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The Journal of Neuroscience, October 4, 2006, 26(40):10129-10140; doi:10.1523/JNEUROSCI.1202-06.2006
 Previous Article | Next Article 
Neurobiology of Disease
Intraneuronal  -Amyloid Aggregates, Neurodegeneration, and Neuron Loss in Transgenic Mice with Five Familial Alzheimer's Disease Mutations: Potential Factors in Amyloid Plaque Formation
Holly Oakley,1
Sarah L. Cole,1
Sreemathi Logan,1
Erika Maus,1
Pei Shao,1
Jeffery Craft,1
Angela Guillozet-Bongaarts,1
Masuo Ohno,2
John Disterhoft,2
Linda Van Eldik,1
Robert Berry,1 and
Robert Vassar1
Departments of 1Cell and Molecular Biology and 2Physiology, The Feinberg School of Medicine, Northwestern University, Chicago, Illinois 60611
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Abstract
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Mutations in the genes for amyloid precursor protein (APP) and presenilins (PS1, PS2) increase production of  -amyloid 42 (A42) and cause familial Alzheimer's disease (FAD). Transgenic mice that express FAD mutant APP and PS1 overproduce A42 and exhibit amyloid plaque pathology similar to that found in AD, but most transgenic models develop plaques slowly. To accelerate plaque development and investigate the effects of very high cerebral A42 levels, we generated APP/PS1 double transgenic mice that coexpress five FAD mutations (5XFAD mice) and additively increase A42 production. 5XFAD mice generate A42 almost exclusively and rapidly accumulate massive cerebral A42 levels. Amyloid deposition (and gliosis) begins at 2 months and reaches a very large burden, especially in subiculum and deep cortical layers. Intraneuronal A42 accumulates in 5XFAD brain starting at 1.5 months of age (before plaques form), is aggregated (as determined by thioflavin S staining), and occurs within neuron soma and neurites. Some amyloid deposits originate within morphologically abnormal neuron soma that contain intraneuronal A. Synaptic markers synaptophysin, syntaxin, and postsynaptic density-95 decrease with age in 5XFAD brain, and large pyramidal neurons in cortical layer 5 and subiculum are lost. In addition, levels of the activation subunit of cyclin-dependent kinase 5, p25, are elevated significantly at 9 months in 5XFAD brain, although an upward trend is observed by 3 months of age, before significant neurodegeneration or neuron loss. Finally, 5XFAD mice have impaired memory in the Y-maze. Thus, 5XFAD mice rapidly recapitulate major features of AD amyloid pathology and may be useful models of intraneuronal A42-induced neurodegeneration and amyloid plaque formation.
Key words: Alzheimer's disease; transgenic mice; A42; amyloid plaques; intraneuronal A; neuron loss
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Introduction
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Amyloid plaques, deposits of the -amyloid (A) peptide (Glenner and Wong, 1984 ), are defining lesions in Alzheimer's disease (AD) brain. A strong genetic association exists between early-onset familial forms of AD (FAD) and the 42 amino acid species of the A peptide (A42) (for review, see Hutton et al., 1998; Younkin, 1998; Sisodia et al., 1999). A is a proteolytic product of the amyloid precursor protein (APP), and autosomal dominant mutations in the genes for APP, presenilin1 (PS1), and presenilin2 (PS2) increase production of A42 and cause FAD. A42 is more fibrillogenic than shorter A peptides, and elevated A42 concentrations are thought to drive the formation of the insoluble fibrils that compose amyloid plaques. The robust association of A42 with FAD argues strongly in favor of a causative role for A42 in the etiology of AD.
A is cleaved from APP by the sequential action of two proteases, the - and  -secretases (for review, see Sisodia et al., 1999; Selkoe, 2001). Initially, the -secretase cuts APP at the N terminus of the A domain to produce the membrane-bound fragment C99 and the secreted APP ectodomain APPs. Subsequently, C99 is cleaved by the -secretase to generate the C terminus of A. -Secretase cleavage is not precise and produces a series of A peptides of 38–43 amino acids in length. Under normal conditions, a higher proportion of A is produced as the 40 amino acid A40, and less is made as A42. FAD mutations in APP that cluster near the - and -secretase cleavage sites either elevate the production of total A, as is the case with the K670N/M671L substitution [Swedish mutation (Mullan et al., 1992a)], or increase the generation of A42 specifically, as occurs with the I716V [Florida mutation (Eckman et al., 1997)] and V717I [London mutation (Goate et al., 1991)] substitutions. PS1 and PS2 appear to be subunits of the -secretase complex (Esler and Wolfe, 2001), and presenilin FAD mutations also elevate A42 generation specifically.
Previous studies have suggested that A42-elevating FAD mutations act in an additive manner to increase A42 generation when incorporated within the same molecule. In particular, the intramolecular combination of I716V and V717I mutations within APP doubled A42 production compared with the individual mutations (Eckman et al., 1997), as did the two PS1 FAD mutations M146L and L286V when introduced together into PS1 (Citron et al., 1998). Moreover, the intermolecular combination of A42-elevating mutations in APP and PS1 also additively increased A42 production (Citron et al., 1998).
To additively drive A42 generation and create a very rapid AD amyloid model, we made transgenic mice that coexpress a total of five FAD mutations [APP K670N/M671L (Swedish) + I716V (Florida) + V717I (London) and PS1 M146L+ L286V]. These "5XFAD" transgenic mice develop cerebral amyloid plaques and gliosis at 2 months of age, achieve massive A42 burdens, and have reduced synaptic markers, increased p25 levels, neuron loss, and memory impairment in the Y-maze. Interestingly, we observe accumulation of intraneuronal A42 before plaques form. Intraneuronal A is aggregated, and amyloid plaques appear to originate from neuron cell bodies with intraneuronal A. Accumulation of intraneuronal A has been observed in the brains of AD (Gouras et al., 2000; Takahashi et al., 2002; Cataldo et al., 2004; Takahashi et al., 2004), Down's syndrome (DS) (Gouras et al., 2000; Gyure et al., 2001; Busciglio et al., 2002; Mori et al., 2002; Cataldo et al., 2004), and AD mouse models (Takahashi et al., 2002; Oddo et al., 2003; Schmitz et al., 2004), implying potential involvement of intraneuronal A in AD pathology (for review, see Echeverria and Cuello, 2002; Tseng et al., 2004; Gouras et al., 2005). Our results with 5XFAD mice suggest that intraneuronal A aggregates may have a role in neurodegeneration, neuron loss, and amyloid plaque formation.
