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The Journal of Neuroscience, May 31, 2006, 26(22):6103-6114; doi:10.1523/JNEUROSCI.4245-05.2006
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Neurobiology of Disease
Tau Aggregation and Progressive Neuronal Degeneration in the Absence of Changes in Spine Density and Morphology after Targeted Expression of Alzheimer's Disease-Relevant Tau Constructs in Organotypic Hippocampal Slices
Neelam Shahani,1 Srinivasa Subramaniam,2 Tobias Wolf,1 Christian Tackenberg,1 andRoland Brandt1 1Department of Neurobiology, University of Osnabrück, 49076 Osnabrück, Germany, and 2Neuroanatomy and Interdisciplinary Center for Neurosciences, University of Heidelberg, 69120 Heidelberg, Germany
Abstract
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Abstract
Introduction
Alzheimer's disease (AD) is characterized by progressive loss of neurons in selected brain regions, extracellular accumulations of amyloid, and intracellular fibrils containing hyperphosphorylated tau. Tau mutations in familial tauopathies confirmed a central role of tau pathology; however, the role of tau alteration and the sequence of tau-dependent neurodegeneration in AD remain elusive. Using Sindbis virus-mediated expression of AD-relevant tau constructs in hippocampal slices, we show that disease-like tau modifications affect tau phosphorylation at selected sites, induce Alz50/MC1-reactive pathological tau conformation, cause accumulation of insoluble tau, and induce region-specific neurodegeneration. Live imaging demonstrates that tau-dependent degeneration is associated with the development of a "ballooned" phenotype, a distinct feature of cell death. Spine density and morphology is not altered as judged from algorithm-based evaluation of dendritic spines, suggesting that synaptic integrity is remarkably stable against tau-dependent degeneration. The data provide evidence that tau-induced cell death involves apoptotic as well as nonapoptotic mechanisms. Furthermore, they demonstrate that targeted expression of tau in hippocampal slices provides a novel model to analyze tau modification and spatiotemporal dynamics of tau-dependent neurodegeneration in an authentic CNS environment.
Key words: Sindbis virus; tauopathy; hippocampus; neurodegeneration; spines; phosphorylation
Introduction
Tau alteration and dysfunction and extensive neuron loss has long been associated with several neurodegenerative diseases now collectively called tauopathies. In tauopathies such as Alzheimer's disease (AD) and frontotemporal dementia and parkinsonism linked to chromosome 17 (FTDP-17), tau is abnormally and hyperphosphorylated and is accumulated as intracellular neurofibrillary tangles (NFTs) (Lee et al., 2001; Shahani and Brandt, 2002
Abnormal phosphorylation of tau is considered one of the earliest signs of neuronal degeneration and appears to precede tau aggregation or amyloid formation (Braak et al., 1994
Glutamate is commonly used as a mimic of phosphoserine or phosphothreonine because of similar steric and electrostatic properties (Huffine and Scholtz, 1996
Slice cultures combine the accessibility and maintenance of in vitro culture systems while preserving intact the hippocampal synaptic circuitry and anatomy. Here we show that tau constructs are efficiently expressed in individual neurons of hippocampal slices using recombinant Sindbis virus. The enhanced green fluorescent protein (EGFP) tag allows an excellent visualization of all cellular compartments down to single dendritic spines of proximal and distal dendrites. We show that tau modifications induce region-specific neurodegeneration, cause accumulation of insoluble tau, induce distinct pathological tau conformations, and affect tau phosphorylation at selected sites. Three-dimensional reconstructions of individual neurons suggest that synaptic integrity is remarkably stable against tau-dependent degeneration.
Materials and Methods
Materials. Chemicals were purchased from Sigma (Deisenhofen, Germany). Cell culture media and supplements were obtained from Sigma and Invitrogen (Gaithersburg, MD), and culture flasks, plates, and dishes were obtained from Nunc (Roskilde, Denmark), unless stated otherwise.Construction of Sindbis virus expression vectors. Eukaryotic expression plasmids for adult [441 amino acids (aa)] and fetal (352 aa) human tau with N-terminally fused EGFP were constructed in pHSV expression vectors. PHP tau was constructed by changing the codons for S198, S199, S202, T231, S235, S396, S404, S409, S413, and S422 to glutamate as described previously (Eidenmüller et al., 2000
pSinRep5–EGFP–tau constructs, pSinRep5–EGFP, and helper DH (26S) DNA (which encodes the structural proteins of the Sindbis virus; S. Schlesinger) were then transcribed in vitro (mMessage Machine SP6 kit; Ambion, Huntingdon, UK). The recombinant RNA and helper DH (26S) RNA were coelectroporated into baby hamster kidney (BHK) cells using the Gene Pulser II electroporation system (Bio-Rad, München, Germany). The recombinant RNA encoding EGFP–tau or EGFP alone was packaged and enveloped by the structural proteins produced by the helper RNA. The replication-incompetent pseudovirions thus produced and released into the extracellular medium were harvested after 24 h and filtered and stored at –80°C. The titer tested on BHK cells ranged from 1.7 to 3.0 x 108 infectious particles per milliliter for different constructs.
