Cholinergic Changes in the APP23 Transgenic Mouse Model of Cerebral Amyloidosis

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The Journal of Neuroscience, April 15, 2002, 22(8):3234-3243

Cholinergic Changes in the APP23 Transgenic Mouse Model of Cerebral Amyloidosis
Sonia Boncristiano¹^,^*, Michael E. Calhoun¹^,^*, Peter H. Kelly², Michelle Pfeifer¹, Luca Bondolfi¹, Martina Stalder¹, Amie L. Phinney¹, Dorothee Abramowski², Christine Sturchler-Pierrat², Albert Enz², Bernd Sommer², Matthias Staufenbiel², and Mathias Jucker¹
¹ Neuropathology, Institute for Pathology, University of Basel, CH-4003 Basel, Switzerland, and ² Novartis Pharma AG, Nervous System Research, CH-4002 Basel, Switzerland

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Alzheimer's Disease (AD) is a neurodegenerative disorder that is characterized by extracellular deposits of amyloid- $beta$ peptide(A $beta$ ) and a severe depletion of the cholinergic system, althoughthe relationship between these two events is poorly understood.In the neocortex, there is a loss of cholinergic fibers and receptorsand a decrease of both choline acetyltransferase (ChAT) and acetylcholinesteraseenzyme activities. The nucleus basalis of Meynert (NBM), whichprovides the major cholinergic input to the neocortex, undergoesprofound neuron loss in AD. In the present study, we have examinedthe cholinergic alterations in amyloid precursor protein transgenicmice (APP23), a mouse model of cerebral $beta$ -amyloidosis. In agedAPP23 mice, our results reveal modest decreases in cortical cholinergicenzyme activity compared with age-matched wild-type mice. Totalcholinergic fiber length was more severely affected, with 29 and35% decreases in the neocortex of aged APP23 mice compared withage-matched wild-type mice and young transgenic mice, respectively.However, there was no loss of cholinergic basal forebrain neuronsin these aged APP23 mice, suggesting that the cortical cholinergicdeficit in APP23 mice is locally induced by the deposition ofamyloid and is not caused by a loss of cholinergic basal forebrainneurons. To study the impact of cholinergic basal forebrain degenerationon cortical amyloid deposition, we performed unilateral NBM lesionsin adult APP23 mice. Three to 8 months after lesioning, a 38%reduction in ChAT activity and significant cholinergic fiber losswere observed in the ipsilateral frontal cortex. There was a 19%decrease in A $beta$ levels of the ipsilateral compared with contralateralfrontal cortex with no change in the ratio of A $beta$ 40 to A $beta$ 42. Weconclude that the severe cholinergic deficit in AD is caused byboth the loss of cholinergic basal forebrain neurons and locallyby cerebral amyloidosis in the neocortex. Moreover, our resultssuggest that disruption of the basal cholinergic forebrain systemdoes not promote cerebral amyloidosis in APP23 transgenicmice.

Key words: Alzheimer's disease; APP; amyloid; basal forebrain; cholinergic system; ChAT; AChE; neurodegeneration; nucleus basalis of Meynert; neocortex; lesion; mouse; stereology; hippocampus; aging

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Alzheimer's disease (AD) is a progressive neurodegenerative disorder that affects a large proportion of elderly people. Althoughgenetic factors seem to strongly contribute to disease susceptibility,only a small number of cases are caused by dominant mutations(Selkoe, 1999). To date, all such mutations alter processing ofthe amyloid precursor protein (APP), leading to changes in theproduction or fibrillization of amyloid- $beta$ (A $beta$ ), the major constituentof amyloid plaques found in AD brain (Hardy, 1997; Selkoe, 1997;Haass and Steiner, 2001).

Besides the extracellular deposition of A $beta$ , the AD brain is characterized by intracellular neurofibrillary tangles and profoundchanges in the cholinergic system (Bartus et al., 1982; Coyleet al., 1983; Goedert, 1993). In both neocortex and hippocampusof AD brain, a loss of cholinergic fibers and terminals, decreasesin cholinergic receptors and/or signal transduction, and significantreductions in choline acetyltransferase (ChAT) and acetylcholinesterase(AChE) enzyme activities have been reported (Coyle et al., 1983;Perry et al., 1992; Ransmayr et al., 1992; Bierer et al., 1995;Jope et al., 1997; Geula et al., 1998; Ladner and Lee, 1998).

The major cholinergic innervation to the cerebral cortex originates from the nucleus basalis of Meynert (NBM), together withthe horizontal limb of the diagonal band of Broca, the ventralpallidum, the magnocellular preoptic area, the substantia innominata,and the nucleus of the ansa lenticularis (hereafter referred toas the NBM complex). Cholinergic innervation to the hippocampusis mainly provided by the medial septum (MS) and the verticallimb of the diagonal band of Broca (VDB) (McKinney et al., 1983;Gaykema et al., 1990; Kitt et al., 1994). In AD brain, a profoundloss of these cholinergic basal forebrain neurons has been reported(Whitehouse et al., 1982; Vogels et al., 1990; Jope et al., 1997;Cullen and Halliday, 1998). This neuron loss may be caused secondarilyas a result of A $beta$ neurotoxicity to the cholinergic terminals followedby retrograde degeneration. Alternatively, degeneration of cholinergicbasal forebrain neurons may be the primary lesion with subsequentloss of cortical cholinergicinnervation.