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Materials and Methods
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Generation of transgenic mice.
The FAD mutations APP K670N/M671L (770 residue isoform numbering) + I716V + V717I and PS1 M146L + L286V were introduced into APP(695) and PS1 cDNAs by site-directed mutagenesis, then subcloned into exon 2 of the mouse Thy1 transgene cassette (Moechars et al., 1996), and sequenced following standard procedures. The APP transgene includes the 5' untranslated region, which contains a putative interleukin-1 (IL-1) translational enhancer element (Rogers et al., 1999). After purification of the transgenes from vector sequence, the transgenes were added together in equal proportions and microinjected into the pronuclei of single-cell C57/B6XSJL hybrid embryos by the staff at the Northwestern University Transgenic and Targeted Mutagenesis Laboratory (Hogan et al., 1994; Jankowsky et al., 2001; Oddo et al., 2003). Founder transgenic mice were identified by PCR and confirmed by Southern blot analysis. The three highest APP and PS1 transgene coexpressing lines (Tg6799, Tg7031, and Tg 7092) were bred with B6/SJL F1 hybrids (Taconic Farms, Germantown, NY) for additional analysis.
Immunoblot analysis.
Mice were anesthetized with pentobarbital (50 mg/kg) and transcardially perfused with PBS (Invitrogen, Carlsbad, CA) buffer containing protease inhibitor cocktail (Calbiochem, La Jolla, CA). Brains were removed and bisected down the midline; one hemibrain was used for biochemical analysis and the other for histological analysis. For immunoblots and ELISAs, hemibrains were homogenized in four volumes of PBS (Invitrogen) containing protease inhibitor cocktail (Calbiochem). Brain homogenates were then aliquoted into two equal portions, one for immunoblot analysis and the other for ELISA. Two times concentrated radioimmunoprecipitation assay buffer (100 mM NaCl, 1% NP-40, 0.25% sodium deoxycholate, 1% SDS, 1 mM EDTA, and 50 mM Tris HCl, pH 7.4) was added to the homogenate for immunoblotting and briefly sonicated. Protein concentrations were determined using a BCA kit (Pierce, Rockford, IL), and 10–20 µg of protein was run on 10 or 10–14.5% Tris-HCl SDS-PAGE gels (Bio-Rad, Hercules, CA). After transfer onto polyvinylidene difluoride membrane, blots were incubated in the following primary antibodies: anti-APP (22C11; Chemicon, Temecula, CA), 1:10,000; anti-PS1 N terminal (PS1NT) (gift from Gopal Thinakaran, University of Chicago, Chicago, IL) (Thinakaran et al., 1998), 1:5000; and anti-actin (Sigma, St. Louis, MO), 1:10,000. Peroxidase-conjugated secondary antibodies were applied, and immunoblot signals were detected by enhanced chemiluminescence [Amersham Biosciences (Arlington Heights, IL) or Pierce] and quantified using an Eastman Kodak (Rochester, NY) Image Analyzer.
For neuron marker and neurodegeneration pathway immunoblots, cortex homogenates were prepared in 1% Triton X-100, PBS, protease inhibitor cocktail (Calbiochem), and Halt Phosphatase Inhibitor Cocktail (Pierce). Protein concentrations were determined using a BCA kit (Pierce), and 5–15 µg of protein was run on 4–12% Bis–Tris gels (Invitrogen), immunoblotted as above, and incubated with the following antibodies: postsynaptic density-95 (PSD-95) (Chemicon), 1:1000; syntaxin (Chemicon), 1:1000; and p35 (Santa Cruz Biotechnology, Santa Cruz, CA), 1:1000. Detection was performed as described above.
A40 and A42 ELISAs.
For A ELISAs, PBS/protease inhibitor brain homogenates were supplemented with guanidine HCl to a final concentration of 5 M, sonicated briefly, and serially diluted with ELISA sample buffer. Final guanidine HCl concentrations were below 0.1 M. Protein concentrations were determined using a BCA kit (Pierce). Sample duplicates were then run on A40 and A42 specific sandwich colorimetric ELISAs following the protocol of the manufacturer (BioSource, Camarillo, CA). Optical densities at 450 nm of each well were read on a Victor 1420 plate reader (Wallac, Gaithersburg, MD), and sample A40 and A42 concentrations were determined by comparison with the A40 and A42 standard curves. All readings were in the linear range of the assay. Finally, sample A40 and A42 concentration values were normalized to total brain protein concentrations and expressed in nanograms of A per milligram total protein. The average of the duplicates was determined, and then the mean and SEM for each age of a given line was calculated.
Synaptophysin ELISA.
Synaptophysin levels in whole-brain homogenates were quantified with a capture ELISA as described previously (Schlaf et al., 1998), with the following modifications. The SY38 monoclonal synaptophysin antibody (Chemicon) was used to coat plates at the concentration of 1.75 µg/ml, whereas a rabbit polyclonal synaptophysin antibody (0.35 µg/ml; Calbiochem) and an HRP-conjugated goat anti-rabbit IgG antibody (1:10,000; Jackson ImmunoResearch, West Grove, PA) were used for detection with a tetramethylbenzidine development system (Sigma). Because of the lack of purified synaptophysin, a mouse corticohippocampal homogenate served as a standard, as described previously (Craft et al., 2004).
Histology and immunostaining.
After perfusion and dissection, one hemibrain of each mouse was fixed in paraformaldehyde/PBS and cryopreserved in 30% sucrose/PBS containing 0.01% sodium azide. Brains were sectioned sagittally on a freezing microtome at 30 µm. Serial sections were collected in 0.1 M phosphate buffer, pH 7.6. Free-floating sections (in most cases adjacent) were then incubated overnight at room temperature with the following primary antibodies: rabbit anti-A42 (1:2500; BioSource), rabbit anti-A40 (1:2500; BioSource), biotinylated mouse anti-A (4G8, 1:10,000; Signet Laboratories, Dedham, MA), rabbit anti-A (R1282, 1:500; gift from Dennis Selkoe, Harvard Medical School, Brigham & Women's Hospital, Boston, MA), rabbit anti-GFAP (G9269, 1:10,000; Sigma), rat anti-F4/80 (MCAP497, 1:10,000; Serotec, Oxford, UK), and anti-neuronal-specific nuclear protein (NeuN) (1:500; Sigma). After washes, the sections were incubated with secondary biotinylated goat anti-rabbit or goat anti-mouse at 1:2000 for 2 h at room temperature. The Vector Laboratories (Burlingame, CA) ABC kit was used with DAB as chromogen to visualize the reaction product. The sections were then mounted on charged slides, counterstained with hematoxylin, dehydrated in a series of alcohols, cleared in xylene, and coverslipped. In some cases, after primary antibody incubation, sections were prepared for immunofluorescence microscopy by incubating with FITC- or tetramethylrhodamine isothiocyanate-labeled goat anti-rabbit or goat anti-mouse secondary antibodies. Thioflavin S or thiazin red staining was also used to visualize amyloid. Cresyl violet was used to stain Nissl substance for visualizing neurons for estimating neuronal loss. Light microscopy was performed on a Nikon (Tokyo, Japan) E800 microscope with a Spot Advanced digital camera for capturing images, and confocal images were captured on a LSM510 META system (Zeiss, Oberkochen, Germany).
