other relevant comparisons were not significant (NS). The inset shows an immunoblot of expression of wild-type and FAD APPs expressed by the different HSV vectors. B, Quantitative analysis of DNA synthesis in cortical neurons expressing FAD APPs shows a significant increase in the number of BrdU-positive nuclei relative to controls. Significant between-group differences were confirmed by a single-factor ANOVA (F_(3,36) = 44.9; p < 0.0001). Post hoc t tests were done using the Bonferroni multiple comparisons test. Significant differences were seen between SWE 695 versus lac or mock and V642I-751 versus lac or mock (p < 0.001). All other relevant comparisons were NS. C, Equal titers of either high- or low-expressing HSV-APP vectors cause the same level of neuronal apoptosis 16 hr after infection. There was no significant difference in the number of condensed nuclei between cultures infected with high-expressing HSV-SWE695 or the low-expressing vector HSV-SWE695-IRESGFP (SWE695IRES). Significant between-group differences were confirmed by a single-factor ANOVA (F_(4,44) = 70.4; p < 0.0001). Post hoc t tests were done using Bonferroni multiple comparisons test. Significant differences were seen between SWE695 and lac or mock, and between SWE695-IRES and lac or mock (p < 0.001 for all comparisons). There was no significant difference in the number of condensed nuclei among the HSV-IRESGFP (IRES), HSV-Lac, and mock groups.

Cortical cells infected with the HSV vectors or mock-infectedcells were fixed 16 hr after infection, and bisbenzamide stainingwas used to detect apoptotic nuclei. The results of a representativeexperiment were quantified and are shown in Figure 1A. Cellsinfected with HSV vectors expressing the Swedish mutant ofAPP-695 or a London mutant (V642I) of APP-751 showed a significantincrease over control ( $~$ 13 and $~$ 15% apoptotic nuclei, respectively,vs $~$ 4%) in the number of apoptotic cells. Cells infected withHSV vectors expressing wild-type APP-695 or APP-751 gave anintermediate phenotype, with $~$ 9% apoptotic nuclei. This intermediateapoptotic effect of overexpression of wild-type APP is consistentwith our previous data (Bursztajn et al., 1998).
In mammalian neurons, certain types of death, including apoptosis,have been linked to the re-expression of cell cycle markers(for review, see Copani et al., 2001). Moreover, Yang et al.(2001) have demonstrated that a significant number of neuronsin vulnerable regions of AD brain have undergone full or partialDNA replication, showing that they have completed the S phase.Therefore, we tested whether FAD APPs could cause entry ofneurons into the cell cycle, as evidenced by DNA synthesis.This turned out to be the case, as shown in Figure 1B. Primary neurons were infected with HSV expressing the Swedish or theLondon mutant of APP in the presence of BrdU, and 16 hr laterthey were fixed and stained with an antibody to BrdU (Zymed).A significant increase in BrdU-positive cells is seen afterinfection with HSV-SWE695 or HSV-V642I-75 ( $~$ 40%) relative to HSV-Lac- or mock-infected controls ( $~$ 18%). To confirm that theenhancement of BrdU incorporation by FAD APP expression iscaused by DNA replication rather than DNA repair, we repeatedthe experiment in the presence or absence of cytosine arabinoside(Ara-C), a DNA replication inhibitor. In the presence of Ara-C(10 µM), which is incorporated into DNA to terminate DNA duplication, FAD APP-induced BrdU incorporation was reducedto control levels (data not shown).
Because the HSV vectors were overexpressing FAD APPs at quitehigh levels, the possibility existed that we might be causingartifactual neuronal death. To test this possibility, we createdvectors expressing FAD APPs at lower levels, to test thesevectors for their ability to cause apoptosis. We placed theFAD APP cDNAs upstream of an IRES-GFP cassette taken from theStratagene (La Jolla, CA) vector pIRES-hrGFP-2a, since we hadpreviously observed (unpublished data) reduced expression ofcDNAs cloned into that position. We infected primary corticalneurons with equal MOIs of HSV-SWE695 and HSV-SWE695-IRES-GFP,and 16 hr later we harvested the neurons for immunoblot analysis(Fig. 1C, inset). It can be seen, by comparison with the HSVlac-and mock-infected lanes (which express only endogenous APP),that the new vector conferred lower levels of expression ofAPP relative to endogenous than did the original HSV-SWE695vector (left lane). We therefore tested these constructs fortheir ability to cause neuronal apoptosis (Fig. 1C). Whenthe cultures were all infected at an MOI of 1 per virus andstained with bisbenzamide after 16 hr, the lower-expressing vectors, which expressed a level of transgene approximatelyequal to endogenous levels of APP, were shown to cause thesame degree of neuronal apoptosis as did the higher-expressingvectors. We conclude that the neuronal apoptosis caused bythe original vectors is not an artifact of high expression but reflects a specific effect of expression of FAD APP on theneurons. It is interesting that the decreased expression doesnot cause a lower level of apoptosis. We infer from these datathat a threshold level of FAD APP expression beyond endogenouswill trigger apoptosis in a given neuron and that levels ofexpression that exceed this threshold will not cause a greater number of neurons to show DNA fragmentation or nuclear condensationat this particular snapshot in time (16 hr after infection).Remember that these vectors decrease the amount of transgenethat is expressed per cell but do not decrease the numbersof neurons that are expressing the transgene, because we infectedwith an equal MOI.
The C terminus of APP interacts with PAK3
We sought to identify proteins that interacted with the intracellular C-terminal end of APP, which might mediate the apoptosis andDNA synthesis caused by FAD mutants of APP. The portion ofthe human APP cDNA encoding the C-terminal 100 amino acidsof APP (APP-C100) was used for in vitro transcription and translationas described (Kozlowski et al., 1992). The resulting radiolabeledAPP-C100 was used as a ligand to screen expression rat braincDNA libraries. Successive rounds of screening and purificationof positive clones yielded a single rat brain cDNA encodinga putative binding protein for APP-C100. The 1965 bp cDNA containeda partial (1352 bp) open reading frame followed by a presumptive3' untranslated region (3' UTR). It was used to reprobe ratbrain cDNA libraries, and numerous cDNA clones overlappingwith the original clone and extending it at the 5' end wereisolated.
At least three of these cDNAs contained a full-length codingsequence. Sequence analysis of these clones revealed a 1632bp open reading frame encoding a 544 amino acid protein identicalto the previously reported ${beta}$ -PAK (Manser et al., 1997), therat homolog of the mouse cDNA encoding mPAK-3 (Bagrodia etal., 1995); this protein is now most commonly referred to asPAK3. The putative APP binding protein is therefore a memberof the p21(Cdc42/Rac)-activated kinase (PAK) family, whichincludes the Saccharomyces cerevisiae STE20 gene product (Lebereret al., 1992; Ramer and Davis, 1993), ${alpha}$ -PAK (also known asPAK1; Manser et al., 1995), and ${gamma}$ -Pak (Teo et al., 1995), which corresponds to hPAK65 (Martin et al., 1995) and PAK2 (Jakobiet al., 1996). The greatest homology among the members of thefamily occurs in the C-terminal serine-threonine kinase domain(70% between PAK3 and STE20; >90% between PAK3 and PAK1).In addition, these kinases share, in their N-terminal domains,a peptide motif (amino acids 70-85) representing the p21-bindingdomain (Burbelo et al., 1995). The PAK proteins are activatedby the Rho family p21 proteins Cdc42 and Rac1, which participatein cytoskeletal-mediated events in the cell.
We performed solid phase binding assays to confirm the interactionof PAK3 with APP. In "pull-down" assays (Chow et al., 1996), glutathione S-transferase (GST) fusion proteins of APP-695,APP-751, and APP-C100 were immobilized on glutathione-agarosebeads and incubated with in vitro-synthesized radiolabeledPAK3. The beads were pelleted, washed, and subjected to SDS-PAGE.Autoradiograms of the gels (Fig. 2A, lanes 1-3) demonstratethe precipitation of radiolabeled PAK3 by GST-APP-695 and GST-APP-C100,but not by GST alone. GST-APP-751 also precipitated radiolabeled PAK3 (data not shown).