Organotypic hippocampal slice cultures and Sindbis virus infections. Organotypic slice cultures from hippocampus were prepared according to the technique described by Stoppini et al. (1991)
Antibodies. The following primary antibodies were used, and specificity and sources are given in parentheses: phosphorylation-independent human tau antibodies: Tau-5 (mouse; PharMingen, San Diego, CA), anti-human tau protein antiserum (rabbit; Biosource, Camarillo, CA); phosphorylation-dependent and site-specific tau antibodies: AT270 (Thr-181; mouse; Pierce, Rockford, IL), pT205 (Thr-205; rabbit; Biosource), pT212 (Thr-212; rabbit; Biosource), pS214 (Ser-214; rabbit; Biosource), pS262 (Ser-262; rabbit; Biosource), pS356 (Ser-356; rabbit; Biosource); conformation-dependent tau antibodies: Alz-50 (7–9, 312–342; mouse; a generous gift from Peter Davies, Albert Einstein College of Medicine, Bronx, NY), MC1 (7–9, 312–342; mouse; P. Davies); anti-GFP antibody (rabbit; Invitrogen). As secondary antibodies, cyanine 3 (Cy3)-coupled anti-rabbit antibody (Dianova, Hamburg, Germany) and peroxidase-conjugated anti-mouse and anti-rabbit antibodies (Jackson ImmunoResearch, West Grove, PA) were used.
Immunohistochemistry. Infected hippocampal slices were left attached on the insert membranes throughout the immunostaining protocol to preserve the hippocampal structure and to ensure even penetration of antibodies inside the tissue. Slices were first washed with PBS and fixed with 4% paraformaldehyde in PBS containing 4% sucrose for 1 h at 4°C. After washing with PBS, slices were treated with 0.4% Triton X-100 in PBS for 90 min and then 50 mM ammonium chloride for 45 min at room temperature and blocked with PBS containing 5% fetal calf serum, 1% BSA, 0.1% Triton X-100, and 0.02% NaN3 at 4°C overnight. Slices were then incubated for 2–3 d at 4°C with primary antibodies diluted in PBS containing 5% fetal calf serum, 1% BSA, 0.1% Triton X-100, and 0.1% NaN3. After washing with PBS, they were incubated with Cy3-coupled anti-rabbit antibody for 2 d at 4°C. The slices were then washed in PBS, mounted in Confocal-Matrix (Micro-Tech-Lab, Graz, Austria) or Vectashield (Vector Laboratories, Burlingame, CA), and coverslipped.
Confocal imaging of fixed and live hippocampal slices. All images were acquired on Nikon (Tokyo, Japan) laser scanning microscope (Nikon Eclipse TE2000-U inverted), equipped with C1 confocal laser scanning unit, argon (Ar; 488 nm), helium/neon (He/Ne; 543 nm), and blue diode (405 nm) lasers, and EZ-C1 software. Neurons expressing EGFP or EGFP–tau were visualized using the 488 nm argon laser line and 510–540 nm bandpass emission filter. Cy3 was imaged using He/Ne 543 laser excitation and 570–610 nm emission filter. Microscope objectives (Nikon) used were a dry 4x [numerical aperture (NA), 0.13], a dry 20x (NA, 0.45; ELWD), an oil–water–glycerine 20x (NA, 0.75), an oil-immersion 60x (NA, 1.4), and an oil-immersion 100x (NA, 1.3). The microscope was enclosed in an incubation chamber maintained at 37°C and 5% CO2 (Solent Scientific, Sagensworth, UK). For two-channel imaging of EGFP and Cy3, images were acquired via sequential scanning. Image stacks (typically 10–35 optical sections per stack; 1024 x 1024 pixels) were collected for the whole hippocampal slice (30.45 µm z-axis steps) and different hippocampal subfields [CA1, CA3, and dentate gyrus (DG); 0.9–2.5 µm z-axis steps] of the infected hippocampal slice fixed at day 3 postinfection. Maximum projection images were generated from the resulting Z stacks.
Live imaging of infected neurons expressing EGFP alone or EGFP–tau constructs in CA1, CA3, and DG regions of organotypic hippocampal slices was performed over a period of 4 d (day 2 to day 5 postinfection). For these experiments (n = 3), culture inserts were transferred to a glass-bottom culture dish (MatTek, Ashland, MA) after the last change of medium. Image stacks (20–35 optical sections per stack; 1024 x 1024 pixels) were collected at 0.45 µm z-axis steps. Images were taken with lowest practical laser (Ar; 488 nm) intensity and shortest practical illumination time to limit photodynamic damage. By carefully marking the culture plate orientation, the same region was scanned at different days. Two-dimensional maximum projection images were reconstructed for each region. For the quantitation of the extent of degeneration, the number of nondegenerating neurons (i.e., neurons without any swellings having processes without any beading) was determined over time (day 3 and 4) and expressed relative to the number at day 2 postinfection from the same microscopic field in different regions for all constructs. Evaluations were performed blindly by a coworker without knowledge of the identity of the samples.
For morphological analysis of spines, two neurons per construct and per hippocampal subregion were completely imaged at high resolution. Image stacks were captured in a montage manner by translating the x–y stage to adjacent microscopic fields until the cell was completely contained within the stacks (pixel size, 0.086 x 0.086 x 0.25 µm; one channel at 12 bit; 60x oil objective; NA, 1.4). To yield a complete map of the neurons, two-dimensional projections of the image stacks were generated, aligned using Adobe Photoshop (Adobe Systems, San Jose, CA), and dendritic segments assigned to subclasses according to the criteria of Megias et al. (2001)
Assessment of cell death. Lactate dehydrogenase (LDH) release into the culture media was determined fluorimetrically using the CytoTox-ONE Homogeneous Membrane Integrity Assay kit (Promega, Madison, WI) according to the manufacturer's protocol. The assay was performed on 96-well microplates and read on Fluostar OPTIMA plate reader (BMG Lab Technologies, Offenburg, Germany) at 544 nm excitation and 590 nm emission. LDH activity was normalized to the EGFP fluorescence, which was determined from the respective fusion protein lysates (from caspase-3 experiments) at different times after infection.