Spontaneous alternation Y-maze task.
Spontaneous alternation performance was tested as described previously (Ohno et al., 2004). Each mouse was placed in the center of the symmetrical Y-maze and was allowed to explore freely through the maze during an 8 min session. The sequence and total number of arms entered was recorded. Experiments were done blind with respect to the genotype of the mice. Percentage alternation is as follows: number of triads containing entries into all three arms/maximum possible alternations (the total number of arms entered – 2) x 100.
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Results
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Transgenic strategy and generation of 5XFAD mice
The majority of AD transgenic mouse models take  6–12 months, or longer, to form amyloid plaques (for review, see Spires and Hyman, 2005). Because many types of investigations would be facilitated by more rapid plaque development, we endeavored to accelerate amyloid deposition by combining multiple FAD mutations in transgenic mice. Previous studies have shown that mice coexpressing FAD mutant APP and PS1 transgenes exhibit additive increases in A42 production (Borchelt et al., 1996, 1997; Citron et al., 1997; Holcomb et al., 1998), although rarely have more than two A42-elevating FAD mutations been combined in transgenic animals. Intrigued by the reports that intramolecular combination of FAD mutations in either APP or PS1 act additively to increase A42 generation (Eckman et al., 1997; Citron et al., 1998), we established transgenic mouse lines that co-overexpress human APP695 with the Swedish (K670N, M671L), Florida (I716V), and London (V717I) FAD mutations in the same APP molecule and human PS1 harboring two FAD mutations, M146L and L286V (Fig. 1 A). The Swedish mutation increases the production of total A, whereas APP Florida and London, and PS1 M146L and L286V, specifically increase the production of A42 (for review, see Sisodia et al., 1999; Selkoe, 2001). From the previous studies, it seemed likely that coexpression of these A42-elevating mutations, in both intermolecular and intramolecular combination, would increase A42 generation in an additive manner in transgenic mice. Because A42 is thought to drive amyloid plaque formation and AD pathogenesis, we reasoned that these transgenics might exhibit more rapid amyloid deposition than previous models and allow us to investigate the overall effects of very high A42 levels in the brain.
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Figure 1. 5XFAD transgenes and expression levels. A, Schematic diagram of 5XFAD APP and PS1 transgenes. FAD mutations in Thy1–APP and Thy1–PS1 transgenes are indicated by arrowheads. Sw, Swedish mutation; Lon, London mutation; Fl, FL mutation. Small gray rectangles represent Thy1 exons. Coding regions of APP and PS1 are represented by larger rectangles and are shown inserted into Thy1 exon 2 of the mouse Thy1 transgene expression cassette (Moechars et al., 1996). The APP transgene has the 5' untranslated region (5'UTR) of APP containing an IL-1 responsive translational element (Rogers et al., 1999). B, Immunoblot analysis of 5XFAD lines showing expression levels of transgene-derived APP and PS1. Whole-brain homogenate (15 µg) from 6-month-old 5XFAD lines (Tg6799, Tg7092, and Tg7031), Tg2576, and nontransgenic controls were run on SDS-PAGE and immunoblotted, followed by detection with APP (22C11; top row) and PS1 (PS1NT; middle row) antibodies. Blots were stripped and incubated with actin antibody (bottom row) as a loading control. A representative selection of male and female mice for each line is shown. Note that 5XFAD lines express less APP than Tg2576, yet all develop amyloid deposits much earlier than Tg2576 (see Figs. 3, 4).
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Transgenic lines were produced by pronuclear coinjection of APP and PS1 transgenes, each using the neuron-specific mouse Thy1 promoter to drive overexpression in the brain (Moechars et al., 1996). Previous work has demonstrated that coinjection results in efficient transgene cointegration, often together at the same genomic locus, thus enabling stable germ-line transmission and transgene coinheritance (Jankowsky et al., 2001; Oddo et al., 2003). Of 17 total founders, four were positive for the APP transgene only, two were positive for the PS1 transgene only, and 11 were positive for both APP and PS1 transgenes (data not shown). Transgenic offspring of most of the bigenic founders were double positive for APP and PS1 transgenes, indicating stable genomic cointegration and germ-line transmission of both transgenes. Because the bigenics carry five FAD mutations, we collectively refer to them as 5XFAD mice.
To determine the levels of APP and PS1 transgene expression, hemizygous transgenic offspring of the 5XFAD founders were killed, and brain homogenates were prepared for immunoblot analysis with anti-APP (22C11) and anti-PS1NT (Thinakaran et al., 1998) antibodies (Fig. 1 B). After initial analyses, we chose for additional study three APP and PS1 coexpressing 5XFAD lines that overexpress APP at high (Tg6799), medium (Tg7092), and low (Tg7031) levels. The well established Tg2576 mouse model of AD, which overexpresses APP with the Swedish mutation (Hsiao et al., 1996), was used as a control in these studies and makes slightly more APP than our highest expressing line, Tg6799. The three 5XFAD lines have been maintained as hemizygotes on a B6/SJL hybrid background for more than 10 generations and show stable germ-line transmission and expression of both APP and PS1 transgenes, demonstrating that the 5XFAD mice breed as single transgenics.
5XFAD mice rapidly accumulate massive A42 levels in brain
To determine whether 5XFAD mice exhibited additively increased A42 production, we measured cerebral levels of A40 and A42 in whole-brain homogenates using specific sandwich ELISAs. As predicted, the three 5XFAD transgenic lines had dramatically higher levels of A42 than those of A40 (Fig. 2). A42 levels increased in a nearly linear manner as 5XFAD mice aged. The A42 load and the rate of the A42 increase were proportional to the level of APP transgene expression for a given line. For example, Tg6799 had the highest APP expression level, the greatest A42 burden (140 ng/mg total brain protein), and the fastest rate of A42 accumulation (Fig. 2A). In contrast, Tg7031 had the lowest levels of both APP and A42 (60 ng/mg total brain protein) and had the slowest rate of A42 increase (Fig. 2C).