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Figure 2. PAK3 interacts with APP both in vitro and in vivo. A, Lanes 1-3, Precipitation of radiolabeled PAK3 by APP-695 and APP-C100 GST fusion proteins. The 61 kDa PAK3 in vitro translation product is indicated. Lane 4, Precipitation of radiolabeled C-terminal-truncated PAK3-13.5 with the APP-751-GST fusion protein. The band at 31 kDa likely represents a dimer of PAK3-13.5. B, PAK3 specifically coimmunoprecipitates with APP in neurons. Primary cortical neurons were coinfected with HSV-myc-PAK3 alone or together with HSV vectors expressing FAD APPs. Immunoprecipitations were with anti-APP antibody 369. The blot was probed with 9E10, specific for the myc epitope. The specific myc-PAK3 band immunodetected by 9E10 is indicated with an arrow and comigrates with the myc-PAK3 band in the lysate from a culture infected with HSV-SWE695+HSV-myc-PAK3. Note the absence of the band in the preimmune serum control. HSV-myc-rab5 was used as a control to demonstrate that antibody 369 does not interact with the myc tag. The bottom panel shows the expression levels of the different myc-tagged proteins in the lysates before immunoprecipitation.

The original cDNA retrieved by screening the library with APP-C100encoded amino acid residues 93-544 of PAK3, comprising a shortregion adjacent to but not including the Rac1/Cdc42 bindingdomain (residues 70-85), together with the C-terminal kinasedomain of PAK3. To determine whether the binding site for APP-C100lay in the former region, we synthesized in vitro a C-terminal-truncatedversion of PAK3 (amino acid residues 1-126, termed PAK3-13.5because of its calculated molecular mass of 13.5 kDa) that includes the Rac1/Cdc42 binding domain and the region immediately C-terminalto it but not the kinase domain. PAK3-13.5 was precipitatedby the APP-GST fusion proteins (Fig. 2A, lane 4), suggestingthat APP binds to PAK3 in the region immediately adjacent tothe Rac1/Cdc42 binding domain, between amino acid residues 93and 126.
To demonstrate a physiologically relevant interaction of APPwith PAK3 in neurons, we expressed PAK3 together with APP-695or APP-751 in rat primary cortical neurons in culture usingHSV vectors. Rat cortical cultures were coinfected with HSV-SWE695or HSV-V642I-751 and HSV-myc-PAK3 (PAK3 with an N-terminalmyc epitope), or with HSV-SWE695 or HSV-V642I-751 and an HSVvector expressing an irrelevant myc-tagged protein (myc-rab5).APP was immunoprecipitated with anti-APP antibody 369, andthe immunoprecipitated material was blotted with the anti-mycantibody 9E10 (Fig. 2B). 9E10 immunodetected a specific proteinband in the immunoprecipitated fraction (arrow) that comigrateswith myc-PAK3 in the lysate from a culture infected with HSV-SWE695+HSV-myc-PAK3(leftmost lane). This band was not detected in immunoprecipitatesfrom cultures infected with HSV-SWE695 or HSV-V642I-751 togetherwith HSV-myc-rab5. The presence of the band in cultures infectedwith HSV-myc-PAK3 alone indicates that PAK3 interacts withendogenous wild-type APP. These data suggest that PAK3 interactswith APP in cells in rat primary cortical cultures.
APP and PAK3 colocalize in rab5- and rab11-positive structures in neurons
To determine whether APP and PAK3 were present in the same subcellular compartments, we coinfected primary cultures of rat corticalneurons with HSV vectors expressing each of the two proteins.Immunocytochemical analysis of the cultures with antibodiesto APP and PAK3 revealed significant overlap in their subcellulardistributions, primarily in punctate endosome-like structures(Fig. 3). To identify the compartments in which they colocalized,we performed triple-labeling immunocytochemistry of HSV-APP-695-and HSV-PAK3-infected neuronal cultures, using APP and PAK3antibodies together with a battery of antibodies for specificcellular organelles. The greatest degree of colocalizationof APP and PAK3 (Fig. 3A) was seen in rab11-positive endosomes,which are a subset of rab5-containing endosomes (Ulrich etal., 1996; Ren et al., 1998). Subcellular fractionation ofuninfected primary cortical neurons confirmed the localizationof APP and PAK3 in the fractions that were enriched in rab11-containingendosomes (Fig. 3B). A significant but lower degree of localizationof APP and PAK3 in fractions enriched in rab5-containing endosomeswas also observed. Little colocalization was seen in the othersubcellular locations examined (data not shown).

