Distinct FTDP-17 Missense Mutations in Tau Produce Tau Aggregates and Other Pathological Phenotypes in Transfected CHO Cells

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager


Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Vogelsberg-Ragaglia, V.
	Articles by Lee, V. M.-Y.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Vogelsberg-Ragaglia, V.
	Articles by Lee, V. M.-Y.

Vol. 11, Issue 12, 4093-4104, December 2000

Distinct FTDP-17 Missense Mutations in Tau Produce Tau Aggregates and Other Pathological Phenotypes in Transfected CHO Cells

Vanessa Vogelsberg-Ragaglia,^* Jennifer Bruce,^* Christiane Richter-Landsberg, Bin Zhang,^* Ming Hong,^* John Q. Trojanowski,^* and Virginia M.-Y. Lee^*

^*The Center for Neurodegenerative Disease Research, Department of Pathology and Laboratory Medicine, University of Pennsylvania, Philadelphia, Pennsylvania 19104; and Department of Biology, Molecular Neurobiology, University of Oldenburg, Oldenburg, Germany D-26111

Submitted May 23, 2000; Revised August 16, 2000; Accepted September 28, 2000
Monitoring Editor: Ted Salmon

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Multiple tau gene mutations are pathogenic for hereditary frontotemporal dementia and parkinsonism linked to chromosome 17(FTDP-17), with filamentous tau aggregates as the major lesionsin the CNS of these patients. Recent studies have shown that bacteriallyexpressed recombinant tau proteins with FTDP-17 missense mutationscause functional impairments, i.e., a reduced ability of mutanttau to bind to or promote the assembly of microtubules. To investigatethe biological consequences of FTDP-17 tau mutants and assesstheir ability to form filamentous aggregates, we engineered Chinesehamster ovary cell lines to stably express tau harboring one orseveral different FTDP-17 mutations and showed that differenttau mutants produced distinct pathological phenotypes. For example, $Delta$ K, but not several other single tau mutants (e.g., V337 M, P301L,R406W), developed insoluble amorphous and fibrillar aggregates,whereas a triple tau mutant (VPR) containing V337M, P301L, andR406W substitutions also formed similar aggregates. Furthermore,the aggregates increased in size over time in culture. Significantly,the formation of aggregated $Delta$ K and VPR tau protein correlatedwith reduced affinity of these mutants to bind microtubules. Reducedphosphorylation and altered proteolysis was also observed in R406Wand $Delta$ K tau mutants. Thus, distinct pathological phenotypes, includingthe formation of insoluble filamentous tau aggregates, resultfrom the expression of different FTDP-17 tau mutants in transfectedChinese hamster ovary cells and implies that these missense mutationscause diverse neurodegenerative FTDP-17 syndromes by multiplemechanisms.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Tau is an abundant microtubule-associated protein of the CNS that is expressed primarily in neurons and is implicated in thepathogenesis of Alzheimer's disease and related neurodegenerativediseases known as tauopathies (reviewed in Vogelsberg-Ragagliaet al., 1999). The major neuropathological characteristics oftauopathies are numerous neuronal and/or glial cytoplasmic inclusionsformed by aggregated paired helical filaments (PHFs) and/or straightfilaments composed of aberrantly phosphorylated tau proteins (PHF-tau)in widespread CNS regions (Spillantini and Goedert, 1998; Vogelsberg-Ragagliaet al., 1999). Six alternatively spliced tau isoforms are expressedin the adult human CNS (Goedert et al., 1989; Andreadis et al.,1992), and are localized predominantly in axons (Binder et al.,1985). Tau proteins bind to and stabilize microtubules (MTs) inthe polymerized state (Weingarten et al., 1975; Drechsel et al.,1992), but the formation of PHF-tau results in a loss of theseimportant functions (Bramblett et al., 1993; Yoshida and Ihara,1993). Moreover, unlike normal tau, PHF-tau is insoluble, accumulatesin the somatodendritic domain of neurons, and assembles into abnormalfilaments that aggregate as neurofibrillary tangles (NFTs; Leeet al., 1991; Goedert et al., 1997). However, the mechanism(s)whereby normal soluble tau assembles into PHFs and aggregatesinto NFTs remains unknown. This is due, in part, to the inabilityto develop cell culture and animal models that produce PHFs andNFTs.

Although the massive degeneration of neurons and extensive gliosis associated with progressive accumulations of PHF-tau lesionsprovided circumstantial evidence implicating filamentous tau pathologyin the onset/progression of neurodegenerative disease, the discoveryof multiple pathogenic tau gene mutations in many different familieswith FTDP-17 showed unequivocally that tau abnormalities causeneurodegenerative disease (reviewed in Vogelsberg-Ragaglia etal., 1999). The FTDP-17 tau gene mutations (i.e., missense substitutions,in-frame deletions, intronic substitutions) occur in exons andintrons of the tau gene (Clark et al., 1998; Hutton et al., 1998;Poorkaj et al., 1998; Spillantini et al., 1998; D'Souza et al.,1999; Iijima et al., 1999; Rizzu et al., 1999). They may causeFTDP-17 by altering the functions or levels of specific tau isoformsand/or promoting tau aggregation in the CNS (Hong et al., 1998;Hutton et al., 1998; D'Souza et al., 1999). Indeed, several FTDP-17missense tau mutations, including $Delta$ 280K ( $Delta$ K), V337M (VM), P301L(PL), and R406W (RW) have been demonstrated to reduce the abilityof bacterially expressed recombinant tau protein to bind to andpromote the assembly of MTs (Hong et al., 1998; D'Souza et al.,1999). Therefore, they may cause neurodegenerative disease byinducing a loss of normal tau functions. Other studies showedthat recombinant tau with the PL mutation aggregates into filamentsmore readily than recombinant wild-type (Wt) tau (Goedert et al.,1999; Nacharaju et al., 1999; Gamblin et al., 2000), supportingthe idea that some missense mutations may also cause neurodegenerativedisease by inducing a gain of toxic function. However, it hasnot been possible to produce tau aggregates in intact cells evenafter massively overexpressing Wt tau in cultured neuronal andnon-neuronal cells (Kanai et al., 1989; Bramblett et al., 1993;Ebneth et al., 1998).

Thus, to more precisely define how these missense mutations cause tau dysfunction and to assess whether they can cause tauaggregation, we generated stably transfected Chinese hamster ovary(CHO) cell lines that expressed tau harboring one or several topographicallydistinct FTDP-17 missense mutations. Here, we report that differenttau mutants produce distinct pathological phenotypes in transfectedCHO cells. More importantly, filamentous tau aggregates were detectedin CHO cells expressing the $Delta$ K and VPRmutations.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Site-directed Mutagenesis of Tau40 to Generate Tau Mutants

Site-directed mutagenesis (Quikchange kit; Stratagene, La Jolla, CA) was used to create a series of single missense mutations(N279K, $Delta$ 280K, P301L, S305N, V337M, R406W and a triple mutation,VPR, containing P301L, V337M, and R406W) in the longest humantau isoform (designated Tau40). The sequences of the mutagenizedoligonucleotides were as follows: N279K: 5'-GGT GCA GATAAT TAA GAA GAA GCT GGA TCT TAG C-3', $Delta$ 280K: 5'-GGG AAGGTG CAG ATA ATT AAT AAG CTG GAT CTT AGC AAC GTC C-3', P301L:5'-GGA TAA TAT CAA ACA CGT CCT GGG AGG CGG CAG TGT GC-3', S305N:5'-CCC GGG AGG CGG CAA TGT GCA AAT AGT CTA C-3', V337M:5'-CCA GGA GGT GGC CAG ATG GAA GTA AAA TCT GAG AAG C-3', and R406W:5'-GGG GAC ACG TCT CCA TGG CAT CTC AGC AAT GTC TCC-3'. In general,two synthetic oligonucleotide primers containing the desired mutationand complimentary to opposite strands of the vector were incubatedwith wild-type Tau40 in a pSG5 vector (Stratagene) and Pfu DNApolymerase. After the polymerase chain reaction reaction, thetemplate DNA was digested with DpnI and the remaining mutatedcDNA was used to transform Escherichia coli. Each tau constructwas subjected to sequence analysis, and the position of each mutationin the largest 441-amino-acid-long tau isoform is shown in Figure1.

