Protein Kinase MARK/PAR-1 Is Required for Neurite Outgrowth and Establishment of Neuronal Polarity

doi:10.1091/mbc.02-03-0046

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Originally published as MBC in Press, 10.1091/mbc.02-03-0046 on September 24, 2002

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Vol. 13, Issue 11, 4013-4028, November 2002

Protein Kinase MARK/PAR-1 Is Required for Neurite Outgrowth and Establishment of Neuronal Polarity

Jacek Biernat,^* Yong-Zhong Wu,^* Thomas Timm, Qingyi Zheng-Fischhöfer, Eckhard Mandelkow, Laurent Meijer, and Eva-Maria Mandelkow^§

Max-Planck-Unit for Structural Molecular Biology, Hamburg, Germany; and Centre National de la Recherche Scientifique, Station Biologique, F-29682 Roscoff, France

Submitted March 26, 2002; Revised July 25, 2002; Accepted August 21, 2002
Monitoring Editor: Richard J. McIntosh

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Protein kinases of the microtubule affinity-regulating kinase (MARK) family were originally discovered because of their abilityto phosphorylate certain sites in tau protein (KXGS motifs inthe repeat domain). This type of phosphorylation is enhanced inabnormal tau from Alzheimer brain tissue and causes the detachmentof tau from microtubules. MARK-related kinases (PAR-1 and KIN1)occur in various organisms and are involved in establishing andmaintaining cell polarity. Herein, we report the ability of MARK2to affect the differentiation and outgrowth of cell processesfrom neuroblastoma and other cell models. MARK2 phosphorylatestau protein at the KXGS motifs; this results in the detachmentof tau from microtubules and their destabilization. The formationof neurites in N2a cells is blocked if MARK2 is inactivated, eitherby transfecting a dominant negative mutant, or by MARK2 inhibitorssuch as hymenialdisine. Alternatively, neurites are blocked ifthe target KXGS motifs on tau are rendered nonphosphorylatableby point mutations. The results suggest that MARK2 contributesto the plasticity of microtubules needed for neuronal polarityand the growth ofneurites.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The establishment of neuronal polarity and the generation of cell processes require the interplay between signaling mechanisms(from extracellular cues to the cytoplasm and to the nucleus),which enable the cell to decide when and where to grow a neurite,and mechanochemical elements (cytoskeleton, motors, and membranes)that allow the neurite to push outward. The actin network in thecell cortex tends to resist gross shape changes, and consequentlyactin-disassembly drugs facilitate neurite outgrowth (Edson etal., 1993; Knowles et al., 1994; Bradke and Dotti, 1999), whereasmicrotubules provide the core for a growing cell process, andtherefore microtubule-disassembly poisons prevent the outgrowth(Baas and Ahmad, 1993; Rochlin et al., 1996). In addition microtubulesmust be dynamically unstable to allow growth cone formation, andtherefore both microtubule-stabilizing and -destabilizing drugscan inhibit neurite outgrowth (Liao et al., 1995; Tanaka et al.,1995; Jordan and Wilson, 1998; Kaverina et al., 1998; Waterman-Storerand Salmon, 1999; Goode et al., 2000; Kabir et al., 2001). Inthis study, we focus on the neuronal microtubule-associated proteintau, its role in neurite outgrowth, and its regulation by phosphorylation.Tau is a mixture of six splicing isoforms (Figure 1; Lee et al.,1988; Goedert et al., 1989) that become largely axonal duringdevelopment (Binder et al., 1985; Hirokawa et al., 1996). Theaccepted role of tau is that of a microtubule stabilizer (Clevelandet al., 1977; Drubin and Kirschner, 1986; Butner and Kirschner,1991; Gustke et al., 1994; Panda et al., 1999), although otherroles such as a regulator of axonal traffic (Ebneth et al., 1998;Stamer et al., 2002), anchor for kinases and phosphatases (Leeet al., 1998; Liao et al., 1998; Sontag et al., 1999), or membranelinker (Brandt et al., 1995) have recently emerged. Tau stronglypromotes neurite outgrowth during differentiation (Caceres andKosik, 1990; Esmaeli-Azad et al., 1994; Leger et al., 1994; Hirokawaet al., 1996), and even in nonneuronal cells tau induces cellprocesses with a cytoskeletal organization reminiscent of neurites(Kanai et al., 1989; Knops et al., 1991; Barlow et al., 1994;Biernat and Mandelkow, 1999). The interaction between tau andmicrotubules is regulated by phosphorylation. This aspect hasbeen studied intensely because hyperphosphorylation of tau, detachmentfrom microtubules, and abnormal aggregation are hallmarks of Alzheimer'sdisease (reviewed in Delacourte and Buee, 2000). One would thereforeexpect that phosphorylation of tau at sites that cause its detachmentfrom microtubules would counteract neurite formation. However,other observations complicate this view of tau's role. One isthat the concentration of tau along an axon seems to be greatestnear the tip where the microtubules are few and of lower stabilityin spite of the presence of tau (Black et al., 1996). This poolof tau is also thought to be in a state of low phosphorylationthat would be expected to favor association with microtubules(Mandell and Banker, 1996). Thus, there is no simple correlationbetween the concentration of tau, its phosphorylation, and thelocal stability of microtubules. Other counterintuitive resultscome from nonneuronal cell models such as Sf9 cells transfectedwith tau, which induces them to develop neurite-like cell processes(Baas et al., 1991; Knops et al., 1991). In this case, the typeof phosphorylation that most potently detaches tau from microtubulesin vitro (at KXGS motifs in the repeat domain) is necessary forcell process outgrowth, rather than inhibitory (Biernat and Mandelkow,1999).

