Dynamic Regulation of Expression and Phosphorylation of Tau by Fibroblast Growth Factor-2 In Neural Progenitor Cells from Adult Rat Hippocampus

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The Journal of Neuroscience, July 1, 1999, 19(13):5245-5254

Dynamic Regulation of Expression and Phosphorylation of Tau by Fibroblast Growth Factor-2 In Neural Progenitor Cells from Adult Rat Hippocampus
Yoshitaka Tatebayashi , Khalid Iqbal, and Inge Grundke-Iqbal
New York State Institute for Basic Research in Developmental Disabilities, Staten Island, New York 10314

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The nature of the extracellular signals that regulate the expression and the phosphorylation of the microtubule-associatedprotein tau, which is aberrantly hyperphosphorylated in Alzheimerdisease and other adult-onset neurodegenerative diseases, is notknown. We have found that neural progenitor cells from adult rathippocampus express adult isoforms of tau and that the expressionand the phosphorylation of tau are regulated by fibroblast growthfactor-2 (FGF-2). Astrocytes that are differentiated from thesecells by stimulation with ciliary neurotrophic factor expressphosphorylated tau similarly when cultured in the presence ofFGF-2. In fetal progenitor cells that express only the fetal tauisoform, expression, but not the phosphorylation, of this proteinis regulated by FGF-2 in cultures of higher passages. The FGF-2-mediatedtau hyperphosphorylation is inhibited by lithium, an inhibitorof glycogen synthase kinase-3 (GSK-3), but not by inhibitors ofmitogen-activated protein kinase or the cyclin-dependent kinases.Furthermore, both GSK-3 activity and the phosphorylation of tauincrease when the concentration of FGF-2 is increased up to 40ng/ml. These results demonstrate that proliferating adult rathippocampal progenitor cells express adult isoforms of tau stablyand that FGF-2 upregulates the expression and, by upregulatingGSK-3 activity, the phosphorylation oftau.

Key words: tau; fibroblast growth factor-2; glycogen synthase kinase-3; neural progenitor cells; phosphorylation; adult tau isoforms; Alzheimer Disease

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Neural progenitor (or stem) cells are multipotential precursor cells that can give rise to both neurons and glia in the fetaland adult CNS (for review, see McKay, 1997). Most of the progenitorcells from adult hippocampus expanded by fibroblast growth factor-2(FGF-2) are immunohistochemically positive for the intermediatefilament nestin, the neuronal marker microtubule-associated protein-2C(MAP-2C), neuron-specific enolase, and the immature glial markerO4, but only a few of the cells have been found to be positivefor markers of differentiation such as glial fibrillary acidicprotein (GFAP), myelin basic protein, or neurofilament H (Gageet al., 1995; Palmer et al., 1997). However, little is known aboutthe expression of the neuronal MAP tau in these progenitor cells.The expression of tau is regulated developmentally; i.e., whereasin adult mammalian brain several isoforms are produced from asingle gene by alternative splicing, in fetal brain only a singleisoform is expressed that corresponds to the smallest of the tauisoforms (Lee et al., 1988; Goedert et al., 1989; Kosik et al.,1989). One of the most important post-translational modificationsof tau is phosphorylation, because the degree of phosphorylationregulates its biological activity (Lindwall and Cole, 1984). Normaladult tau, which contains two to three phosphate groups, promotesthe assembly of microtubules in vitro, and fetal tau, which ishyperphosphorylated to an intermediate degree, has less activity(Yoshida and Ihara, 1993). In Alzheimer disease (AD), tau is hyperphosphorylatedabnormally (Grundke-Iqbal et al., 1986a,b; Iqbal et al., 1986).It contains up to 9 mol of phosphate per mole of the protein (Köpkeet al., 1993) and is microtubule assembly-incompetent (Alonsoet al., 1994; Iqbal et al., 1994).

In the present study, using adult hippocampal progenitor cells expanded by FGF-2, we demonstrate for the first time that thesecells express adult isoforms of tau that are phosphorylated, especiallyat Ser 195/198/199/202, the Tau-1 site. Interestingly, in thesecells, FGF-2 upregulates the expression and phosphorylation oftau at the Tau-1 site. We show that the mechanism of the hyperphosphorylationof tau by FGF-2 involves the upregulation of the glycogen synthasekinase-3 (GSK-3) activity; the mitogen-activated protein kinase(MAPK) and cyclin-dependent kinase (cdk) pathways are not involvedin this mechanism. On the other hand, fetal hippocampal progenitorcells expanded by FGF-2 express only the fetal isoform of taufor which the expression is regulated by FGF-2, but only in thelate passages, and FGF-2 has no effect on its phosphorylation.Thus, FGF-2 is the first identified extracellular regulator forexpression and phosphorylation of tau in neural cells derivedfrom adultCNS.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Antibodies, enzyme inhibitors, isolation of tau. The following phosphorylation-dependent, site-specific monoclonal and phosphorylation-independentpolyclonal antibodies to tau were used: Tau-1 (to unphosphorylatedSer 195, 198, 199, or 202; numbers according to the longest humantau isoform, corresponding to Ser 186, 189, 190, or 193 in thelongest rat tau isoform; ascites, 1:50,000) (Binder et al., 1985;Grundke-Iqbal et al., 1986a; Szendrei et al., 1993); PHF-1 (tophosphorylated Ser 396/404 in human and Ser 387/395 in rat; culturesupernatant, 1:100) (Greenberg et al., 1992; Otvos et al., 1994);M4 (to phosphorylated Thr 231/Ser 235 in human and Thr 222/Ser226 in rat; ascites, 1:2000) (Hasegawa et al., 1993); 12E8 (tophosphorylated Ser 262/356 in human and Ser 253/347 in rat; 1µg/ml) (Seubert et al., 1995); rabbit antisera to isolated bovinetau, 92e (1:5000; Grundke-Iqbal et al., 1988); and to recombinanthuman tau ₄₁₀, 134d [1:5000; raised according to the method inGrundke-Iqbal et al. (1988)]. Other primary antibodies used weremonoclonal antibody SMI 33 to dephosphorylated neurofilamentsH and M (1:1000; Sternberger Monoclonals, Baltimore, MD); monoclonalantibody DM1A to $alpha$ -tubulin (1:2000; Sigma, St. Louis, MO); polyclonalantibody 972 to dephosphorylated MAP-2A-C (1:10,000; Sánchezet al., 1995); monoclonal and polyclonal antibodies to GFAP, mono-GFAP(1:1000; Boehringer Mannheim, Indianapolis, IN), poly-GFAP (1:2000;Dako, Carpinteria, CA), monoclonal antibodies to nestin, Rat-401(1:1000; PharMingen, San Diego, CA), and rabbit antiserum to nestin#130 (1:1000; Tohyama et al., 1992); and rabbit antiserum R133dto GSK-3 (1:500; Pei et al., 1997). The secondary antibodies usedwere goat anti-mouse IgG (1:100), followed by Clono PAP (1:100),both purchased from Sternberger (Jarrettsville, MD); ¹²⁵I-conjugated anti-mouse and anti-rabbit IgG antibodies (0.1 µg/ml;Amersham, Arlington Heights, IL) for radio immunoblots; OregonGreen 488-labeled goat anti-mouse (1:1000; Molecular Probes, Eugene,OR) and Texas Red-labeled goat anti-rabbit IgG antibodies (1:2000;Molecular Probes) for immunocytochemistry. PD 98059, butyrolactoneI, and LiCl were purchased from Calbiochem (La Jolla, CA), BIOMOL">Biomol(Plymouth Meeting, PA), and Sigma, respectively. Recombinant humantaus, tau₄₁₀ (tau 39, three-repeat tau with two N-terminal inserts),tau₃₈₃ (tau 24, four-repeat tau without N-terminal inserts), andtau₃₅₂ (tau 23, three-repeat tau without N-terminal inserts) wereprepared as previously described (Singh et al., 1995b). Hyperphosphorylatedtau (AD P-tau) was purified from Alzheimer brain as describedpreviously (Köpke et al., 1993).