The relationship between cerebral amyloidosis and cholinergic depletion in AD remains poorly understood (Roberson and Harrell,1997; Auld et al., 1998; Geula et al., 1998). It has been demonstratedthat stimulation of muscarinic acetylcholine receptor subtypesincreases non-amyloidogenic APP processing (Nitsch et al., 1992).It has also been reported that AChE accelerates the assembly ofA $beta$ into insoluble amyloid fibrils (Inestrosa et al., 1996). Accordingly,dysfunction of the cholinergic system may influence cerebral amyloidosis.Vice versa, it has been demonstrated that A $beta$ is neurotoxic tocholinergic neurons and that low concentrations of A $beta$ can directlyinhibit cholinergic signaling (Auld et al., 1998; Pettit et al.,2001). Thus, increased A $beta$ levels may contribute physiologicallyand/or pathologically to the cholinergic changes in ADbrain.

Several APP transgenic mouse models have been generated that exhibit age-related A $beta$ deposition in plaques and vessels predominantlyin the neocortex and hippocampus (Games et al., 1995; Hsiao etal., 1996; Sturchler-Pierrat et al., 1997). The amyloid depositsdisplay major characteristics of human AD plaques and human cerebralamyloid angiopathy including congophilic A $beta$ cores, amyloid-associatedcell death, dystrophic neurites, activated microglia, and reactiveastrocytes (Masliah et al., 1996; Frautschy et al., 1998; Calhounet al., 1999; Phinney et al., 1999; Stalder et al., 1999; VanDorpe et al., 2000; Winkler et al., 2001; Bondolfi et al., 2002).These mouse models offer the opportunity to study cholinergicalterations that result from, or lead to, cerebral amyloidosis.To this end we have used biochemical and morphological techniquesto assess cholinergic changes in neocortex and basal forebrainof APP23 transgenic mice. Moreover, to test the hypothesis thatcortical cholinergic depletion has an effect on amyloid plaqueformation we have lesioned the NBM in APP23mice.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animals. The generation of the B6,D2-TgN(Thy1-APP_Swe) transgenic mouse line (APP23) is described elsewhere (Sturchler-Pierratet al., 1997). In brief, APP₇₅₁ cDNA with the Swedish mutation(K670N-M671L) was inserted into an expression cassette comprisinga murine Thy-1.2 gene construct, and mice were generated by pronuclearinjection. The founder mice were then back-crossed with C57BL/6mice. APP23 mice of generations F5-F10 and corresponding wild-typemice were used. The wild-type control mice were either littermatesor nontransgenic age-matched mice from another litter of the samegeneration ofbackcrossing.

ChAT and AChE enzyme activities. Mice were killed by decapitation, and the frontal cortex was dissected on ice. The tissuewas weighed, snap-frozen on dry ice, and stored at $-$ 80°C untilanalysis. Tissue was homogenized 1:50 (w/v) in 10 mM EDTA containing0.5% Triton X-100 at pH 7.4. ChAT enzyme activity was measuredby a slight modification (Kelly and Moore, 1978) of the methodof Fonnum (1975). In brief, tissue homogenates were incubatedin a water bath at 37°C in an incubation mixture containing (inmM): 300 NaCl, 8 choline iodide, 20 EDTA, 0.1 eserine hemisulfate,and 0.2 acetyl-[1-¹⁴C]-coenzyme A in 50 mM phosphate buffer, pH 7.4 (final concentrations).After stopping the production of radioactively labeled acetylcholinewith ice-cold 10 mM sodium dihydrogen phosphate, pH 7.4, the solutionswere transferred into scintillation vials, and sodium tetraphenylboron(0.5% in acetonitrile; Merck, Darmstadt, Germany) and the scintillant(0.05% PPO in toluene) were added. Labeled acetylcholine was determinedby liquid scintillation counting in the biphasic aqueous, toluenescintillation solution mixture. ChAT enzyme activity was expressedin micromoles per 100 mg of protein per hour. Protein concentrationwas measured using the Bio-Rad (Munich, Germany) proteinassay.

For AChE activity, samples of the same homogenates were sonicated, and aliquots were assayed for AChE activity by colorimetricdetermination by the method of Ellman et al. (1961) and Cutleret al. (1998). In short, after centrifugation for 15 min (15,000rpm, 4°C), aliquots from the clear supernatant were used as enzymesource. Twenty microliters of supernatant (quadruplicates) wereplaced in a 96-well flat-bottom micro-test plate. The reactionwas started by adding the following substrate-reagent mixture,using an automatic plate dispenser (Titertek Autodrop): 0.5 mMacetylthiocholine iodide (Fluka, Buchs, Switzerland), 1 mM tetraisopropylpyrophosphoramide(iso-OMPA; Sigma, Buchs, Switzerland), and 0.25 mM 5,5'-dithiobis-2-nitrobenzoate(Fluka) in 0.1 M phosphate buffer, pH 7.4. The plate was thenplaced in the automatic Micro-Reader (Molecular Devices, PaloAlto, CA; UVmax) that recorded the occurrence of the yellow reactionproduct at 405 nm. The data were processed by a program (Softmax;Molecular Devices) controlled by the plate reader. The calculationof the enzymatic activity (performed by the computer program)is based on a change in optical density in the linear range overtime using the molar extinction coefficient of the reaction product(13.3 cm²/mmol). AChE enzyme activity was expressed in nanomoles per milligramof protein perminute.