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Figure 1. Bar diagram of human tau, phosphorylation sites, and antibody epitopes. (a) N-terminal half is the "projection domain" because it projects from the microtubule surface but does not bind itself. The C-terminal half is the "assembly domain" because it binds to microtubules and promotes their assembly. The binding is mediated by the three to four pseudorepeats (~31 residues each) and the flanking domains (shaded). Compared with the longest isoform in the CNS (htau40, 441 residues), the fetal isoform htau23 (352 residues) lacks the second repeat (exon 10) and two inserts near the N terminus (58 residues). The SP or TP motifs (outside the repeat domain, 14 in htau23, 17 in htau40) are marked; in the AP-htau23 mutants the S or T residues are replaced by A so that they cannot be phosphorylated by proline-directed kinases. The KXGS motifs (one per repeat) are the targets of MARK; in the KXGA-htau23 mutant the S residues are replaced by A, making them nonposphorylatable. (b) Antibody epitopes in htau40 sensitive to phosphorylation are indicated. The main targets of cdk5 or cdc2 on htau40 are the double motifs T231/S235 (epitope of antibody AT-180), S202/T205 (antibody AT-8), and S404 (only weak reaction with PHF-1); the main targets of GSK-3 $beta$ are S396/S404 (strong reaction with antibody PHF-1), and S202/T205 (AT-8 epitope) (Illenberger et al., 1998

); the main target of MARK is S262 (epitope of antibody 12E8).

These observations require a critical evaluation of the kinases of tau and their role in neurite outgrowth. Tau contains manyphosphorylation sites targeted by several kinases. One can broadlydistinguish two classes of sites: 1) Tau contains many Ser-Proor Thr-Pro motifs phosphorylated by proline-directed kinases suchas GSK-3 $beta$ , cdc2, cdk5, or mitogen-activated protein (MAP) kinase.These sites account for the major fraction of tau phosphorylation(Figure 1; Illenberger et al., 1998; Biernat and Mandelkow, 1999)and have received attention because they are prominent in taufrom Alzheimer brain (Morishima-Kawashima et al., 1995). 2) Othersites can be phosphorylated by nonproline-directed kinases suchas protein kinase A (PKA), protein kinase C, calcium/calmodulin-dependentprotein kinase II, or microtubule affinity-regulating kinase (MARK).Some sites have pronounced effects on tau's binding to microtubules,notably, the KXGS motifs in the repeats that can be phosphorylatedby MARK (Biernat et al., 1993; Drewes et al., 1997). Similar KXGSmotifs occur in other MAPs (MAP2 and MAP4), suggesting a generalizedmechanism of regulation (Illenberger et al., 1996; Ozer and Halpain,2000). There is a family of MARK kinases in mammals with homologyto kinases in other organisms (par-1, kin1+; reviewed in Dreweset al., 1998; Nelson and Grindstaff, 1997; Kemphues, 2000), membersof the SNF1/AMPK subfamily of kinases (Hanks and Hunter, 1995).They are important for the establishment of cell polarity in differentcontexts, e.g., asymmetric distribution of P-granules in the Caenorhabditiselegans zygote (par-1; Guo and Kemphues, 1995), polar growth ofSchizosaccharomyces pombe (kin1+; Levin and Bishop, 1990), axisformation in the Drosophila embryo (Shulman et al., 2000; Tomancaket al., 2000), or the polar structure of epithelial cell layers(Böhm et al., 1997). Kinases of the MARK/PAR-1 family seem tobe elevated in fetal tissue (Lopez and Sheetz, 1995; Drewes etal., 1997; Jenkins and Johnson, 1997; Brown et al., 1999). Wetherefore studied whether MARK plays a role in neurite developmentand whether it operates through its target tau. The results shownherein suggest that this is indeed thecase.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Cells and Viruses

