Modulation of Alzheimer-Like Synaptic and Cholinergic Deficits in Transgenic Mice by Human Apolipoprotein E Depends on Isoform , Aging, and Overexpression of Amyloid beta  Peptides But Not on Plaque Formation

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The Journal of Neuroscience, December 15, 2002, 22(24):10539-10548

Modulation of Alzheimer-Like Synaptic and Cholinergic Deficits in Transgenic Mice by Human Apolipoprotein E Depends on Isoform , Aging, and Overexpression of Amyloid $beta$ Peptides But Not on Plaque Formation
Manuel Buttini¹, Gui-Qiu Yu¹, Kristina Shockley¹, Yadong Huang¹, Brian Jones¹, Eliezer Masliah³, Margaret Mallory³, Tracy Yeo²^,⁴, Frank M. Longo²^,⁴, and Lennart Mucke¹^,²
¹ Gladstone Institute of Neurological Disease, and ² Department of Neurology, University of California, San Francisco, California 94141-9100, ³ Departments of Neurosciences and Pathology, University of California at San Diego, La Jolla, California 92093-0624, and ⁴ Veterans Affair's Medical Center, San Francisco, California 94121

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The most frequent human apolipoprotein (apo) E isoforms, E3 and E4, differentially affect Alzheimer's disease (AD) risk (E4> E3) and age of onset (E4 < E3). Compared with apoE3, apoE4 promotesthe cerebral deposition of amyloid $beta$ (A $beta$ ) peptides, which arederived from the amyloid precursor protein (APP) and play a centralrole in AD. However, it is uncertain whether A $beta$ deposition intoplaques is the main mechanism by which apoE isoforms affect AD.We analyzed murine apoE-deficient transgenic mice expressing intheir brains human APP (hAPP) and A $beta$ together with apoE3 or apoE4.Because cognitive decline in AD correlates better with decreasesin synaptophysin-immunoreactive presynaptic terminals, cholineacetyltransferase (ChAT) activity, and ChAT-positive fibers thanwith plaque load, we compared these parameters in hAPP/apoE3 andhAPP/apoE4 mice and singly transgenic controls at 6-7, 12-15,and 19-24 months of age. Brain aging in the context of high levelsof nondeposited human A $beta$ resulted in progressive synaptic/cholinergicdeficits. ApoE3 delayed the synaptic deficits until old age, whereasapoE4 was not protective at any of the ages analyzed. Old hAPP/apoE4mice had more plaques than old hAPP/apoE3 mice, but synaptic/cholinergicdeficits preceded plaque formation in hAPP/apoE4 mice. Moreover,despite their different plaque loads, old hAPP/apoE4 and hAPP/apoE3mice had comparable synaptic/cholinergic deficits, and these deficitswere found not only in the hippocampus but also in the neocortex,which in most mice contained no plaques. Thus, apoE3, but notapoE4, delays age- and A $beta$ -dependent synaptic deficits througha plaque-independent mechanism. This difference could contributeto the differential effects of apoE isoforms on the risk and onsetofAD.

Key words: acetylcholine; aging; Alzheimer's disease; amyloid; apolipoprotein E; cholinergic; neurodegeneration; synapses; transgenic

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Alzheimer's disease (AD) is an age-dependent neurodegenerative disorder that is characterized by a progressive cognitive declineand by characteristic morphological CNS alterations, includingdeposition of amyloid $beta$ peptides (A $beta$ ) in parenchymal plaques andcerebral blood vessels; intraneuronal formation of neurofibrillarytangles; and loss of neuronal subpopulations, synaptophysin-immunoreactive(SYN-IR) presynaptic terminals, and cholinergic fibers (Terryet al., 1999). Different gene products have been implicated inthe pathogenesis of this disease. Early-onset autosomal dominantforms of familial AD (FAD) have been linked to mutations in genesencoding amyloid precursor protein (APP), presenilin 1, and presenilin2 (Selkoe, 2001). Mutations in these genes alter the processingof APP such that increased amounts of either total A $beta$ or A $beta$ endingat residue 42 (A $beta$ 42) are produced (Selkoe, 2001).

Although mutations in APP or presenilin genes account for only a fraction of AD cases, inheritance of the apolipoprotein (apo)E $epsilon$ 4 allele is the major known genetic risk factor for the mostcommon type of AD (Farrer et al., 1997). ApoE is a 34 kDa lipidcarrier protein that participates in the maintenance and repairof neurons (Mahley and Huang, 1999). It is expressed at high levelsin the brain and can be produced by diverse cell types, includingneurons, astrocytes, and microglia (Boyles et al., 1985; Stoneet al., 1997; Buttini et al., 1999; Xu et al., 1999, 2000; Dekroonand Armati, 2001). In humans, apoE occurs in three major isoforms,which are associated with different risks of developing AD (E4> E3 > E2) (Corder et al., 1993; Farrer et al., 1997). The twomost frequent isoforms differ not only in their effects on A $beta$ deposition (E4 > E3) (Rebeck et al., 1993; Schmechel et al., 1993;Berr et al., 1994; Heinonen et al., 1995; Hyman et al., 1995;Gearing et al., 1996; Ishii et al., 1997; Johnson et al., 1998;McNamara et al., 1998; Holtzman et al., 2000a,b) but also in theircapacity to protect the brain against diverse injuries, includingthose elicited by excitotoxins, ischemia, and trauma (E3 > E4)(Sheng et al., 1998; Buttini et al., 1999, 2000; Horsburgh etal., 2000; Sabo et al., 2000). Although any or all of these effectsmight play a role in AD, some studies have suggested that themain effect of apoE isoforms is through plaque formation (Holtzmanet al., 2000a,b), whereas others have provided evidence for plaque-independentmechanisms (Raber et al., 2000).