Cerebral A42 levels began rising at very young ages in 5XFAD mice: 1.5, 2, and 4 months for Tg6799, Tg7092, and Tg7031, respectively (Fig. 2). For example, in the highest expressing line, Tg6799, at 1.5 months (the earliest age we tested), brain A42 levels were 0.3–0.7 ng/mg protein (background is 0.1 ng/mg), but, by 2 months, A42 levels rose to 9–21 ng/mg protein, a very steep increase in just 2 weeks. Interestingly, young 5XFAD mice produced A42 almost exclusively. With age, A40 levels also began to rise in transgenic brains, but the A40 increase typically lagged 2–3 months behind the A42 increase for a given line. In addition, the rate of the A40 increase was less than that of A42 for all lines. The A42/A40 ratios were very high in young mice, averaging 25, but decreased to 5 as a result of the increasing A40 levels with age.
Levels of A42 in the 5XFAD lines far exceeded those in Tg2576, which had 0.1–0.5 ng A42/mg total brain protein up to 9 months, 2 ng A42/mg total brain protein at 12 months, and 10 ng A42/mg total brain protein at 16 months (Fig. 2D). Moreover, the A42/A40 ratio of Tg2576 was much lower than that of the 5XFAD lines, reaching a maximum of 0.1–0.2 at 9–16 months. Finally, we noted that young female Tg6799 and Tg7092 mice tended to have slightly higher A42 levels than age-matched males, but this trend appeared to diminish at older ages. Together, our data demonstrate that 5XFAD mice accumulate massive amounts of cerebral A42 at young ages and generate much more A42 than A40, suggesting cumulative effects of the five FAD mutations on A42 production.
5XFAD mice display very early amyloid deposition and gliosis
Given the very high levels of A42 that rapidly accumulated in 5XFAD brains, we anticipated that 5XFAD mice would show abundant amyloid deposition at young ages. Indeed, 5XFAD brain sections processed for histological detection of amyloid exhibited robust plaque deposition that was proportional to cerebral A42 levels for a given line. Deposits were immunoreactive with 4G8 (anti-Atotal) (Fig. 3A–C), anti-A42, and anti-A40 end-specific antibodies (Fig. 4A–H) and were positive after staining with thioflavin S (Fig. 3E,F) and thiazin red (Fig. 3G), demonstrating that the deposits are composed of aggregated -pleated sheet amyloid.
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Figure 3. Amyloid deposition and gliosis in 5XFAD lines. Parasagittal serial sections of brains from Tg6799 (A, E–G), Tg7031 (B), Tg7092 (C), and nontransgenic control (D) mice were stained with anti-A (4G8; A–D), thioflavin S (E, F), or anti-GFAP and thiazin red (G) and imaged by bright-field (A–D) or confocal (E–G) microscopy. Ages of mice were 2 (E), 6 (A–D), and 7 (F, G) months. A–D, Shown are sections including the hippocampus and cortex of representative 6-month-old 5XFAD mice from each line stained with anti-A (brown) and hematoxylin (blue). Across the 5XFAD lines, the relative amounts of amyloid burden (and gliosis; data not shown) correlated with A42 levels as measured by ELISA (Fig. 2). Scale bar (in D): A–D, 1 mm. E, F, Brain sections of representative 2-month-old (E) and 7-month-old (F) Tg6799 mice were stained with thioflavin S (green). Amyloid deposits labeled strongly with thioflavin S, indicating that A was in an aggregated -pleated sheet conformation. Note that plaque sizes (20 µm) are similar to those of large neuron cell bodies (data not shown). Scale bar (in F): E, F, 20 µm. G, Activated astrocytes around a Tg6799 plaque. Brain section of a representative 7-month-old Tg6799 mouse costained with thiazin red (to label -pleated sheet amyloid) and anti-GFAP antibody (green). The astrocytes adjacent to the amyloid plaque display ramified processes and express GFAP, indicative of an activated phenotype associated with inflammation. Scale bar, 50 µm.
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Figure 4. Rapid cerebral amyloid deposition and gliosis in 5XFAD line Tg6799. Parasagittal serial sections of brains from 2 (A, E, I, M), 4 (B, F, J, N), 6 (C, G, K, O), and 9 (D, H, L, P) month Tg6799 mice were stained with antibodies recognizing A42 C terminus (A–D), A40 C terminus (E–H), GFAP (I–L), and F4/80 (M–P) and counterstained with hematoxylin. Shown are sections including the hippocampus and cortex of representative Tg6799 mice from each age. Amyloid deposition began in the deep cortex and subiculum at 2 months in this line and then spread into other brain regions at older ages. Note that A42 staining is much stronger than that of A40 at every age and that the densities of astrocytes (GFAP) and microglia (F4/80) parallel that of the A42 staining. Scale bar, 1 mm.
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Tg6799, the line with the highest A42 levels, showed the earliest amyloid deposition by anti-A42 immunohistochemistry and thioflavin S staining, starting at 2 months (Figs. 3E, 4A) and following closely the initial rise in A42 level by ELISA observed at 1.5 months (Fig. 2A). Deposition in Tg7092 and Tg7031 was delayed relative to that in Tg6799, beginning at 4 months (data not shown) and 6 months (Fig. 3B), respectively, reflecting the correspondingly lower A42 levels for these lines. In contrast, Tg2576 mice did not begin to deposit amyloid until 9–12 months of age (data not shown) (Hsiao et al., 1996). As expected, the rate of deposition and the total amyloid burden in 5XFAD mice were directly proportional to cerebral A42 levels for a given line; amyloid deposition increased rapidly in Tg6799 with age, reaching massive levels by 6 months (Fig. 4C), whereas the plaque loads in Tg7092 and Tg7031 increased more slowly and were quantitatively less than that of Tg6799 (data not shown). We also performed anti-A40 immunohistochemistry on Tg6799 brain sections and observed substantially weaker A40 immunoreactivity than that of A42 in amyloid deposits (Fig. 4E–H), thus paralleling the lower A40 levels as measured by ELISA (Fig. 2A).