N2a neuroblastoma cells were grown in minimal essential medium Earle's medium supplemented with 10% fetal calf serum, 2 mMglutamine (Biochrom, Berlin, Germany), and 0.1% nonessential aminoacids (Sigma Chemie, Deisenhofen, Germany), at 37°C and 5% CO₂in a humidified chamber. Cells were seeded onto coverslips ata density 2 × 10⁴ cells/cm² in 24-well culture dishes, transfected with 1 µg of plasmid DNAby Effectene (QIAGEN, Hilden, Germany) or N-[1-(2,3-dioleoyloxy)propyl]-N,N,N-trimethylammoniummethylsulfate (Roche Applied Science, Mannheim, Germany) accordingto the manufacturer's protocol. N2a cells were differentiatedand transfected (before or afterward) with plasmids encoding tau,MARK2, or their mutants. Differentiation of N2a cells was inducedby serum deprivation and 1 µM retinoic acid (Sigma Chemie) for24 h. The N2a/htau40 cell line stably transfected with htau40was described previously (Ebneth et al., 1998). Sf9 cells wereobtained from Invitrogen (San Diego, CA) and were grown at 27°Cin monolayer culture Grace's medium (Invitrogen, Carlsbad, CA)supplemented with 10% fetal bovine serum, 50 µg/ml gentamicin,and 2.5 µg/ml amphotericin. BaculoGold was obtained from BD PharMingen(San Diego, CA) and pVL1392 was from Invitrogen. Concentrationsof tau were determined by an enzyme-linked immunosorbent assaydescribed previously (Ackmann et al., 2000).

Plasmids and Recombinant Baculoviruses Containing Mutated Tau Genes

The cDNAs of tau and tau mutants were inserted into a derivative of pRc/CMV vector (Invitrogen, Leek, The Netherlands) byusing NdeI and BamHI restriction sites to yield vectors for tau(htau23) or tau mutants AP (all SP or TP motifs changed to AP)or KXGA (all KXGS motifs changed to KXGA). The same procedurewas used for the kinase MARK2 or its inactive mutant MARK2/T208A/S212A(numbering as in Drewes et al., 1997). The construction of recombinantbaculoviruses containing mutated tau genes was described previously(Biernat and Mandelkow, 1999)

Quantitation of Tau-induced Process Formation in Sf9 Cells

The frequency of cell processes was determined in monolayer culture. Cells (3 × 10⁶) were plated on 60-mm Petri dishes, infected with recombinantbaculoviruses at a multiplicity of infection (MOI) of 1-5, andincubated at 27°C. The morphological analysis was performed onunfixed cells because the cells have the tendency to detach andprocesses are lost during the fixation procedure. Process morphologywas quantitated in three independent experiments, scoring 200cells each. To determine the effects of the kinase inhibitorshymenialdisine (HD), flavopiridol (FL), H89, or LiCl on cell processes,Sf9 cells were allowed to express tau for 48 h (at this time arobust growth of processes is observed in transfected cells),and then treated with 50 µM HD or FL inhibitors or 50 mM LiCl,or 10 µM H89, for 3 h and scoredsubsequently.