View larger version (13K):
[in this window]
[in a new window]

Figure 1. Topography of FTDP-17 missense mutations in tau- and epitope-specific anti-tau antibodies. Schematic representation of the longest tau isoform, designated Tau40, containing 441 amino acids. The locations of six FTDP-17 missense mutations studied here are identified in the schematic diagram of tau. The two 29-amino-acid-long inserts are defined by white boxes at the amino-terminal region and the MT binding repeats appear as four black blocks near the carboxy terminal of tau. Each MT repeat is numbered 1-4. The defined epitopes recognized by each of the anti-tau antibodies used in this study are shown below the tau schematic with their corresponding amino acid length and position as well as the code name of the specific antibody that recognizes each epitope. The exact site(s) of phosphorylation detected by the phosphorylation-dependent anti-tau MAbs are shown here below the code names.

Stable Expression of Wt and Mutant Tau40 in Transfected CHO Cells

CHO cells were maintained in $alpha$ -minimum essential medium supplemented with 10% fetal bovine serum, 2 mM glutamine, 100 IU/mlpenicillin, and 100 µg/ml streptomycin (Life Technologies, Rockville,MD) as previously described (Bramblett et al., 1993). CHO Pro5cells were cotransfected with either the Wt or mutant Tau40 cDNAand pcDNA3 containing the neomycin gene, by using the calciumphosphate precipitation method (Chen and Okayama, 1987) as previouslydescribed (Bramblett et al., 1993). After selection in $alpha$ -minimumessential medium containing 0.8 mg/ml G418, the cells were screenedfor tau expression by Western blot and indirect immunofluorescence(see below), followed by subcloning. Stably transfected CHO celllines were established from subclones expressing Wt or mutanttau in >90% of cells at approximately equivalent tau protein levels,and these cell lines were used in the studies reported below unlessotherwisestated.

Preparation and Western Blot Analyses of Lysates from Transfected CHO Cells

Transfected CHO cells were washed once with phosphate-buffered saline (PBS) and lysed in ice-cold high salt RAB buffer [0.1M 2-(N-morpholino)ethanesulfonic acid, 0.5 mM MgSO₄, 1 mM EGTA,2 mM dithiothreitol, and 0.75 M NaCl, pH 6.8] supplemented with0.1% Triton X-100 and a mixture of protease and phosphatase inhibitors(2 mM phenylmethylsulfonyl fluoride; 20 mM NaF; 0.5 mM sodiumorthovanadate; and L-1-tosylamide-2-phenylethylchloromethyl, N-tosyl-L-lysinechloromethyl ketone, leupeptin, pepstatin, and soybean trypsininhibitor, each at 1 µg/ml). Cell lysates were incubated on icefor 10 min, sonicated, and centrifuged for 20 min at 50,000 ×g at 4°C. The supernatants were collected, boiled for 10 min,and then centrifuged for 10 min at 12,000 × g at 4°C. Proteinconcentration was determined by using the bicinchoninic acid method(Pierce, Rockford, IL). Samples were resolved on 7.5% SDS-PAGEgels and the tau proteins expressed in these cell lines were probedby Western blot analysis by using a variety of epitope-specificanti-tau antibodies (see below). Antibody binding was detectedwith horseradish peroxidase-conjugated secondary antibody (JacksonLaboratories, West Grove, PA) and the blots were developed eitherby the enhanced chemiluminescence (Amersham, Piscataway, NJ) or3,3'-diaminobenzidine method. For quantification, ¹²⁵I-labeled goat anti-mouse IgG was used as secondary antibody andthe blots were exposed to PhosphorImager plates. Quantitativeanalysis was performed with ImageQuant software (Molecular Dynamics,Sunnyvale, CA). Recombinant tau protein corresponding to the largesttau isoform was prepared as described in Hong et al. (1998).

Dephosphorylation and Proteolysis of Tau from Transfected CHO Cells

Heat-stable, high-salt CHO cell lysates were dialyzed overnight in 50 mM Tris, pH 8.0, 0.2 mM EDTA, and protease inhibitorsto remove the high salt, inhibit proteolysis, and establish anoptimal environment for dephosphorylating tau with alkaline phosphatase(Sigma, St. Louis, MO) as described in Hong et al. (1998). Increasedproteolysis was achieved by eliminating protease inhibitors fromthe high-salt RAB extractionbuffer.

Metabolic Labeling and Western Blot Studies of Tau from Transfected CHO Cells

Transfected CHO cells stably expressing Wt or mutant tau proteins were incubated with methionine-free medium for 15 min andpulsed with 100 µCi/ml [³⁵S]methionine (NEN, Boston, MA) for 30 min as described in Merricket al. (1996). The radiolabeled CHO cells were chased for differentlengths of time and harvested in ice-cold RIPA buffer (50 mM Tris,pH 7.4, 150 mM NaCl, 1% NP-40, 5 mM EDTA, 0.5% sodium deoxycholate,0.1% SDS). Radiolabeled tau in cell lysates was immunoprecipitatedwith a rabbit polyclonal anti-tau antibody (17026), followed byprotein A-Sepharose (Pharmacia Biotech, Peapack, NJ) and the antigen-antibodycomplex was resolved by SDS-PAGE. After the radiolabeled gelswere dried, they were exposed to PhosphorImager plates for subsequentanalysis.

MT Binding Assay of Tau from Transfected CHO Cells

To determine whether the point mutations alter interactions of tau with tubulin in the MTs of intact cells, an MT bindingassay was performed as described in Bramblett et al. (1993) andMerrick et al. (1996). Briefly, CHO cells were harvested in RABbuffer supplemented with 0.1% Triton X-100, 20 µM Taxol, 2 mMGTP, and a mixture of protease inhibitors (as mentioned above)at 37°C. Cell lysates were homogenized with 15 strokes in a warmDounce homogenizer, and then immediately centrifuged for 20 minat 50,000 × g at 25°C. The supernatant containing unbound tauwas removed and the protein concentration determined by the bicinchoninicacid method (Pierce). The remaining pellet was resuspended ina 2× volume of sample buffer corresponding to the total volumeof supernatant after normalizing to total protein. The sampleswere resolved on 7.5% SDS-PAGE gels, transferred onto nitrocellulosereplicas, and the amounts of tau and $alpha$ -tubulin protein were quantifiedusing ¹²⁵I-labeled secondary antibody. The ratio of tau bound to MTs (pellet)versus soluble or unbound tau (supernatant) was determined bycomparing the tau immunoreactivities in these twofractions.

Isolation of Insoluble Tau from Transfected CHO Cells

Low-density CHO cell transfectants were grown to 80% confluency and extracted with high-salt RAB containing 0.1% Triton X-100.The cell lysates were subjected to two or more freeze-thaw cyclesto remove tau bound to MTs. The homogenate was centrifuged at50,000 × g for 20 min to generate a supernatant and a pellet.The supernatant was removed, boiled, and then centrifuged at 50,000× g for 20 min. The pellet from the original spin was sonicatedin 2× sample buffer. Samples containing both the supernatant andthe pellet were resolved on 7.5% SDS-PAGE gels and transferredonto nitrocellulose replicas for Western blotanalyses.