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Figure 3. APP and PAK3 colocalize in rab5- and rab11-positive structures in neurons. A, Neuronal cultures were infected with both HSV-PAK3 and HSV-APP-695. The first column of cells represents APP immunofluorescence, the middle column PAK3 immunofluorescence, and the last column rab5, rab7, or rab11 immunofluorescence, as indicated by the row label. Note overall colocalization of APP and PAK3. Rab11 shows slightly more specific colocalization with APP than does rab5. Rab7 localization shows minimal overlap with that of APP or PAK3. Scale bar, 20 µm. B, Immunoblots of endosomal fractionation of rat brain lysates demonstrates that PAK3 and APP cofractionate into rab-11 and rab-5 positive fractions. The three lanes of each blot are designated L, E, and H: L, the membrane fraction that is enriched in late endosomes; E, the membrane fraction that is enriched in early endosomes; H, the fraction that contains heavy membranes.

PAK3 is expressed selectively in the nervous system
PAK3 mRNA is enriched in the brain in rodents (Manser et al.,1995). To determine the tissue specificity of PAK3 mRNA expressionin the human, its cDNA was used to probe an RNA blot containingRNA from a range of human fetal (20-22 week) tissues (Fig. 4A). An $~$ 11 kb mRNA was detected only in the brain, confirmingthat expression of the PAK3 gene is restricted to the nervoussystem in the human as well as in the rodent.

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Figure 4. RNA blot and in situ hybridization analyses of PAK3 gene expression in the nervous system. A, The PAK3 cDNA was used to probe an RNA blot containing RNA from a range of human fetal (20-22 week) tissues (Sp, spleen; T, thymus; M, muscle; K, kidney; Liv, liver; L, lung; SI, small intestine; H, heart; AG, adrenal gland; Br, brain). B, In situ hybridization analysis of PAK3 mRNA expression in the rat nervous system. Panels show coronal sections of adult brain (a-d), sagittal sections of adult brain (e-g), a coronal section through E18 body (h), and a low-power sagittal section of rat brain (i). a, Hippocampus with intense signal in CA1 through CA4; b, brainstem; c, temporal cortex; d, cerebral cortex with cell layer containing intense signal (arrows); e, amygdala; f, olfactory bulb; g, striatum containing dispersed, heavily labeled cells (arrows); h, spinal cord; i, sagittal section through postnatal day 21 rat brain. dg, Dentate gyrus; th, lateral dorsal thalamic nucleus; aq, aqueduct; rn, raphe nucleus; ent, entorhinal cortex; sub, subiculum; bm, basomedial amygdaloid nucleus; ah, amygdalohippocampal area; co, posterolateral cortical amygdaloid nucleus; gl, glomerular cell layer; mcl, mitral cell layer; gr, granule cell layer; sc, spinal cord; drg, dorsal root ganglion. Scale bar, 500 µm.

To localize PAK3 mRNA more precisely in the rat brain, in situhybridization was performed using an antisense riboprobe correspondingto the region of PAK3 cDNA that shares least homology withthe ${alpha}$ -PAK cDNA. Consistent with the expression of PAK3 mRNAobserved on blots, the expression of PAK3 mRNA in rat brainwas robust in some areas and restricted in others (Fig. 4i).Very high levels of PAK3 mRNA were observed in brain regionsincluding the hippocampus, amygdala, piriform and entorhinalcortex, and olfactory bulb. A robust signal was also observedin discrete brainstem nuclei, including the raphe nucleus.Moderate levels of signal were found in neocortex and thalamus. In some brain regions with an overall low level of signal, includingthe caudate nucleus, dispersed intensely labeled cells werenonetheless observed. The cerebellum was devoid of detectablesignal. Control hybridizations with sense riboprobe gave nospecific signal (data not shown).
To determine whether PAK3 mRNA was localized outside the brain, in situ hybridization of antisense PAK3 riboprobe to coronal sections of E18 rats was performed. PAK3 mRNA was found in spinal cord and dorsal root ganglia, as well as in brain (Fig. 4h),suggesting that it is expressed in both the central and peripheralnervous systems. Non-neural tissues, including gut, bone, andmuscle, were not labeled (data not shown).
Coexpression of a dominant-negative mutant of PAK3 blocks FAD APP-mediated neuronal apoptosis and DNA synthesis; this block is independent of p21 binding and is specific to PAK3
To find out whether the interaction between APP and PAK3 playsa role in FAD APP-mediated apoptosis and/or DNA synthesis,we tested the effects of dominant-negative (K297R) and dominant-positive(T421E) mutants (Sells et al., 1997) of PAK on FAD APP-inducedapoptosis and DNA synthesis. Primary rat cortical cultures at 5 d in vitro were infected with HSV vectors expressing myc-taggedPAK and the mutant PAKs; 16 hr later the infected cells wereharvested, and their proteins were analyzed by immunoblot analysisto confirm equal expression of the transgenes (Fig. 5A, inset).We then coinfected neurons with specific combinations of APPand PAK3 vectors and quantified apoptotic nuclei and BrdU incorporationin the infected neurons (Fig. 5A-C). Coexpression of the dominant-negativemutant of PAK3 (K297R) with wild-type and FAD APPs caused asignificant inhibition of APP-induced apoptosis, almost tobasal levels (Fig. 5A). Coexpression of the dominant-positivemutant of PAK3 (T421E) slightly enhanced the apoptosis causedby the Swedish mutant of APP, but did not significantly increasethe apoptosis caused by the V642I mutant of APP. Expressionof wild-type or mutant PAK3 cDNAs alone did not cause a significantchange in apoptosis relative to basal levels (Fig. 5B).