Quantitation of Neurite Outgrowth in N2a Cells Transfected with tau23 Constructs

N2a cells were allowed to differentiate for 24 h by treatment with retinoic acid in the presence of 0.1% fetal calf serumand subsequently transfected with plasmids encoding tau constructs.Twenty-four hours after transfection the coverslips were fixedwith methanol and incubated with the rabbit polyclonal pan-tauantibody K9JA (Dako Diagnostika, Hamburg, Germany) and the mousemonoclonal anti-tubulin antibody DM1A (Sigma Chemie). Tau-containingcells were scored for cell processes only when they reached alength of more than two cell diameters (>40 µm; three independentexperiments, 100 cellseach).

Quantitation of Neurite Outgrowth in N2a Cells Treated with Kinase Inhibitors

Control N2a/htau40 cells were differentiated by serum deprivation and treatment with 1 µM retinoic acid, fixed with 4% paraformaldehyde,and stained for immunofluorescence with tau antibody K9JA. N2a/htau40cells differentiated for 12 h by serum deprivation and treatmentwith retinoic acid were incubated for 2-5 h in the presence of50 µM FL, an inhibitor of cdk5 and GSK-3 $beta$ (Leclerc et al., 2001)or of 50 µM HD, also an inhibitor of GSK-3 $beta$ and cdk5 (Meijer etal., 2000), fixed, and stained for immunofluorescence with tauantibody K9JA. Cells with extended neurites were counted and scoredas the percentage of totalcells.

Transfection of N2a Cells with MARK2, Mutant MARK2, and Cotransfection with tau23-KXGA

N2a cells were transiently transfected with plasmids encoding MARK2 or dominant negative mutant of MARK2. Twenty-four hoursafter transfection the coverslips were fixed with methanol andincubated with monoclonal antibody 12CA5 (staining for MARK2)and with the mouse monoclonal anti-tubulin antibody DM1A. MARK2-or dnMARK2-containing cells were counted for extended neuritesand scored as the percentage of total transfected cells. In cotransfectionexperiments, the N2a cells were cotransfected transiently withplasmids encoding green fluorescent protein (GFP)-MARK2 and KXGA/htau23and after 16 h differentiated for 24 h, fixed with 4% paraformaldehydfor 5 min and incubated with the rabbit polyclonal pan-tau antibodyK9JA and the mouse monoclonal anti-tubulin antibody (DM1A). Doubletransfected cells with extended neurites were counted and scoredas the percentage of total transfectedcells.

Western Blot Analysis

Sf9 cells were infected with recombinant virus at an MOI of 1-5. Cell lysates were prepared in hypotonic lysis buffer (50mM Tris-HCl pH 7.4, 120 mM NaCl, 10% glycerol, 1% Nonidet-P40,5 mM dithiothreitol, 1 mM EGTA, 20 mM NaF, 1 mM orthovanadate,5 µM microcystin, 100 µg/ml each of protease inhibitors leupeptin,aprotinin, and pepstatin). The lysed cells were centrifuged at16,000 × g for 15 min, and the supernatant and pellet were separated.The supernatant was adjusted to 500 mM NaCl, boiled for 10 min,and centrifuged at 16,000 × g for 15 min. Then 1- to 3-µg aliquotsof proteins in the supernatant were electrophoresed by SDS-PAGE,transferred to a polyvinylidene difluoride membrane, and blottedwith the following monoclonal antibodies: 12E8 (1:5000; a giftof P. Seubert, Elan Pharma, South San Francisco, CA), AT-8 (stock1 mg/ml, diluted 1:2000), AT-180 (1 mg/ml, 1:2000), AT-100 (1mg/ml, 1:500 (Innogenetics, SA, Ghent, Belgium), PHF-1 (1:600;a gift of P. Davies, Albert Einstein College, Bronx, NY), polyclonalrabbit anti-tau antibody K9JA (1:2000, Dako Diagnostika), andpolyclonal rabbit antibody SA6941, raised against the regulatoryloop peptide of MARK2 phosphorylated at T208 and S212. The antibodywas affinity purified. The immunostaining was visualized usingenhanced chemiluminescence (Amersham Biosciences, Braunschweig,Germany).