Isolation of adult hippocampal progenitor cells. Approximately 3-month-old rats were killed by lethal injection of Nembutal(200 mg/kg body weight; Abbott Laboratories, North Chicago, IL);the hippocampus was dissected, and the cells were dissociatedaccording to the slightly modified method of Brewer (1997). Dissectedhippocampus was cut into small (~0.5 mm³) pieces with a razor blade in Hibernate A containing 2% B27 supplementand 0.5 mM glutamine at 4°C (all of which were purchased fromLife Technologies, Grand Island, NY). The tissue pieces were digestedwith 2 mg/ml papain (Worthington, Freehold, NJ) in Hibernate A/B27for 30 min at 30°C with shaking on a reciprocal shaker at 170rpm, washed gently with warm Hibernate A/B27 once, and dissociatedin three 2 ml volumes of Hibernate A/B27 by brief mechanical triturationwith a siliconized Pasteur pipette. To remove debris, we layeredthe resulting 6 ml of cell suspension over a 4 ml step densitygradient (Optiprep, Life Technologies; at 7, 9.4, 11.7, and 16.4%,1 ml each, in Hibernate A/B27) and centrifuged it at 800 × g atroom temperature for 15 min. The top 7 ml of the supernatant thatcontained only debris was discarded, and the remaining 3 ml ofsupernatant, including the dense band of cells and some debrisand the pellet, were collected together and diluted in 5 ml ofHibernate A/B27. After 5 min of centrifugation at 800 × g, thecell pellet was resuspended in Neurobasal A (12.5 mM NaCl plusNeurobasal; Life Technologies) containing 2% B27 supplement and0.5 mM glutamine, and 1 × 10⁶ of cells were plated onto glass slides precoated with 0.01% poly-L-lysine(135 kDa; Sigma). Cultures were incubated at 37°C with 5% CO₂for 1 hr. Then the slides were washed once with warm NeurobasalA/B27 to remove debris and were cultured with Neurobasal A/B27containing 0.5 mM glutamine, 100 IU/ml of penicillin, 100 µg/mlof streptomycin, and 5 ng/ml FGF-2 (Life Technologies). Half ofthe medium was changed to new medium with a double amount of freshFGF-2 every 3-4 d, and the cells were passaged at 70-90% confluencyby incubating them briefly in warm PBS and scraping them witha cell scraper. After the third passage the plates were precoatedwith 1 µg/ml of fibronectin (Life Technologies) in addition to0.01% poly-L-lysine; the FGF-2 concentration in the medium wasincreased to 10 ng/ml. Cultures from the fifth to eleventh passageswere used for thisstudy.

Isolation of fetal hippocampal progenitor cells. Fetal hippocampal progenitor cells were isolated and expanded according tothe slightly modified method of Johe et al. (1996). Briefly, ratfetal hippocampus (gestation day 16; day of conception is day1) was dissected in Hibernate A/B27 and dissociated by brief triturationin the same medium. The cells were collected by centrifugationas above and resuspended in Neurobasal containing 2% B27 supplement,0.5 mM glutamine, 100 IU/ml penicillin, 100 µg/ml streptomycin,and 10 ng/ml FGF-2. Cells (1 × 10⁶) were plated on 10 cm plastic tissue culture plates precoatedwith 0.01% poly-L-lysine and 1 µg/ml fibronectin. The medium waschanged every 3-4 d. Cells were passaged at 50-75% confluenceby incubating them briefly in warm PBS and scraping them witha cellscraper.

Immunocytochemistry. For immunofluorescence double-staining the cells were cultured on Lab-Tek slides (Nunc, Naperville, IL)that had been precoated with 0.01% poly-L-lysine and 1 µg/ml fibronectin.The cells were fixed with 4% paraformaldehyde in PBS for 10 minand permeabilized with 0.5% Triton X-100 in PBS for 5 min; thenthey were blocked in 5% bovine serum albumin in Tris-bufferedsaline (TBS) for 10 min and incubated with primary antibodiesat 37°C overnight, followed by Oregon Green-conjugated anti-mouseantibody and Texas Red-conjugated anti-rabbitantibody.