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Figure 5. Coexpression of a dominant-negative mutant (K297R) of PAK3 blocks FAD APP-mediated neuronal apoptosis and DNA synthesis. A, Quantitative analysis of condensed nuclei in neurons coinfected with HSV-SWE695 or HSV-V642I-751 and HSV vectors expressing myc-PAK3 or mutants of myc-PAK3 demonstrates that the dominant-negative mutant of PAK3, PAK3-K297R, protects against apoptosis caused by FAD mutants of APP. A dominant-positive mutant (T421E) of PAK3 enhances the apoptosis caused by FAD APPs. Wild-type PAK3 has no effect on the apoptosis caused by FAD APPs. Note that HSV-Lac was used to equalize virus amounts among the conditions. Data are expressed as percentages (mean ± SEM). The inset shows an immunoblot of expression in neurons of myc-tagged PAK3 and PAK3 mutants. Significant between-group differences were confirmed by a single-factor ANOVA (F_(9,90) = 26.4; p < 0.0001). Post hoc t tests done using the Bonferroni multiple comparisons test reveal significant differences in the number of cells with condensed nuclei between the following groups: SWE695+lac or SWE695+myc-PAK3 versus SWE695+myc-PAK3-K297R (p < 0.001), SWE695+lac versus SWE695+myc-PAK3-T421E (p < 0.05), V642I-751+ lac or V642I-751+myc-PAK3 versus V642I-751+myc-PAK3-K297R (p < 0.001), SWE695+lac or V642I-751+lac versus lac or mock (p < 0.001). All other relevant comparisons were NS. B, Expression of wild-type or mutant PAK3 alone does not result in apoptosis. Data are expressed as in A. A single-factor ANOVA showed no significant differences among the groups. C, Quantitative analysis of BrdU-positive nuclei in neurons coinfected with HSV-SWE695 or HSV-V642I-751 and HSV-myc-PAK3-K297R demonstrates a significant reduction in the number of BrdU-stained nuclei in neurons coexpressing myc-PAK3-K297R. Significant between-group differences were confirmed by a single-factor ANOVA (F_(5,53) = 41.9; p < 0.0001). Post hoc t tests done using the Bonferroni multiple comparisons test reveal significant differences in the number of BrdU-positive nuclei between the following groups: SWE695+lac versus SWE695+myc-PAK3-K297R, V642I-751+lac versus V642I-751+myc-PAK3-K297R, and SWE695+lac or V642I-751+lac versus lac or mock (p < 0.001 for all comparisons). Other relevant comparisons were NS. D, Abrogation of FAD APP-mediated apoptosis by dominant-negative PAK3 is independent of p21 binding. Dominant-negative mutants of PAK3 both with and without functional p21 binding domains both significantly decreased the number of condensed nuclei in cultures expressing SWE-695 (HSV-SWE695 added in lanes with plus signs). Significant differences were confirmed by ANOVA (F_(4,44) = 34.6; p < 0.0001). Post hoc t tests done using the Bonferroni multiple comparisons test reveal significant reductions in the number of condensed nuclei in cultures coexpressing SWE695+myc-PAK3-K297R or SWE695+myc-PAK3-K297R (no p21) versus SWE695+lac (p < 0.001). E, There is no change in in vitro PAK kinase activity after coexpression of wild-type or FAD APPs with either myc-PAK1 (top panel, lanes with plus signs) or myc-PAK3 (bottom panel, lanes with plus signs). The final lane in each panel demonstrates that the dominant-negative of each isoform of PAK is in fact kinase-dead. F, Coexpression of dominant-negative (K299R) PAK1 has the opposite effect of dominant-negative PAK3 on FAD APP-mediated apoptosis in cortical neurons, whereas coexpression of dominant-negative (K278R) PAK2 has no effect, indicating individual isoform-specific effects of PAKs on FAD APP-mediated apoptosis. Quantitative analysis of condensed nuclei in neurons coinfected with HSV-V642I-751 (lanes with plus signs) and HSV vectors expressing myc-tagged wild-type or dominant-negative PAK1, PAK2, or PAK3 demonstrates a significant reduction in condensed nuclei in neurons coexpressing wild-type myc-PAK1, but no reduction in condensed nuclei in neurons coexpressing myc-PAK1-K299R. Neither wild-type or dominant-negative PAK2 affects apoptosis mediated by V642I-751. Significant differences were confirmed by ANOVA (F_(12,116) = 28.1; p < 0.0001). Post hoc t tests done using the Bonferroni multiple comparisons test reveal significant differences in the number of condensed nuclei between V642I-751+lac versus V642-751+myc-PAK3-K297R or V642I-751+myc-PAK1 (p < 0,001). All other relevant comparisons were NS.