Indirect Immunofluorescence Studies of Tau and MTs in Transfected CHO Cells

CHO cell transfectants were fixed with 0.3% glutaraldehyde in PEM buffer [80 mM piperazine-N,N'-bis(2-ethanesulfonic acid),pH 6.8, 5 mM EGTA, 1 mM MgCl₂] for 10 min, and permeabilized with0.5% Triton X-100 in phosphate-buffered saline (PBS) for 15 minbefore quenching the glutaraldehyde with 10 mg/ml sodium borohydridein PBS for 7 min followed by 0.1 M glycine in PBS for 20 min (Blacket al., 1996). After a final rinse in PBS, the cells were incubatedwith 17026, a rabbit polyclonal anti-tau antibody and a monoclonalantibody (MAb) to $alpha$ -tubulin (Blose et al., 1984) for 2 h at roomtemperature. Secondary antibodies were fluorescent-labeled donkeyanti-rabbit IgG and Texas Red-labeled donkey anti-mouse IgG (JacksonLaboratories).

Transmission and Immuno-electron Microscopy (EM) of Transfected CHO Cells

Transmission and pre-embedding immuno-EM was performed on representative samples of CHO cells expressing Wt or mutant tau(VPR and $Delta$ K; n = 3 samples of each) after fixation with 4% paraformaldehydeand 2% glutaraldehyde or 4% paraformaldehyde and 0.25% glutaraldehydein PBS buffer, respectively, for 60 min, followed by quenchingin 0.1% sodium borohydride in Tris-buffered saline for 10 minand treatment for another 10 min with 20% ethanol. For transmissionEM, staining and ultrastructural analysis were performed as describedpreviously (Tu et al., 1995). To facilitate the identificationof fibrils in aggregates of mutant tau, grids were also treatedwith 30% formic acid for 90 s before examination by EM. For immuno-EM,fixed cells were blocked in 5% donor horse serum in PBS with 0.2%cold water fish skin gelatin and 1% ovalbumin for 60 min beforeincubation with 17026, the anti-tau antiserum (dilution 1:500),in 0.1% BSA and PBS overnight at 4°C. A goat anti-rabbit nanogold-IgG(1:40; Nanoprobes Inc., Yaphank, NY) secondary antibody was appliedfor 2 h at room temperature. Silver enhancement was performedby incubating cells with silver enhancement reagent (NanoprobesInc.) for 8 min in the dark. For the diaminobenzidine (DAB) plussilver-gold-enhancement immuno-EM method (Teclemariam-Mesbah etal., 1997), biotinylated goat anti-rabbit IgG (1:100; Vector,Houston, TX) secondary antibody was applied for 2 h at room temperaturefor each set of cells. After visualizing the DAB-positive cellslabeled by routine immuno-EM methods, silver-gold intensificationwas performed by incubating the samples in silver methenaminedeveloper (3% methenamine, 5% silver nitrate, and 1% sodium tetraborate)at 60°C for 5 min as described in Teclemariam-Mesbah et al. (1997).The reaction was stopped with 2% sodium acetate and then stabilizedin 3% sodium thiosulphate for 5 min. Gold toning was obtainedby incubating the cells in 0.1% gold chloride for 5 min, followedby the stabilizationstep.

CHO cells prepared for immuno-EM by using nanogold and DAB plus silver enhancement were fixed with 2% glutaraldehyde in PBSbuffer overnight. Cells were collected and spun down at 1000 ×g for 5 min. The pellet from nanogold-labeled cells were postfixedin 0.5% osmium tetroxide for 30 min at 4°C, whereas the pelletsof DAB plus silver-gold enhancement-labeled cells were treatedin 2% osmium tetroxide for 60 min at 4°C. After dehydration withgraded alcohols and propylene oxide, the pellets were embeddedin Epon-812 and polymerized at 70°C for 48 h. Sixty-five nanometerthin sections were cut and mounted on 200-mesh copper grids, stainedwith 1% uranyl acetate in 50% ethanol by bismuth subnitrite andexamined with a JEM1010 electron microscope at 80kV.

Properties of the Epitope Specific Anti-Tau Antibodies Used in These Studies

The following antibodies to tau proteins, including some that recognize specific epitopes in tau, were used in this study:17026 (a rabbit polyclonal antibody made against the largest humanrecombinant tau; Ishihara et al., 1999); T3P (a rabbit polyclonalantibody raised to a synthetic peptide containing the phosphorylatedSer396; Lee et al., 1991); MAbs T14 and T46 are phosphorylation-independentanti-tau antibodies (Kosik et al., 1988; Trojanowski et al., 1989);MAb T1 (Binder et al., 1985; Szendrei et al., 1993); MAb PHF1(specific for phosphorylated serine 396/404; Greenberg and Davies,1990; Otvos et al., 1994); MAb AT8 (specific for phosphorylatedserine 202 and threonine 205; Goedert et al., 1993, 1994); MAb12E8 (specific for phosphorylated Ser262; Seubert et al., 1995);MAb PHF6 (specific for phosphorylated Thr231; Hoffmann et al.,1997), and MAb AT270 (specific for phosphorylated serine 181;Goedert et al., 1994). The position of the epitope locations forthe anti-tau antibodies used in this study are illustrated inFigure 1. T1 was obtained from Dr. L. Binder, PHF1 from Dr. P.Davies, and AT8 and AT270 from Innogenetics (Alharetta, GA). Themouse MAb to $alpha$ -tubulin was purchased from Amersham (Blose et al.,1984).

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Phosphorylated RW and VPR Mutant Tau40 Isoforms Do Not Exhibit Slower SDS-PAGE Mobility

To examine the effects of FTDP-17 mutations on the properties of mutant versus Wt tau, we subjected stably transfected CHOcell lines to SDS-PAGE. Although most of the tau mutants comigratedwith Wt tau, the RW and VPR tau mutants predominantly exhibiteda faster electrophoretic mobility on SDS-PAGE gel (Figure 2A).To determine whether the faster migrating tau containing the RWmutation corresponded to a reduction in the extent of phosphorylation,high-salt extracts of Wt tau and all of the tau mutants, exceptthe NK and SN, were subjected to enzymatic dephosphorylation withalkaline phosphatase followed by SDS-PAGE (Figure 2B). The NKand SN mutations were not examined in these studies because theyalter exon 10 splicing rather than other properties of tau (Honget al., 1998; D'Souza et al., 1999). Dephosphorylation resultedin the comigration of Wt tau and all the tau mutants examinedhere, suggesting that CHO cell lines expressing tau with an RWmutation is less phosphorylated than Wt and the other tau transfectantswith a single point mutation (Figure 2B).

View larger version (44K):
[in this window]
[in a new window]

Figure 2. SDS-PAGE analysis of the electrophoretic mobility of Wt and mutant tau expressed in CHO cells. Western blot analysis of cell lysates from CHO cells stably expressing either the Wt or mutant tau proteins and probed with a cocktail of MAbs T14 and T46 (T14/46; A). Tau proteins harboring the RW and the triple mutation (VPR) migrate rapidly and nearly in parallel with Wt recombinant tau (R). Extracted Wt and mutant tau proteins were either untreated ( $-$ ) or treated (+) with alkaline phosphatase (Alk Phos) and probed with T14/46 (B). Note that after treatment with Alk Phos all tau proteins migrate as one strong band with R.