For dephosphorylation, fixed cells were treated after the blocking step with 256 U/ml alkaline phosphatase (Sigma) at 37°Covernight. After incubation the cells were washed with warm TBS,reblocked with 5% bovine serum albumin in TBS for 5 min, and incubatedwith primary and secondary antibodies asabove.

Preparation of cell samples and rat brain homogenate. Cells were cultured up to ~70-90% confluence in 10-cm-diameter dishes.For harvesting, the culture medium first was changed to cold (4°C)PBS, and the cells were collected immediately with a cell scraperand centrifuged at 800 × g at 4°C for 5 min. In most cases theresulting cell pellets were lysed in 0.4% SDS and 0.4% $beta$ -mercaptoethanol(BME) solution, immediately probe-sonicated, and boiled for 5min. The lysates were aliquoted and stored at $-$ 85°C until use.For detection of tau isoforms and GSK-3 assay, the cells werelysed on ice for 30 min in lysis buffer [50 mM Tris, pH 8.2, fortau isoform analysis and pH 7.4 for GSK-3 assay; 0.1% Triton X-100;20 mM NaCl; 1 mM phenylmethane-sulfonylfluoride (PMSF); and (inµg/ml) 5 leupeptin, 5 aprotinin, 2 pepstatin A, and 50 phosphoramidon],and centrifuged at 200,000 × g for 30 min. The resulting extractswere aliquoted and stored as above. The protein concentrationswere determined by the modified Lowry method of Bensadoun andWeinstein (1976).

For the detection of tau isoforms, cell extracts (15 µg) from adult and fetal progenitor cells and from the cortex of a 3-month-oldrat were mixed with alkaline phosphatase in the proportion of2 µg of sample per 1 U of alkaline phosphatase, adjusted to 156-2000U/ml with lysis buffer, and incubated at 37°C overnight. The incubationwas stopped by adding the appropriate amount of SDS-BME solutionand immediate boiling it for 5min.

Treatment with growth factors. Cells that had been cultured with 10 ng/ml FGF-2 in 10-cm-diameter dishes were used to studythe effects of FGF-2. On the starting day (experimental day 0),the medium was changed to new Neurobasal A/B27 (or Neurobasal/B27for fetal stem cells) containing various concentrations of FGF-2.The medium was changed on experimental days 2, 4, and 6 with thesame medium, and the cells were lysed on experimental day7.

For transformation to astrocytes the cells were cultured with 10 ng/ml FGF-2 on Lab-Tek slides. On experimental day 0 themedium was changed to new Neurobasal A/B27 containing both 10ng/ml ciliary neurotrophic factor (CNTF; Sigma) and FGF-2. Thenext day (day 1) the cells received fresh medium containing either10 ng/ml CNTF alone or CNTF with 20 ng/ml FGF-2. Further mediumchanges were done on experimental days 3, 5, and 7, and the cellswere fixed on experimental day 8 and double-stained as describedabove.

Radio immunoblots. Indicated amounts of protein samples were electrophoresed on at least triplicate SDS-polyacrylamide gels(8 × 6 × 0.75 cm; 6, 10, or 5-10% acrylamide), transferred toImmobilon membranes (Millipore, Bedford, MA), and probed withprimary antibodies. To assay the degree of phosphorylation atthe Tau-1 site, we treated the membranes with or without alkalinephosphatase (196 U/ml) at 37°C for 8 hr in dephosphorylation buffer[containing (in mM) 50 Tris, pH 8.2, 2 MgCl₂, and 1 PMSF plus(in µg/ml) 5 leupeptin, 5 aprotinin, 2 pepstatin A, and 50 phosphoramidon]before the application of Tau-1. Bound antibodies were probedwith ¹²⁵I-conjugated anti-mouse or anti-rabbit IgG. The radio immunoblotswere scanned with a Fuji BAS 1500 Bio Image analyzer (RaytestUSA, Wilmington, DE). Images were processed with the Tina software,and the strength of immunostaining was expressed as pixels persquare length (PSL). Tau levels (micrograms of tau/mg total protein)were determined by comparing the PSLs of known amounts of recombinanttau and of the taus in total cell lysates in the blots treatedwith alkaline phosphatase and stained with Tau-1. Phosphorylationat the Tau-1 epitope (percentage of phosphorylation) was calculatedby the following formula: [PSL of Tau-1 in alkaline phosphatase-treatedblot (total tau) $-$ PSL of Tau-1 in the untreated blot (tau notphosphorylated at the Tau-1 site)]/PSL of Tau-1 in alkaline phosphatase-treatedblot (total tau) ×100.

GSK-3 assay. Activities of GSK-3 were determined as described previously (Pei et al., 1997). Aliquots of 50 µg of cell extractprotein were diluted to 250 µl with lysis buffer and mixed with250 µl of TBS, 300 mM NaCl, and 1 mM PMSF with or without 2 µlof anti-GSK-3 serum R133. After incubation at 4°C for 8 hr, 20µl of immobilized G-protein (Pierce, Rockford, IL) was added tothe mixtures, which were incubated further at 4°C for 2 hr andthen centrifuged. The precipitates were washed three times andsuspended in 50 µl of 50 mM Tris, pH 7.4, containing 10 mM MgCl₂and 1 mM PMSF. Equal amounts (10 µl) of precipitate suspension,800 µM [ $gamma$ -³²P] ATP, 0.4 mg/ml phosphoglycogen synthase peptide 2 (UBI, LakePlacid, NY), and 120 mM Tris, pH 7.4, containing (in mM) 40 MgCl₂,40 NaF, 4 Na₃VO₄, 8 EGTA, and 40 BME were mixed and incubatedat 30°C for 30 min. All assays were performed in triplicate. Reactionswere stopped with 40 µl of 300 mM o-phosphoric acid, and the mixtureswere applied to phosphocellulose units (Pierce). The filters werewashed three times with 75 mM phosphoric acid, dried, and counted.For negative control the precipitates that had been incubatedwithout antibody were used. GSK-3 activity was obtained by subtractingthe counts in the absence of antibody from the counts in the presenceofantibody.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Adult hippocampal progenitor cell cultures express nestin, MAP-2C, and phosphorylated tau

Hippocampal cells were isolated from adult brain and cultured with 5 ng/ml FGF-2 for the first 3 months. In the first fewweeks the cultures were heterogeneous, containing one major typeof cells with small round cell bodies and multiple branched, thinprocesses. A change of FGF-2 from 5 to 10 ng/ml dramatically increasedthe speed of proliferation of thesecells.