Differentiating whether AD-related neuronal deficits are caused by plaques, A $beta$ fibrils, or nonfibrillar A $beta$ species is an importantconundrum in AD research (Klein et al., 2001). Human A $beta$ is neurotoxicwhen added to cultures of neural cells or tissue sections (Pikeet al., 1993; Yankner, 1996; Klein et al., 2001), injected intothe brain (Geula et al., 1998), or produced in neurons of transgenicmice (Games et al., 1995; Masliah et al., 1996, 2001; Nalbantogluet al., 1997; Calhoun et al., 1998; Price et al., 1998; Hsia etal., 1999; Mucke et al., 2000). However, both in vitro and invivo, A $beta$ can exist in diverse conformational states. Which ofthese states is responsible for the dysfunction and degenerationof neurons in AD remains a matter of active study and debate (Terry,1996; Davis and Chisholm, 1997; Hartley et al., 1999; Hsia etal., 1999; Lue et al., 1999; McLean et al., 1999; Mucke et al.,2000; Näslund et al., 2000; Klein et al., 2001). Both depositedand nondeposited forms of A $beta$ might contribute to the pathogenesisof AD, but their relative contributions have been difficult todissect, both in humans and in experimental models. Although neuriticdystrophy appears to be closely linked to plaques (Knowles etal., 1999), evidence is mounting that AD-related synaptic degenerationand functional neuronal impairments may be caused primarily bynondeposited forms of A $beta$ (Lambert et al., 1998; Hartley et al.,1999; Holcomb et al., 1999; Hsia et al., 1999; Lue et al., 1999;McLean et al., 1999; Mucke et al., 2000; Raber et al., 2000; Kleinet al., 2001).

To investigate the effects of apoE isoforms on AD-related deficits in vivo and, in particular, the possible relationship betweenthe development of such deficits and the amyloidogenic effectof apoE4, we analyzed transgenic mice expressing human APP (hAPP)/A $beta$ in combination with either apoE3 or apoE4 in the brain. We focusedour analysis on SYN-IR presynaptic terminals, choline acetyltransferase(ChAT) activity, and cholinergic fibers, because decreases inthese parameters correlate well with cognitive decline in AD (Terryet al., 1991; Samuel et al., 1997; Sze et al., 1997; Brown etal., 1998). ChAT synthesizes the neurotransmitter acetylcholine(ACh) and is produced by cholinergic neurons clustered in a numberof cell groups in the basal forebrain (Cummings, 2000). Its activityis 40-90% lower in AD brains than in control brains, and thisreduction correlates with cognitive decline (Perry et al., 1978;Davies, 1979; Wilcock et al., 1982; Sims et al., 1983; Neary etal., 1986; Bierer et al., 1995; Samuel et al., 1997; Cummings,2000).

In mice, lack of murine apoE or expression of human A $beta$ in the presence of murine apoE is also associated with age-dependentsynaptic and cholinergic deficits (Games et al., 1995; Gordonet al., 1995; Masliah et al., 1995a,b, 1996, 2001; Buttini etal., 1999, 2000; Hsia et al., 1999; Mucke et al., 2000). However,these models did not allow an analysis of potential interactionsbetween human A $beta$ and human apoE. In the current study, we analyzedhAPP/apoE3 and hAPP/apoE4 mice that express human A $beta$ in the contextof human apoE and therefore more closely simulate the situationencountered in the humanbrain.

Previous studies of hAPP/apoE transgenic mice focused primarily on amyloid deposition and plaque-related pathology (Holtzmanet al., 1999, 2000a,b) but did not examine effects of human apoEisoforms on other AD-related deficits, such as loss of SYN-IRpresynaptic terminals, ChAT activity, or cholinergic fibers. Theresults we obtained in the current study suggest that apoE3 butnot apoE4 can delay some age- and A $beta$ -dependent neuronal deficitsthrough a plaque-independent neuroprotectivemechanism.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animals. The generation of murine apoE-deficient transgenic mice expressing FAD-mutant hAPP, directed by the platelet-derivedgrowth factor (PDGF) B chain promoter (line J9), in combinationwith either apoE3 or apoE4, directed by the neuron-specific enolase(NSE) promoter, has been described previously (Raber et al., 1998,2000; Buttini et al., 1999; Hsia et al., 1999; Mucke et al., 2000).For the current study, we used a total of 102 mice, bred to be>95% C57BL/6J. Six genotypes and three age groups were analyzed(Table 1). Each genotype and age group contained approximatelythe same number of males and females. No significant differenceswere identified between age- and genotype-matched male and femalemice with respect to any of the endpoints analyzed. Mice wereanesthetized with chloral hydrate and flush-perfused transcardiallywith 0.9% saline. Brains were removed and divided sagitally. Onehemibrain was postfixed in phosphate-buffered 4% paraformaldehyde,pH 7.4, at 4°C for 48 hr for vibratome sectioning. The neocortex,hippocampus, and medial septum were dissected from the other hemibrainon ice, frozen immediately on dry ice, and stored at $-$ 70°C untilanalysis.


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Table 1. Relative levels of SYN-IR presynaptic terminals in transgenic mice

A $beta$ measurements. Frozen brain tissues were homogenized in guanidine buffer, and human A $beta$ peptides were quantitated by ELISAas described previously (Johnson-Wood et al., 1997). The A $beta$ 1-42ELISA detects only A $beta$ 1-42, whereas the A $beta$ 1-x ELISA detects A $beta$ 1-40,A $beta$ 1-42, A $beta$ 1-43, and C-terminally truncated forms of A $beta$ containingamino acids 1-28.