Immunohistochemistry. Perfusion- or immersion-fixed brains were paraffin embedded according to a previously published procedure(Calhoun et al., 1998a) that involved post-fixation in increasingalcohol concentrations and clearing with Cedarwood oil and methylsalicylate (Aldrich, Buchs, Switzerland). Serial coronal sections(25 µm) were cut with a microtome, and immunohistochemistry wasperformed using the avidin-biotin-peroxidase method (Calhoun etal., 1998a). In brief, paraffin sections were deparaffinized inxylene, then placed in 100% ethanol for 10 min followed by 30min in methanol with 0.3% H₂O₂. Sections were rinsed in PBS andincubated for 1 hr in 5% goat or horse serum (Vector Laboratories,Burlingame, CA) in a humid chamber. Sections were then incubatedovernight with a primary antibody in PBS with 3% serum. Afterrinsing, sections were incubated for 1 hr with biotinylated secondaryantibody (Vector Laboratories) diluted 1:200 in PBS. Sectionswere rinsed again and incubated with the avidin-biotin-peroxidasecomplex (1:50; ABC Elite kit; Vector Laboratories) in PBS. Finally,sections were reacted with 3',3-diaminobenzidine-dihydrochloride(DAB; Sigma; 0.08%) and 0.03% hydrogen peroxide in PBS, rinsed,dehydrated, cleared in xylene, and coverslipped. On NBM-lesionedtissue (see below) immunohistochemistry was done on free-floating,fixed-frozen sections according to a previously published protocol(Phinney et al., 1999), similar to the procedure described above.The following antibodies were used: polyclonal anti-A $beta$ (NT12;1:500 and 1:2000 for paraffin and frozen sections, respectively)(Schrader-Fischer and Paganetti, 1996) and polyclonal anti-ChAT(AB144P; 1:500 for paraffin sections; Chemicon, Temecula,CA).

AChE histochemistry. Mice were deeply anesthetized with an intraperitoneal injection of an overdose of pentobarbital (50 mg/mlNembutal) and transcardially perfused with 4% paraformaldehydein PBS. Brains were removed, post-fixed for 24 hr in 4% paraformaldehyde,cryoprotected in 30% sucrose in PBS, frozen in isopentane at $-$ 25°C,and serially sectioned at 40 µm on a freezing-sliding microtome.AChE immunohistochemistry was performed according to a previouslypublished method (Hedreen et al., 1985). Some sections were alsoimmunostained with a polyclonal antibody to AChE (Marsh et al.,1984) (gift of J. Massoulie, Paris, France). No qualitative differencewas noted between the histochemical and immunohistochemical reactionconfirming previous findings in the rat (Jucker et al., 1996).Histochemical AChE staining was however more reliable and moredistinct and was taken for quantitative analysis of cholinergicfiber length (seebelow).

To study the localization of AChE in more detail, some of the tissue was fixed with paraformaldehyde plus 1% glutaraldehyde,cut on a vibratome (60 µm), stained for AChE, and plastic-embeddedaccording to a previously published protocol (Stalder et al.,1999). Semithin (0.5 µm) and ultrathin (80 nm) sections were cuton a ultramicrotome. Sections were collected on Formvar-coatednickel grids and viewed under high-power light microscopy or electronmicroscopy.

Stereological assessment of cholinergic fiber length. Stereological techniques were used to estimate the total length of AChE-positivefibers in the neocortex (Table 1). To this end, every 16^th section throughout the neocortex was histochemically stainedfor AChE according to the above described protocol. The volumeof the neocortex was estimated by superimposing a point-grid oneach section and counting the points over neocortex, accordingto the Cavalieri principle (West et al., 1991; Calhoun et al.,1998b). AChE-positive fiber density was then estimated by superimposinga system of test lines, and intersections of test lines with fiberswere counted within the volume of disectors systematically spacedthroughout the neocortex using the 100× objective (2756× finalmagnification) with a numerical aperture of 1.3 (Stocks et al.,1996). This number of intersections between fibers and test linesof a known length produces a result directly related to the lengthof the fibers themselves within the disector volume (Howard etal., 1992). Because length measurement was performed on coronalsections in all cases, it is assumed that no overall directionalorientation with respect to the plane of section exists for cholinergicfibers as they innervate the cortex. AChE-positive fiber lengthwas calculated by multiplying the region volume by the fiber lengthdensity (West, 1993). Stereological analysis was performed withthe aid of Stereologer software and a motorized x-y-z stage coupledto a video microscopy system (Systems Planning and Analysis, Alexandria,VA). Post-processing section thickness was measured using a focusdrive accurate to ±0.1 µm (Applied Scientific Instrumentation,Eugene, OR). Coefficient of error was calculated according toWest et al. (1991) and was well below biological variability.Region definitions of neocortex were based on a recent mouse brainatlas (Franklin and Paxinos, 1997).


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Table 1. Stereological parameters for cholinergic fiber, amyloid load, and cholinergic basal forebrain neuron quantification

Stereological assessment of amyloid load. Amyloid load was assessed on every 20^th paraffin section throughout the neocortex immunostained withNT12. The percentage of neocortical volume occupied by amyloid(amyloid load) was determined by sampling through the entire neocortexwith a 20× objective (numerical aperture, 0.45) and counting thepercentage of points from a superimposed point grid that hit amyloid(Table 1) (Calhoun et al., 1998b). Stereological analysis wasperformed with the Stereologer software describedabove.