After the fifth passage, almost all of the cells immunocytochemically stained intensely with polyclonal antibody 134d fortau, which recognizes tau in a phosphorylation-independent manner(Fig. 1Aa,Ab). In contrast, these cells were stained only poorlywith antibody Tau-1, which recognizes only tau that is not phosphorylatedat the Tau-1 epitope (Fig. 1Ac,Ad). However, when the fixed cellswere dephosphorylated with alkaline phosphatase before the applicationof Tau-1 antibody, the staining pattern changed dramatically (Fig.1Af,Ag) in that almost all of the cells were immunostained intensely.Both Tau-1 and 134d antibodies stained cell bodies and processes,but not the nuclei, suggesting that tau in these cells is mostlycytosolic. Most cells also were stained with antibody 972 to dephosphorylatedMAP-2A-C (data not shown), whereas only a rare cell was stainedwith GFAP antibodies (data not shown). Almost all of the cellsalso were stained with monoclonal (data not shown) and polyclonalantibodies to nestin (Fig. 1Ae,Ah), a marker for immature neuralcells. In some instances the nestin staining increased after dephosphorylation(Fig. 1Ah). Presently, it is not known whether this treatmentnonspecifically increased the antibody accessibility to nestinby unmasking it or whether nestin antibody #130 is somewhat phospho-dependent.

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Figure 1. Proliferating adult hippocampal progenitor cells express not only nestin and MAP-2C but also tau, with the Tau-1 site phosphorylated. A, Expression of tau and nestin in proliferating adult hippocampal progenitor cells. Adult hippocampal progenitor cells (passage 7) were cultured with 10 ng/ml FGF-2 on Lab-Tek slides and stained as described in Materials and Methods. a, Phase contrast; b, anti-tau serum R134d. c-h, Cells were double-stained with Tau-1 and nestin (#133) antibodies without (c-e) and with (f-h) alkaline phosphatase pretreatment; (c, f) phase contrast; (d, g) Tau-1; (e, h) nestin (#133). Note that most adult progenitor cells were tau-positive. After alkaline phosphatase treatment most of the nestin-positive cells also became Tau-1-positive, indicating that tau in adult progenitor cells is phosphorylated at the Tau-1 site. Scale bar, 10 µm. B, Western blot analysis of lysates from adult progenitor cells and rat brain. Lysates (15 µg) from a 3-month-old rat brain tissue (1) and adult hippocampal progenitor cells (2) were applied on 5-10% SDS-polyacrylamide gels. Transferred membranes were pretreated with alkaline phosphatase and analyzed with antibodies Tau-1 (anti-dephosphorylated tau), SMI 33 (anti-dephosphorylated neurofilament H and M), and 972 (anti-dephosphorylated MAP-2A-C). Note that adult progenitor cells express tau and MAP-2C, but not the high-molecular-weight MAP-2 (arrow) and neurofilament H and M (arrowheads).

Western blot analysis of the cell lysates with monoclonal antibody Tau-1 after dephosphorylation of the blot revealed severalimmunopositive bands in the 48-62 kDa area but with slightly differentmobilities from the major tau bands in rat brain (Fig. 1B, Tau-1).In contrast to rat brain homogenate, which also contained thehigh-molecular-weight isoforms of MAP-2 and the H and M neurofilamentsubunits, in the cell lysates only MAP-2C (~70 kDa) and a bandof ~90 kDa, most probably a MAP-2C-derivative variant (Kalchevaet al., 1997), but not MAP-2A and MAP-2B, were detected with antibody972 (Fig. 1B, 972). No neurofilament polypeptides were labeledwith antibody SMI 33 in the cell lysates (Fig. 1B, SMI 33). Thesedata demonstrate clearly that the cells we cultured were morphologicallyand immunocytochemically indistinguishable from adult hippocampalprogenitor cells or the stem cells described previously (Gageet al., 1995; Johe et al., 1996; Palmer et al., 1997); these cellswill be called "progenitor cells"below.

Expression of tau isoforms in adult and fetal hippocampal progenitor cells

To study the isoform composition of tau in adult and fetal progenitor cells, we compared polypeptide patterns of tau in cellextracts by Western blots developed with phospho-independent polyclonalantibody 92e. Cell extracts were incubated in vitro with or withoutalkaline phosphatase before application on the gel (Fig. 2A).Without dephosphorylation, tau in the cell extracts from bothadult and fetal progenitor cells showed several immunoreactivebands ranging from 48 to 62 kDa. However, on in vitro dephosphorylation,tau from adult progenitor cells was resolved into three majordistinct bands. In contrast, tau from fetal progenitor cells showedonly a single band of ~43 kDa, suggesting that adult hippocampalprogenitor cells express adult isoforms of tau, whereas fetalhippocampal progenitor cells express only the fetal tau isoform(Fig. 2A). On Western blots that used 6% gradient gels and Tau-1antibody, tau from the adult progenitor cells was resolved intofive isoforms but in different ratios from those seen in rat brain(Fig. 2B). Tau from adult rat brain was resolved into six bandsof 61, 58, 53, 50, 46, and 43 kDa. In contrast, tau from adultprogenitor cells resolved into four major polypeptides of 53,50, 46, and 43 kDa and a weakly labeled polypeptide of 58 kDa,which was visible only when the ¹²⁵I blot was overexposed. An identical Tau-1-immunoreactive bandpattern was observed even after incubation with several-foldsof alkaline phosphatase (1000-2000 U/ml; data not shown). Thesedata show that undifferentiated proliferating adult hippocampalprogenitor cells do express adult isoforms of tau, but the ratioat which the isoforms are expressed is different from that ofrat cerebrum.