Immunohistochemistry for A $beta$ was performed on 50 µm free-floating vibratome sections of paraformaldehyde-fixed brain tissue.Endogenous peroxidase activity was quenched by incubating sectionsin 3% H₂O₂ in PBS with 0.5% Triton X-100 for 20 min. To blocknonspecific binding sites, sections were incubated for 1 hr atroom temperature in 15% goat serum (Vector Laboratories, Burlingame,CA). Sections were then incubated overnight at 4°C with a 1:6000dilution of R1282 antibody (gift from D. Selkoe, Brigham and Women'sHospital, Boston, MA). Sections were then washed twice in PBSand incubated for 1 hr with a 1:200 dilution of biotin-labeledanti-rabbit as a secondary antibody (Vector Laboratories). Secondaryantibody binding was detected with the ABC Elite kit (Vector Laboratories)using diaminobenzidine and H₂O₂ as chromagenic substrates. A $beta$ -immunoreactivedeposits were visualized by bright-field microscopy with a 4×objective and photographed with an Axiocam digital camera (Zeiss,Weimar,Germany).

Although the A $beta$ antibody detects both diffuse and fibrillar amyloid deposits, thioflavin-S (thio-S) detects primarily fibrillaramyloid and, hence, is widely used to detect more mature amyloidplaques (Schmidt et al., 1995). Thio-S-positive amyloid plaqueswere visualized in 50 µm vibratome sections with a staining protocoladapted from Schmidt et al. (1995). Briefly, sections were mountedonto SuperFrost glass slides (Fisher Scientific, Houston, TX)and air-dried. After fixation for 10 min in 3.7% formalin, theywere rinsed twice in PBS and immersed in 0.25% KMnO₄ in PBS for10 min. After another rise in PBS, they were immersed for 5 minin a solution containing 2% K₂O₅S₂ and 1% oxalic acid. After a10 min rinse in water, sections were incubated for 10 min in a0.015% thio-S solution in 50% ethanol, differentiated in 50% ethanol,washed in water, air-dried, and coverslipped. Sections were examinedby confocal microscopy (MRC 1024 or Radiance 2000; Bio-Rad, Hercules,CA) with an FITC filter set. Digitized images were transferredto a computer, and the average percentage area of the hippocampusoccupied by thio-S-positive plaques in three to four sectionsper mouse (plaque load) was determined with NIHImage.

ApoE measurements. ApoE levels in brain tissues were quantitated by Western blot analysis as described previously (Huang etal., 1996, 2001). Briefly, brain tissues were homogenized in 0.3ml of ice-cold lysis buffer containing 50 mM Tris/HCl, pH 8.0,150 mM NaCl, 4% SDS, 1% Nonidet P-40, 1% sodium deoxycholate,and protease inhibitors. After determination of protein concentrationsby the Lowry method, samples (100 µg total proteins per lane)were subjected to SDS-PAGE and analyzed by Western blotting withan anti-human apoE antibody. Sample bands were compared with standardscontaining different amounts of recombinant human apoE3 or apoE4by densitometricanalysis.

ApoE immunohistochemistry was performed on 50 µm vibratome sections. Endogenous peroxidase was quenched by incubation in 3%H₂O₂/10% methanol in PBS for 15 min, and nonspecific binding siteswere blocked with a mixture of 10% rabbit serum, 1% nonfat drymilk, 0.2% gelatin, and 0.2% Triton X-100. Anti-apoE (Calbiochem,San Diego, CA) was diluted 1:28,000, and biotin-labeled anti-goatsecondary antibody was diluted 1:200. Secondary antibody bindingwas detected with the ABC Elite kit (Vector Laboratories) usingdiaminobenzidine and H₂O₂ as chromagenic substrates. The specificityof this immunostain has been documented previously (Buttini etal., 1999). Photomicrographs were taken with an AxioCam digitalcamera (Zeiss) coupled to an Olympus Optical (Tokyo, Japan) BX-60microscope.

SYN-IR presynaptic terminals. Vibratome sections (n = 2 per mouse) labeled first with an anti-synaptophysin monoclonal antibody(diluted 1:40; Boehringer Mannheim, Mannheim, Germany) and thenwith an FITC-coupled anti-mouse antibody (diluted 1:75; VectorLaboratories) were imaged, essentially as described previously(Buttini et al., 1999), with a Radiance 2000 laser scanning confocalmicroscope mounted on an Olympus BX-60 microscope using a 60×oil objective. Sections were assigned code numbers to ensure objectiveassessment, and codes were not broken until the analysis was complete.The density of SYN-IR presynaptic terminals was assessed in thestrata radiatum and lacunosum of the hippocampus (CA1 subfield)and in layers 2-5 of the frontoparietal neocortex. For each mouse,we analyzed three to four optical sections of the stratum radiatumand the stratum lacunosum and four to six optical sections oftheneocortex.

Staining of sections with antibody dilutions that are either too high or too low can obscure differences between experimentaland control groups, yielding false negative results. To avoidthis problem, we injected wild-type mice with saline or kainateas described previously (Buttini et al., 1999) and performed pilotexperiments to determine the dilutions of primary and secondaryantibodies at which differences in the intensity of synaptophysinimmunostaining between these groups were maximal. The optimizedantibody dilutions were then used for the current study as describedabove. To further ensure the reliability of our quantitations,for each experiment, we first determined the linear range of fluorescenceintensity and density of SYN-IR presynaptic terminals in sectionsfrom wild-type mice (data not shown). This setting of the confocalmicroscope was then used to collect all images analyzed in thesame experiment. The density of SYN-IR presynaptic terminals wasexpressed as percentage of the image area occupied by immunoreactivestructures of defined signal intensity. Digitized images weretransferred to a computer (Apple Computers, Cupertino, CA) andanalyzed with the public domain program NIH Image. As reviewedrecently (Buttini et al., 1999), the above approach has been usedsuccessfully in various experimental models of neurodegenerationand diseased human brain and has been validated by comparisonswith quantitative immunoblots, ELISAs, and the optical disectorprobe.