Phosphorylation of Tau with the RW Mutation Is Reduced at Ser396 and Ser404

To identify the exact phosphorylation site(s) affected by the RW mutation, we performed immunoblot analysis with a panel ofphosphorylation site- or epitope-specific anti-tau antibodieson lysates of CHO cells expressing Wt tau and several differenttau mutants (Figure 3). The phosphorylation-independent anti-tauMAbs T14 and T46 were used in combination (T14/46) and detectedat least three distinct phosphoisoforms in cells expressing Wt, $Delta$ K, PL, and the VM mutation, but not in cells expressing the RWand the triple VPR mutations. The pattern of tau immunobands detectedby the phosphorylation-dependent MAbs T1, AT270, PHF1, T3P, 12E8,and PHF6 also do not differ significantly in cells expressingWt versus $Delta$ K, PL, and VM mutations. However, CHO cells expressingthe RW and the triple VPR mutations showed a significant reductionin the extent of phosphorylation at Ser396/404 (as detected byT3P and the PHF1 MAb) without affecting phosphorylation at theThr181 (as detected by AT270), Ser262 (as detected by 12E8), andThr231 (as detected by PHF6) sites, suggesting that the RW mutationselectively reduces tau phosphorylation at Ser396 and Ser404 (Figure3). The greater reduction in PHF1 and T3P immunoreactivities ofthe VPR tau mutant relative to the RW tau mutant suggests thatthe V337 M and P301L mutations act synergistically with the RWmutation to reduce tau phosphorylation at Ser396 and Ser404.

View larger version (64K):
[in this window]
[in a new window]

Figure 3. RW and VPR tau mutants exhibit reduced phosphorylation at Ser396 and Ser404. The phosphorylation of Wt and mutant tau at multiple sites was determined by immunoblot analysis with a panel of anti-tau antibodies. Note that the phosphorylation of the RW and VPR tau mutants expressed in CHO cells is reduced at the Ser 396/404 site (as detected by PHF1 and T3P antibodies), but not at Thr181 (AT270), Ser262 (12E8), or Thr231 (PHF6).

Tau Mutations Do Not Alter the Turnover of Tau Phosphoisoforms in Transfected CHO Cells

We also assessed whether the lack of the slower migrating and more phosphorylated tau isoforms in the RW and VPR mutants mightbe due to the inability of CHO cells to phosphorylate tau at sitesthat lead to the mobility shift or a faster turnover of phosphategroups present in the slower migrating tau isoforms. To do this,we examined the turnover of the phosphoisoforms in Wt and mutanttau transfectants by using a pulse-chase paradigm. After the cellswere pulsed with [³⁵S]methionine for 30 min, they were chased for different lengthsof time (Figure 4). At time zero, the majority of the radiolabeledtau proteins migrated as a single poorly phosphorylated band.However, a chase of 3 h generated slower migrating tau isoformsthat we have shown are more phosphorylated (Merrick et al., 1996).Significantly, these slower migrating tau isoforms were detectedat all chase time points in CHO cells expressing Wt tau, PL, and $Delta$ K, but not RW and VPR tau mutants, suggesting that the lattertau mutants are not phosphorylated by CHO cells to generate thesephosphoisoforms (Figure 4). As with PL and Wt tau, $Delta$ K mutantswere also modified by phosphorylation within 3 h after labeling.However, the slowest species of the $Delta$ K tau mutants were not asprominent, suggesting that these mutant forms of tau are not phosphorylatedto the same extent as Wt and PL tau. Thus, our pulse chase studiessupport the idea that the RW and VPR, as well as the $Delta$ K, tau mutantsare not phosphorylated to the same extent as Wt and PL in CHOcells. Finally, these pulse-chase studies also did not revealany significant differences between the turnover rates of theWt versus the mutant tau isoforms.

View larger version (83K):
[in this window]
[in a new window]

Figure 4. Turnover of Wt and mutant tau in CHO cells is similar. Wt and mutant tau proteins were immunoprecipitated at various times after pulse labeling with [³⁵S]methionine. No significant difference in the turnover rate of mutant versus Wt tau was apparent in these cells. However, although Wt tau and PL tau mutants migrated more slowly over the chase period, an indication of increase phosphorylation, the slower migrating tau isoforms are not detected in cells harboring the RW and VPR mutations.

Proteolytic Processing of Tau Is Altered by the $Delta$ K, RW, and VPR Mutations

The reduction in tau phosphorylation at Ser396 and Ser404 in the RW mutants suggests the possibility that a conformationalchange, due to the substitution of arginine with tryptophan atresidue 406 of the 441-amino-acid-long tau protein, could resultin a differential accessibility of kinases and/or endogenous protease(s)to this mutant form of tau. To test this possibility, we preparedcell lysates from Wt and mutant tau CHO cell transfectants inthe absence of protease inhibitors and analyzed the tau fragmentsby Western blotting with multiple anti-tau antibodies (Figure5, A and B). Overall, the pattern of proteolytic tau fragmentsgenerated were similar among Wt tau and PL mutant-expressing cells,but differed from those detected in cells expressing $Delta$ K, RW, andVPR tau mutants. Specifically, a fragment of ~36 kDa appearedto be absent from the RW and VPR tau mutants, and this 36-kDafragment was most likely derived from the carboxy half of taubecause it was detected by both the T46 and T1 Mabs, which arespecific for epitopes, including residues 404-441 and 189-209,respectively (Figure 5, A and B). Another ~43-kDa tau fragmentcleaved at the carboxy terminus was also not detected in the RW,VPR, and $Delta$ K tau mutants. And a 57-kDa fragment cleaved at thecarboxy terminus (because it was detected by T1, but not T46)was not affected by any of the tau mutations examined here. Thedifferences in the pattern of proteolytic fragments are not dueto the extent of tau phosphorylation because dephosphorylationdid not have any effect on the presence or absence of these fragments(our unpublished results). Taken together, these data supportthe notion that a conformational change induced by the $Delta$ K andRW mutations could account for the changes in phosphorylationand proteolysis of these tau mutants.

View larger version (38K):
[in this window]
[in a new window]

Figure 5. Alteration in proteolytic processing by FTDP-17 tau mutations. Immunoblot analysis of tau extracted from CHO cells expressing Wt and FTDP-17 mutant tau proteins showing the intact, full-length species of each tau isoform and the profile of breakdown products generated, as visualized by the T46 MAb (A) and the T1 MAb (B). The banding pattern is altered for the $Delta$ K, RW, and VPR tau mutants relative to Wt tau, suggesting that these mutations induce a conformational change that modifies the proteolysis of these proteins.

$Delta$ K and VPR Tau Mutants Develop Tau Aggregates as Detected by Indirect Immunofluorescence

To assess whether any of the overexpressed tau mutants in CHO cells develop tau aggregates, indirect immunofluorescence studieswere conducted. As observed previously for Wt tau (Kanai et al.,1989; Bramblett et al., 1993), the expression of RW mutant tauin CHO cells resulted in the bundling of MTs and the formationof MT cables around the nucleus, as detected by anti- $alpha$ -tubulinand anti-tau antibodies (compare Figure 6A with B, and E withF). In fact, the staining of Wt tau and RW tau mutants colocalizedalmost exactly with that of $alpha$ -tubulin (Figure 6, A and B). Moreover,the staining pattern of the PL and VM tau mutant expressing CHOcell clones looked comparable to the CHO cells expressing Wt tau(our unpublished results). However, the tau and MT staining patternwas dramatically different in cells expressing either the $Delta$ K orVPR tau mutants. Specifically, focal tau immunoreactivities weredetected in ~70-80% of the CHO cell transfectants with the $Delta$ Kand the VPR tau mutations, and these tau immunoreactive aggregateswere present throughout the perinuclear cytoplasm, although theyvaried in size and shape (Figure 6, C and D). In addition to thesetau aggregates, tau staining in these cells was mostly diffuseand did not colocalize with the MT network (Figure 6, C and D).Furthermore, the aggregates seen in CHO cells expressing the $Delta$ Kand VPR mutant tau were also immunostained by the MAb Alz50 andother phosphorylation-dependent and -independent anti-tau antibodies(our unpublished results). The inclusions did not contain f-actin(our unpublished results) or $beta$ -tubulin (Figure 8, C and D). Thelack of MT bundling in these CHO cells suggests that the $Delta$ K andVPR tau mutants do not bind very well to MTs (Figure 6, G andH).