All three 5XFAD lines had qualitatively similar spatial patterns of amyloid deposition in the brain. In young mice, plaques first appeared in deep layers of the cortex and in the subiculum (Fig. 4A,B). As mice aged, amyloid deposits spread to fill much of the cortex, subiculum, and hippocampus (Fig. 4C,D). Plaques were also observed in thalamus, brainstem, and olfactory bulb in older mice, but deposits were less numerous in these brain regions (data not shown). Amyloid deposition did not appear in the cerebellum of 5XFAD mice (data not shown). As expected, the spatial pattern of plaques in 5XFAD mice agreed well with those of previously reported Thy1 promoter-driven APP transgenic mice (Sturchler-Pierrat et al., 1997; Moechars et al., 1999; Oddo et al., 2003). Interestingly, amyloid deposits in 5XFAD mice were typically smaller (20 µm) but vastly more numerous than those observed in Tg2576 (data not shown), possibly because elevated A42 levels may have resulted in greater plaque seed density in the 5XFAD lines. Together, our results demonstrate that the very high cerebral A42 levels caused by the five FAD mutations drive the early formation of amyloid deposits that rapidly increase to large numbers, most notably in 5XFAD line Tg6799.
Neuroinflammation is a hallmark of AD brain and is characterized by the presence of activated astrocytes and microglia surrounding amyloid plaques (for review, see Akiyama et al., 2000). Similar to AD, APP transgenic mouse models have elevated inflammation markers and gliosis associated with amyloid deposits (Games et al., 1995; Hsiao et al., 1996; Sturchler-Pierrat et al., 1997). The 5XFAD lines also exhibited neuroinflammation, as demonstrated by astrogliosis and microgliosis (Figs. 3G, 4I–P). Immunostaining for glial activation markers GFAP (astrocytes) and F4/80 (microglia) revealed that gliosis was proportional to A42 levels and amyloid deposition in 5XFAD brains and began at approximately the time when plaques initially appeared in each line. Tg6799 had GFAP-positive astrocytes and F4/80-positive microglia beginning at 2 months of age (Fig. 4I,M), whereas the appearance of activated glia in Tg7092 and Tg7031 started at 4 and 6 months, respectively (data not shown). The number of activated astrocytes and microglia increased with age for each line, paralleling the age-related rise in amyloid burden. By 9 months, Tg6799 had robust gliosis in cortex and hippocampus (Fig. 4L,P), whereas gliosis in Tg2576 did not become significant until after 9 months of age (data not shown). The spatial pattern of gliosis in 5XFAD brain closely followed the distribution of amyloid deposits (Fig. 4I–P). Similar to AD, GFAP-immunoreactive astrocytes were often observed surrounding amyloid deposits in 5XFAD brain (Fig. 3G). As a whole, our data indicate that 5XFAD mice display characteristics of neuroinflammation that appear similar to those observed in AD brain.
In addition to amyloid plaques, neurofibrillary tangles composed of hyperphosphorylated tau are characteristic lesions found in AD brain (Lee et al., 1991). To determine whether our 5XFAD mice exhibited abnormal tau phosphorylation similar to that observed in neurofibrillary tangles, we immunostained sections of Tg6799 brain from aged mice with antibody AT8 (Biernat et al., 1992). We did not observe significant staining of 5XFAD brain sections with this abnormal tau phosphorylation antibody (data not shown), but the presence of other phospho-tau epitopes has not yet been investigated. Similar to other APP single and APP/PS1 double-transgenic mice, we did not notice any neurofibrillary tangles in 5XFAD brain.
5XFAD mice have robust intraneuronal A labeling
Recent studies have reported intraneuronal A in AD, Down's syndrome, and APP transgenic brains (for review, see Echeverria and Cuello, 2002; Tseng et al., 2004; Gouras et al., 2005), suggesting that intraneuronal A may play a role in AD pathology. In some cases, plaques in AD brain have appeared to originate from neuron cell bodies that contained intraneuronal A (Gouras et al., 2000; D'Andrea et al., 2001). Interestingly, we also observed intraneuronal A in the brains of 5XFAD mice, especially in the highest expressing line, Tg6799. Immunostaining of Tg6799 brain sections with anti-A42 C terminus, 4G8, and R1282 (anti-Atotal) (Joachim et al., 1991) antibodies revealed strong subcellular labeling primarily within large pyramidal neurons of cortical layer 5 and the subiculum (Fig. 5A–C,G) (supplemental data, available at www.jneurosci.org as supplemental material). Anti-A42 end-specific immunoreactivity was predominantly punctate, suggesting that A42 accumulation occurred within vesicular compartments (Fig. 5A,C). The anti-A42 C terminus antibody does not recognize full-length APP or APP C-terminal fragments (CTFs); therefore, the staining pattern accurately reflects A42 intraneuronal localization. The intraneuronal A immunostaining first appeared at 1.5 months of age in Tg6799 (Fig. 5A, inset), coinciding with the initial rise in cerebral A42 levels and occurring immediately before the formation of amyloid deposits at 2 months in this line. Staining with 4G8 (Fig. 5B) and R1282 (Fig. 5G) (supplemental data, available at www.jneurosci.org as supplemental material) antibodies also showed punctate intraneuronal labeling, as well as diffuse lower-intensity staining in some neurons. In addition to total A, 4G8 and R1282 also recognize full-length APP and APP CTFs, which may be responsible for this diffuse immunostaining. It is noteworthy that large 4G8-labeled intraneuronal accumulations were observed near the region of the axon hillock (Fig. 5B, black arrows).
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Figure 5. Intraneuronal A accumulation in Tg6799: intracellular A aggregates and plaque formation. Brain sections from representative 1.5- to 6-month-old Tg6799 mice were processed for immunocytochemistry with anti-A antibodies (A–C, G) or stained with thioflavin S (D–F). Some sections were counterstained with hematoxylin (A, B) or with an antibody that recognizes the neuronal marker NeuN (green stain in C, G). Anti-A antibodies used were specific for the C terminus of A42 (A, brown; C, red) or recognized all forms of A (B, 4G8, brown; G, R1282, red). Tg6799 ages were 1.5 (A, inset), 2 (A, C, D, F, G), 3 (E), and 6 (B) months. Intraneuronal A accumulations were primarily observed as small puncta, although occasional large irregular accumulations were seen near the axon hillock (black arrows; B). Importantly, thioflavin S staining revealed intraneuronal A aggregates consisting of -pleated sheet amyloid accumulations within soma (punctate signals; D, E) and neurites (linear structures, white arrows; F). Note the thioflavin S-positive amyloid plaque (right; E). In some sections (G), an amyloid deposit (white arrowhead) was observed to originate from a neuron cell body with abnormal, disrupted-appearing morphology. This neuron had very little anti-NeuN antibody staining (green), indicating that it was likely in the process of degeneration. In addition, other neurons in the section appeared to be in various stages of degeneration (e.g., bottom right; G) and were also in close proximity to amyloid plaques (e.g., far left center; G). Note the presence of A-filled neurites passing through the section (red linear structures, white arrows; G). Interestingly, plaque sizes were typically of the same magnitude as neuronal soma. Additional amyloid plaques can be seen at the bottom left in B and at the top right in G. For a movie of a three-dimensional reconstruction of the Z-stack sections in G, see supplemental material (available at www.jneurosci.org). Scale bars, 20 µm.