As described above, neuronal apoptosis caused by FAD mutantsof APP can be blocked by a dominant-negative mutant of PAK3.Can this same mutant prevent DNA synthesis caused by FAD mutantsof APP? Neurons were coinfected with HSV vectors expressingthe FAD mutants of APP together with a vector expressing PAK3in the presence of BrdU, and 16 hr later they were fixed andstained with an antibody to BrdU. The results (Fig. 5C) showthat a dominant-negative mutant of PAK3 prevents the increasein DNA synthesis caused by the FAD APPs, suggesting that entry into the cell cycle caused by FAD APPs is mediated by the samesignal transduction pathway that mediates the neuronal apoptosiscaused by FAD mutants of APP.
The APP binding site in PAK3 is adjacent to the p21 bindingsite; this raises the question of whether the binding of theRho GTPases Rac1 or Cdc42 to PAK3 modulates its functionalrole in mediating FAD APP-induced apoptosis. One way to testthis is to ask whether the protection against FAD APP-induced apoptosis afforded by PAK3 is affected by p21 binding to PAK3.We made mutated PAK3 so that leucine residues were substitutedfor two highly conserved histidine residues (his78 and his81)within the p21-binding domain. These mutations abolish bindingof PAK3 to Cdc42 or Rac1 (Sells et al., 1997). Neurons werecoinfected with HSV vectors expressing the Swedish mutant ofAPP together with a vector expressing dominant-negative PAK3(K297R) or dominant-negative PAK3 plus the mutated histidineresidues [K297R (no p21)]. The results (Fig. 5D) indicate that the inhibition of FAD APP-mediated apoptosis by PAK3 isindependent of p21 binding. Dominant-negative PAK3, eitherwith or without a functional p21 binding domain, significantlydecreased the number of condensed nuclei in cultures expressingthe Swedish mutant of APP.
The APP binding domain of PAK3 overlaps with a PAK3 autoinhibitorydomain (amino acids 78-144). Thus, one explanation for ourresults is that competition for the autoinhibitory domain ofPAK3 by APP renders PAK active. We tested this possibilityby determining whether PAK activity is influenced by APP coexpression(Fig. 5E). Neurons were infected with HSV vectors expressing myc-PAK1 or myc-PAK3, either alone or in combination with wild-typeor FAD APP. myc-PAK1 and myc-PAK3 were immunoprecipitated fromthe cell lysates and incubated with histone H4, a substratefor PAKs, in the presence of ³³P-ATP. The reactions were subjectedto SDS-PAGE, after which the gels were fixed, dried, and exposedto film to visualize incorporated radioactivity. As shown inFigure 5E, there is no change in in vitro PAK kinase activityafter coexpression of wild-type or FAD APPs with either myc-PAK1(top panel) or myc-PAK3 (bottom panel). Furthermore, note thatneither myc-PAK3(101-126), which represents the APP bindingdomain, nor myc-PAK3(78-144), which represents the PAK3 autoinhibitorydomain, affects the kinase activity of coexpressed PAK3. Notealso that these data confirm that the dominant-negative mutantsof PAK1 and PAK3 are, as expected, kinase-dead.
PAK3 is a member of a family of proteins that contains at leastsix members (for review, see Jaffer and Chernoff, 2002). Wemade dominant-negative mutants of members of the group I PAKs(PAK1, PAK2, PAK3) to test whether they also protected againstFAD APP-mediated neuronal apoptosis. Neurons were infectedwith HSV vectors expressing a London mutant (V642I) of APP-751together with wild-type or dominant-negative mutants of PAK1,PAK2, and PAK3. The results (Fig. 5F) indicate that coexpressionof dominant-negative (K299R) and wild-type PAK1 has the oppositeeffect of dominant-negative (K297R) and wild-type PAK3 on FAD APP-mediated apoptosis in cortical neurons: wild-type PAK1 protectsagainst the apoptosis, whereas dominant-negative PAK1 has noeffect on the apoptosis. Coexpression of dominant-negative(K278R) or wild-type PAK2 has no effect on FAD APP-mediatedapoptosis. These data suggest that there are individual isoform-specificeffects of PAKs on FAD APP-mediated apoptosis.
Dominant-negative PAK3 does not block chemically induced neuronal apoptosis
To ascertain whether the dominant-negative mutant of PAK3 hasa general effect on apoptotic pathways, we tested the effectof expression of K297R-PAK3 on neurons treated with the apoptosis-inducingagents etoposide and staurosporine (Fig. 6A). Both etoposideand staurosporine induced a significant increase in DNA fragmentationin cortical cells. This increase in DNA fragmentation was notprevented by coinfection with HSV expressing the dominant-negativemutant of PAK3. These data suggest either that etoposide and staurosporine act in a distinct apoptotic pathway or that theireffects on apoptosis are distal to the effect of PAK3 in thesame pathway.

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Figure 6. Expression of the PAK3 dominant-negative mutant K297R does not block chemically induced neuronal apoptosis, deletion of the APP binding site in dominant-negative (K297R) PAK3 abrogates its ability to inhibit FAD APP-mediated apoptosis, and coexpression of a peptide representing the APP binding site in PAK3 blocks FAD APP-mediated apoptosis. A, Quantitative analysis of condensed nuclei in neurons treated with staurosporine (S) or etoposide (E) and coinfected with myc-PAK3-K297R shows no significant reduction in the number of condensed nuclei as compared with neurons treated with staurosporine or etoposide alone. Data are expressed as percentages (mean ± SEM). B, Coexpression of myc-PAK3-K297R with SWE695 significantly blocks the FAD APP-mediated apoptosis. However, deletion of the APP binding site (amino acids 101-126) in PAK3-K297R abrogates its ability to inhibit the FAD APP-mediated apoptosis. Expression of myc-PAK3-K297R (del101-126) alone does not result in apoptosis (data not shown). No significant difference in the number of condensed nuclei is seen between SWE695+lac versus SWE695+ PAK3-K297R (del101-126). Coexpression of GFP- or myc-tagged APP binding site peptide PAK (101-126) with the Swedish mutant of APP-695 significantly blocked FAD APP-mediated apoptosis. Data are expressed as percentages (mean ± SEM). Significant differences were confirmed by ANOVA (F_(6.62) = 29.1; p < 0.0001). Post hoc t tests done using the Bonferroni multiple comparisons test reveal significant differences between SWE695+lac versus SWE695+myc-PAK3-K297R. Significant differences also are seen between SWE695+myc-PAK (101-126) or SWE695+GFP-PAK (101-126) versus SWE695+lac (p < 0.001 for both). The comparison of SWE695+lac versus SWE695+myc-PAK3-K297R (del101-126) was NS. All other relevant comparisons were NS. The insets show immunoblots of expression of epitope-tagged PAK (101-126) peptides and of the myc-tagged PAK3 mutations.