Caspase-3 activity was determined fluorimetrically from the lysates of infected hippocampal slices at different times after infection using EnzChek Caspase-3 assay kit number 1 with N-CBZ-L-aspartyl-L-glutamyl-L-valyl-L-aspartic acid/aminomethyl coumarin (AMC) substrate (Invitrogen) according to the manufacturer's protocol. The assay was performed on 96-well microplates and read on Fluostar OPTIMA plate reader at 355–10 nm excitation, 460 nm emission (for AMC) and 485 nm excitation, and 520 nm emission (for EGFP). Caspase-3 activity was normalized to the EGFP fluorescence of the respective fusion protein lysates.
For determination of DNA fragmentation, DNA was extracted from four to eight hippocampal slices using the TACS apoptotic DNA laddering kit from R & D Systems (Wiesbaden, Germany) according to the manufacturer's protocol. Approximately 1 µg of DNA from each sample was electrophoresed through 1.5% agarose in Tris acetic acid buffer, visualized by ethidium bromide staining, and photographed under UV illumination.
Immunoblot analysis. Cultured hippocampal slices (at different times after infection) were harvested and sonicated in radioimmunoprecipitation assay (RIPA) buffer (50 mM Tris/HCl, pH 7.5, 150 mM NaCl, 1 mM EDTA, 1% NP-40, 0.5% deoxycholate, and 0.1% SDS, pH 8.0) containing protease inhibitors (1 mM PMSF, 10 µg/ml each of leupeptin and pepstatin, 1 mM EGTA) and phosphatase inhibitors (1 mM sodium orthovanadate, 20 mM sodium fluoride, and 1 mM sodium pyrophosphate) and centrifuged for 15 min at 13,000 x g at 4°C. The supernatant (lysate) was collected, frozen, and stored at –80°C. Protein concentration of the samples was determined with BCA (Pierce). Samples (10 µg of protein in lysates) or recombinant tau proteins (0.1 µg of protein) were subjected to SDS-PAGE and transferred to Immobilon-P (Millipore) followed by immunoblotting with various antibodies against tau and GFP. As secondary antibody, peroxidase-coupled anti-mouse or rabbit antiserum was used. Detection used enhanced chemiluminescence using SuperSignal West Dura extended duration substrate (Pierce) and was performed according to the manufacturer's protocol. Quantification of the blots was performed with Gel-Pro Analyzer 4.0 (Media Cybernetics, Silver Spring, MD). To determine quantitatively alterations in EGFP–tau phosphorylation/conformation at different epitopes, all data obtained with phosphorylation-dependent/conformation-dependent antibodies were normalized to total tau levels in the samples, and differences in phosphorylation/conformation between EGFP–PHP tau and EGFP–wt tau were determined.
Sequential extraction of EGFP–tau proteins. To study the solubility of tau proteins in infected hippocampal slices, we generated a tau solubility profile by applying a sequential extraction approach on hippocampal slices using buffers of increasing stringency (Zhukareva et al., 2004
Statistical analysis. Data were expressed as means ± SE (n = 3–5). All experiments were performed in triplicates or duplicates and repeated at least three times. Statistical analysis among experimental groups was performed using paired Student's t test (Origin 7.0; Microcal Software, Northampton, MA). p values are */°p < 0.05, **/°°p < 0.01, and ***/°°°p < 0.001.
Results
Targeted expression of EGFP-tagged human tau in organotypic hippocampal slices permits high-resolution imaging of individual neurons
To analyze the behavior of tau in neurons in an authentic CNS environment, we prepared a panel of EGFP-tagged tau constructs and expressed them in cultured mouse hippocampal slices. The constructs were based on the longest adult (441 aa) and fetal (352 aa) CNS tau isoforms (Fig. 1A). Wild-type tau and PHP tau sequences, which mimic key structural and functional aspects of hyperphosphorylated tau protein (Eidenmüller et al., 2000
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Figure 1. Sindbis-virus-mediated expression of EGFP-tagged human tau constructs in organotypic hippocampal slices. A, Schematic representation of EGFP-tagged human tau constructs. The constructs were based on the longest adult (441 aa) and fetal (352 aa) wild-type tau isoforms with an amino terminally fused EGFP sequence (discontinuous gray box). Serine (S)/threonine (T) residues, which have been substituted with glutamate (E) to create a pseudohyperphosphorylation of these residues, are indicated. As a control, EGFP sequence alone was used. The microtubule-binding repeats of tau are indicated by the thick black box. Adult-specific exons are shaded. B, C, Time course of EGFP expression in infected hippocampal slices. B, Lysates of the slices at different times after infection were prepared and separated by 10% SDS-PAGE and immunoblotted with GFP antibody. C, The graph shows the relative amounts of EGFP expressed at days 1–6 (d1–d6) postinfection. EGFP was detected as early as 7 h postinfection (data not shown), peaked at around day 3, and persisted until 1 week. D, E, Time course of EGFP–tau expression in infected hippocampal slices at d2, d4, and d6 postinfection (D) and the quantitation of results (E). Note that the kinetics of expression of the different tau fusion proteins is very similar to EGFP alone. Lysates of slices at different times after infection were prepared and analyzed by immunoblot using phosphorylation-independent antibody (Tau-5). Data are presented as mean ± SEM from three independent experiments.