View larger version (54K):
[in this window]
[in a new window]

Figure 6. FTDP-17 missense mutations induce tau aggregation and disrupt MT bundling. CHO cells expressing Wt and mutant tau were plated onto glass coverslips and allowed to settle overnight. After fixation in 0.3% glutaraldehyde, cells were permeabilized with Triton X-100 and immunostained with recombinant tau (17026) (A-D and I-L) and $alpha$ -tubulin (E-H and I-L). Colocalization and bundling of tau and tubulin are readily apparent in cells with Wt (A, E, and I) and RW (B, F, and J) tau. This pattern is completely disrupted with the expression of the $Delta$ K and VPR tau mutants. Note that in CHO cells expressing these tau mutants, tau and tubulin no longer colocalize (K and L), the tubulin network is not bundled (G and H), and aggregates of tau are apparent (C and D). Bar, 30 µm at 20×.

$Delta$ K and VPR Mutant Tau Show Significantly Reduced MT Binding

To further confirm that $Delta$ K and VPR tau mutants expressed in CHO cells lead to reduced binding to MTs, we compared the abilityof Wt and mutant tau proteins extracted from CHO cells to bindto endogenous MTs. As shown in Figure 7, A and B, the amount oftau bound to MTs and recovered from the pellets comprised ~75%of the total tau in CHO cell transfectants expressing the Wt tau,and PL, VM, and RW tau mutants, whereas only 48 and 40% of boundtau proteins were recovered from cells expressing the $Delta$ K and VPRtau mutants, respectively. The specific reduction of the VPR taumutants to MTs was further substantiated by similar data fromthree different subclones of VPR transfectants (Figure 7, C andD). Finally, we showed that ~80% of the tubulin was recoveredin the pellet in all tau transfectants (Figure 7, A and C).

View larger version (25K):
[in this window]
[in a new window]

Figure 7. FTDP-17 missense mutations decrease the binding of tau to MT. Cell lysates from CHO cells stably expressing Wt or mutant tau were separated into cytoskeletal (P) and soluble fractions (S) after MT assembly. The amount of tau and $alpha$ -tubulin present in each fraction was determine by immunoblot analysis with I¹²⁵-conjugated secondary antibody for quantification (A and C). (B and D) Quantitation of the percentage of tau in the soluble fraction relative to the total amount of tau present. Note that the $Delta$ K and VPR mutations significantly reduce the binding of tau to MT, leaving more of these mutant proteins free in the soluble fraction. (n = 4, *p < 0.01), and that the dramatic loss of MT binding was evident in three different CHO cell clones that expressed the VPR tau mutants (C and D).

Abundant Tau Aggregates Are Present in $Delta$ K- and VPR-Expressing CHO Cells

To further investigate the inclusions formed by the $Delta$ K and VPR tau mutants, transfected CHO cells were maintained on coverslipsfor either 1 or 3 d. After 1 d in culture, numerous small tau-positiveaggregates were detected (Figure 8A), which did not disrupt theMT network (Figure 8B). However, after 3 d in culture, much larger,variably shaped tau-positive aggregates (~1-3 per cell) appearedin >80% of the CHO cells expressing the $Delta$ K and VPR tau mutations(Figure 8C). These tau aggregates also did not perturb the MTnetwork (Figure 8D). To determine whether tau filaments were foundin the small and large tau inclusions, transmission EM and immuno-EMstudies were conducted. Strong tau-positive staining was localizedto both the small and large tau aggregates (Figure 8, E-H). Occasionalfilaments were also detected in the aggregates by transmissionEM (Figure 9, A and B), but they were better visualized afterformic acid extraction (Figure 9, C and D). The tau-positive aggregateswere not detected by histochemical dye such as Thioflavin S, indicatingthat there is probably not sufficient numbers of filaments formedand/or that there is insufficient cross $beta$ -pleated sheet structuresin these inclusions.

View larger version (100K):
[in this window]
[in a new window]

Figure 8. Aggregates of FTDP-17 tau mutants grow larger with time. CHO cells stably expressing Wt tau and mutant tau protein were plated at low density on coverslips and grown for either 1 or 3 d. (A-D) Double-labeled immunofluorescence images of CHO cells expressing the VPR tau mutants immunostained with rabbit antirecombinant tau (17026; A and C) and a MAb to $alpha$ -tubulin (B and D) in cells grown for 1 d (A and B) or 3 d (C and D). (E-H) Immuno-EM detection of tau by using 17026 as the primary antibody visualized either with secondary antibody and silver-enhanced DAB (E and F) or nanogold conjugated secondary antibody (G and H). Bar, 10 µm at 60× for immunofluorescence photomicrographs; bar, 100 nm for immuno-EM.

View larger version (211K):
[in this window]
[in a new window]

Figure 9. Aggregates with fibrillar structures are detected in CHO cells expressing the VPR tau mutants. Transmission EM of tau aggregates at low (A and C) and corresponding high (B and D) magnifications. (C and D) Images of aggregates that were treated with formic acid. The image in D is a higher magnification of the lower left portion of the inclusion seen in C. Arrowheads in C correspond to the same region that is marked by arrowheads at higher magnification in D. Arrows in B and D highlight fibril-like structures within the aggregates. Bar, 100 nm.

Tau with $Delta$ K and VPR Mutations Becomes More Insoluble than Other Tau Isoforms Expressed in Transfected CHO Cells

To assess whether the formation of tau aggregates correlated with the accumulation of insoluble mutant tau proteins, we comparedthe amount of insoluble tau recovered from tau transfectants expressingeither Wt tau or the $Delta$ K or VPR tau mutants after extraction withhigh-salt RAB buffer containing 0.1% Triton X-100. We found asignificant increase in the amount of insoluble tau recoveredfrom CHO cells expressing the $Delta$ K (~5 fold) and the VPR tau mutants(~17 fold) compared with the amount detected in Wt tau-expressingCHO cells (Figure 10, A and B).

View larger version (14K):
[in this window]
[in a new window]

Figure 10. FTDP-17 tau mutant become increasingly insoluble in CHO cells. Soluble and insoluble fractions of tau from CHO cells expressing Wt and FTDP-17 mutant tau protein were isolated and evaluated by immunoblot analysis with Tau14/46 (A). Quantitative analysis (n = 3) of the percentage of insoluble tau relative to the soluble fraction in Wt-, $Delta$ K-, and VPR-expressing CHO cells (B). There is an increase in the amount of insoluble tau present in cells expressing the $Delta$ K and VPR tau mutants relative to Wt tau.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Our study demonstrates for the first time that the overexpression of specific FTDP-17 tau mutants in CHO cells leads to theformation of intracytoplasmic tau aggregates that can be detectedby indirect immunofluorescence, transmission EM, and immuno-EM.Furthermore, the presence of tau aggregates correlates with mutanttau proteins that remain insoluble in nonionic detergents suchas Triton X-100. Other evidence also supports the view that topographicallyseparate missense mutations in the tau gene pathogenic for FTDP-17differentially alter the biochemical properties and/or functionsof the corresponding tau mutants in transfected non-neuronal cells.Specifically, our data show that some missense mutations alterthe phosphorylation of tau at specific sites and other mutationsreduce the MT binding ability of tau. Although evidence is emergingto suggest that topographically distinct intronic and exonic FTDP-17tau gene mutations result in losses of different tau functionsand/or gains of toxic properties by tau isoforms (Clark et al.,1998; Hasegawa et al., 1998; Hong et al., 1998; Hutton et al.,1998; D'Souza et al., 1999; Dayanandan et al., 1999; Matsumuraet al., 1999), the study reported here comprehensively analyzedand compared the consequences of diverse FTDP-17 missense substitutionson the biochemical and functional properties of tau mutants expressedin stably transfected cells. Significantly, we demonstrated adirect correlation between missense substitutions that reducethe ability of the corresponding tau mutants to bind MTs and theformation of intracytoplasmic accumulations of insoluble tau aggregates.Thus, our findings support the hypothesis that a reduction inthe binding of tau to MTs, concomitant with increased levels ofunbound tau proteins, could initiate a pathological cascade leadingto the aggregation and assembly of tau into abnormalfilaments.