ChAT activity and immunoreactivity. ChAT activity in the medial septum of 3-10 mice per genotype was determined by previouslydescribed procedures (Yeo et al., 1997). Medial septum tissuewas sonicated in 50 mM Tris/0.2% Triton X-100 buffer, pH 7.4 (diluted1:20, wet w/v), and centrifuged at maximum speed in an Eppendorfcentrifuge. The supernatant was transferred to another tube, andsoluble protein levels were determined by bicinchoninic acid assay(Pierce, Rockford, IL). Samples from each mouse were diluted 1:5with 50 mM Tris/0.5 M sodium-phosphate buffer, pH 7.0, to a finalvolume of 50 µl, mixed with 50 µl of reaction buffer (0.4 M NaCl,80 µg/ml eserine, 12 mM choline chloride, 10 µg/ml albumin, and0.05 µCi ¹⁴C-labeled acetyl CoA in Na-phosphate buffer), and incubated at37°C for 30 min. Background readings for each mouse were obtainedby boiling duplicate tissue samples for 5 min before mixing themwith the reaction buffer. Reactions were stopped with 500 µl ofice-cold H₂O and loaded onto a column with 1 inch of Dowex 1X-Abeads (Bio-Rad). Columns were washed twice with 600 µl of H₂O,and all of the column effluents were collected and counted ona Beckman (Fullerton, CA) scintillation counter. The amount ofACh synthesized was calculated and expressed as nanomoles permilligram of protein perhour.

Immunohistochemistry for ChAT was performed on 50 µm free-floating vibratome sections of paraformaldehyde-fixed brain tissue.Endogenous peroxidase activity was quenched by incubating sectionsin 3% H₂O₂ in PBS with 0.5% Triton X-100 for 20 min. To blocknonspecific antibody binding, sections were incubated for 15 minin Superblock (Scytek, Logan, UT). Sections were then incubatedovernight at 4°C with anti-ChAT antibody (diluted 1:3500; Chemicon,Temecula, CA). Sections were then washed twice in PBS and incubatedfor 1 hr with biotin-labeled anti-goat secondary antibody (diluted1:200; Vector Laboratories). Secondary antibody binding was detectedwith the ABC Elite kit using diaminobenzidine and H₂O₂ as chromagenicsubstrates. For all sections, the development reaction was stoppedafter 2 min by transferring the sections into 0.1 M Tris, pH 7.5.After two washes in the same buffer, sections were mounted, air-dried,and coverslipped. Digitized images of the immunostained sectionswere obtained with a DEI-450 Optronics digital camera (Coleta,CA) mounted on a BX-60 microscope (Olympus Optical) using a 20×magnification lens, and the integrated optical density of theimmunoperoxidase product over defined areas was quantitated withthe BioQuant Image Analysis package (R& M Biometrics, Nashville,TN). For each mouse, three to four measurements per brain regionwere obtained and averaged. Four to seven animals were analyzedper group. Dilutions of primary and secondary antibodies and developmenttimes for the chromagenic reaction were optimized in pilot experimentsto maximize the reliability of the immunostain (see also above).To further standardize our measurements, control sections fromthe same three wild-type mice (two sections per mouse) were includedin each staining experiment, and all sections were processed andmeasured under similar conditions. Measurements in experimentalmice were expressed as the percentage of integrated optical densityreadings obtained in corresponding regions of the wild-type controlsections.

Statistical analyses. Statistical analyses were performed with the StatView 5.0 program (SAS Institute, Cary, NC). Differencesamong means were assessed by Mann-Whitney U test or by one-wayANOVA followed by Tukey-Kramer post hoc test asappropriate.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Generation of hAPP/apoE doubly transgenic mice lacking murine apoE

To study the influence of human apoE isoforms on AD-related neuropathological alterations, we bred murine apoE-deficient PDGF-hAPPtransgenic mice from line J9 (Hsia et al., 1999; Mucke et al.,2000; Raber et al., 2000) (hAPP mice) with murine apoE-deficientNSE-apoE mice (apoE mice) that express apoE3 or apoE4 in the brainat levels similar to those in human cortex (Buttini et al., 1999).These crosses yielded six groups of mice, all of which lackedmurine apoE (Apoe^/): doubly transgenic mice (hAPP/apoE3 or hAPP/apoE4), singly transgenicmice (hAPP, apoE3, or apoE4), and mice lacking human transgenes.ApoE3 and apoE4 singly transgenic mice show similar levels anddistributions of human apoE in the brain (Raber et al., 1998;Buttini et al., 1999), and 6-month-old hAPP/apoE3 and hAPP/apoE4mice have comparable levels of A $beta$ 1-42 and A $beta$ 1-x (approximatestotal A $beta$ ) in the hippocampus (Raber et al., 2000). In the currentstudy, we made similar observations (data not shown) and extendedthese findings to another brain region and an older age group(Fig. 1).