To determine the time course of expression, virus was applied onto the hippocampal slices by the droplet method and lysates of the slices at different times after infection were prepared and analyzed by immunoblot. As a control, a construct with EGFP sequence alone was used. EGFP was detected as early as 7 h postinfection (data not shown), peaked at3 d, and persisted until 1 week (Fig. 1B,C). The kinetics of expression of the different tau fusion proteins was very similar to EGFP alone (Fig. 1D,E).
Efficient infection of neurons in all regions of the hippocampal slice was observed 3 d after application of the virus as indicated by the intense EGFP fluorescence (Fig. 2A). At higher magnification, many individual infected CA1 and CA3 pyramidal neurons as well as DG granule neurons were identified by their characteristic morphology and location (Figs. 2B–D). In addition, some interneurons in all regions were also infected. EGFP fluorescence was present in cell bodies, processes, and dendritic spines of the proximal and distal dendrites and allowed high-resolution imaging at the level of individual spines for several days (Fig. 2E–G). At later time points after infection (>5 d), many fluorescent cells appeared to have died in all hippocampal regions (data not shown).
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Figure 2. Distribution of infected neurons in cultured hippocampal slices. A–D, Immunofluorescence micrographs of the whole slice (A), CA1 region (B), CA3 region (C), and DG region (D) of EGFP–tau-infected slices 3 d postinfection. Note efficient infection of neurons in all regions. E–G, High-power magnifications of a single CA3 pyramidal neuron (E) and sections of the proximal (F) and distal (G) dendrites. Note intense EGFP fluorescence in all cellular compartments. Slices were fixed and processed for immunofluorescence as described in Materials and Methods. so, Stratum oriens; sp, stratum pyramidale; sr, stratum radiatum; slm, stratum lacunosum-moleculare; sm, stratum moleculare; sg, stratum granulosum. Scale bars: A, 300 µm; B–E, 50 µm; F, G, 10 µm.
Tau-dependent neurodegeneration occurs region specifically in organotypic culture
To determine a potential cytotoxic effect of tau expression in cultured hippocampal slices, release of LDH as a marker for plasma membrane damage was analyzed fluorimetrically at different times after infection. LDH activity was normalized to the EGFP fluorescence, which was determined from the respective lysates. In most experiments, expression of adult or fetal wt tau caused only a small increase in LDH release compared with EGFP alone at 3 and 4 d postinfection (Fig. 3A). In contrast, PHP tau expression resulted in anTo determine the mechanisms that are associated with the PHP tau-induced neurodegeneration, activation of caspase-3 as a marker for apoptotic events was assayed fluorimetrically and normalized to the EGFP fluorescence of the respective fusion protein. Caspase-3 activity was significantly increased for the PHP tau constructs compared with wt tau or EGFP alone in the infected hippocampal slices (Fig. 3B). The pattern of caspase-3 activation for the different isoforms and time points after infection was very similar to that of LDH release, indicating that the neurodegenerative effect of PHP tau is closely associated with apoptotic mechanisms. Support for an apoptotic contribution to PHP tau-induced cell death was provided by the appearance of DNA fragmentation revealed by agarose gel electrophoresis (Fig. 3C). The fragmentation pattern was very similar to the fragmentation induced by the typical apoptosis inducer staurosporine (Gianinazzi et al., 2004
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Figure 3. Effect of tau expression on LDH release, caspase-3 activity, and DNA fragmentation. A, Release of LDH from the infected hippocampal slices at 3 (left) and 4 (right) days postinfection. Both adult (441) and fetal (352) PHP tau induce a significant increase compared with the respective wt isoform or EGFP alone. B, Caspase-3 activity after 3 (left) and 4 (right) days postinfection. Caspase-3 activity is significantly increased for the PHP tau constructs compared with wt tau or EGFP alone in the lysates of infected hippocampal slices at different times after infection (day 3–4). C, DNA fragmentation after 3 d postinfection or treatment with staurosporine (Stp). The pattern of DNA damage for the PHP tau constructs was similar to that induced by the typical apoptosis inducer staurosporine (10 µM; 6 h). LDH and caspase-3 activity were assayed fluorimetrically and normalized to the EGFP fluorescence of the respective fusion protein. All values are shown as the mean ± SEM from at least three independent experiments. Data for EGFP–wt or PHP tau are expressed as percentage of the value for EGFP alone. Data were analyzed using Student's t test and considered to be significantly different from EGFP–wt tau at *p < 0.05, **p < 0.01, and ***p < 0.001. For the assay for DNA fragmentation, samples were separated by agarose gel electrophoresis on 1.5% agarose. Similar results were obtained by two independent experiments. M, Marker.