Number and volume of ChAT-positive basal forebrain neurons. For estimation of the number (West et al., 1991) and volume (Jensenand Gundersen, 1993) of ChAT-positive cells in the basal forebrain,systematic random series of ChAT-stained paraffin sections wereanalyzed using a fractionator sampling scheme. For quantitativeanalysis ChAT-positive neurons in the NBM complex that providethe major cholinergic innervation to the neocortex were combined.Similarly cholinergic neurons in the MS and VDB, that providethe cholinergic innervation to the hippocampus were combined foranalysis. Every eighth section throughout the NBM complex andevery fourth section throughout the MS-VDB were collected. Oneach section a point grid was placed randomly over the regionto determine the systematic-random placement of the optical disectors.The total number of ChAT-positive neurons within the three-dimensionaloptical disectors throughout the region were then counted. Objectswere counted by focusing through the counting frame using a 63×objective with a numerical aperture of 1.25. The nuclei of ChAT-positivecells were the selected objects for counting (Table 1). Additionally,the volume of each counted cell was estimated. For practical reasons,the tissue could not be randomly rotated during sectioning, andit was thus assumed that there is no change in preferred orientationof the cells in the basal forebrain (Gundersen et al., 1988).A vertical line with three perpendicular grid lines were superimposed,and intersections of grid lines with the cell soma were identified.The mean length of these lines is proportional to neuron volume(Jensen and Gundersen, 1993), although in this case the valueis orientation-dependent. Stereological analysis was performedwith the Stereologer software describedabove.

NBM Lesions. Animals were deeply anesthetized using a combination of ketamine (10 mg/kg body weight; Ketalar; Parke-Davis,Ann Arbor, MI) and xylazine (20 mg/kg body weight; Rompun, Bayer,Germany) in saline administered intraperitoneally. Using stereotaxicsurgery, the scalp was cut, a hole was drilled, and an electrodewas lowered into the NBM [anteroposterior (bregma), $-$ 0.2 mm; lateral,1.5 mm; dorsoventral (dura), $-$ 4.5 mm]. A current flow of 0.5 mAwas passed for 15 sec. Half of the mice received an additionalsham lesion on the contralateral side, in which the electrodewas lowered, but no current was passed through. The lesion sidewas alternated evenly over thegroups.

Mice were killed 3-8 months later by decapitation. Brains were removed, and a small piece of the ipsilateral and contralateralfrontal neocortex was dissected and combined with a small piecefrom the ipsilateral and contralateral motor-somatosensory cortexas previously described (Kelly and Moore, 1978). The dissectedtissue was weighed, snap-frozen on dry ice, and assayed for ChATenzyme activity (described above) and APP/A $beta$ (see below). Therest of the brain was immersion-fixed in 4% paraformaldehyde,cryoprotected in 30% sucrose, and frozen. Serial coronal 40 µmsections were cut throughout the frontal cortex, and alternatesections were stained for A $beta$ and AChE or double-stained for both.Amyloid load was then determined stereologically on the A $beta$ -stainedsections (see above), discarding the sections missing the dissectedpieces. This yielded a total of 5-15 A $beta$ -stained sections throughthe frontal cortex per mouse. Percentage of amyloid load was determinedfor both hemispheresseparately.

A $beta$ load and APP processing using Western blotting. It has previously been demonstrated that amyloid cores in APP23 mice arecompletely soluble in SDS (Kuo et al., 2001). Thus, the tissuesamples used to determine ChAT activities (see above) were diluted1:3 (weight/volume) in 1.5× SDS-sample buffer (containing 1% SDS)and separated using a 10% SDS-polyacrylamide gel containing 8M urea (Klafki et al., 1996). For amyloid quantification 2 µlwas loaded from the unlesioned and lesioned side. After separation,proteins were transferred to Immoblin-P (Millipore, Bedford, MA)with a Bio-Rad semidry transfer apparatus for 1 hr at 25 V, accordingto Wiltfang et al. (1997). Membranes were blocked in 5% nonfatmilk in PBS with 0.1% Tween 20 (PBS-T) and reacted overnight at4°C with A $beta$ antibody 6E10 (Signet, Dedham, MA) at 1:2000 in PBS-Tfollowed by a goat anti-mouse peroxidase conjugate (Chemicon,Temecula, CA) at 1:2500 in PBS-T for 30 min at room temperature.Bands were visualized using Supersignal (Pierce, Rockford, IL)and developed onto Kodak X-OMAT AR film (Rochester, NY). Differentexposures of the film were digitized, and band density measurementsfor A $beta$ 40 and A $beta$ 42 were made using NIH Image version 1.61 (NationalInstitutes of Health, Bethesda, MD). Each sample pair was runat least three times, and the mean was taken. Only bands withinthe linear range of the film wereanalyzed.

To analyze APP processing in more detail, the $beta$ -secretase cut, the N terminal secreted fragment (sAPP $beta$ ), and the correspondingC terminal fragment C99 were additionally analyzed. For the analysisof sAPP $beta$ , proteins were separated on a 8% SDS-polyacrylamide geland transferred to Immobilon-P membranes as described previously(Andra et al., 1996). The blot was reacted with rabbit neoepitopeantiserum 852 against the C terminus of sAPP $beta$ (P. Paganetti andM. Staufenbiel, unpublished observations). As an internal control,an antibody to tubulin wasused.