It is well known that phosphorylation regulates the binding of tau to MTs, that increased phosphorylation at specific sitesin tau reduces MT binding, and that hyperphosphorylated PHF-tauis completely unable to bind MTs, but that this function can berestored by enzymatic dephosphorylation of PHF-tau (Bramblettet al., 1993; Yoshida and Ihara, 1993). However, it is unclearwhether phosphorylation plays a role in the pathogenesis of thetopographically separate FTDP-17 missense tau mutations. Indirectevidence from our studies showed that a change in the secondarystructure of tau rather than phosphorylation mediates the pathogenicityof some of the missense mutations. For example, we demonstratedthat the RW mutation causes a selective reduction in tau phosphorylationat Ser396 and Ser404 and that this reduction is most likely aconsequence of altered secondary structure around the site ofR406W mutation. The data to support this idea are as follows.First, the Ser396 and Ser404 residues are the only phosphorylationsites that are affected and they are located close to the R406Wresidue. This implies that a change in local secondary structurecould impede phosphorylation by specific kinases. Second, differencesin the pattern of proteolytic fragments generated from the RWmutant compared with Wt tau suggest differential accessibilityof Wt and RW mutant tau to endogenous proteases. Third, the observationthat nonphosphorylated, bacterially expressed recombinant RW mutanttau bind less well to MTs compared with Wt tau suggests that phosphorylationis not responsible for this reduction (Hasegawa et al., 1998;Hong et al., 1998). Fourth, because the R406W mutation is notlocated on a MT binding repeat or an inter-repeat region, it shouldnot alter MT binding directly. Finally, the reduction in phosphorylationat Ser396, which we observed in tau proteins extracted from thebrains of affected members of a kindred with a RW tau gene mutation,lend further support to our experimental results (Reed et al.,1997; our unpublished observation). Thus, our data are consistentwith a change in the secondary structure induced by the RWmutation.

Previous in vitro studies have shown that recombinant PL, VM, RW, and $Delta$ K tau mutants isolated from genetically engineeredE. coli have a reduced binding affinity for MTs (Hasegawa et al.,1998; Hong et al., 1998; D'Souza et al., 1999). However, whenexpressed in transfected CHO cells, none of these tau mutants,except for the $Delta$ K tau mutant, exhibited reduced MT binding. Thereason for this discrepancy is most likely due to technical limitationsin the ability to control precisely the expression of tau proteinin transfected cells such that a small reduction in the affinityof tau for MT cannot be detected. This hypothesis is supportedby the observation that introduction of three mutations (VPR)in a single tau isoform amplifies this reduction to levels thatcan be readily observed. In contrast, the single $Delta$ K mutation causeda significant reduction in the MT binding ability of the correspondingtau mutant. Indeed, the 280K residue, which is located in theinter-repeat region of tau between MT binding repeat 1 and 2,was identified previously as one of three lysine residues thatis most critical in modulating the binding of tau to MTs (Goodeand Feinstein, 1994). Furthermore, our previous in vitro dataon MT binding showed that the $Delta$ K mutation caused the most dramaticreduction in the MT binding affinity of tau compared with othertau mutants harboring one of several different missense substitutions(Hong et al., 1998; D'Souza et al., 1999). Additionally, the $Delta$ Kmutation perturbs the alternative splicing of tau resulting inthe diminished inclusion of exon 10 (D'Souza et al., 1999). Thus,the $Delta$ K missense mutation may be pathogenic for FTDP-17 by disruptingmechanisms that regulate the expression of the tau gene and/orby altering biochemical properties of tau isoforms that are criticalfor the function and viability of CNS neurons andglia.

Indeed, multiple pathogenic mechanisms have been proposed for the diverse FTDP-17 mutations and several FTDP-17 mutationsappear to cause tau dysfunction by reduced MT binding and/or promotingfilament formation. We speculate that the reduced binding of tauto MTs is an initiating event that leads to the formation of abnormaltau filaments and/or the aggregation of tau. This hypothesis issupported by several lines of evidence from our studies of the $Delta$ K and VPR tau mutants. First, the $Delta$ K and VPR tau mutants werethe only two mutants that evidenced a reduction in the abilityto bind MTs, and they also were the only tau mutants that aggregatedinto tau-rich inclusions in the cytoplasm of CHO cells. Second,although other FTDP-17 missense mutations (e.g., PL) were shownto facilitate the aggregation of bacterially expressed recombinanttau in the presence of heparin (Goedert et al., 1999; Nacharajuet al., 1999; Gamblin et al., 2000), none of the other tau mutants(including PL) we studied in CHO cells developed detectable intracytoplasmictau aggregates by using the criteria established here. Finally,because the turnover rate of Wt tau and all the tau mutants inCHO transfectants was similar, it seems unlikely that the taupathologies caused by the $Delta$ K and VPR mutations are the resultof decreased turnover of the mutant tau proteins. Instead, ourdata are consistent with the interpretation that these mutationsmay be pathogenic because they cause a reduction in the bindingof tau to MTs, resulting in an increase in the cytosolic concentrationof tau that culminates in aggregation of tau in the cytoplasm.However, we cannot rule out the possibility that these specificmutations also could promote tau aggregation and filament formationby othermechanisms.

Although filaments were detected within aggregates that also were decorated by anti-tau antibodies, these filaments are notidentical to authentic PHFs in Alzheimer's disease or tau filamentsin tangles of FTDP-17 patients. This is not surprising becausetau tangles undoubtedly develop over a long period of time andthey are found in postmitotic neurons and nondividing glial cells.Indeed, our observations that the aggregates become larger inmutant CHO transfectants cultured for 3 versus 1 d support theidea that the formation of tau tangles may be a slow process.Nevertheless, our ability to demonstrate the formation of somefilaments within the tau aggregates in dividing non-neuronal CHOcells provides proof of the concept that increasing levels ofcytosolic mutant tau proteins can lead to the assembly of tauthat aggregate into inclusions, and the identification of specifictau mutants that form insoluble fibrillar aggregates will facilitatefuture efforts to develop in vitro models of PHFs in postmitoticneurons and glial cells. Finally, because we link the formationof tau aggregates to reduced MT binding caused by specific mutations,these data support the hypothesis that both gains of toxic propertiesand losses of normal tau functions are involved in the onset/progressionof neurodegenerative tauopathies. Thus, the CHO cell mutant taumodel system described here will be useful in studies designedto further elucidate mechanisms leading to the formation of taupathology in thesediseases.

	ACKNOWLEDGMENTS

We thank the Biomedical Imaging Core Facility of the University of Pennsylvania for their assistance in the EM studies. Supportedin part by grants from the National Institute on Aging and theJohn H. Ware III Endowed Chair for Alzheimer's DiseaseResearch.

	FOOTNOTES

Corresponding author. E-mail address: vmylee{at}mail.med.upenn.edu.