To determine the spatiotemporal dynamics of tau-induced neurodegeneration, we performed live imaging of infected neurons expressing the EGFP-tagged constructs in the CA1, CA3, and DG regions over a period of 4 d. We observed a time-dependent loss of individual neurons in all hippocampal regions and with all constructs (Fig. 4A,B, asterisks). In addition, in CA3 and DG, many PHP tau-expressing neurons developed a "ballooned" phenotype characterized by a swollen neuronal perikaryon starting at day 3 postinfection for the adult isoform (Fig. 4B, arrowheads) and day 4 for the fetal isoform. Ballooned neurons with and without apparent processes were observed. It was not possible to preserve ballooned neurons by standard fixation procedures, suggesting that they had lost their contacts and cytoskeletal integrity. It should be noted that the development of a ballooned phenotype is considered to be distinct from apoptosis (Gleckman et al., 1999
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Figure 4. Live imaging of the effect of tau expression on the survival of individual neurons in hippocampal slices. A, B, Fluorescence micrographs of the CA1 region (A) and CA3 region (B) of living hippocampal slices 2 and 3 d postinfection. Time-dependent loss of individual neurons was observed in all hippocampal regions (A, B, asterisks) and with all constructs, which appeared higher in the CA3 region for PHP tau (B). In addition, in CA3 and DG, many PHP tau expressing neurons developed a ballooned phenotype characterized by a swollen neuronal perikaryon with or without processes (arrowheads). Scale bars: A, B, 50 µm. C–E, Percentage of nondegenerating neurons (i.e., neurons with unaffected perikarya and processes) at days 2, 3, and 4 postinfection and expressed relative to the number at day 2 postinfection. In CA3 (D) and DG (E) regions, but not in the CA1 (C) region, the number of nondegenerating neurons expressing the PHP tau isoforms dramatically decreased compared with neurons expressing EGFP alone or wt tau isoforms. All values are shown as the mean ± SEM from at least three independent experiments (C–E). The data for EGFP alone or EGFP–wt or EGFP–PHP tau (at day 3 or day 4) are expressed as percentage of the respective value for day 2 postinfection. Data were analyzed using Student's t test and considered to be significantly different from EGFP alone at *p < 0.05, **p < 0.01, and ***p < 0.001 or from EGFP–wt tau at °p < 0.05, °°p < 0.01, and °°°p < 0.001.
To quantitate the extent of degeneration, the number of nondegenerating neurons (i.e., neurons without any swelling having processes without beading) was determined over time (day 3 and 4) and expressed relative to the number at day 2 postinfection from the same microscopic field in different regions for all constructs (Fig. 4C–E). In the CA1 region, tau expression resulted in a slight reduction of the number of nondegenerating neurons compared with neurons expressing EGFP alone (Fig. 4C). We did not observe a difference between wt tau- and PHP tau-expressing neurons. In contrast, in CA3 and DG regions, the number of nondegenerating neurons expressing the PHP tau isoforms dramatically decreased compared with neurons expressing EGFP alone or wt tau isoforms (Fig. 4D,E). Neurons expressing the adult isoform of PHP tau degenerated earlier (day 3) than fetal PHP tau-expressing neurons, in which the majority of neurons were degenerated only at day 4.Collectively, the data indicate that the PHP modification induces a region-specific neurodegeneration in the CA3 and DG subfields of hippocampal slices and that cell death involves both apoptotic and nonapoptotic mechanisms.
Spine density and spine morphology are stable against tau-induced degeneration
In AD, alterations in synaptic integrity and plasticity have been reported as an early event (Selkoe, 2002
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Figure 5. Spine density and spine morphology of tau-expressing neurons in hippocampal slices. A, Complete map of an individual neuron of the CA1 (left) and CA3 (right) region infected with EGFP–tau. Segments are assigned to dendritic subclasses. Scale bar, 100 µm. B, Representative dendritic segments after deconvolution from stratum radiatum thick and thin subclasses from CA1 and CA3 pyramidal neurons expressing tau constructs as indicated. Each frame has a width of 30 µm. C, Spine density in dendritic subclasses of CA1 and CA3 pyramidal neurons expressing adult (441) and fetal (352) wt and PHP tau constructs. Data are based on the analysis of the complete dendritic arbor of two neurons per construct and per hippocampal region. Mean and range are indicated. D, Spine length and volume in stratum radiatum thick and thin subclasses of CA1 and CA3 pyramidal neurons expressing adult (441) and fetal (352) wt and PHP tau constructs. Data were analyzed as described in Materials and Methods from a total of 747 dendritic segments. All values are shown as the mean ± SEM. St. Or, Stratum oriens; st. Luc, stratum lucidum; st. Rad., stratum radiatum; st. L-M, stratum lacunosum-moleculare; prox, proximal; med, medial; dist, distal.
The data suggest that synaptic integrity is remarkably stable against tau-dependent degeneration, providing evidence that alterations in synaptic plasticity in AD are directly caused by the amyloid pathology rather than by tau-mediated mechanisms.Disease-like tau modifications cause accumulation of insoluble tau, induce pathological tau conformation, and affect tau phosphorylation at selected sites
Filamentous tau aggregates that can be biochemically isolated from diseased brain tissue are hallmarks of tauopathies such as Alzheimer's disease (Selkoe et al., 1982
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Figure 6. Accumulation of insoluble tau and induction of pathological tau conformation after targeted tau expression. A, Tau solubility profile from lysates of infected hippocampal slices. The profile was generated using buffers of increasing stringency: high salt, 1% Triton, RIPA buffer, 2% SDS, and 70% formic acid. In wt tau (441 and 352 isoform)-infected slices, the majority of tau was soluble and present in the high salt extract with almost no insoluble tau. In contrast, a significant portion of PHP tau isoforms was insoluble. No tau was detected in the 70% formic acid fraction. An equal amount of the material from each extraction step was loaded, and Tau-5 antibody was used for immunoblot analysis. B, Schematic representation that indicates the epitopes of the conformational-dependent antibodies Alz50 and MC1. C, Immunoblot of lysates of infected hippocampal slices. The PHP tau proteins showed a strong increase in immunoreactivity for Alz50 and MC1 antibodies compared with the respective wt proteins. D, E, Quantitation of the immunoblots. Conformational alteration for PHP tau was increased for both adult and fetal tau isoforms at different times after infection (day 3 and day 4). To determine quantitatively the alterations in EGFP–tau conformation, all data obtained with conformation-dependent antibodies were normalized to total tau (Tau-5) levels in the samples, and then the difference in conformation between EGFP–PHP tau and EGFP–wt tau was determined. Data for EGFP–PHP tau are expressed as percentage of the value for EGFP–wt tau (wt tau set as 100%). All values are shown as the mean ± SEM from three independent experiments. Data were analyzed using Student's t test and considered to be significantly different from EGFP-wt tau at *p < 0.05, **p < 0.01, and ***p < 0.001. F, Double immunofluorescence staining of all infected neurons stained with the MC1 antibody showed a subcellular distribution closely reflecting the EGFP fluorescence. Scale bar, 100 µm.