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Figure 1. Comparable levels of human A $beta$ and apoE in brain tissues of hAPP/apoE3 and hAPP/apoE4 mice. A-E, Snap-frozen neocortex from 12- to 15-month-old hAPP/apoE3 mice and hAPP/apoE4 mice (n = 4-7 per genotype) was homogenized and analyzed for human A $beta$ 1-x or A $beta$ 1-42 by ELISA and for human apoE by quantitative Western blot analysis. hAPP/apoE3 (open bars) and hAPP/apoE4 (filled bars) mice had comparable A $beta$ 1-x levels (A), A $beta$ 1-42 levels (B), A $beta$ 1-42/A $beta$ 1-x ratios (C), and apoE levels (D). Values in A-D represent group means ± SEM. E depicts a representative Western blot demonstrating similar apoE levels in hAPP/apoE3 mice (lanes 1-6) and hAPP/apoE4 mice (lanes 7-10). F-H, The distribution of human apoE in the hippocampus of 12- to 15-month-old mice was determined by anti-apoE immunoperoxidase staining of paraformaldehyde-fixed vibratome sections in a hAPP/apoE3 mouse (F) and a hAPP/apoE4 mouse (G). An Apoe^/ mouse served as a control (H). Scale bar, 400 µm (applies to F-H).

ApoE3 but not apoE4 delays the age-dependent decline in SYN-IR presynaptic terminals in hAPP mice expressing high levels of soluble human A $beta$

On the murine apoE wild-type background, hAPP mice develop an age-dependent loss of SYN-IR presynaptic terminals that is associatedwith major deficits in synaptic transmission strength (Hsia etal., 1999; Mucke et al., 2000). To detect potential apoE isoform-specificeffects on age-related synaptic impairments in the context ofhuman A $beta$ production, we determined the levels of SYN-IR presynapticterminals in the neocortex (layers 2-5, frontoparietal region)and hippocampus (strata radiatum and lacunosum) by computer-assistedconfocal image analysis. Six genotypes were analyzed at threeage ranges (Table 1).

On the murine apoE-deficient background, hAPP mice also developed an age-related decline in SYN-IR presynaptic terminals inall three brain regions analyzed (Fig. 2). ApoE3 significantlydelayed this decline, whereas apoE4 did not (Table 1, Figs. 2,4). At 6-7 (neocortex) and 12-15 (neocortex and hippocampus) monthsof age, hAPP/apoE3 mice had higher levels of SYN-IR presynapticterminals than hAPP/apoE4 mice, hAPP mice, or Apoe^/ mice lacking human transgenes (Table 1, Figs. 2, 4). The levelsof SYN-IR presynaptic terminals in hAPP/apoE3 mice at these ageswere normal (i.e., similar to those of age-matched wild-type controlswithout human transgenes) (Masliah et al., 1995b; Buttini et al.,1999, 2000; Hsia et al., 1999; Mucke et al., 2000) (data not shown).The levels of SYN-IR presynaptic terminals in hAPP/apoE4 micewere abnormally low and comparable to those in age-matched hAPPmice with or without murine apoE expression and to those in Apoe^/ mice lacking human transgenes (Fig. 2) (Masliah et al., 1995b;Buttini et al., 1999, 2000; Hsia et al., 1999; Mucke et al., 2000).

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Figure 2. Age-related changes in presynaptic terminals of apoE singly transgenic (left) and hAPP/apoE doubly transgenic (right) mice lacking murine apoE. Littermates expressing neither human nor murine apoE served as additional controls. The density of SYN-IR presynaptic terminals in the strata radiatum and lacunosum of the hippocampus and in the neocortex was determined by confocal microscopy and computer-assisted image analysis. ApoE4 mice and hAPP/apoE4 mice showed a significant loss of SYN-IR presynaptic terminals at 12-15 and 19-24 months in all three brain regions. Like nontransgenic, wild-type (Apoe^+/+) mice (Buttini et al., 1999, 2000) (data not shown), apoE3 mice had no significant age-dependent loss of SYN-IR presynaptic terminals. In hAPP/apoE3 mice, the loss of SYN-IR presynaptic terminals was delayed until 19-24 months of age, when it was comparable to that in age-matched hAPP/apoE4 mice. ApoE-deficient mice with or without hAPP/A $beta$ expression developed an age-related loss of SYN-IR presynaptic terminals similar to that of apoE4 or hAPP/apoE4 mice. Results represent means ± SEM; n = 4-7 mice per genotype and age range; *p < 0.05, age-matched mice expressing apoE3 versus apoE4 (Tukey-Kramer test).

Although apoE3 was able to protect hAPP/apoE3 mice against synaptic deficits at 6-7 and 12-15 months of age, it failed todo so at 19-24 months of age (Table 1, Figs. 2, 4). By 19-24months of age, levels of SYN-IR presynaptic terminals had declinedto similar levels in hAPP/apoE3 and hAPP/apoE4 mice (Figs. 2,4). In the absence of hAPP/A $beta$ , apoE3 was able to protect eventhe oldest murine apoE-deficient mice against synaptic deficits(Fig. 2). In contrast, apoE4 failed to protect against synapticdeficits at all ages tested, compared with apoE-deficient controlswith or without hAPP/A $beta$ expression (Table 1, Fig. 2).

ApoE3 protects murine apoE-deficient mice against age-dependent cholinergic deficits but only if they do not produce human A $beta$

To investigate the effect of apoE isoforms on ChAT in the presence or absence of human A $beta$ , we analyzed ChAT activity in themedial septum, which contains cell bodies of ACh-producing neurons,and ChAT-IR fibers in the neocortex and hippocampus, which containcholinergic terminals. Murine apoE-deficient mice developed anage-dependent loss of ChAT activity and ChAT-IR fibers that wasprevented by apoE3 but not by apoE4 (Fig. 3). However, this protectiveeffect of apoE3 was not seen in mice expressing high levels ofhuman A $beta$ , consistent with results obtained in hAPP mice expressingwild-type murine apoE (Boncristiano, 2002). Both hAPP/apoE4 andhAPP/apoE3 mice showed a comparable age-dependent loss of ChATactivity and ChAT-IR fibers (Figs. 3, 4).