Binding of APP to PAK3 regulates FAD APP-induced apoptosis
We then performed a set of experiments using two different strategiesto test whether an interaction between FAD APP and PAK3 wasnecessary for FAD APP-induced apoptosis (Fig. 6B). First,a deletion of the putative APP-binding domain of PAK3 [101-126;these residues were chosen to not interfere with p21 binding to PAK3 (Zhao et al., 1998)] was introduced into the dominant-negativemutant of PAK3. This double mutant, unlike the K297R mutantalone, did not inhibit apoptosis caused by the Swedish mutantof APP-695. Then we coexpressed with the Swedish mutant of APP-695, myc- or GFP-tagged peptides representing the PAK3-binding domainof APP (101-126). Expression of the 101-126 peptide, whetherit was fused to the myc tag or to GFP, inhibited FAD APP-inducedapoptosis to the same degree that it was inhibited by expressionof the dominant-negative mutant of PAK3.
Pertussis toxin blocks FAD APP-mediated neuronal apoptosis and DNA synthesis
It has been shown that APP interacts with the G-protein G_o (Nishimoto et al., 1993; Brouillet et al., 1999), specificallyvia G ${beta}$ ${gamma}$ (Giambarella et al., 1997), and that members of theSTE20/PAK family interact with heterotrimeric G-proteins (Leeuwet al., 1998). Therefore we tested whether pertussis toxin,an inhibitor of G_o and G_i, had an effect on APP- or FAD APP-induced apoptosis (Fig. 7A). In the presence of pertussis toxin, nosignificant increase in apoptosis above basal levels was detectedin cultures infected with HSV recombinants expressing FAD (Swedish-695or V642I-751) mutants of APP. If the pertussis toxin-treatedcultures were coinfected with a pertussis toxin-insensitive mutant of G_o (G_o ${alpha}$ ptx), the apoptosis caused by the Swedish mutantof APP was partially "rescued" (Fig. 7C), suggesting thatit is the specific inhibition of G_o, rather than that of G_i,by pertussis toxin that blocks FAD APP-mediated neuronal apoptosis.Pertussis toxin inhibits not only FAD APP-mediated apoptosis,but also FAD APP-mediated DNA synthesis in neurons (Fig. 7B).These data suggest that G_o interaction with APP is essentialfor both apoptosis and DNA synthesis mediated by FAD APPs.

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Figure 7. Pertussis toxin blocks FAD APP-mediated neuronal apoptosis and DNA synthesis. This block is prevented by coexpression of a pertussis toxin-insensitive mutant (G ${alpha}$ _o^*), by deletion of the G_o binding domain of APP, or by deletion of the putative G_o binding domain of PAK3. A, Pertussis toxin (PTX) treatment of cultures infected with HSV vectors expressing FAD mutants of APP significantly reduces apoptosis to basal levels. Data are expressed as percentages (mean ± SEM). Significant differences were confirmed by ANOVA (F_(7,72) = 14.9; p < 0.0001). Post hoc t tests done using the Bonferroni multiple comparisons test reveal significant differences between SWE695 versus SWE695+PTX and between V642I-751 versus V642I-751+PTX (p < 0.001). Other relevant comparisons were NS. B, PTX treatment of cultures infected with HSV vectors expressing FAD mutants of APP significantly reduces DNA synthesis to basal levels. Data are expressed as percentages (mean ± SEM). Significant differences were confirmed by ANOVA (F_(7,71) = 34.1; p < 0.0001). Post hoc t tests done using the Bonferroni multiple comparisons test reveal significant differences between SWE695 versus SWE695+PTX and between V642I-751 versus V642I-751+PTX (p < 0.001). All other relevant comparisons were NS. C, Coexpression of the PTX-insensitive mutant G ${alpha}$ _o^* significantly prevents the PTX block of FAD APP-mediated apoptosis. Significant differences were confirmed by ANOVA (F_(3,35) = 12.3; p < 0.0001). Post hoc t tests done using the Bonferroni multiple comparisons test reveal significant differences between the following groups: SWE695+lac versus SWE695+lac+PTX and SWE695+lac+PTX versus either SWE695+G ${alpha}$ _o^* or SWE695+ G ${alpha}$ _o^*+PTX (p < 0.001). SWE695+lac versus either SWE695+G ${alpha}$ _o^* or SWE695+G ${alpha}$ _o^*+PTX were NS. D, Deletion of the G_o binding domain (amino acids 657-676) in APP or the putative G_o binding domain in PAK3 significantly blocks FAD APP-mediated apoptosis. Significant differences were confirmed by ANOVA (F_(9,88) = 18.1; p < 0.0001). Post hoc t tests done using the Bonferroni multiple comparisons test reveal significant differences between the following groups: SWE695 versus SWE695 (del657-676), V642I-751 versus V642I-751 (del657-676), SWE695+lac versus SWE695+mycPAK3 (noG_o), or V642I-751+ lac versus V642I-751+mycPAK3 (no G_o) (p < 0.001 for all comparisons). All other relevant comparisons were NS.