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Figure 2. Adult hippocampal progenitor cells express adult isoforms of tau, and fetal cells express only the fetal tau isoform. A, Tau isoforms expressed by adult and fetal hippocampal progenitor cells. Extracts (15 µg) from adult ( $---$ a $---$ ) and fetal ( $---$ f $---$ ) progenitor cells were incubated in vitro with (+) or without ( $-$ ) alkaline phosphatase and analyzed by Western blots with phospho-independent polyclonal antibody 92e. h $tau$ , Recombinant human tau 39, 24, and 23 (10 ng each). Bars indicate their apparent molecular weights (from top to bottom) of 62, 52, and 48 kDa, respectively. Note that, after treatment with alkaline phosphatase in vitro, tau from fetal cells was resolved into a single band, but tau from adult cells still showed several major bands. B, Comparison of the tau isoform profiles of adult hippocampal progenitor cells and rat brain tissue. Extracts (15 µg) from a 3-month-old rat (1) and adult hippocampal progenitor cells (2) were incubated in vitro with alkaline phosphatase, applied on a 6% gel, and analyzed with the Tau-1 antibody. Bars left and right indicate the apparent molecular weights of tau isoforms (from top to bottom) of 61, 58 (only on left), 53, 50, 46, and 43 kDa, respectively. The 58 kDa tau isoform in the progenitor cells could be observed only if the membrane was overexposed (data not shown).

Regulation of expression and phosphorylation of tau by FGF-2

Adult progenitor cells
To determine the effect of FGF-2 on tau expression, we incubated cells with increasing concentrations of FGF-2, ranging from0 to 40 ng/ml for 7 d, and we determined the levels of tau inthe cell lysates by [¹²⁵I] Western blots as described in Materials and Methods. Usingphospho-independent tau antibody 134d, we found that FGF-2 markedlyincreased, in a concentration-dependent manner, the level of totaltau expression (Fig. 3A,B). This effect also was observed in Tau-1blots treated with alkaline phosphatase. In cultures without FGF-2,the tau level was ~0.45 µg/mg of total protein. This amount increasedwith an increase in FGF-2 concentration and reached ~1.5 µg/mgat 40 ng/ml of FGF-2 concentration (Fig. 3B). Furthermore, inaddition to the FGF-2-dependent increase of total tau, tubulinlevels also increased (Fig. 3C).

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Figure 3. FGF-2 increases the tau and tubulin expressions and the degree of tau phosphorylation at the Tau-1 site in adult hippocampal progenitor cells. A, Western blot analysis of cell lysates from adult hippocampal progenitor cells cultured with increasing concentrations of FGF-2. Adult progenitor cells (passage 8) cultured with 0, 2, 5, 10, 20, and 40 ng/ml of FGF-2 for 7 d were lysed and analyzed with phosphorylation-independent antibody 134d and with phosphorylation-dependent antibodies Tau-1 without (Tau-1) or with (Tau-1 dp) alkaline phosphatase treatment on the membranes, 12E8, PHF-1, and M4. Lane 1, AD P-tau, 3 µg; lane 2, mixture of recombinant human tau 23, 24, and 39, 10 ng each. Lanes 3-8, Cell lysates, 12.5 µg, from the cultures with different concentrations of FGF-2: lane 3, 0 ng/ml; lane 4, 2 ng/ml; lane 5, 5 ng/ml; lane 6, 10 ng/ml; lane 7, 20 ng/ml; lane 8, 40 ng/ml. B, Tau levels increase, depending on the FGF-2 concentrations. Tau levels in adult hippocampal progenitor cells (passage 8) were determined from the radio immunoblots as described in Materials and Methods (n = 3). Absolute tau amounts (micrograms of tau per milligram total protein) were derived by using recombinant human tau as a standard. Similar results also were obtained with adult progenitor cells that had been passaged five times. C, Tubulin levels increase with increased FGF-2 concentration. Cell lysates (6 µg) were analyzed by Western blots with tubulin monoclonal antibody DM1A (inset). The percentage of increase in immunoreactivity was calculated on the basis of the value of FGF-2 at 0 ng/ml (n = 3), which was taken as 0%. D, The phosphorylation of tau at the Tau-1 site increases with increased FGF-2 concentration. The degree of phosphorylation at the Tau-1 site was determined from the Western blots as described in Materials and Methods (n = 3). Note that FGF-2 had a strong effect on the phosphorylation of tau at the Tau-1 site in adult progenitor cells.

As shown in Figure 1 by immunocytochemistry, tau in adult progenitor cells is phosphorylated at the Tau-1 site. This alsowas confirmed by immunoblot analysis (Fig. 3A). Radio immunoblotassays demonstrated that the degree of phosphorylation at theTau-1 site also is regulated strongly by the concentration ofFGF-2 (Fig. 3D). In FGF-2-depleted cultures the phosphorylationat the Tau-1 site was only ~20% but increased to close to 80%at an FGF-2 concentration of 40 ng/ml. A small increase in phosphorylationalso was seen at the 12E8 and PHF-1 sites concurrent with increasedFGF-2 (Fig. 3A). However, this increase in phosphorylation wasnot observed when normalized against total tau (as determinedwith Tau-1 after dephosphorylation), suggesting that the increasedtau is in the form of the protein phosphorylated at the 12E8 andPHF-1 sites. Antibody M4 recognized tau weakly with the immunostaining,even slightly decreasing with increasing tau concentrations. Thusit is indicated that this site is not phosphorylated significantlyin adult hippocampal progenitor cells as a response to FGF-2 (Fig.3A).