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The observation of intense intraneuronal A42 immunostaining in Tg6799 suggested that A42 concentrations within intracellular puncta may have been high and implied the possibility that intraneuronal A42 could have been aggregated. To investigate this hypothesis, we examined thioflavin S-stained Tg6799 brain sections for labeled intraneuronal puncta. Indeed, thioflavin S staining revealed a punctate, subcellular pattern within cell bodies of large pyramidal neurons of Tg6799 brain (Fig. 5D,E), demonstrating that intraneuronal A42 had formed -pleated sheet aggregates. These thioflavin S-positive puncta were of similar number and spatial pattern as the intraneuronal A42-immunostained puncta and were not observed in negative control mice (data not shown). The approximate 1:1 ratio of thioflavin S-positive and A42-positive puncta suggested that much of the intraneuronal A42 was in an aggregated state. In addition to puncta within neuron cell bodies, thioflavin S-positive linear structures appearing to be neurites were observed in Tg6799 cortex (Fig. 5F). Together, these observations suggest that intraneuronal A42 concentrations are high enough in intracellular compartments to form aggregates within the cell bodies and neurites of large pyramidal neurons in Tg6799 mice.
The presence of thioflavin S-positive intracellular A42 aggregates within Tg6799 neurons suggested the possibility of an "inside-out" process in which intraneuronal A42 aggregates lead to neurodegeneration and amyloid plaque formation. If so, we reasoned that we might observe neurons at a stage of degeneration with plaques appearing to originate from cell bodies. Indeed, Tg6799 brain sections stained with anti-A antibody occasionally showed intraneuronal A-containing soma in close physical association with amyloid deposits (Fig. 5G, arrowhead) (supplemental plaque seed movie, available at www.jneurosci.org as supplemental material). These neurons stained weakly with antibodies that recognize the neuronal marker NeuN and had abnormal morphologies, suggesting that the neurons were in the process of degeneration. Plaque-associated neurons were relatively rare within Tg6799 brain sections, implying that only a few neurons had made the transition to this stage at the time of fixation.
In support of the hypothesis that some plaques may form from intraneuronal A aggregates within degenerating neurons, we observed that the highest density of amyloid deposits occurred in deep cortical layers and subiculum, the same regions that had the greatest number of intraneuronal A-containing neurons in Tg6799 brain. Some neurites were also labeled with anti-A antibody (Fig. 5G, arrows). As a whole, our results show that (1) 5XFAD mice accumulate intraneuronal A before the start of amyloid deposition, (2) intraneuronal A aggregates occur mainly in large pyramidal neurons of deep cortical layers and subiculum, and (3) some amyloid plaques appear to originate from intracellular A-containing neurons that have abnormal, degenerated morphologies.
5XFAD mice exhibit neurodegeneration and neuron loss
Given our observations that some 5XFAD neurons contained intraneuronal A aggregates, displayed disrupted-appearing morphologies, and were in close physical contact with amyloid deposits, we hypothesized that intraneuronal A might be associated with neurodegeneration and neuron loss in 5XFAD brain. To initially investigate this possibility, we measured synaptophysin levels in whole-brain homogenates of Tg6799 mice by ELISA, which has greater accuracy and precision than immunoblot analysis. We observed that whole-brain synaptophysin levels decreased in Tg6799 brains beginning at 4 months of age and that, by 9 months, synaptophysin levels were 75% of those in age-matched nontransgenic controls (Fig. 6A), demonstrating significant degeneration of synapses in 5XFAD mice. To confirm these results, we performed immunoblot analysis of homogenates from cortexes of 3-, 9-, and 12-month-old Tg6799 mice with antibodies against syntaxin and PSD-95 (Fig. 6B,C) and found that the levels of these synaptic markers were also reduced at 9 and 12 months of age compared with control. Together, these results demonstrate synaptic degeneration in Tg6799 brain.
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Figure 6. Reduced synaptophysin, syntaxin, and PSD-95 levels in Tg6799: synaptic degeneration. A, Whole-brain homogenates from 2- to 12-month-old Tg6799 and 9-month-old nontransgenic control (9C) mice were analyzed for synaptophysin by ELISA. Synaptophysin levels are expressed as the percentage of 9-month-old control whole-brain synaptophysin levels (9C is 100%). No significant gender differences were observed in Tg6799 synaptophysin levels at any given age (data not shown), so values from age-matched males and females were pooled (3 mice for each gender and age). Note the steady decline in synaptophysin levels starting at 4 months in Tg6799, eventually falling to 75% of control levels at 9 months. B, C, Immunoblot analysis of synaptic markers syntaxin and PSD-95 in cortex homogenates (15 mg) from Tg6799 (Tg) and nontransgenic (wild type, WT) mice (3, 9, and 12 months old). Equal loading was determined by ponceau red staining of the blots (data not shown). Immunoblot signals were captured using a PhosphorImager (B), quantified, and expressed as percentage of age-matched control (C). Note that synaptic markers are significantly reduced by 9 months of age in Tg6799, indicating neurodegeneration. Error bars represent SEM.
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Because of the spatial pattern of intraneuronal A, we suspected that degeneration in Tg6799 may be restricted to specific neuronal populations. We reasoned that we might observe loss of certain neuron subpopulations in Tg6799 brain and that loss would most likely occur in the intracellular A-containing neuron populations. To test this, we stained brain sections of 9-month-old Tg6799 and nontransgenic controls with cresyl violet and examined them for evidence of neuron loss. As predicted, we found that large pyramidal neurons in cortical layer 5 were visibly reduced in number in Tg6799 compared with control (Fig. 7A–D). Moreover, cortical layer 1 was significantly thinner in Tg6799 relative to control (Fig. 7A,B), most likely attributable to the loss of layer 5 neuron dendrites that project to and ramify in layer 1. In addition, neurons in Tg6799 subiculum appeared very pale or were missing entirely (Fig. 7F). Neurons in other cortical layers, hippocampus, and elsewhere in the brain appeared relatively intact by visual inspection, although we did not perform neuron counting and it is possible that additional neuron populations were also affected.