The G_o binding domain within APP [amino acids 657-676 usingthe numbering of APP-695, as defined by Nishimoto et al. (1993)and Lang et al. (1995)], was deleted from the Swedish andLondon mutants of APP. These mutants were expressed in neurons using HSV vectors; 16 hr after infection the neurons were fixedand stained with bisbenzamide to detect condensed nuclei. Asseen in Figure 7D, deletion of the G_o binding domain fromeither of the FAD APPs reduces their ability to cause neuronalapoptosis almost to control levels. These data suggest thatinteraction of FAD APPs with G_o is required for them to causeneuronal apoptosis and are consistent with our data demonstrating that pertussis toxin inhibits FAD APP-mediated apoptosis.
The data described thus far suggest that APP interacts withPAK3 both directly, at a region between amino acids 93 and126, and indirectly, via activation of G_o and presumably G ${beta}$ ${gamma}$ .Furthermore, it appears that both direct and indirect interactionsare necessary to get activation, because blocking either one(with a peptide representing amino acids 101-126 of PAK3 orwith pertussis toxin) prevents apoptosis. This differs fromheptahelical G-protein-coupled receptors, for which there is believed to be only the indirect, G-protein-mediated interactionbetween the receptor and the effector. The interaction betweenPAK3 and G ${beta}$ ${gamma}$ most likely occurs in the last 10-12 residues atthe C terminus of PAK3 (Leeuw et al., 1998). To test whethera direct interaction between PAK3 and G ${beta}$ ${gamma}$ is also necessary forFAD APP-mediated apoptosis to occur, we constructed a mutantof PAK3 [PAK3(del G_o)] with the last 12 amino acids deleted.This mutant should be unable to interact with G ${beta}$ ${gamma}$ . Neurons wereinfected with HSV vectors expressing FAD mutants of APP, bothalone and together with an HSV vector expressing PAK3(del G_o).Analysis of the results (Fig. 7D) showed that PAK3(del G_o)behaved in a dominant-negative manner, inhibiting the apoptosiscaused by the FAD mutants of APP. These data indicate that adirect interaction between PAK3 and G ${beta}$ ${gamma}$ is necessary for FADAPP-mediated apoptosis to occur.
Antibody 22C11, which binds to the extracellular domain of APP, causes neuronal apoptosis that is inhibited by dominant-negative PAK3
Okamoto et al. (1995) showed that an antibody to the extracellulardomain of APP (22C11) that may act as a ligand mimetic causesactivation of G_o, reinforcing the idea that APP may be a G-protein-coupledreceptor. Subsequently, Rohn et al. (2000) showed that thissame antibody induces neuronal apoptosis. We tested whether22C11-induced neuronal apoptosis activated the same signalingpathway or pathways that are activated by FAD APPs. The antibody22C11 (2 µg/ml) was added to primary neuronal culturesfor 16 hr, in the presence of HSV vectors expressing dominant-negativePAK3 (K297R) or the PAK3 APP binding domain, after which the cells were fixed and stained with bisbenzamide. Figure 8A showsthat 22C11 causes neuronal apoptosis in our paradigm and thatthis apoptosis is prevented by coexpression of mutants of PAK3that inhibit FAD APP-mediated apoptosis. 22C11 also causesDNA synthesis to occur in neurons (Fig. 8B). These data indicatethat a similar signaling pathway is activated by 22C11 as is activated by FAD mutants of APP. Whereas 22C11 could act byblocking the cell survival promoting effect of secreted formsof APP, this possibility is unlikely because we changed themedium, thereby removing secreted APP, immediately before adding22C11.

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Figure 8. Treatment of neurons with antibody 22C11 causes apoptosis and DNA synthesis and expression of C57 or C31 causes neuronal apoptosis and DNA synthesis. A, Sustained treatment of neurons with 1 µl/ml of 22C11, a ligand mimetic for APP, causes neuronal apoptosis. Expression of either myc-PAK3-K297R or peptide myc-PAK3 (101-126) significantly abrogates 22C11-mediated neuronal apoptosis. Significant differences were confirmed by ANOVA (F_(6,62) = 28.0; p < 0.0001). Post hoc t tests done using the Bonferroni multiple comparisons test reveal significant differences between the following groups: 22C11 or 22C11+lac versus 22C11+mycPAK3K297R, 22C11+mycPAK3 (101-126), 22C11 versus lac (no 22C11), mock (no 22C11) or 9E10 (p < 0.001 for all comparisons). B, Sustained treatment of cortical neurons with 22C11 leads to a significant increase in the number of neurons showing DNA synthesis. Significant differences were confirmed by ANOVA (F_(5,53) = 95.4; p < 0.0001). Post hoc t tests done using the Bonferroni multiple comparisons test reveal significant differences between the following groups: 22C11 (1 µl) or 22C11 (2 µl) versus 9E10 (1 µl), 9E10 (2 µl), lac, or mock (p < 0.001 for all comparisons), and 22C11 (1 µl) versus 22C11 (2 µl) (p < 0.01). All other relevant comparisons were NS. C, Infection of neurons with HSV vectors expressing myc-tagged C57 or C31 causes an increase in the number of apoptotic nuclei relative to infection of neurons with control HSV-Lac. Coexpression of dominant-negative PAK3 or addition of PTX causes a significant reduction in the number of apoptotic nuclei in cultures expressing myc-C57 or myc-C31. Significant differences were confirmed by ANOVA (F_(8,81) = 34.95; p < 0.0001). Post hoc t tests done using the Bonferroni multiple comparisons test reveal significant differences between the following groups: mycC57 versus mycC57+mycPAK3K297R, mycC57+PTX or lac, and mycC31 versus mycC31+mycPAK3K297R, mycC31+PTX or lac (p < 0.001 for all comparisons). Other relevant comparisons were NS. D, Expression of myc-tagged C57 or C31 leads to a significant increase in the number of neurons showing DNA synthesis. Significant differences were confirmed by ANOVA (F_(3,36) = 12.98; p < 0.0001). Post hoc t tests done using the Bonferroni multiple comparisons test demonstrated a significant increase in the number of BrdU-positive nuclei in cultures infected with HSV-myc-C57 or HSV-myc-C31 versus lac or mock (p < 0.001). Other relevant comparisons were NS.