Statistics. All statistical analysis was done using StatView 5.0.1. The mean ± SEM is indicated. Significance level was setat p < 0.05.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Disruption and loss of cholinergic fibers in neocortex of aged APP23 mice

To study the impact of cerebral amyloidosis on the cholinergic system, we have analyzed AChE-positive fiber length and ChAT-positiveboutons in neocortex of APP23 mice. Three age groups with similarnumbers of male and female APP23 mice were examined: young (6months; n = 6), adult (15 months; n = 5), and aged (24 months;n = 7). Corresponding controls were young (6 months; n = 6), adult(15 months; n = 8), and aged (24 months; n = 5) wild-type mice.Quantitative analysis of the amyloid load revealed no amyloiddeposition in the young APP23 mice, 4.0 ± 1.8% in adult APP23mice, and 28.6 ± 1.4% in aged APP23 mice (Fig. 1A,B). Consistentwith previous reports, the majority of the amyloid depositionin APP23 mice was compact in nature and congophilic (Calhoun etal., 1998b; Stalder et al., 1999). Amyloid deposits were alsofound in vessels and as extracellular diffuse amyloid (Fig. 1B).Neocortical volume did not differ between the groups at any age(mean volume for all mice = 17.4 mm³; one hemisphere).

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Figure 1. Amyloid deposits and cholinergic disruption in neocortex of aged APP23 mice. A, No amyloid is detected in 24-month-old wild-type mice. B, Immunostaining for A $beta$ reveals numerous compact amyloid plaques, diffuse amyloid (arrowheads), and amyloid deposits in vessels (arrow) in neocortex of a 24-month-old APP23 mouse. C, D, Histochemical staining for AChE reveals a disruption and a decrease in cholinergic fiber density in neocortex of 24-month-old APP23 mice (D) compared with 24 month-old control mice (C). The disruption is most evident around plaques but occurs throughout the neocortex. Scale bars, 120 µm.

Histochemical staining for AChE revealed a dense laminated network of cholinergic fibers throughout the neocortex of wild-typemice and young APP23 mice. In adult and aged APP23 mice, however,there was a loss and often dramatic disruption of the cholinergicfiber network (Fig. 1C,D). In particular in the aged APP23 mice,a loss of AChE-positive fibers throughout the entire neocortexwas evident with intense staining of dystrophic structures atthe plaque periphery and diffuse staining of the amyloid cores(Fig. 2A). High-power microscopic analysis identified these dystrophicstructures as fibers that often formed loops ending in dystrophicboutons (Fig. 2A). Semithin and ultrathin sectioning through thediffusely stained AChE-positive amyloid cores demonstrated thatAChE immunoreactivity was associated with amyloid fibrils (Fig.2B).

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Figure 2. Cholinergic disruption and dystrophy in APP23 neocortex. A, AChE-positive fibers around an amyloid plaque with diffuse staining of the amyloid cores in the neocortex of an aged APP23 mouse (arrowhead). Inset, High-power analysis of the abnormal and often swollen AChE-positive fibers with terminal large boutons in vicinity of the amyloid plaque (arrowheads). Fibers frequently grow toward the amyloid but then form loops or sharply turn around to grow away from the amyloid to turn later again toward the amyloid (arrow). B, High-power analysis of diffuse AChE-staining associated with the amyloid cores. Inset, AChE staining in semithin sections suggests an association of AChE with the amyloid core. Subsequent ultrastructural analysis confirms that AChE reactivity (arrow) is associated with amyloid fibers (a). C, Immunostaining for ChAT reveals dense punctate staining of cholinergic boutons in the frontal cortex of an aged wild-type mouse. D, In contrast, a loss of cholinergic boutons is apparent in aged APP23 mice. Dystrophic ChAT-positive boutons and neuritic structures are present around amyloid plaques (arrowheads). Scale bars: A, 50 µm; B, 1.6 µm; C, D, 50 µm.

ChAT immunohistochemistry revealed punctate staining of cholinergic boutons throughout the neocortex (Fig. 2C,D). Punctatestaining was often very dense revealing the shape of individualcholinergic fibers with their immunostained boutons. No qualitativedifference in staining was noted between wild-type and young APP23mice. In contrast, in adult and aged APP23 mice a reduction ofChAT-positive boutons was observed in neocortical areas with ahigh amyloid burden, such as entorhinal and frontal cortex (Fig.2D). Large dystrophic ChAT-positive structures were present atthe periphery of the amyloid plaques and resembled the AChE-positivedystrophic fibers describedabove.

For quantification of cholinergic fiber length, AChE histochemistry was chosen because of robust staining and significantpenetration of the stain into the tissue sections, both prerequisitesfor stereological analysis. Results for total length of AChE-positivefibers in neocortex revealed the astonishing length of 600 m perhemisphere and was similar for all three groups of wild-type mice(Fig. 3). In contrast to this lack of age effect in wild-typemice, there was a clear reduction in fiber length with aging inthe APP23 mice that reached 35% compared with young APP23 miceand 25% compared with adult APP23 mice. In comparison with age-matchedwild-type mice there was a 29% reduction. Consistently, ANOVArevealed a significant age effect (F_(2,31) = 6.40; p < 0.01),a significant transgene effect (F_(1,31) = 4.59; p < 0.05), anda significant age × transgene interaction (F_(2,31) = 4.30; p <0.05). Newman-Keuls post hoc analysis indicated that the fiberloss in aged APP23 mice was statistically significant comparedwith aged wild-type mice (p < 0.01) and to young (p < 0.01) andadult (p < 0.05) APP23 mice (Fig. 3A). A significant negativecorrelation between AChE-positive fiber length and amyloid loadwas apparent when adult and aged APP23 mice were combined (R² = 0.46; p < 0.05) (Fig. 3B). Males and females were combinedfor AChE-fiber length analysis because previous ANOVA analysisdid not reveal any significance for, or interaction with, gender.