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Andreadis, A., Brown, W.M., and Kosik, K.S. (1992). Structure and novel exons of the human tau gene. Biochemistry 31, 10626-10633[Medline].
Binder, L.I., Frankfurter, A., and Rebhun, L.I. (1985). The distribution of tau in the mammalian central nervous system. J. Cell Biol. 101, 1371-1378[Abstract/Free Full Text].
Black, M.M., Slaughter, T., Moshiach, S., Obrocka, M., and Fischer, I. (1996). Tau is enriched on dynamic microtubules in the distal region of growing axons. J. Neurosci. 16, 3601-3619[Abstract/Free Full Text].
Blose, S.H., Meltzer, D.I., and Feramisco, J.R. (1984). 10 nm Filaments are induced to collapse in living cells microinjected with monoclonal and polyclonal antibodies against tubulin. J. Cell Biol. 98, 847-858[Abstract/Free Full Text].
Bramblett, G.T., Goedert, M., Jakes, R., Merrick, S.E., Trojanowski, J.Q., and Lee, V.M.-Y. (1993). Abnormal tau phosphorylation at Ser396 in Alzheimer's disease recapitulates development and contributes to reduced microtubule binding. Neuron 10, 1089-1099[Medline].
Chen, C., and Okayama, H. (1987). High-efficiency. transformation of mammalian cells by plasmid DNA. Mol. Cell. Biol. 7, 2745-2752[Abstract/Free Full Text].
Clark, L.N., Poorkaj, P., Wszolek, Z.K., Geschwind, D.H., Nasreddine, Z.S., Miller, B., Payami, H., Awert, F., Markopoulou, K., D'Souza, I., Lee, V.M.-Y., Reed, L.A., Trojanowski, J.Q., Zhukareva, V., Bird, T.D., Schellenberg, G.D., and Wilhelmsen, K. (1998). Pathogenic implications of mutations in the tau gene in pallido-ponto-nigral degeneration and related chromosome 17-linked neurodegenerative disorders. Proc. Natl. Acad. Sci. USA 95, 13103-13107[Abstract/Free Full Text].
D'Souza, I., Poorkaj, P., Hong, M., Nochlin, D., Lee, V.M.-Y., Bird, T.D., and Schellenberg, G.D. (1999). Missense and silent tau gene mutations cause frontotemporal dementia with parkinsonism-chromosome 17 type, by affecting multiple alternative RNA splicing regulatory elements. Proc. Natl. Acad. Sci. USA 96, 5598-5603[Abstract/Free Full Text].
Dayanandan, R., Van, S.M., Mack, T.G., Ko, L., Yen, S.H., Leroy, K., Brion, J.P., Anderton, B.H., Hutton, M., and Lovestone, S. (1999). Mutations in tau reduce its microtubule binding properties in intact cells and affect its phosphorylation. FEBS Lett. 446, 228-232[Medline].
Drechsel, D.N., Hyman, A.A., Cobbs, M.H., and Kirschner, M.W. (1992). Modulation of the dynamic instability of tubulin assembly by the microtubule-associated protein tau. Mol. Biol. Cell 3, 1141-1154[Abstract].
Ebneth, A., Godemann, R., Stamer, K., Illenberger, S., Trinczek, B., and Mandelkow, E. (1998). Overexpression of tau protein inhibits kinsesin-dependent trafficking of vesicles, mitochondria, and endoplasmic reticulum: implication for Alzheimer's disease. J. Cell Biol. 143, 777-794[Abstract/Free Full Text].
Gamblin, T.C., King, M.E., Dawson, H., Vitek, M.P., Kuret, J., Berry, R.W., and Binder, L.I. (2000). In vitro polymerization of tau proteins monitored by laser light scattering: method and application to the study of FTDP-17 mutants. Biochemistry 39, 6136-6144[Medline].
Goedert, M., Jakes, R.A., and Crowther, R.A. (1999). Effects of frontotemporal dementia FTDP-17 mutations on heparin-induced assembly of tau filaments. FEBS Lett. 450, 306-311[Medline].
Goedert, M., Jakes, R., Crowther, R.A., Cohen, P., Vanmechelen, E., Vandermeeren, M., and Cras, P. (1994). Epitope mapping of monoclonal antibodies to the paired helical filaments of Alzheimer's disease: identification of phosphorylation sites in tau protein. Biochem. J. 301, 871-877.
Goedert, M., Jakes, R., Crowther, R.A., Six, J., Lubke, U., Vandermeeren, M., Cras, P., Trojanowski, J.Q., and Lee, V.M.-Y. (1993). The abnormal phosphorylation of tau protein at Ser²⁰² in Alzheimer disease recapitulates phosphorylation during development. Proc. Natl. Acad. Sci. USA 90, 5066-5070[Abstract/Free Full Text].
Goedert, M., Spillantini, M.G., Jakes, R., Rutherford, D., and Crowther, R.A. (1989). Multiple isoforms of human microtubule-associated protein tau: sequences and localization in neurofibrillary tangles of Alzheimer's disease. Neuron 3, 519-526[Medline].
Goedert, M., Trojanowski, J.Q., and Lee, V.M.-Y. (1997). The neurofibrillary pathology of Alzheimer's disease. In: The Molecular and Genetic Basis of Neurological Diseases, ed. S.B. Prusiner, R.N. Rosenberg, S. Di Mauro, and R.L. Barchi, Boston: Butterworth Heineman Press, 613-627.
Goode, B.L., and Feinstein, S.C. (1994). Identification of a novel microtubule binding and assembly domain in the developmentally regulated inter-repeat region of tau. J. Cell Biol. 124, 769-782[Abstract/Free Full Text].
Greenberg, S.G., and Davies, P. (1990). A preparation of Alzheimer paired helical filaments that displays distinct tau proteins by polyacrylamide gel electrophoresis. Proc. Natl. Acad. Sci. USA 87, 5827-5831[Abstract/Free Full Text].
Hasegawa, M., Smith, M.J., and Goedert, M. (1998). Tau proteins with FTDP-17 mutations have a reduced ability to promote microtubule assembly. FEBS Lett. 437, 207-210[Medline].
Hoffmann, R., Lee, V.M.-Y., Leight, S., Varga, I., and Otvos, L.J. (1997). Unique Alzheimer's. disease paired helical filament specific epitopes involve double phosphorylation at specific sites. Biochemistry 36, 8114-8124[Medline].
Hong, M., Zhukareva, V., Vogelsberg-Ragaglia, V., Wszolek, Z., Reed, L., Miller, B.I., Geschwind, D.H., Bird, T.D., McKeel, D., Goate, A., Morris, J.C., Wilhelmsen, K.C., Schellenberg, G.D., Trojanowski, J.Q., and Lee, V.M.-Y. (1998). Mutation-specific functional impairments in distinct tau isoforms of hereditary FTDP-17. Science 282, 1914-1917[Abstract/Free Full Text].
Hutton, M., Lendon, C.L., Rizzu, P., Baker, M., Froelich, S., Houlden, H., Pickering-Brown, S., Chakraverty, S., Isaacs, A., Grover, A., Hackett, A., Adamson, J., Lincoln, S., Dickson, D., et al. (1998). Association of missense and 5'-splice-site mutations in tau with the inherited dementia FTDP-17. Nature 393, 702-705[Medline].
Iijima, M., Tabira, T., Poorkaj, P., Schellenberg, G.D., Trojanowski, J.Q., Lee, V.M.-Y., Schmidt, M.L., Takahashi, K., Nabika, T., Matsumoto, T., Yamashita, Y., Yoshioka, S., and Ishino, H. (1999). A. distinct familial presenile dementia with a novel missense mutation in the tau gene. NeuroReport 10, 497-501[Medline].
Ishihara, T., Hong, M., Zhang, B., Nakagawa, Y., Lee, M.K., Trojanowski, J.Q., and Lee, V.M.-Y. (1999). Age-dependent emergence and progression of a tauopathy in transgenic mice overexpressing the shortest human tau isoform. Neuron 24, 751-762[Medline].
Kanai, Y., Takemura, R., Oshima, T., Mori, H., Ihara, Y., Yanagisawa, M., Masaki, T., and Hirokawa, N. (1989). Expression of multiple tau isoforms and microtubule bundle formation in fibroblasts transfected with a single tau cDNA. J. Cell Biol. 109, 1173-1184[Abstract/Free Full Text].
Kosik, K.S., Orecchio, L.D., Binder, L., Trojanowski, J.Q., Lee, V.M.-Y., and Lee, G. (1988). Epitopes that span the tau molecule are shared with paired helical filaments. Neuron 1, 817-825[Medline].
Lee, V.M.-Y., Balin, B.J., Otvos, L., Jr., and Trojanowski, J.Q. (1991). A68. A major subunit of paired helical filaments and derivatized forms of normal tau. Science 251, 675-678[Abstract/Free Full Text].
Matsumura, N., Yamazaki, T., and Ihara, Y. (1999). Stable expression in Chinese hamster ovary cells of mutated tau genes causing frontotemporal dementia and parkinsonism linked to chromosome 17 (FTDP-17). Am. J. Pathol. 154, 1649-1656[Abstract/Free Full Text].
Merrick, S.E., Demoise, D.C., and Lee, V.M.-Y. (1996). Site-specific dephosphorylation of tau protein at Ser²⁰²/Thr²⁰⁵ in response to microtubule depolymerization in cultured human neurons involves protein phosphatase 2A. J. Biol. Chem. 271, 5589-5594[Abstract/Free Full Text].
Nacharaju, P., Lewis, J., Easson, C., Yen, S., Hackett, J., Hutton, M., and Yen, S.H. (1999). Accelerated filament formation from tau protein with specific FTDP-17 missense mutations. FEBS Lett. 447, 195-199[Medline].
Otvos, L., Jr., Feiner, L., Lang, E., Szendrei, G.I., Goedert, M., and Lee, V.M.-Y. (1994). Monoclonal antibody PHF-1 recognizes tau protein phosphorylated at serine residues 396 and 404. J. Neurosci. Res. 39, 669-673[Medline].
Poorkaj, P., Bird, T.D., Wijsman, E., Nemens, E., Garruto, R.M., Anderson, L., Andreadis, A., Wiederholt, W.C., Raskind, R., and Schellenberg, G.D. (1998). Tau is a candidate gene for chromosome 17 frontotemporal dementia. Ann. Neurol. 43, 815-825[Medline].
Reed, L.A., Grabowski, T.J., Schmidt, M.L., Morris, J.C., Goate, A., Solodkin, A., Van, H.G., Schelper, R.L., Talbot, C.J., Wragg, M.A., and Trojanowski, J.Q. (1997). Autosomal dominant dementia with widespread neurofibrillary tangles. Ann. Neurol. 42, 564-572[Medline].
Rizzu, P., Van Swieten, J.C., Joosse, M., Hasegawa, M., Stevens, M., Tibben, A., Niermeijer, M.F., Hillebrand, M., Ravid, R., Oostra, B.A., Goedert, M., Van, D.C., and Heutink, P. (1999). High prevalence of mutations in the microtubule-associated protein tau in a population study of frontotemporal dementia in the Netherlands. Am. J. Hum. Genet. 64, 414-421[Medline].
Seubert, P., Mawal-Dewan, M., Barbour, B., Jakes, R., Goedert, M., Johnson, G.V.W., Litersky, J.M., Schenk, D., Lieberburg, I., Trojanowski, J.Q., and Lee, V.M.-Y. (1995). Detection of phosphorylated Ser²⁶² in fetal tau, adult tau, and paired helical filament tau. J. Biol. Chem. 270, 18917-18922[Abstract/Free Full Text].
Spillantini, M.G., and Goedert, M. (1998). Tau protein pathology in neurodegenerative diseases. Trends Neurosci. 21, 428-433[Medline].
Szendrei, G.I., Lee, V.M.-Y., and Otvos, L.J. (1993). Recognition of the minimal epitope of monoclonal antibody Tau-1 depends upon the presence of a phosphate group but not its location. J. Neurosci. Res. 34, 243-249[Medline].
Teclemariam-Mesbah, R., Wortel, J., Romijn, H.J., and Buijs, R.M. (1997). A simple silver-gold intensification procedure for double DAB labeling studies in electron microscopy. J. Histochem. Cytochem. 45, 619-621[Free Full Text].
Trojanowski, J.Q., Schuck, T., Schmidt, M.L., and Lee, V.M.-Y. (1989). Distribution of tau proteins in the normal human central and peripheral nervous system. J. Histochem. Cytochem. 37, 209-215[Abstract].
Tu, P.-H., Elder, G., Lazzarini, R.A., Nelson, D., Trojanowski, J.Q., and Lee, V.M.-Y. (1995). Overexpression of the human NFM subunit in transgenic mice modifies the level of endogenous NFL and the phosphorylation state of NFH subunits. J. Cell Biol. 129, 1629-1640[Abstract/Free Full Text].
Vogelsberg-Ragaglia, V., Trojanowski, J.Q., and Lee, V.M.-Y. (1999). Cell biology of tau and cytoskeletal pathology in Alzheimer's disease. In: Alzheimer's Disease, ed. R.D. Terry, R. Katzman, K.L. Bick, and S.S. Sisodia, Philadelphia: Lippincott, Williams & Wilkins, 359-371.
Weingarten, M.D., Lockwood, A.H., Hwo, S.Y., and Kirschner, M.W. (1975). A protein factor essential for microtubule assembly. Proc. Natl. Acad. Sci. USA 72, 1858-1862[Abstract/Free Full Text].
Yoshida, H., and Ihara, Y. (1993). Tau in paired helical filaments is functionally distinct from fetal tau: assembly incompetence of paired helical filament-tau. J. Neurochem. 61, 1183-1186[Medline].