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Figure 7. Neuron loss in cortical layer 5 and subiculum of Tg6799. Parasagittal sections of representative 9-month-old nontransgenic (Non-Tg) control (A, C, E) and Tg6799 (B, D, F) brains were stained with cresyl violet and micrographed to image layer 5 cortex (A–D) and subiculum (E, F). Numbers indicate cortical layers, and dashed lines identify boundaries between layers. Boxes in A and B delineate areas of cortex shown at higher magnification in C and D, respectively, to clearly visualize layer 5. B, D, Note that large pyramidal neurons in cortical layer 5 are visibly reduced in number in Tg6799. Moreover, layer 1 of Tg6799 cortex (B) is thinner than that of nontransgenics (A). Neuron loss is also visible in Tg6799 subiculum (oval, F) compared with that of nontransgenics (oval, E). In addition, note the large number of glia in Tg6799 subiculum (small darkly staining cells, F). Neurons are distinguishable from glial cells because of the larger size of neuronal cell body and the usual appearance of a prominent nuclear nucleolus. Layer 5 and subiculum exhibited the highest levels of both intraneuronal A accumulation and amyloid deposition in Tg6799 (for A42 immunostaining of a section adjacent to that in B, see Fig. 4D) Scale bar (in B): A, B, 1 mm; C–F, 100 µm.
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It is important to note that the neuron loss in cortical layer 5 and subiculum occurred in the brain regions with the highest levels of both intraneuronal A accumulation and amyloid plaque burden (Fig. 4D). We also observed that glial cells, identified by small nuclei that stained darkly with cresyl violet, were present in much larger numbers throughout the plaque-bearing regions of Tg6799 brain (Fig. 7F) compared with nonplaque regions and control. Neurons were easily distinguished from glial cells based on the larger neuron cell body and the prominent nuclear nucleolus. Together, our results indicate that 5XFAD mice exhibit significant neurodegeneration and loss of large pyramidal neurons, which appear to correlate with intraneuronal A and amyloid plaques, respectively.
To gain insight into the molecular mechanism of synaptic degeneration and neuron loss in Tg6799, we performed immunoblot analysis of cortex homogenates from 3-, 9-, and 12-month-old mice using an antibody against the neurodegeneration pathway marker p25. We found that levels of p25 were increased to 150% of control in Tg6799 cortex at 9 and 12 months, with an upward trend at 3 months when intraneuronal A aggregates were present (Fig. 8A,B). Thus, elevated p25 correlates with synaptic degeneration and neuron loss in 5XFAD brain and may be associated with intraneuronal A aggregates.
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Figure 8. p25 levels are increased in Tg6799 mice. Immunoblot analysis of the cdk5 activating subunit p25 in cortex homogenates (15 mg) from Tg6799 (Tg) and nontransgenic (wild-type, WT) mice (3, 9, and 12 months old). Equal loading was determined by ponceau red staining of the blots (data not shown). Immunoblot signals were captured using a PhosphorImager (A), quantified, and expressed as percentage of age-matched control (B). Note that p25 levels are significantly elevated by 9 months of age in Tg6799 but that a trend toward higher values can be seen at 3 months. Error bars represent SEM.
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5XFAD mice develop spatial memory deficits
AD is an amnestic disorder, and it has been shown that high cerebral A levels correlate with memory impairments in APP transgenic mice (for review, see Ashe, 2001). To determine whether our 5XFAD mice also develop behavioral deficits, we tested 2-month-old and 4- to 5-month-old Tg6799 mice for spontaneous alternation performance in the Y-maze (Ohno et al., 2004). This learning task does not involve any training, reward, or punishment and allowed us to assess hippocampus-dependent spatial working memory in Tg6799. At 2 months of age, spontaneous alternation in the Y-maze for Tg6799 was similar to that for age-matched nontransgenic littermates. However, by 4–5 months of age, Tg6799 mice were significantly impaired in this task compared with nontransgenic control mice (Fig. 9A). The number of arms entered during the test was comparable for Tg6799 and control mice at both ages, indicating that Tg6799 had normal motor function and exploratory activity (Fig. 9B). Tg6799 mice have also been tested in trace and contextual fear conditioning paradigms and the Morris water maze, and they also exhibited deficits in these other hippocampus-dependent memory tasks (Ohno et al., 2006). These results demonstrate that, similar to other AD transgenic models, 5XFAD mice develop memory deficits with age.
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Figure 9. Memory deficits in Tg6799 mice with age. A, Spatial working memory of Tg6799 and nontransgenic littermate (Wild-type) mice was assessed by spontaneous alternation in the Y-maze (n = 12–20). Tg6799 mice showed normal alternation performance in the Y-maze at 2 months of age, but they performed poorly at 4–5 months of age (only slightly >50% chance levels) compared with nontransgenic littermate mice (F(3,62) = 13.96; p < 0.01). B, The total number of arm entries was not different between Tg6799 and nontransgenic (Wild-type) control mice, indicating similar levels of motor and exploratory activity in the Y-maze (n = 12–21). Each column represents the mean ± SEM. **p < 0.01 versus nontransgenic compared by ANOVA and post hoc Fisher's PLSD test.
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Discussion
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5XFAD mice: rapid amyloid pathology models
To substantially accelerate amyloid deposition in vivo, we made transgenic mouse lines that co-overexpress APP with three FAD mutations (K670N/M671L, I716V, and V717I) and PS1 with two FAD mutations (M146L and L286V) with the neuron-specific Thy1 promoter. 5XFAD mice breed as single transgenics and produce massive levels of cerebral A42, far exceeding those of A40. Other AD transgenic mice have demonstrated that A42-elevating FAD mutations in APP and PS1 additively increase A42 production and accelerate amyloid deposition when in intermolecular combination (for review, see Spires and Hyman, 2005). Here, we show that FAD mutations when combined together both intramolecularly and intermolecularly act in an additive manner to markedly increase the generation of A42 in vivo. As a consequence, 5XFAD mice develop AD-like amyloid pathology starting at a very young age (2 months, in line Tg6799). The 5XFAD pathologic phenotype consists of amyloid plaques, gliosis, neurodegeneration, and memory deficits. In addition, 5XFAD mice exhibit intraneuronal A and obvious neuron loss, a fundamental characteristic of AD lacking in most AD transgenic models.