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Figure 3. Age-related changes in ChAT activity (top row) and ChAT-IR fibers (bottom rows) in apoE singly transgenic (left) and hAPP/apoE doubly transgenic (right) mice lacking murine apoE. Littermates expressing neither human nor murine apoE served as additional controls. ChAT activity was measured in the medial septum. Levels of ChAT-IR fibers in the strata radiatum and lacunosum of the hippocampus and in the neocortex were expressed as percentage of corresponding levels in nontransgenic, wild-type (Apoe^+/+) control mice. Compared with apoE3 mice, apoE4 mice showed a loss of ChAT activity and ChAT-IR fibers at 12-15 and 19-24 months of age but not at 6-7 months of age. hAPP/apoE mice showed an age-related loss of ChAT regardless of whether they expressed apoE3 or apoE4. Age-related losses of ChAT in apoE-deficient mice with or without hAPP expression were similar to those in apoE4 mice. Results represent means ± SEM; n = 3-10 (ChAT activity) and n = 4-7 (ChAT-IR fibers) mice per genotype and age range; *p < 0.05, age-matched mice expressing apoE3 versus apoE4 (Tukey-Kramer test). ChAT activity measurements for one 19-month-old apoE3 mouse and one 12-month-old apoE4 mouse were excluded from the statistical analysis because they were well outside of the range of the other values.

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Figure 4. Age-dependent progression of neuropathological alterations in hAPP/apoE3 and hAPP/apoE4 mice. SYN-IR presynaptic terminals (stratum lacunosum) and ChAT-IR fibers (strata lacunosum and radiatum) of defined signal intensity were measured in the hippocampus. Age-dependent decreases in SYN-IR presynaptic terminals developed later in hAPP/apoE3 mice than in hAPP/apoE4 mice. Thio-S-positive plaques and A $beta$ -IR deposits in the hippocampus were detected only in the oldest age group, with more deposits found in hAPP/apoE4 mice than in hAPP/apoE3 mice. Note that 12- to 15-month-old hAPP/apoE4 mice had decreased levels of SYN-IR presynaptic terminals and ChAT-IR fibers but no amyloid deposits, and that 19- to 24-month-old hAPP/apoE4 mice had a larger amyloid burden than hAPP/apoE3 mice (Fig. 5), although at this age both groups had comparable decreases in SYN-IR presynaptic terminals and ChAT-IR fibers (Figs. 2, 3). Scale bars: top row, 30 µm; second row, 65 µm; third row, 250 µm; fourth row, 400 µm.

The effects of apoE3 and apoE4 on synaptic deficits in hAPP/apoE mice are not attributable to their differential effects on plaque formation

To assess the age-dependent formation of amyloid plaques, we stained brain sections of murine apoE-deficient hAPP/apoE3 mice,hAPP/apoE4 mice, and hAPP mice with thio-S. No thio-S-positiveplaques were detected at 6-7 and 12-15 months of age in any ofthese mice (Figs. 4, 5). By 19-24 months of age, numerous plaqueswere found in the hippocampus of hAPP/apoE4 mice (Figs. 4, 5),whereas only few plaques were detected in the hippocampus of age-matchedhAPP/apoE3 mice (Figs. 4, 5) or hAPP mice lacking apoE (data notshown). Plaques were most numerous in the stratum lacunosum inhAPP/apoE4 mice and almost completely restricted to this regionin hAPP/apoE3 mice (Fig. 4). Thio-S-positive plaques were detectedin the neocortex in one of seven hAPP/apoE4 mice and none of eighthAPP/apoE3 mice (data not shown).

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Figure 5. Age-dependent formation of thio-S-positive plaques in the hippocampus of hAPP/apoE mice. Brain sections were stained with thio-S and imaged by confocal microscopy (FITC filter setting). The hippocampal area occupied by thio-S-positive plaques was determined (y-axis on left, solid symbols and lines). Thio-S-positive amyloid plaques were detected only in the 19-24 month age group. hAPP/apoE4 mice had a significantly higher plaque load than hAPP/apoE3 mice. Results represent means ± SEM; n = 4-7 mice per genotype and age range; *p < 0.05 by Mann-Whitney U test. Synaptophysin data (stratum lacunosum) from Figure 2 were superimposed (y-axis on right, open symbols and dashed lines) to highlight that the differential effects of apoE isoforms on plaques and SYN-IR presynaptic terminals occur at different ages.

To detect amyloid deposits that might be too diffuse to stain with thio-S, we stained brain sections of hAPP/apoE3 and hAPP/apoE4mice with a polyclonal anti-A $beta$ antibody (R1282). Like thio-S-positiveplaques, A $beta$ -IR deposits were detected only at 19-24 months ofage but not at 6-7 or 12-15 months of age (Fig. 4). A $beta$ -IR depositswere detected primarily in the strata radiatum, oriens, and lacunosumof the hippocampus and were more numerous and dense in hAPP/apoE4mice than in hAPP/apoE3 mice (Fig. 4). Only two of seven hAPP/apoE4and none of eight hAPP/apoE3 had A $beta$ -IR deposits in the neocortex(data notshown).