To test whether the accumulation of insoluble tau is associated with an induction of pathological tau conformation, immunoblots with Alz50 and MC1 antibodies were performed. Both antibodies recognize a conformational epitope in AD brains that depends on two discontinuous portions of the tau sequence as shown in Figure 6B (Jicha et al., 1997Abnormal phosphorylation may be involved to generate a conformational state that is typical for the disease. To determine whether pseudohyperphosphorylation of tau induces abnormal phosphorylation in hippocampal slices expressing tau constructs, immunoblot analysis using a panel of phosphorylation-dependent and site-specific antibodies against selected serine and threonine residues was performed (Fig. 7A). None of these antibodies was reactive against recombinant wt or PHP tau with the exception of an antibody against phosphorylated S356, which was less reactive with PHP tau isoforms compared with wild-type tau (10–40% for the fetal and adult isoform, respectively). In lysates of infected hippocampal slices, we observed a change in phosphorylation at several sites compared with the respective wt tau constructs (Fig. 7B). A strong increase in phosphorylation was seen with both adult and fetal PHP tau isoforms at T212, S214, and S262. In contrast, a marked decrease was observed at T205. The amount of total tau as determined using a phosphorylation-independent antibody (Tau-5) was very similar for both isoforms (wt and PHP tau). Quantitative analysis confirmed increased phosphorylation for PHP tau (30–150% compared with the respective wt tau isoform) at T212, S214, and S262 for both adult and fetal tau isoforms at different times after infection (Figs. 7C–F). A significant increase in phosphorylation at S356 (50–60%) was observed for the fetal PHP tau isoform (Fig. 7D,F). A slight increase (10–30%) was also observed for T181. At all conditions, phosphorylation at T205 was strongly decreased (40–70%) for PHP tau.
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Figure 7. Phosphorylation state of tau in infected neurons. A, Schematic representation that indicates the epitopes of phosphorylation-sensitive antibodies detecting serine (S) and threonine (T) residues that were not mutated in PHP tau. B, Immunoblot of lysates of infected hippocampal slices with different phosphorylation-sensitive antibodies. Note that some antibodies show a strong increase in the staining of the PHP isoforms relative to total tau (Tau-5). C–F, Quantitation of the immunoblots. An increased phosphorylation for PHP tau was detected at T212, S214, and S262 for both adult and fetal tau isoforms compared with the respective wt tau isoform at different times after infection. At all conditions, phosphorylation at T205 was strongly decreased for PHP tau. To determine quantitatively the alterations in EGFP–tau phosphorylation at different epitopes, all data obtained with phosphorylation-dependent antibodies were normalized to total tau (Tau-5) levels in the samples, and then the difference in phosphorylation between EGFP–PHP tau and EGFP–wt tau was determined. The data for EGFP–PHP tau are expressed as percentage of the value for EGFP–wt tau (wt tau set as 100%). All values are shown as the mean ± SEM from three independent experiments. Data were analyzed using Student's t test and considered to be significantly different from EGFP–wt tau at *p < 0.05, **p < 0.01, and ***p < 0.001.
To determine the distribution of exogenously expressed tau and the different phosphoisoforms, immunohistochemistry of infected hippocampal slices was performed. Tau was present in all infected (EGFP-positive) neurons and exhibited a strong staining in processes and cell bodies as detected using a phosphorylation-independent polyclonal antibody against human tau (Fig. 8A). Immunostainings with the phosphorylation-dependent and site-specific antibodies confirmed phosphorylation of the exogenously expressed tau proteins at the respective sites. With all antibodies, only infected neurons in all regions were immunoreactive (Fig. 8B–D and data not shown). Within the population of stained neurons, marked differences in the antibody stainings compared with the EGFP fluorescence were observed. In particular, most interneurons in different zones (e.g., in the CA1 region) showed only weak or no immunoreactivity against selected antibodies (Fig. 8B–D, arrowheads); however, exceptions were also observed (Fig. 8B, asterisk). For some antibodies, staining was prominent only in cell bodies (Fig. 8C), whereas others also showed staining in processes (Fig. 8B,D).
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Figure 8. Distribution of the infected neurons that were immunoreactive with different phosphorylation-sensitive antibodies. A–D, Representative images for the CA1 region of hippocampal slices with EGFP fluorescence (left), stained for the respective antibodies (middle) and overlay (right). With all antibodies, only infected neurons were immunoreactive (B–D). Note that most interneurons in different zones in the CA1 region showed only weak or no immunoreactivity against selected antibodies (B–D, arrowheads) with some exceptions (B, asterisk). Some antibodies stained most prominently the cell bodies (C), whereas others showed staining also in processes (B, D). Scale bars, 100 µm.