Recent studies have described intraneuronal A accumulation in AD and DS brain and have reported that amyloid plaques appear to originate from neuron cell bodies or processes (for review, see Echeverria and Cuello, 2002; Tseng et al., 2004; Gouras et al., 2005). Some AD transgenic mice also display intraneuronal A (Takahashi et al., 2002; Oddo et al., 2003; Schmitz et al., 2004). Importantly, 5XFAD intraneuronal A aggregates into -pleated sheet amyloid, as determined by thioflavin S staining, and it labels with anti-A42 end-specific antibody and can appear physically associated with amyloid plaques originating from neurons, similar to AD and DS.
We did not expect 5XFAD mice to develop neurofibrillary tangles, because tangle pathology has not been reported in APP single- or APP/PS1 double-transgenic mice. However, unlike other APP transgenic mice, 5XFAD did not display abnormally phosphorylated tau epitopes (Sturchler-Pierrat et al., 1997). The reason for the lack of phospho-tau immunoreactivity in 5XFAD brain is unclear, and additional analyses of pathologic tau epitopes in 5XFAD are required. Transgenic mice expressing human tau with the P301L frontotemporal dementia mutation develop neurofibrillary tangles when coexpressing an FAD mutant APP transgene (Lewis et al., 2001; Oddo et al., 2003) or after injection with A42 (Gotz et al., 2001), indicating that A42 promotes tangle formation. Crosses of 5XFAD with P301L tau mice will be valuable for investigating the effects of very high A42 levels on the development of neurofibrillary tangles.
Although 5XFAD mice recapitulate major characteristics of AD-relevant amyloid pathology, caveats must be considered when interpreting the 5XFAD phenotype and its relationship to human AD. First, no cases of AD are caused by multiple FAD mutations, and unanticipated effects on APP processing could potentially occur as a consequence of the mutation combination in 5XFAD mice. Second, the A42/A40 ratio appears to be higher in 5XFAD than in human AD, thus raising the possibility that a greater level of A42 toxicity exists in 5XFAD than is typical in AD brain. In general, all AD transgenic mouse models face similar criticisms because of the overexpression of one or more FAD mutations, yet they have provided invaluable insight into AD pathogenesis and therapeutic strategies. The fact that 5XFAD amyloid pathology is similar to, but more rapid than, that found in AD and other AD transgenics indicates that 5XFAD mice are potentially relevant and useful models of AD-like amyloidosis, although, like all animal models, caution should be exercised when relating the 5XFAD phenotype to human AD.
Intraneuronal A, neurodegeneration, and amyloid plaque formation
In the highest expressing 5XFAD line, Tg6799, intraneuronal A is evident at 1.5 months of age, just before the first appearance of amyloid deposits at 2 months. In DS and APP transgenics, intraneuronal A accumulation has also been observed before the formation of plaques (Gyure et al., 2001; Busciglio et al., 2002; Oddo et al., 2003; Cataldo et al., 2004; Schmitz et al., 2004), suggesting the possibility that build-up of A within neurons may play a role in plaque formation and neurodegeneration. Importantly, intraneuronal A42 was observed in the brains of young (3–4 years old) DS patients (Gouras et al., 2000; Mori et al., 2002), years before plaques develop. In Tg6799, intraneuronal A accumulation is prominent within large pyramidal neurons of layer 5 cortex and subiculum, possibly a result of the Thy1 transgene promoter expression pattern (Feng et al., 2000). Much of the intraneuronal A is within soma, although intracellular A is also observed in neuronal processes. Immunoreactivity with anti-A42 end-specific antibodies demonstrates that intraneuronal staining identifies bona fide A42 rather than APP or APP CTFs.
Intraneuronal A labeling in 5XFAD brain is primarily punctate, suggesting vesicular compartmentalization. We have not yet determined the subcellular compartments in which intraneuronal A inclusions occur. Based on extensive intracellular localization studies of APP and the secretases, we speculate that aggregated intraneuronal A likely occurs within acidic compartments such as endosomes. Interestingly, Takahashi et al. (2002) have identified multi-vesicular bodies, or late endosomes, as compartments in which intracellular A accumulates in AD and APP transgenic brains. We also observe large intraneuronal A accumulations occurring near the axon hillock. This latter observation, together with anti-A antibody and thioflavin S staining in neurites, suggests that aggregated intraneuronal A may interfere with axonal and/or dendritic transport. Future studies will determine the subcellular compartments in which A accumulates and the effects of intraneuronal A aggregates on intracellular trafficking in 5XFAD mice.
-Sheet-structured A may be neurotoxic (Urbanc et al., 2002), and several observations suggest that the thioflavin S-positive intraneuronal A aggregates in 5XFAD mice may cause neurodegeneration: (1) presynaptic markers synaptophysin and syntaxin are reduced; (2) postsynaptic marker PSD-95 is reduced; (3) intraneuronal A-containing neurons frequently exhibit weak NeuN immunostaining and abnormal morphologies and sometimes are physically associated with amyloid deposits; (4) large pyramidal neurons of layer 5 cortex and subiculum are markedly lost, exhibit prominent intraneuronal A staining, and are located in regions of high plaque burden; and (5) p25 levels are increased. Importantly, p25 elevation may be an early event in 5XFAD brain, trending upward by 3 months of age and temporally coinciding with the accumulation of intraneuronal A. By 9 months of age, the p25 increase in 5XFAD brain is significant and correlates with marked synaptic degeneration and neuron loss. Calpain cleavage generates p25, which in turn activates cyclin-dependent kinase 5 (cdk5), a potential player in the connection between A toxicity, neurodegeneration, and neurofibrillary tangle formation in AD (for review, see Cruz and Tsai, 2004). Although our work does not unequivocally prove that intraneuronal A aggregates cause neuronal degeneration, it provides initial insights into a potential molecular mechanism that may link intraneuronal A and neurodegeneration. Taken as a whole, our results suggest that intraneuronal A42 aggregates may play a role in neurodegeneration, neuron loss, and the formation of amyloid plaques.
Robust neuronal loss has not been observed in most APP transgenic mouse models. However, a recent APP/PS1 line coexpressing APP K670N/M671L plus V717I and PS1 M233T plus L235P (APPSLPS1KI) exhibits significant neuron death in CA1/2 of the hippocampus (Casas et al., 2004; Schmitz et al., 2004). Like 5XFAD mice, the neuron loss in APPSLPS1KI mice is preceded by intraneuronal A, although intraneuronal A does not appear to cause amyloid plaque formation in this model. Other APP transgenics also display intraneuronal A but do not have significant neuron death (Takahashi et al., 2002; Oddo et al., 2003 |
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Abstract
Introduction