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Figure 3. AChE-positive fiber length and amyloid load in neocortex of APP23 mice. A, Total length of AChE-positive fibers in neocortex of young (6 months), adult (15 months), and aged (24 months) APP23 mice (black bars) and age-matched wild-type mice (open bars). Aged transgenic mice had a significant loss of fiber length compared with aged wild-type mice (**p < 0.01) and with young transgenic mice (**p < 0.01). Indicated is the mean ± SEM for one hemisphere only. B, A significant negative correlation between AChE-positive fiber length and amyloid load was apparent when adult (circles) and aged (squares) APP23 mice were combined.

ChAT and AChE activities in the frontal cortex of APP23 mice

ChAT and AChE enzyme activities were measured in the frontal cortex (Table 2). Three age groups consisting of similar numbersof both sexes of APP23 mice (6 months, n = 8; 19 months, n = 11;24 months, n = 6) and age-matched wild-type control mice (6 months,n = 8; 19 months, n = 9; 24 months, n = 7) were used. Becauseof logistical issues, the young, adult, and aged mice were analyzedseparately, thus preventing comparison between age groups. Becauseno difference between males and females was apparent, male andfemales were combined. Results revealed a modest but significantdecrease of ChAT activity in the frontal cortex of aged APP23mice as compared with age-matched controls (t₍₁₁₎ = 2.27; p <0.05) (Table 2). Differences in AChE activities did not reachsignificance, although there was a trend toward decreased activitiesin transgenic mice in all three groups (Table 2).


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Table 2. ChAT and AChE enzyme activities in the frontal cortex

Number and volume of ChAT-positive neurons in the basal forebrain

Two age groups of APP23 mice (young: 8 months, n = 8; aged: 27 months, n = 8) and corresponding wild-type mice (young: 8 months,n = 7; aged: 27 months, n = 6) were used with sex equally balancedwithin groups and treated as one group. ANOVAs for ChAT-positiveneuron number were calculated separately for the NBM complex andthe MS-VDB (Fig. 4). Results did not reveal a significant effectof age or transgene on neuron number (p > 0.05) (Fig. 5A,B). Therewas also no change in volume of ChAT-positive cells in the NBMcomplex (Fig. 5C). Rather unexpectedly, a significant transgeneeffect (F_(1,25) = 8.76; p < 0.05) with a nonsignificant age ×transgene interaction was found for the volume of ChAT-positivecells in the MS-VDB, indicating that both young and aged APP23mice have smaller cholinergic neurons in the MS-VDB (Fig. 5D).

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Figure 4. ChAT-positive neurons in the basal forebrain of APP23 mice. A, B, No apparent difference in neuron number was observed in the NBM of 27-month-old APP23 mice (A) compared with aged-matched wild-type mice (B). C, D, Similarly, no apparent difference in ChAT-positive neuron number in the MS was noted between 27-month-old APP23 (C) mice and age-matched control mice (D). For quantification, see Figure 5. Scale bar, 50 µm.

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Figure 5. Number and volume of cholinergic neurons in the basal forebrain of APP23 mice. Number (A) and volume (C) of ChAT-positive neurons in the NBM complex in APP23 mice (black bars) and wild-type mice (open bars). No significant difference between transgenic and wild-type mice was noted. A similar analysis was done for the number (B) and volume (D) of ChAT-positive neurons in the MS-VDB in APP23 mice (black bars) and wild-type mice (open bars). For neuron volume, a significant reduction of 38 and 42% was found in the 8-month-old and 27-month-old APP23 mice, respectively (*p < 0.05). Data are mean ± SEM. Indicated values are for one hemisphere only.

Lesions of the nucleus basalis of Meynert reduce neocortical A $beta$ load

Groups of male and female mice were lesioned at 5, 7, 10, and 13 months of age and were killed at 9, 15, 13, and 20 monthsof age, respectively. Only mice with a complete lesion of theNBM complex and a >20% ChAT decrease in the ipsilateral comparedwith contralateral frontal cortex were included in the analysis(n = 11; mean ChAT decrease: 38 ± 4%). Histologically, in thesemice there was a considerable loss of AChE-positive fibers inthe ipsilateral frontal cortex (Fig. 6).

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Figure 6. Amyloid load in the frontal cortex after NBM lesions. A, B, Double labeling for AChE (brown) and A $beta$ (blue) in a 13-month-old APP23 mouse 3 months after a unilateral NBM lesion reveals a considerable loss of cholinergic fibers in the ipsilateral (B) compared with contralateral (A) frontal cortex. Stereological assessment revealed a 22% reduction of amyloid deposition in the ipsilateral compared with contralateral side. Scale bar: A, B, 90 µm. C, Western blotting of cortex homogenates. Samples were run in pairs, i.e., contralateral side (c) versus ipsilateral side (i). Shown are three mice. Results for all the mice revealed a 19% decrease of A $beta$ 40 between the two sides. No difference in the ratio between A $beta$ 40 and A $beta$ 42 was found between contralateral and ipsilateral side.