The data indicate that abnormal phosphorylation at selected sites, induction of pathological tau conformation and formation of tau aggregates are closely associated.
Discussion
Imaging and evaluation of synaptic morphology
We expressed the cytoskeletal protein tau tagged with EGFP using the neurotropic, recombinant Sindbis virus, which provides an efficient, transient expression of the fusion proteins in individual neurons of hippocampal slices. Because EGFP expression revealed the detailed morphology of living neurons, we were able to follow and image structural changes of the same neuron over a time course of several days. EGFP labeling also allowed us a high-resolution imaging and algorithm-based evaluation of the neuronal morphology at the level of individual spines in fixed tissue.A number of studies have indicated alterations in synaptic integrity and plasticity as an early phenotypic manifestation in the pathogenesis of AD (Selkoe, 2002
Mechanisms of cell death
AD and other neurodegenerative diseases are characterized by progressive cell loss of specific neuronal populations, but the underlying molecular mechanisms that are responsible for the temporally and spatially defined cell death are still unresolved. Postmortem analysis of human brain has shown apoptotic DNA fragmentation (Su et al., 1994bWe observed that disease-like tau modification induced extensive cell death in organotypic hippocampal cultures, which is associated with apoptotic mechanisms as indicated by an increase in caspase-3 activity and typical DNA fragmentation. In addition, many neurons specifically degenerated by establishing a ballooned phenotype, as has also been reported for patients with AD and other tauopathies (Dickson et al., 1986
We observed that neurodegeneration induced by PHP tau occurs predominantly in the CA3 and DG region of the hippocampal slices. This indicates that disease-relevant tau modification do not cause general toxicity but exert their neurodegenerative effect in a region- and neuron-type specific manner. In AD and after hypoxic/ischemic insults, CA1 region typically demonstrates profound vulnerability to neuronal cell death (Schmidt-Kastner and Freund, 1991
The neurotoxic effect of PHP tau may be caused by a selective disturbance of signal transduction cascades in CA3 pyramidal neurons and DG granule neurons; however, the precise molecular events and the relationship to AD remain to be shown. It should be taken into account that our approach results in the presence of tau in all neuronal compartments, whereas endogenous tau is enriched in the axon. This may cause the slight toxicity observed after expression of wt tau but would not explain the obvious difference between wt tau and PHP tau. Furthermore, a relocation of tau from the axonal to the somatodendritic compartment where neurofibrillary tangles become apparent is a characteristic event during the development of tau pathology. Thus, the presence of tau in the "wrong" compartment could well be relevant for disease progression.
Although PHP tau mimics key aspects of hyperphosphorylation, including the induction of structural and functional changes, it does not longer participate in the complex phosphorylation/dephosphorylation events occurring with "normal" tau protein. Whether this is relevant for tau-mediated toxicity in disease in which dephosphorylation of tau is drastically reduced (Matsuo et al., 1994
Abnormal phosphorylation and tau aggregation
Constructs with pseudophosphorylated residues provide a tool to determine the effect of disease-like tau modifications on tau phosphorylation at selected sites. Here, we show that pseudohyperphosphorylation increases phosphorylation at several other sites including T181, T212, S214, S262, and S356. Some of these sites are known to be abnormally hyperphosphorylated in AD, constitute recognition sites for some AD diagnostic antibodies, and are also known to correlate with the severity of neuronal pathology (Augustinack et al., 2002The contribution of tau modification and tau aggregation to the neurodegenerative process remains elusive. Both neuronal loss and NFTs increase in parallel with the duration and severity of illness, but the amount of neuronal loss exceeds by manyfold the amount of NFTs accumulated (Gomez-Isla et al., 1997
Footnotes
Received Oct. 5, 2005; revised April 18, 2006; accepted April 19, 2006.This work was supported by the Ministry for Science and Culture of Lower Saxony. We thank Dr. Sondra Schlesinger (Washington University School of Medicine, St. Louis, MO) for the generous gift of pSinRep5 vector and helper DH (26S) DNA and Dr. Peter Davies (Albert Einstein College of Medicine, Bronx, NY) for Alz-50 and MC1 antibody. We thank Dr. Brent Lindquist (Stony Brook University, Stony Brook, NY) for providing the source code for 3DMA-Neuron and Dr. Christina Weaver (Mount Sinai School of Medicine, NY) for helpful suggestions on the usage of the software. We appreciate the help of Nataliya Golovyashkina, Julian Heidelberg, Ann-Theres Lütkhoff, Jörg Rathert, and Christian Stößel with morphological analyses.
Correspondence should be addressed to Dr. Neelam Shahani or Dr. Roland Brandt, Department of Neurobiology, University of Osnabrück, Barbarastraße 11, D-49076 Osnabrück, Germany. Email: neelam.shahani{at}biologie.uni-osnabrueck.de or Brandt{at}biologie.uni-osnabrueck.de
DOI:10.1523/JNEUROSCI.4245-05.2006
Copyright © 2006 Society for Neuroscience 0270-6474/06/266103-12$15.00/0
References
Allen B, Ingram E, Takao M, Smith MJ, Jakes R, Virdee K, Yoshida H, Holzer M, Craxton M, Emson PC, Atzori C, Migheli A, Crowther RA, Ghetti B, Spillantini MG, Goedert M (2002) Abundant tau filaments and nonapoptotic neurodegeneration in transgenic mice expressing human P301S tau protein. J Neurosci 22:9340–9351.