Notably, at 12-15 months of age, hAPP/apoE4 mice already had a significant loss of SYN-IR presynaptic terminals and ChAT-IRfibers in the stratum lacunosum, although they had not yet formedplaques or diffuse amyloid deposits (Figs. 2-5). In 19- to 24-month-oldhAPP/apoE4 mice, plaque load did not correlate with levels ofSYN-IR presynaptic terminals or ChAT-IR fibers (Spearman's rankcorrelation). Furthermore, hAPP/apoE3 and hAPP/apoE4 mice showedmarked differences in plaque load in the stratum lacunosum at19-24 months of age but very similar losses of SYN-IR presynapticterminals and ChAT-IR fibers (Table 1, Figs. 2-5). hAPP/apoE3 andhAPP/apoE4 mice showed an age-dependent decline in SYN-IR presynapticterminals and ChAT-IR fibers in the neocortex (Figs. 2, 3), althoughA $beta$ -IR deposits were detected in this region in only two hAPP/apoE4mice and thio-S-positive plaques were detected in only one hAPP/apoE4 mouse (data not shown). Lastly, no A $beta$ -IR deposits or plaqueswere found in the medial septum and nucleus basalis magnocellularis(data not shown), which give rise to the ChAT-IR fibers of theneocortex and hippocampus,respectively.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The current study demonstrates that brain aging in the context of high levels of nondeposited human A $beta$ is associated witha progressive loss of SYN-IR presynaptic terminals, ChAT activity,and ChAT-IR fibers. The pace of the synaptic but not of the cholinergicdecline was critically influenced by which isoform of human apoEwas expressed in the brain. ApoE3 delayed the synaptic declineuntil old age, whereas apoE4 had no significant protective effectson synapses at any of the ages analyzed. Because synaptic deficitscorrelate well with the development of cognitive deficits in AD(DeKosky and Scheff, 1990; Terry et al., 1991; Langlais et al.,1993; Samuel et al., 1997; Sze et al., 1997; Brown et al., 1998),the differential effects of apoE3 and apoE4 identified here mightrelate closely to the effects of these isoforms on AD risk (E4> E3) and age of onset (E4 < E3) (Corder et al., 1993; Farreret al., 1997).

Studies of AD brains have identified a higher plaque burden in people with apoE4 than in people with apoE3 (Berr et al., 1994;Heinonen et al., 1995; Hyman et al., 1995; Ishii et al., 1997;Johnson et al., 1998; McNamara et al., 1998), and these observationshave been confirmed in transgenic models expressing these humanapoE isoforms in astrocytes (Holtzman et al., 2000a,b) or neurons(this study). These associations have widely been interpretedas evidence that apoE4 increases AD risk through its effect onamyloid deposition (Holtzman et al., 2000a,b; Selkoe, 2001). However,there are several reasons to consider alternativepossibilities.

ApoE4 accelerates AD onset and worsens age-related neuronal decline during the early stages of aging but appears to have relativelylittle impact on the severity and progression of neuronal deficitsin old age and during later stages of AD (Farrer et al., 1997;Bookheimer et al., 2000; Greenwood et al., 2000; Small et al.,2000; Yaffe et al., 2000; Caselli et al., 2001; Chapman et al.,2001; Reiman et al., 2001). In contrast, the effect of apoE4 onamyloid deposition is most prominent in advanced age, both inhumans (Berr et al., 1994; Heinonen et al., 1995; Hyman et al.,1995; Ishii et al., 1997; Johnson et al., 1998; McNamara et al.,1998) and in transgenic mice (Holtzman et al., 2000a,b) (thisstudy). ApoE4 increases the plaque burden not only in people withAD but also in nondemented individuals (Berr et al., 1994), underliningthe potential dissociation between its effects on amyloid depositionand AD risk/onset. ApoE3 and apoE4 have differential effects onA $beta$ -dependent memory deficits in hAPP/apoE transgenic mice wellbefore these mice develop amyloid deposits (Raber et al., 2000).Studies in human AD cases and in hAPP transgenic mice have demonstratedthat AD-related synaptic and functional neuronal deficits correlatebetter with levels of nondeposited A $beta$ than with plaque load (Holcombet al., 1999; Hsia et al., 1999; Lue et al., 1999; McLean et al.,1999; Mucke et al., 2000; Raber et al., 2000). In addition, severalrecent studies of people with one or two APOE $epsilon$ 4 alleles but withoutovert AD revealed decreased brain activity, decreased visual attention,and subtle memory impairments in $epsilon$ 4 carriers compared with peoplewith other APOE alleles (Caselli et al., 1999; Bookheimer et al.,2000; Greenwood et al., 2000; Small et al., 2000; Reiman et al.,2001). These findings lend support to the notion that the criticaleffects of apoE isoforms on AD risk precede the clinical manifestationof AD by many years and, hence, are most likely independent ofthe prominent plaque formation that occurs during the later stagesof theillness.

In the current study, we also detected a higher plaque load in old hAPP/apoE4 mice than in old hAPP/apoE3 mice. However, severalfindings suggest that this difference does not account for thedifferential effects of apoE isoforms on age- and A $beta$ -dependentsynaptic and cholinergic decline. First, loss of SYN-IR presynapticterminals and ChAT-IR fibers in hAPP/apoE4 mice clearly precededplaque formation. Second, old hAPP/apoE3 and hAPP/apoE4 mice hadcomparable synaptic and cholinergic deficits but markedly differentplaque loads. Third, the age-dependent loss of SYN-IR presynapticterminals and ChAT-IR fibers also affected the neocortex, whichwas mostly devoid of plaques and A $beta$ deposits. Thus, it is likelythat a plaque-independent mechanism accounts for the differentialneuroprotective effects observed in ourstudy.