Stereological analysis of the amyloid load on A $beta$ -immuno-stained sections revealed a mean decrease in the amyloid load of 22± 8% in the ipsilateral versus contralateral frontal cortex (Fig.6A,B). The individual changes ranged from +14 to $-$ 63% with a decreasein 8 of 11 mice. This difference did not reach statistical significance(p = 0.11, Wilcoxon signed rank test). In contrast, a significantdecrease was observed when A $beta$ 40 was analyzed using densitometryof Western blots. The mean decrease was 19 ± 9% with a range from+30% to $-$ 61% (Fig. 6C). Eight of 11 mice revealed a decrease (p= 0.04, Wilcoxon signed rank test). The ratio between A $beta$ 42 andA $beta$ 40 was not significantly different between the ipsilateral (0.29)and contralateral side (0.26).

To further study APP processing we have analyzed sAPP $beta$ and C99, the two cleavage products of $beta$ -secretase. No significant differencewas found for sAPP $beta$ between ipsilateral and contralateral side( $-$ 7%; p = 0.15; paired t test), and this difference was identicalto the one found for tubulin. Consistently, no apparent differencefor C99 between ipsilateral versus contralateral was found (resultsnot shown). These results indicate that cholinergic denervationdoes not lead to a globally detectable shift of APP metabolismto the amyloidogenic pathway in APP23mice.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cerebral amyloidosis is a hallmark lesion of AD, and genetic analysis has demonstrated that A $beta$ is central to AD pathogenesis(Selkoe, 1999). Similarly, depletion of the cholinergic systemis a robust finding in AD and correlates with cognitive impairment(Collerton, 1986; DeKosky et al., 1992; Bierer et al., 1995).Yet, the link between cerebral amyloidosis and the cholinergicdeficit remains poorlyunderstood.

The present study was undertaken to investigate alterations in the cholinergic system in the APP23 mouse model of cerebralamyloidosis. The mice develop amyloid plaques and cerebrovascularamyloid throughout the neocortex and hippocampus with only modestamyloid deposition in the basal forebrain (Sturchler-Pierrat etal., 1997; Calhoun et al., 1998b). Individual amyloid depositsin APP23 mice are also morphologically similar to those in ADbrain and include congophilic amyloid cores, amyloid-associateddystrophic neurites, astrocytosis, and microgliosis (Jucker etal., 2001). A difference between amyloid plaques in mouse comparedwith AD brain is the lack of paired helical filaments in plaque-associateddystrophic neurites (Sturchler-Pierrat et al., 1997). Moreover,there is a difference in solubility and chemical composition ofthe amyloid (Kuo et al., 2001).

Results of the present study reveal a robust 30% decrease in cholinergic fiber length with distorted and dystrophic cholinergicfibers surrounding the amyloid very similar to that in AD brain(Geula et al., 1998). Because fiber loss in the mice correlatedwith cortical A $beta$ load and because we did not find a loss or shrinkageof cholinergic neurons in the NBM, our results suggest that thecortical cholinergic deficit in APP23 mice is locally inducedby A $beta$ deposition. These results are also consistent with earlierobservations that retrograde degeneration in the NBM only occursafter more severe cortical tissue damage (Sofroniew et al., 1983;Liberini et al., 1994). In other transgenic mouse models, a lackof neuron loss in the basal forebrain has also been reported.However, in these mouse models, no significant cortical cholinergicdeficits have been observed possibly because of the age of themice and/or the lower neocortical amyloid burden (Wong et al.,1999; Bronfman et al., 2000; Hernandez et al., 2001; Jaffar etal., 2001), although in one plaque-burdened mouse line a decreasein vesicular acetylcholine transporter-positive bouton area anddensity in frontal cortex was reported (Wong et al., 1999).

Rather unexpectedly, our results reveal that cholinergic neurons in the MS/VDB of APP23 mice are significantly smaller comparedwith wild-type mice. Amyloid deposition is unlikely to accountfor this observation, because a decrease in neuron volume wasalso found in the 8-month-old APP23 mice that exhibited negligibleamyloid deposition in hippocampus and no deposition in the MS-VDB.It has been reported that in SN56 cells (N18TG2 neuroblastomacells fused with mouse primary septal neurons), low concentrationsof A $beta$ can induce long-lasting downregulation of the cholinergicactivities without evidence of neurotoxicity (Pedersen et al.,1996; Auld et al., 1998). Thus, it is possible that A $beta$ levelsin the 8-month-old APP23 mice are high enough to induce cholinergichypoactivity and shrinkage of MS-VDB neurons, although it is unclearwhy this region would be preferentially affected. Interestingly,in another APP transgenic mouse model, a selective decrease insize of MS cholinergic neurons, but not NBM cholinergic neurons,has also been reported (Bronfman et al., 2000). In this modelhowever, shrinkage was observed in aged transgenic mice but notin young transgenic mice without amyloid deposition. This differencemay be explained by the much lower levels of APP expression/A $beta$ in this latter model. In AD a shrinkage of basal forebrain cholinergicneurons has also been reported (Vogels et al., 1990).

Cholinergic fiber loss in AD neocortex displays considerable regional variability with reductions exceeding 50% in some corticalareas (Mesulam, 1996; Geula et al., 1998). In addition, thereis a poor correlation between amyloid plaques and fiber loss,suggesting that amyloid deposition in neocortex cannot be theexclusive cause of the cholinergic loss. Thus, it is likely thatin AD brain the significant loss of cholinergic basal forebrainneurons contributes to the cortical cholinergic deficit and accountsfor the more pronounced fiber loss as compared with APP23 mice.NBM cholinergic neurons are among the first neuronal groups withneurofibrillary tangle formation and among the first neurons thatare lost in AD (Mesulam, 1996; Cullen and Halliday, 1998; Sassinet al., 2000).