[Abstract/Free Full Text] Arendt T, Holzer M, Grossmann A, Zedlick D, Bruckner MK (1995) Increased expression and subcellular translocation of the mitogen activated protein kinase kinase and mitogen-activated protein kinase in Alzheimer's disease. Neuroscience 68:5–18.[CrossRef][Medline]
Augustinack JC, Schneider A, Mandelkow EM, Hyman BT (2002) Specific tau phosphorylation sites correlate with severity of neuronal cytopathology in Alzheimer's disease. Acta Neuropathol (Berl) 103:26–35.[CrossRef][Medline]
Braak H, Braak E, Strothjohann M (1994) Abnormally phosphorylated tau protein related to the formation of neurofibrillary tangles and neuropil threads in the cerebral cortex of sheep and goat. Neurosci Lett 171:1–4.[CrossRef][ISI][Medline]
Brandt R, Hundelt M, Shahani N (2005) Tau alteration and neuronal degeneration in tauopathies: mechanisms and models. Biochim Biophys Acta 1739:331–354.[Medline]
Coleman PD, Yao PJ (2003) Synaptic slaughter in Alzheimer's disease. Neurobiol Aging 24:1023–1027.[CrossRef][ISI][Medline]
Davis BG (2004) Mimicking posttranslational modifications of proteins. Science 303:480–482.
[Abstract/Free Full Text] Dickson DW, Yen SH, Suzuki KI, Davies P, Garcia JH, Hirano A (1986) Ballooned neurons in select neurodegenerative diseases contain phosphorylated neurofilament epitopes. Acta Neuropathol (Berl) 71:216–223.[CrossRef][Medline]
Drewes G, Lichtenberg-Kraag B, Doring F, Mandelkow EM, Biernat J, Goris J, Doree M, Mandelkow E (1992) Mitogen activated protein (MAP) kinase transforms tau protein into an Alzheimer-like state. EMBO J 11:2131–2138.[ISI][Medline]
Ehrengruber MU, Lundstrom K, Schweitzer C, Heuss C, Schlesinger S, Gahwiler BH (1999) Recombinant Semliki Forest virus and Sindbis virus efficiently infect neurons in hippocampal slice cultures. Proc Natl Acad Sci USA 96:7041–7046.
[Abstract/Free Full Text] Eidenmüller J, Fath T, Hellwig A, Reed J, Sontag E, Brandt R (2000) Structural and functional implications of tau hyperphosphorylation: information from phosphorylation-mimicking mutated tau proteins. Biochemistry 39:13166–13175.[CrossRef][Medline]
Eidenmüller J, Fath T, Maas T, Pool M, Sontag E, Brandt R (2001) Phosphorylation-mimicking glutamate clusters in the proline-rich region are sufficient to simulate the functional deficiencies of hyperphosphorylated tau protein. Biochem J 357:759–767.[CrossRef][ISI][Medline]
el Hachimi KH, Foncin JF (1990) [Loss of dendritic spines in Alzheimer's disease]. C R Acad Sci III 311:397–402.[Medline]
Fath T, Eidenmüller J, Brandt R (2002) Tau-mediated cytotoxicity in a pseudohyperphosphorylation model of Alzheimer's disease. J Neurosci 22:9733–9741.
[Abstract/Free Full Text] Ferrer I, Gullotta F (1990) Down's syndrome and Alzheimer's disease: dendritic spine counts in the hippocampus. Acta Neuropathol (Berl) 79:680–685.[CrossRef][Medline]
Fujino Y, Delucia MW, Davies P, Dickson DW (2004) Ballooned neurones in the limbic lobe are associated with Alzheimer type pathology and lack diagnostic specificity. Neuropathol Appl Neurobiol 30:676–682.[Medline]
Gervais FG, Xu D, Robertson GS, Vaillancourt JP, Zhu Y, Huang J, LeBlanc A, Smith D, Rigby M, Shearman MS, Clarke EE, Zheng H, Van Der Ploeg LH, Ruffolo SC, Thornberry NA, Xanthoudakis S, Zamboni RJ, Roy S, Nicholson DW (1999) Involvement of caspases in proteolytic cleavage of Alzheimer's amyloid-beta precursor protein and amyloidogenic A beta peptide formation. Cell 97:395–406.[CrossRef][ISI][Medline]
Gianinazzi C, Grandgirard D, Simon F, Imboden H, Joss P, Tauber MG, Leib SL (2004) Apoptosis of hippocampal neurons in organotypic slice culture models: direct effect of bacteria revisited. J Neuropathol Exp Neurol 63:610–617.[Medline]
Gleckman AM, Jiang Z, Liu Y, Smith TW (1999) Neuronal and glial DNA fragmentation in Pick's disease. Acta Neuropathol (Berl) 98:55–61.[CrossRef][Medline]
Gomez-Isla T, Hollister R, West H, Mui S, Growdon JH, Petersen RC, Parisi JE, Hyman BT (1997) Neuronal loss correlates with but exceeds neurofibrillary tangles in Alzheimer's disease. Ann Neurol 41:17–24.[CrossRef][ISI][Medline]
Götz J, Chen F, van Dorpe J, Nitsch RM (2001) Formation of neurofibrillary tangles in P301l tau transgenic mice induced by Abeta 42 fibrils. Science 293:1491–1495.
[Abstract/Free Full Text] Holzer M, Holzapfel HP, Zedlick D, Bruckner MK, Arendt T (1994) Abnormally phosphorylated tau protein in Alzheimer's disease: heterogeneity of individual regional distribution and relationship to clinical severity. Neuroscience 63:499–516.