This article has been cited by other articles:

B. Bandyopadhyay, G. Li, H. Yin, and J. Kuret
Tau Aggregation and Toxicity in a Cell Culture Model of Tauopathy
J. Biol. Chem., June 1, 2007; 282(22): 16454 - 16464.
[Abstract] [Full Text] [PDF]

A. I. Iliev, S. Ganesan, G. Bunt, and F. S. Wouters
Removal of Pattern-breaking Sequences in Microtubule Binding Repeats Produces Instantaneous Tau Aggregation and Toxicity
J. Biol. Chem., December 1, 2006; 281(48): 37195 - 37204.
[Abstract] [Full Text] [PDF]

J. M. Bunker, K. Kamath, L. Wilson, M. A. Jordan, and S. C. Feinstein
FTDP-17 Mutations Compromise the Ability of Tau to Regulate Microtubule Dynamics in Cells
J. Biol. Chem., April 28, 2006; 281(17): 11856 - 11863.
[Abstract] [Full Text] [PDF]

				A. I. Iliev, S. Ganesan, G. Bunt, and F. S. Wouters Removal of Pattern-breaking Sequences in Microtubule Binding Repeats Produces Instantaneous Tau Aggregation and Toxicity J. Biol. Chem., December 1, 2006; 281(48): 37195 - 37204. [Abstract] [Full Text] [PDF]

				J. M. Bunker, K. Kamath, L. Wilson, M. A. Jordan, and S. C. Feinstein FTDP-17 Mutations Compromise the Ability of Tau to Regulate Microtubule Dynamics in Cells J. Biol. Chem., April 28, 2006; 281(17): 11856 - 11863. [Abstract] [Full Text] [PDF]