In contrast to the significant fiber loss in APP23 mice, our results revealed only a modest loss of ChAT and AChE enzyme activities.Correlative analysis of ChAT and AChE enzyme activities and amyloidload in AD brain have revealed conflicting findings. Some studieshave found negative correlations (Perry et al., 1981; Mountjoyet al., 1984; Zubenko et al., 1989; Beach et al., 2000a), whereasothers have found no relation (Wilcock et al., 1982; DeKosky etal., 1992; Geula et al., 1998). In AD and in APP23 mice, a significantamount of ChAT and AChE staining is associated with dystrophicneurites surrounding amyloid plaques (Benzing et al., 1993; Moranet al., 1993). Moreover, in both AD and APP23 mice, AChE is acomponent of amyloid-containing plaques, and it has been suggestedthat AChE accelerates amyloid fibril formation (Gomez-Ramos etal., 1992; Mesulam et al., 1992; Inestrosa et al., 1996). It ispossible that this notable accumulation of ChAT and AChE withinand around plaques in APP23 mice accounts for the only modestoverall decrease in enzymeactivities.

It has been hypothesized that cholinergic depletion in AD contributes to cerebral amyloidosis. This hypothesis is based onthe observation that activation of protein kinase C through muscarinicreceptor binding stimulates the nonamyloidgenic pathway of APPprocessing by increasing sAPP $alpha$ production and reducing A $beta$ generation(Buxbaum et al., 1992; Nitsch et al., 1992; Hung et al., 1993).Thus, the loss of the cholinergic innervation may lead to increasedproduction of A $beta$ and amyloid deposition. In vivo support for alteredAPP processing has been provided in both NBM-lesioned rats andin rats after muscarinic agonist treatment (Rossner et al., 1997;Lin et al., 1999). However, A $beta$ levels were not assessed in thesestudies. In contrast, A $beta$ levels were assessed 6 months after NBMlesions in rabbits and resulted in a 2.5- and 8-fold increasein neocortical A $beta$ 40 and A $beta$ 42, respectively, however no depositionof amyloid was found (Beach et al., 2000b). Based on these findingswe initiated similar NBM lesions in APP23 mice that develop cerebralamyloidosis withaging.

ChAT reduction after NBM lesions in APP23 mice was 38% and is similar to the reduction reported in NBM-lesioned mice, rats,and rabbits (Smith, 1988; Beach et al., 2000b). However, we failedto see increased A $beta$ levels or deposition in the lesioned hemispherein APP23 mice. Perhaps it is difficult to further shift the processingof transgenic APP toward the $beta$ -secretase pathway because the Swedishdouble mutation in APP23 mice already greatly favors this pathway(Citron et al., 1992).

The observation that NBM lesions in APP23 mice actually result in a decrease in neocortical amyloid deposition may be explainedby the finding that AChE accelerates the assembly of amyloid peptideinto amyloid fibrils (Inestrosa et al., 1996). Accordingly, thecholinergic deficit in APP23 mice may result in reduced amyloidformation. However, the observations of amyloid plaque reductionafter NBM lesions may also be the result of enhanced clearingmechanisms in a lesioned-deafferented brain tissue and not bespecific to the cholinergic system. It has been reported thattraumatic brain injury results in a 30% regression of amyloidburden in the hippocampus of PDAPP transgenic mice (Nakagawa etal., 2000). Moreover, entorhinal cortex lesions appear to inhibitamyloid plaque formation in the deafferented dentate gyrus (S.Sisodia, personal communication). The mechanism is not clear butmay involve enhanced microglia clearance of amyloid in the denervated-lesionedbrainareas.

In conclusion, our results suggest that the cerebral amyloidosis in neocortex of APP23 mice causes significant cholinergicfiber loss and severe disruption of the cholinergic fiber network.Because the mice do not lose basal cholinergic forebrain neurons,these results suggest that the cholinergic deficit in APP23 miceis locally induced by the amyloid in neocortex. In light of therole and importance of the neocortical cholinergic system forcognition (Winkler et al., 1995), the cholinergic changes in APP23mice may contribute to the recently described cognitive impairmentof these mice (Kelly et al., 2002). Importantly, our lesion resultssuggest that in the APP23 mouse model, loss of cholinergic forebrainneurons and a subsequent loss of cortical cholinergic activitydoes not promote amyloiddeposition.

  FOOTNOTES

Received Oct. 10, 2001; revised Jan. 31, 2002; accepted Feb. 7, 2002.

^* S.B. and M.E.C. contributed equally to thiswork.

This work was supported by grants from the Swiss National Science Foundation and the VerUm Foundation (Munich, Germany). Wethank J. Massoulie for providing antibodies, P. Mouton for helpfulcomments regarding stereological procedures, D. Hunziker for technicalassistance, and T. Schürch and H. Zysset for assistance inphotography.

Correspondence should be addressed to Mathias Jucker, Institute of Pathology, University of Basel, Schönbeinstrasse 40, CH-4003Basel, Switzerland. E-mail: mjucker{at}uhbs.ch.

M. E. Calhoun's present address: Kastor Neurobiology of Aging Laboratories, Mount Sinai School of Medicine, New York, NY10029.

A. L. Phinney's present address: University of Toronto, Center for Research in Neurodegenerative Diseases, Toronto, OntarioM5S 3H2,Canada.

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