C57 and C31 cause apoptosis that is mediated by PAK3 and G_o
We suggested previously (McPhie et al., 2001) that the C-terminal31 amino acids of APP (C31), which is generated by intracellularcaspase cleavage, is responsible for the apoptosis caused byFAD mutants of APP. Moreover, it has been shown that the APP intracellular domain (AICD) generated by ${gamma}$ -secretase cleavageof APP can cause apoptosis in neuroglioma cells (Kinoshitaet al., 2002). We asked whether apoptosis caused by C31 orC57 (one of the fragments released intracellularly by ${gamma}$ -secretasecleavage) is mediated by PAK3 and G_o. Neurons in culture wereinfected with HSV vectors expressing myc-tagged C57 or C31,alone or in combination with dominant-negative PAK3 or pertussistoxin. The results (Fig. 8C) show that both C57 and C31 directlycause neuronal apoptosis and that both forms of apoptosis areinhibited by dominant-negative PAK3 or pertussis toxin. Thus,PAK3 and G_o mediate apoptosis caused by C57 or C31. We thenasked whether C57 and C31 also caused neuronal DNA synthesis.The results (Fig. 8D) indicate that both of these fragments,when expressed ectopically in primary neurons in culture, causeDNA synthesis to occur.
FAD APP-mediated DNA synthesis precedes FAD APP-mediated apoptosis in neurons
Is FAD APP-mediated apoptosis caused by entry into the cellcycle, or is the converse true? To begin to answer this question,we treated neurons expressing FAD APPs with the cell cycleG1/S blockers mimosine and deferoxamine (Farinelli and Greene, 1996). First we tested whether these compounds block FAD APP-mediatedDNA synthesis. Neurons were infected with HSV vectors expressing the Swedish or the London mutant of APP; at the same time, mimosineor deferoxamine was added to the cultures, along with 10 µMBrdU. 16 hr later the cultures were fixed and stained withantibody to BrdU. The data in Fig. 9A show that mimosine blocksDNA synthesis completely in primary neuronal cultures. Deferoxamineinterestingly appears to block FAD APP-induced DNA synthesisbut not basal synthesis as measured in mock- or HSV-lacz-infectedcultures.

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Figure 9. FAD APP-mediated DNA synthesis precedes FAD APP-mediated apoptosis in neurons. A, The G1/S blockers mimosine and deferoxamine block the FAD APP-mediated increase in DNA synthesis in primary neuronal cultures. A significant decrease in the number of BrdU-positive nuclei is seen after treatment of HSV-FAD APP-infected cultures with either 400 µM mimosine or 1 mM deferoxamine as confirmed by ANOVA (F_(11,107) = 54.8; p < 0.0001). Post hoc t tests done using the Bonferroni multiple comparisons test reveal significant differences between the following groups: SWE695 versus SWE695+mimosine, SWE695+deferoxamine, lac or mock; V642I-751 versus V642I-751+mimosine, V642I-751+deferoxamine, lac or mock (p < 0.001). All other relevant comparisons were NS. B, The G1/S phase blockers mimosine and deferoxamine block FAD APP-mediated apoptosis. Addition of 400 µM mimosine or 1 mM deferoxamine to HSV-FAD APP-infected cortical neurons significantly blocked the FAD APP-mediated increase in condensed nuclei. Significant differences were confirmed by ANOVA (F_(11,107) = 7.3; p < 0.0001). Post hoc t tests done using the Bonferroni multiple comparisons test reveal significant differences between the following groups: SWE695 versus SWE695+mimosine, SWE695+deferoxamine, lac, or mock; and V642I-751 versus V642I-751+mimosine, V642I-751+ deferoxamine, lac or mock (p < 0.001). All other relevant comparisons were NS. C, The pan-caspase inhibitor Boc-DFMK significantly blocks FAD APP-mediated apoptosis. Significant differences were confirmed by ANOVA (F_(7,72) = 40.3; p < 0.0001). Post hoc t tests done using the Bonferroni multiple comparisons test reveal significant differences between the following groups: SWE695+DMSO versus SWE695+BocDFMK, lac+DMSO, or mock+DMSO; and V642I-751+DMSO versus V642I-751+BocDFMK, lac+DMSO or mock+DMSO (p < 0.001). All other relevant comparisons were NS. D, The pan-caspase inhibit or Boc-DFMK does not block FAD APP-mediated DNA synthesis. No significant differences in the number of BrdU-positive nuclei were seen between SWE695+DMSO versus SWE695+BocDFMK or between V642I-751+DMSO versus V642I-751+BocDFMK.

We then assessed whether these same compounds inhibited FADAPP-mediated apoptosis. As shown in Figure 9B, both mimosineand deferoxamine significantly inhibited apoptosis mediatedby the Swedish and London mutants of APP. Both compounds appearedto increase basal levels of apoptosis slightly (see the datafor mock- and HSV-LacZ-infected cultures), but significantlydecrease FAD APP-induced apoptosis. These data suggest thatblocking entry into the cell cycle inhibits neuronal apoptosiscaused by FAD APPs. Interestingly, the DNA synthesis inhibitoraphidicolin did not block neuronal apoptosis caused by FAD APPs (data not shown), implying that inhibiting DNA synthesisper se does not provide protection against apoptosis.
We then asked whether inhibition of neuronal apoptosis in HSV-FAD-APP-infectedcultures would inhibit DNA synthesis. Neurons were infectedwith HSV vectors expressing the Swedish or the London mutantof APP; at the same time, the pan-caspase inhibitor Boc-D-FMKwas added to the cultures (BrdU was also added at this timeto samples in which DNA synthesis was to be assessed). Sixteenhours later, the levels of apoptosis or DNA synthesis in thecultures were measured (Fig. 9C). As expected, the pan-caspaseinhibitor blocked neuronal apoptosis caused by the FAD APPs.In contrast, however, Boc-D-FMK had no effect on DNA synthesis caused by the Swedish and London mutants of APP (Fig. 9D).^</