Immunofluorescence

Cells were washed in MTSB buffer (80 mM HEPES, pH 6.9, 1 mM MgCl₂, 1 mM EGTA, 4% polyethylene glycol) and subsequently fixedwith methanol at $-$ 20°C for 5 min, washed with phosphate-bufferedsaline, and treated with 5% bovine serum albumin in phosphate-bufferedsaline and 0.1% Triton X-100 for 1 h. Fixed cells were incubatedwith rabbit polyclonal pan-tau antibody K9JA (1:500; Dako Diagnostika),rat monoclonal anti-tubulin antibody YL1/2 (1:200; Serotec, Oxford,United Kingdom), mouse monoclonal anti-hemagglutinin (HA) tagantibody 12CA5 (1:200; Roche Applied Science) or rhodamine-labeledphalloidin (Molecular Probes, Eugene, OR). Fluorescently labeled(fluorescein isothiocyanate and tetramethylrhodamine B isothiocyanate)secondary antibodies were obtained from Dianova (Hamburg, Germany).Samples were examined using an LSM510 confocal microscope or anAxioplan fluorescence microscope equipped with a cooled charge-coupleddevice camera (Zeiss, Jena,Germany).

Kinase Preparations and Assays

Recombinant MARK2 was expressed in Escherichia coli (BL21, DE3 pLys) with a C-terminal His-tag. Cells were lysed in bufferA (50 mM Tris-HCl, pH 7.5, 200 mM NaCl, 50 mM imidazole, 5 mM3-[(3-cholamidopropyl)dimethylammonio]propanesulfonate, 2 mM benzamidine,1 mM $beta$ -mercaptoethanol, 1 mM phenylmethylsulfonyl fluoride [PMSF])with a French press. The supernatant was loaded onto a Ni²⁺-NTA column (QIAGEN). After washing with 10 column volumes ofbuffer A the protein was eluted with a short gradient (5 columnvolumes) to buffer B (as buffer A, but 500 mM imidazole). Fractionsthat contained MARK2 were pooled and dialyzed against buffer C(50 mM Tris-HCl pH 7.5, 200 mM NaCl, 2 mM benzamidine, 1 mM $beta$ -mercaptoethanol,1 mM PMSF, 50% glycerol) and stored at $-$ 20°C. The purity of theobtained kinase was higher than 95%. Kinase activities were assayedin 50 mM Tris-HCl, pH 7.5, 5 mM MgCl₂, 2 mM EGTA, 0.5 mM PMSF,0.5 mM dithiothreitol, 0.5 mM benzamidine for 30 min at 30°C.The final concentration of [³²P]ATP (7.4 × 10⁵ MBq/mmol) and substrate peptides was 15 µM. As substrates weused the synthetic tau-repeat1-peptide ₂₅₅NVKSKIGSTENLK₂₇₆ (Dreweset al. 1997) for recombinant MARK2 and the pCreb-peptide (prephosophorylatedby PKA) for GSK3 $beta$ (Upstate Biotechnology, Lake Placid, NY). Reactionswere stopped by addition of one-half the reaction volume of 30%(wt/vol) trichloroacetic acid. After centrifugation, the supernatantwas applied to phosphocellulose-paper discs, five times washedwith 0.1 M phosphoric acid, dried by air, and counted in a scintillationcounter. Blank values were subtracted and activities expressedin percentage of the maximal activity, i.e., without inhibitors.IC₅₀ values were estimated from the dose-response curves. Brainextract kinase activity for phosphorylating and activating MARK2was prepared as described previously (Biernat et al., 1993).

In Vivo Labeling of Tau Derivatives in Sf9 Cells and Phosphopeptide Mapping

Metabolic labeling of Sf9 cells with ³²P was performed using 0.5 mCi of ³²Pi/ml TNM FH cell medium lacking phosphate and supplemented withdialyzed fetal calf serum. Sf9 cells were infected with recombinantbaculovirus at an MOI of 10. At 36 h postinfection cells weresupplemented with 0.5 mCi of ³²P_i per milliliter of medium and incubated for 3 h. After labelingcells were washed, resuspended in lysis/boiling buffer, and immediatelyboiled. After centrifugation the supernatant was subjected forSDS-PAGE and radioactive tau bands were eluted and precipitatedby trichloroacetic acid. The radioactive Tau derivatives werefurther used for peptide mapping. Two-dimensional (2D) phosphopeptidemapping (on thin layer cellulose plates) was performed accordingto Boyle et al. (1991) and Illenberger et al. (1998). Note thatthe absolute degree of tau phosphorylation in Sf9 cells cannotbe obtained from the radioactive labeling experiments becausethe efficiency of conversion of ³²P to [ $gamma$ -³²P]ATP in the cells is not known; however, it can be estimatedfrom the molecular weight shifts and the known specificities ofthe phosphorylation-sensitiveantibodies.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Neurite Outgrowth in N2a Cells Requires Phosphorylation at KXGS Motifs in the Repeat Domain of Tau