Fetal progenitor cells
The effect of FGF-2 on the expression and the phosphorylation of tau also was investigated in progenitor cells from fetalrat hippocampus. During the first three passages the total tauappeared to decrease in the fetal progenitor cells (data not shown),as described previously (Sah et al., 1997). The tau level in thecells from the third passage was ~0.1 µg/mg of total protein,and FGF-2 had no effect on the total tau expression or phosphorylationat the Tau-1 site (Fig. 4A,B). However, in the fifth passage eventau from cells that had been grown for 1 week in FGF-2-depletedmedium was increased fivefold to approximately the same levelas the similarly treated adult progenitor cells (compare Figs.3B, 4B). The addition of FGF-2 to these cultures resulted in anincrease in the tau level, but this increase was only one-halfof that seen in the adult cells, even at 20 ng FGF-2/ml, the maximalpoint of increase. At 40 ng/ml of FGF-2 the tau content decreased.The reason for this negative switch is not understood at present.A possibility is that the inhibition of tau expression beyonda certain maximal point represents a regulatory mechanism by thefetal cells. In contrast to adult cells, 50% of tau already wasphosphorylated at the Tau-1 site in the FGF-2-depleted fetal cells,and the addition of FGF-2 did not have any effect on Tau-1 phosphorylation(Fig. 4C). Thus, the regulation of expression and phosphorylationof tau by FGF-2 between adult and fetal hippocampal progenitorcells was different.

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Figure 4. In fetal hippocampal progenitor cells, FGF-2 increases the expression of tau only in cultures of higher passages but has no effect on the phosphorylation at the Tau-1 site. A, Western blot analysis of cell lysates from fetal hippocampal progenitor cells. Fetal hippocampal progenitor cells, passage 3 (P3) and passage 5 (P5), cultured with increasing concentrations of FGF-2 for 7 d were lysed and analyzed with Tau-1 without (Tau-1) or with (Tau-1 dp) alkaline phosphatase treatment on the membranes. Lane 1, AD P-tau, 3 µg; lane 2, mixture of recombinant human tau 23, 24, and 39, 10 ng each. Lanes 3-7, Cell lysates (12.5 µg) from the cultures with increasing concentrations of FGF-2: lane 3, 0 ng/ml; lane 3', 2 ng/ml; lane 4, 5 ng/ml; lane 5, 10 ng/ml; lane 6, 20 ng/ml; lane 7, 40 ng/ml. Note that fetal progenitor cells in P3 cultures expressed fetal tau very weakly, and FGF-2 had no effect on its expression or phosphorylation. In contrast, the cells in P5 cultures expressed tau abundantly, and FGF-2 increased its expression. B, Tau levels in fetal hippocampal progenitor cells increase with increased concentration of FGF-2 only in later passages. Tau levels were analyzed from the Western blots and expressed by using the same methods as for Figure 3B. Tau levels increased 5- to 10-fold in P5 cultures as compared with P3 cultures. Moreover, FGF-2 altered tau expression only in P5 culture. C, Degree of phosphorylation at the Tau-1 site in fetal hippocampal progenitor cells is independent of the concentration of FGF-2. The degree of phosphorylation in the P5 cultures was determined as described in Materials and Methods. Similar results also were obtained in P3 cultures (data not shown). Note that FGF-2 had no effect on tau phosphorylation at the Tau-1 site.

Even cultures grown for up to 3 months with multiple passages expressed mostly fetal tau, suggesting that factors other thanFGF-2 are required to induce adult isoforms of tau in fetal hippocampalprogenitorcells.

Differentiated astrocytes
To elucidate whether the effect of FGF-2 on tau is limited to undifferentiated progenitor cells or also might extend to cellsdifferentiated into astrocytes, we stimulated progenitor cellswith 10 ng/ml of CNTF with or without the addition of FGF-2 (20ng/ml), as described in Materials and Methods. CNTF converts adultneural progenitor cells to astrocytes (Johe et al., 1996). Afterstimulation for 8 d the cells were double-stained with monoclonalantibody to GFAP and polyclonal tau antibody 134d. In culturesstimulated with only CNTF on alternate days, ~30-40% of the cellswere GFAP-positive. The GFAP-positive cells contained no or onlyvery low tau immunoreactivity (Fig. 5b,c). In cultures that werestimulated simultaneously with CNTF and FGF-2, the same proportionof cells was stained with GFAP. However, most of the GFAP-positiveastrocytes also were strongly tau-positive, at approximately thesame intensity as in undifferentiated progenitor cells (Fig. 5e,f).Immunocytochemistry with Tau-1 antibody with or without alkalinephosphatase treatment showed that, as in the undifferentiatedadult progenitor cells, the Tau-1 site was hyperphosphorylated(data not shown). These findings indicate that FGF-2 affects tauexpression and phosphorylation even in adult differentiated astrocytes.

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Figure 5. Effect of FGF-2 on the expression of tau in differentiated astrocytes. Adult hippocampal progenitor cells cultured with 10 ng/ml CNTF alone (a-c) or, in addition, with 20 ng/ml FGF-2 (d-f) for 8 d as in Materials and Methods were double-stained with mono-GFAP and 134d. a, d, Phase contrast; b, e, mono-GFAP; c, f, 134d. In the cultures stimulated with CNTF alone, differentiated astrocytes were tau-negative (c) or very weakly tau-positive (data not shown). In contrast, in cultures stimulated with both CNTF and FGF-2, most astrocytes expressed tau strongly with the same intensity as undifferentiated progenitor cells. Asterisks show differentiated astrocytes. The tau-positive cells in c and f most probably represent undifferentiated progenitor cells (GFAP-negative). Scale bar, 10 µm.