At 12-15 months of age, neocortical levels of SYN-IR presynaptic terminals were significantly lower in hAPP/apoE4 mice thanin hAPP/apoE3 mice, although these groups had similar levels ofhuman A $beta$ 1-x, A $beta$ 1-42, and apoE in the neocortex. Thus, the differencein synaptic integrity in hAPP/apoE3 and hAPP/apoE4 mice was notcaused by differences in the abundance of these transgene products.Neuroprotective activities of apoE3 that might allow it to delayage- and A $beta$ -dependent synaptic deficits include promotion of neuriteextension (Nathan et al., 1994; Holtzman and Fagan, 1998) andsynapse formation (Mauch et al., 2001), stabilization of microtubules(Strittmatter et al., 1994; Nathan et al., 1995) and endosomal-lysosomalmembranes (Ji et al., 2002), and protection against oxidativestress (Miyata and Smith, 1996). Additional studies are neededto determine which of these mechanisms is most important in relationto age- and A $beta$ -dependent neuronal deficits in vivo.

Like the neuronal deficits identified in the current study, behavioral deficits in hAPP/apoE4 mice were seen in both malesand females (Raber et al., 2000). In contrast, behavioral deficitsin singly transgenic mice expressing apoE4 in the absence of hAPP/A $beta$ were seen only in females (Raber et al., 1998, 2000). Recent findingssuggest that endogenous androgens protect singly transgenic malemice against apoE4-dependent behavioral deficits, and that thisprotection is relative rather than absolute (Raber et al., 2002).

Although apoE4 failed to prevent the age-dependent synaptic and cholinergic decline that occurs in murine apoE-deficient mice(with or without A $beta$ expression), it did not worsen it. This findingmay be consistent with a loss of neuroprotective functions ofapoE4 compared with apoE3. However, it could also reflect thegain of an adverse activity that counteracts or interferes withbeneficial activities of the holoprotein (Raber et al., 1998,2000; Tolar et al., 1999; Buttini et al., 2000; Huang et al.,2001). The 112_CysArg substitution, which differentiatesapoE4 from apoE3, affects many aspects of apoE, including itsconformation, stability, and binding to lipids and other molecules(Dong and Weisgraber, 1996; Ji et al., 1998; Huang et al., 2001;Raffaï et al., 2001). Determining whether these or other factorsaccount for the lack of neuroprotective effects of apoE4 and itsrole in AD is an importantobjective.

Interestingly, overexpression of human A $beta$ failed to further augment the age-related synaptic and cholinergic deficits in micelacking apoE. This finding may be consistent with the notion thatthe formation of neurotoxic A $beta$ species depends on the associationof A $beta$ with "pathological molecular chaperones," such as apoE andapoJ (Wisniewski and Frangione, 1992; Oda et al., 1995; Ma etal., 1996; Permanne et al., 1997). In the presence of murine apoE(Hsia et al., 1999; Mucke et al., 2000; Masliah et al., 2001)or human apoE (this study), A $beta$ clearly did affect the integrityor function of presynaptic terminals and cholinergic neurons.Here, A $beta$ interfered with the ability of apoE3 to prevent lossof SYN-IR presynaptic terminals in the oldest group of mice andto prevent loss of ChAT-IR fibers at all agesanalyzed.

It is interesting to speculate how these results might relate to findings obtained in epidemiological and clinicopathologicalstudies in humans. As in our mouse models, the differential effectsof apoE3 and apoE4 on the development of AD manifestations wereapparent primarily during early but not late stages of the agingprocess (Farrer et al., 1997; Bookheimer et al., 2000; Greenwoodet al., 2000; Small et al., 2000; Yaffe et al., 2000; Chapmanet al., 2001; Reiman et al., 2001). The therapeutic effect ofacetylcholinesterase inhibitors during early stages of AD suggestsan early impairment of cholinergic functions (Cummings, 2000;Nakano et al., 2001), and there is evidence that the responsivenessto these compounds is influenced by apoE genotype (Farlow et al.,1998). However, biochemical and neuropathological alterationsof the cholinergic system have been detected primarily in laterstages of the disease, and their modification by apoE isoformsremains controversial (Poirier et al., 1995; Soininen et al.,1995; Allen et al., 1997; Arendt et al., 1997; Salehi et al.,1998; Gilmor et al., 1999; Bronfman et al., 2000; Corey-Bloomet al., 2000; Tiraboschi et al., 2000; Sjögren et al., 2001).Some of the reported discrepancies probably reflect genuine differencesin the brain regions, AD populations, or disease models analyzed,but technical differences may also play a role (see MaterialsandMethods).

In conclusion, apoE3 and apoE4 have differential effects not only on amyloid deposition and plaque-associated neuritic dystrophybut also on AD pathologies that appear to be primarily plaqueindependent, particularly loss of SYN-IR presynaptic terminals.Differences in the ability of these apoE isoforms to protect thebrain against nondeposited toxic A $beta$ species could contribute totheir effects on AD risk and onset. Drugs that simulate apoE3activities or convert apoE4 into a molecule with apoE3-like functionmight delay both plaque-dependent and plaque-independent neuronaldeficits in the many APOE $epsilon$ 4 carriers afflicted with or at riskforAD.

  FOOTNOTES

Received April 17, 2002; revised Aug. 29, 2002; accepted Sept. 4, 2002.

This work was supported by National Institutes of Health Grants AG11385 and NS41787 and by a Zenith Award (99-1847) from theAlzheimer's Association. We thank D. Selkoe for the 1282 antibody,J. Carroll and S. Gonzales for preparation of graphics, G. Howardand S. Ordway for editorial assistance, and D. McPherson for administrativeassistance.

Correspondence should be addressed to Dr. Lennart Mucke, P.O. Box 419100, San Francisco, CA 94141. E-mail: lmucke{at}gladstone.ucsf.edu.

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