One aim of our studies was to determine the role of tau protein, its phosphorylation, and its protein kinases on the elaborationof neurites. To achieve this one needs an experimental systemthat allows both cell biological and biochemical observations.We focused on the mouse neuroblastoma cell line N2a because itcan be readily differentiated with retinoic acid after serum deprivationto form neurite-like cell processes (Figure 2). Differentiationof neuronal cells requires endogenous tau (Drubin and Kirschner1986; Caceres and Kosik, 1990; Esmaeli-Azad et al., 1994); inN2a cells tau is only present at low concentrations, below thedetectability by immunofluorescence. We transfected human fetaltau isoform htau23 (352 residues) transiently into wild-type N2acells that induces them to develop long neurites after a differentiationstimulus. In the example of Figure 2a, ~60% of transfected cellshave processes longer than twice the cell body diameter. As acontrol, among cells not expressing exogenous htau23 only 20%develop extended processes (Figure 2, a, b, and f).

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Figure 2. Neurite outgrowth by N2a cells and dependence on tau phosphorylation. N2a cells were differentiated by serum withdrawal and retinoic acid and then transiently transfected with tau or tau mutants, and scored for the development of extended neurites longer than two cell body diameters (>40 µm). (a and c) Tau staining (antibody K9JA). (b and d) Tubulin staining (DM1A). (a and b) Cells transfected transiently with htau23 (50% efficiency). Among the cells not expressing exogenous tau, only 20% develop extended neurites (control; Figure 2e). In contrast, among the cells expressing exogenous htau23 the fraction with extended neurites rises to 60% (Figure 2, a and b, arrows, and f). (c and d) Cells transfected with the KXGA mutant of htau23: Among the cells expressing exogenous tau mutant (three cells highlighted by arrows in 2, c and d) only few develop neurites longer than two cell body diameters (compare other untransfected cells in d). This shows that the phosphorylation at KXGS motifs is important for neurite outgrowth. (e) Differentiated control N2a cells (no transfection with tau). (f) Histogram of neurite formation with different tau constructs: Only 20% of control cells show extended neurites, but 60% of cells transfected with htau23. Cells transfected with the KXGA mutant of htau23 are comparable with controls (20%, no phosphorylation by MARK2 possible). Cells transfected with the AP mutant are comparable with transfection by htau23 (60%, no phosphorylation by proline-directed kinases). The data show that transfection with htau23 and the AP mutant are similarly efficient in promoting neurite outgrowth, whereas transfection with the KXGA mutant has no effect. Error bars show SE.

Tau contains many Ser or Thr residues that can be phosphorylated by several kinases. To probe whether the outgrowth of neuritesdepends on the phosphorylation of tau we generated several tauconstructs in which certain Ser or Thr residues were mutated intoAla, thus making them inaccessible to phosphorylation. Among thephosphorylation sites one can distinguish different classes: 1)The S-P or T-P motifs (14 in isoform htau23, mostly in the domainsflanking the repeats; Figure 1) can be phosphorylated by proline-directedkinases such as GSK-3 $beta$ and cdk5. They are thought to play a rolein neurodegeneration (Imahori and Uchida, 1997; Mandelkow andMandelkow, 1998), they induce the epitopes of several antibodiescharacteristic of Alzheimer tau (e.g., AT-8, AT-100, AT-180, andPHF-1), but have only a modest influence on tau-microtubule interactions(Biernat et al., 1993). 2) The KXGS motifs (one per repeat, threein htau23, four in htau40; Figure 1) are targets of nonproline-directedkinases, primarily MARK (and less efficiently PKA; Biernat etal., 1993; Drewes et al., 1997), which has a pronounced effecton detaching tau from microtubules (particularly Ser262 in thefirst repeat) and render them dynamic in vitro and in vivo (Ebnethet al., 1999). We therefore made modified constructs of htau23,one with all 14 S-P or T-P motifs mutated into A-P (AP-tau), andone with the KXGS motifs mutated into KXGA (nonphosphorylatableKXGA-tau) (Figure 1). When AP-tau was transfected into N2a cells,the effect was similar to that of wild-type tau, i.e., a stronginduction of neurites, with about one-half of the transfectedcells displaying extended processes (Figure 2f). Because proline-directedkinases are active in the cells (see below), this result meansthat the phosphorylation at SP or TP motifs is of lesser importancefor neuriteoutgrowth.