Mechanism of the phosphorylation of tau by FGF-2 in adult progenitor cells

To date, MAPK, GSK-3, and Cdk-5 are the three major candidate kinases that have been reported to induce tau phosphorylationat the Tau-1 site in vitro (Drewes et al., 1992; Hanger et al.,1992; Vulliet et al., 1992; Singh et al., 1995b). Therefore, toidentify the protein kinase(s) that might be involved in the FGF-2-inducedtau hyperphosphorylation in adult progenitor cells, we examinedthe effect of inhibitors specific to the above kinases. Afterthe indicated periods of incubation with each kinase inhibitorand 10 ng/ml FGF-2, the cells were lysed and analyzed with Tau-1antibody on Western blots that had been treated or untreated withalkaline phosphatase (Fig. 6A). PD 98059, which inhibits the activationof MAPK/MAPK kinase (Alessi et al., 1995), and butyrolactone I,which inhibits the activities of cdks (Hosoi et al., 1995), failedto inhibit the phosphorylation of tau induced by FGF-2 (Fig. 6A).However, lithium, which inhibits GSK-3 activity (Klein and Melton,1996), inhibited the phosphorylation of tau and resulted in amobility shift of tau bands (see Fig. 6A; compare lane 2 withlanes 1, 3, 4). For further confirmation the cells were treatedat different concentrations of LiCl for 6 hr, and the percentageof phosphorylation was determined as described in Materials andMethods (Fig. 6B). The degree of phosphorylation at the Tau-1site was decreased by increasing concentrations of LiCl in a dose-dependentmanner, suggesting that GSK-3 is the kinase involved in the FGF-2signaling pathways.

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Figure 6. Phosphorylation of tau induced by FGF-2 is mediated by GSK-3. A, Effect of kinase inhibitors on the phosphorylation of tau induced by FGF-2. Adult progenitor cells treated with butyrolactone I (30 µg, 6 hr), PD98059 (50 µg, 60 min), or LiCl (30 mM, 3 hr) and 10 ng/ml FGF-2 were lysed and analyzed on Western blots that had been treated with (Tau-1 dp) or without (Tau-1) alkaline phosphatase. Lane 1, Untreated; lane 2, LiCl; lane 3, butyrolactone I; lane 4, PD98059. Note that the phosphorylation at the Tau-1 site induced by FGF-2 was inhibited only by lithium, an inhibitor of GSK-3 (no upward mobility shift in lane 2 in top panel as compared with lanes 1, 3, 4). B, Dose-dependent inhibitory effect of lithium on FGF-2-mediated tau phosphorylation. Adult progenitor cells treated with indicated concentrations of LiCl for 6 hr in 10 ng/ml FGF-2 were lysed, and the percentage of phosphorylation was determined from Western blots as described in Materials and Methods. The data points without LiCl are from Figure 3D. The percentage of phosphorylation was decreased by lithium in a dose-dependent manner. C, FGF-2 increases GSK-3 activity. GSK-3 activities were measured by using extracts from the cells that had been cultured in the indicated concentrations of FGF-2 for 7 d. The GSK-3 activity (%) was calculated on the basis of the value of FGF-2 at 0 ng/ml (n = 3). FGF-2 increases GSK-3 activity in a dose-dependent manner.

To confirm the involvement of GSK-3 in the FGF-2-mediated hyperphosphorylation of tau, we assayed the GSK-3 activity, usingphosphoglycogen synthase peptide 2 as the specific substrate.GSK-3 was immunoprecipitated from the cell extracts, and its kinaseactivity was assayed. As expected, FGF-2 increased GSK-3 activityin a dose-dependent manner (Fig. 6C), again supporting the conceptthat FGF-2 induces tau phosphorylation by activating GSK-3.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The nature of the extracellular signal that regulates the expression and phosphorylation of tau is not understood. The presentstudy shows for the first time that (1) neural proliferating progenitorcells from adult rat brain stably express adult isoforms of tau,(2) that the expression and the phosphorylation at the Tau-1 siteof the adult tau isoforms are regulated by FGF-2, (3) that thekinase responsible for the FGF-2-mediated tau phosphorylationis GSK-3, and (4) that FGF-2 induces expression and phosphorylationof tau in differentiated astrocytes. In contrast, fetal progenitorcells express mostly fetal tau, and FGF-2 regulates only its expression,but not its phosphorylation. The production of adult tau isoformstogether with the ability to differentiate, on stimulation, intoneuronal and/or glial cells indicates the potential of adult progenitorcells as a cell culture model to study adult neurodegenerativediseases that are characterized by an accumulation of hyperphosphorylatedtau.

No tau immunoreactivity has been reported previously in undifferentiated adult progenitor cells. In this study, however, wefound that these cells express abundantly the adult isoforms oftau, with the Tau-1 site highly phosphorylated. This phosphorylationwas the very reason that the presence of tau in these cells hadbeen overlooked previously. Most of the previous studies had usedTau-1 antibody, which recognizes tau only when it is dephosphorylatedat the Tau-1 site. Indeed, the same results were obtained in thepresent study when Tau-1 was used without any previous treatmentwith alkaline phosphatase (see Fig. 1A).

The present study gives rise to several issues. First, tau expression not only is restricted to differentiated neurons butalso occurs in actively dividing progenitor cells and astrocytesderived from them. Second, the expression of adult tau isoformsdoes not necessarily indicate the maturity of a cell. This pointis demonstrated in the progenitor cells from adult hippocampus,which, although immature (nestin-positive), still produce mostof the adult tau isoforms but in different proportions from thosein adult rat brain tissue. On the other side of the spectrum arethe progenitor cells from fetal brain, which do not seem to switchto adult tau. In contrast, in primary cultures of neonatal ratbrain, changes in tau mRNA splicing and production of adult tauisoforms have been observed during 6-12 d in culture (Pizzi etal., 1995). Most likely, fetal progenitor cells are too immaturedevelopmentally and lack the factors to make in vitro the switchfrom fetal to adulttau.

The marked effect of FGF-2 on the expression of tau in progenitor cells from adult rat brain indicates the role of FGF-2 asa regulator of tau. This effect of FGF-2 on tau might be acquiredduring later stages of the development, because the increase intau expression in the progenitor cells from fetal brain couldnot be observed until the fifth passage. The dynamic effect ofFGF-2 on tau expression also may be of importance for postmitoticneurons. FGF-2 has been reported to have an effect on axonal formation(Walicke et al., 1986), especially axonal branching (Miyagawaet al., 1993) and in vivo sprouting in cholinergic neurons (Faganet al., 1997). Tau is one of the major MAPs in mature neuronsand is expressed abundantly in axons (Binder et al., 1985). Therefore,FGF-2 possibly may have an effect on the regulation of axonalformation, generation, and, especially, regeneration after injuryby affecting tau expression and phosphorylation in adultbrain.

It has been shown previously that progenitor cells differentiate into astrocytes by stimulation with CNTF, both in the presenceor absence of FGF-2 (Johe et al., 1996). We studied the effectof FGF-2 on tau in astrocytes derived from CNTF-treated adultprogenitor cells. As shown in Figure 5, tau is present in culturedastrocytes when they are treated with FGF-2. The tau proteinsin these differentiated astrocytes also are regulated by FGF-2as well as those in undifferentiated progenitor cells, suggestingthat the effect of FGF-2 on the expression of adult tau may bemore general in adult CNS. Although the mechanisms are still unclear,in some pathological conditions, including progressive supranuclearpalsy, corticobasal degeneration, Pick's disease, dementia pugilistica,and Alzheimer Disease, abnormally phosphorylated tau-positiveastrocytes or astrocytic processes have been reported to appearin the affected areas of the brain (for review, see Chin and Goldman,1996), sometimes in parallel with overexpression of FGF-2 (Stopaet al., 1990).

In the present study we found that FGF-2 upregulates the phosphorylation of tau at the Tau-1 site in progenitor cells fromadult hippocampus. This increase in tau phosphorylation is attributablemainly to the increased levels of phosphorylated tau (Fig. 3A,compare Tau-1 with Tau-1 dp). Interestingly, this pattern of increasein phosphorylated tau is similar to that in AD brain (see Khatoonet al., 1992). Furthermore, the present study shows that the increasein tau phosphorylation at this site corresponded to an increasein the activity of GSK-3 but neither MAPK nor cdks, suggestingthat GSK-3 activity might be regulated by the FGF-2 signalingpathway. Unlike adult progenitor cells, these cells from fetalbrain did not reveal any increase in tau phosphorylation in responseto FGF-2 treatment, suggesting that the FGF-2 signaling pathwaythat regulates the GSK-3 activity is probably not developed inthe fetalcells.

GSK-3 is believed to be a key kinase in AD involved in the hyperphosphorylation of tau, because it can induce Alzheimer-likephosphorylation in COS cells transfected with tau (Lovestone etal., 1994). In vitro Alzheimer-type phosphorylation of tau isinduced by GSK-3 only in the presence of heparin or when tau isprephosphorylated with certain nonproline-dependent kinases (Morenoet al., 1995; Singh et al., 1995a,b; Sengupta et al., 1998). Thatnot all characteristic AD tau epitopes are hyperphosphorylatedin the progenitor cells with the conditions used in the presentstudy may be attributable to differences in the kinase/phosphataseratios or exogenous factors such as neurotrophins or lymphokines.However, in AD, with its decreased protein phosphatase activity(Gong et al., 1993, 1995), FGF-2 might be one of the factors thatplay an important role in the increased tau levels (Khatoon etal., 1992) and the formation and accumulation of highly phosphorylatedtau in brain (Grundke-Iqbal et al., 1986a; Iqbal et al., 1989;Lee et al., 1991; Köpke et al., 1993). Indeed, in AD brain theFGF-2 level is elevated when compared with age-matched controlbrain (Stopa et al., 1990), and strong FGF-2 immunoreactivityhas been observed in tau lesions such as neurofibrillary tanglesand dystrophic and degenerating neurites of neuritic plaques (Cummingset al., 1993). Moreover, brain injury, one of the major risk factorsof AD and probably the cause of dementia pugilistica, also isknown to increase the expression of FGF-2 (Finklestein et al.,1988; Frautschy et al., 1991; Logan et al., 1992). Furthermore,continuous upregulation of FGF-2 in brain might be critical becauseit can induce not only an initial accumulation of hyperphosphorylatedtau but also continuous activation of GSK-3. Increased GSK-3 activityhas been reported to induce cholinergic dysfunction in primarycultured neurons (Hoshi et al., 1996) and apoptosis in PC12 cells(Pap and Cooper, 1998), both reported to occur in AD neuropathology.GSK-3 also is involved in the regulation of diverse transcriptionfactors, which also might be affected by increased GSK-3activity.

In conclusion, FGF-2 upregulates the expression and phosphorylation of tau in progenitor cells and differentiated astrocytesfrom adult, but not fetal, rat hippocampus. The hyperphosphorylationof tau produced by FGF-2 in these cells occurs via upregulationof GSK-3 activity but neither MAPK nor cdks activities. Thesefindings identify a new role of FGF-2 both in normal neurobiologyand in neurodegenerative diseases characterized by the accumulationof hyperphosphorylatedtau.

  FOOTNOTES

Received Nov. 11, 1998; revised March 23, 1999; accepted April 13, 1999.

These studies were supported in part by funds from the New York State Office of Mental Retardation and Developmental Disabilitiesand National Institutes of Health Grants NS18105, AG05892, andAG08076. We thank Tanweer Zaidi and Qiongli Wu of our laboratoryfor the preparation of AD P-tau and recombinant human tau isoforms.We gratefully acknowledge Dr. Ronald D.G. McKay (National Instituteof Neurological Disorders and Stroke, Bethesda, MD) for a giftof polyclonal antibody to nestin #133, Dr. Lester I. Binder (Universityof Alabama, Birmingham, AL) for a generous supply of monoclonalantibody Tau-1, Dr. Peter Davies (Albert Einstein College of Medicine,Bronx, NY) for PHF-1, Dr. Jesus Avila (Universidad Autónoma deMadrid, Madrid, Spain) for antibody 972, Dr. Yasuo Ihara (Universityof Tokyo, Tokyo, Japan) for M4 antibody, and Dr. Dale Schenk (AthenaNeurosciences, San Francisco, CA) for 12E8 antibody. We also thankthe Biomedical Photography Unit for the preparation of the figures,Ms. Maureen Marlow for editorial assistance, and Ms. Janet Biegelsonand Ms. Sonia Warren for secretarialassistance.
Correspondence should be addressed to Dr. Inge Grundke-Iqbal, New York State Institute for Basic Research in DevelopmentalDisabilities, 1050 Forest Hill Road, Staten Island, NY10314.

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