In contrast, when repeating the experiment with KXGA-tau the outgrowth of extended neurites after a differentiation stimuluswas nearly abolished. As a control, the effect was limited tothe cells that actually express the tau mutant (Figure 2c, cellswith arrows), whereas the others obtain normal processes afterdifferentiation (Figure 2d, cells without arrows). Thus, the KXGAmutations in the repeats essentially abrogate tau's ability toinduce neurites (Figure 2f). We note that the KXGA mutant hasthe same ability to bind and polymerize microtubules as wild-typeunphosphorylated tau, in contrast to tau phosphorylated at KXGSmotifs (Biernat et al., 1993; our unpublished data). These resultssuggest that N2a cells contain active kinase(s) that phosphorylatethe KXGS motifs and that the phosphorylation at these motifs isimportant for neuriteoutgrowth.

Neurite Outgrowth Is Promoted by Activity of MARK2

Given that the KXGS motifs of tau are important for neurite outgrowth, the next question was to identify the responsible kinase(s).We had shown previously that the kinase that phosphorylates theKXGS motifs in tau and related MAPs most efficiently is MARK (Dreweset al., 1995; Illenberger et al., 1996). We therefore approachedthe identification of the kinase by asking how MARK influencesneurite outgrowth and the phosphorylation of tau in N2a cells.Surprisingly, transient transfection of MARK2 into N2a cells causeddifferentiation without further stimuli (such as serum withdrawaland retinoic acid; Figure 3a, b, and e), although the transfectionrate was low (1-2%). In contrast, the majority of N2a cells expressingthe dominant negative mutant of MARK2 (Figure 3, c, d, and e)were not able to form extended neurites, even after a differentiationstimulus. As shown previously (Drewes et al., 1997), this mutantwas rendered inactive in vitro and in cells by replacing phosphorylatableresidues in the regulatory loop by alanines (T208A and S212A).Wild-type N2a cells contain endogenous tau only at the low levelof 24 ng/10⁷ cell (using an enzyme-linked immunosorbent assay developed byAckmann et al., 2000). We therefore generated N2a cells stablyexpressing htau40, the largest tau isoform in the CNS, at a ~40-foldhigher level (~1 µg/10⁷ cells), to analyze the phosphorylation state of tau biochemically.These cells were transiently transfected with dnMARK2. Cells expressingthe inactive mutant of MARK2 could not form neurites (Figure 4,a-d, arrows), whereas cells not expressing dnMARK2 were able todifferentiate (Figure 4, a-d, asterisks). This argues that MARK2or a closely related isoform might be important for neurite outgrowthand for the phosphorylation of the KXGS motifs in tau. To verifythat MARK2 operates via tau phosphorylation, N2a cells were cotransfectedwith GFP-MARK2 and KGXA-htau23 (Figure 4, e-h). In the cases wherethe cells express the KXGA mutant of tau, or both MARK2 and theKXGA mutant, formation of extended neurites is strongly reduced.In other words, the neurite-promoting effects of tau can be obliteratedeither by mutating the KXGS target motif on tau (KXGA-tau; Figures2c and 4, e-g), or by inactivating the kinase MARK2 (Figure 3,c-e).

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Figure 3. Transfection of N2a cells with MARK2 promotes neurite formation, and dominant negative MARK2 inhibits it. N2a cells were transiently transfected with MARK2 (a and b) or a dominant negative mutant of MARK2 (c and d). (a and c) Staining for MARK2 (antibody 12CA5). (b and d) Staining for tubulin (antibody DM1A). (a and b) Although cells containing only the low levels of endogenous tau show no neurites in serum before differentiation (see rounded-up cells in b, asterisks) and would require differentiation conditions to develop processes (serum withdrawal, retinoic acid, etc), transfection with MARK2 overcomes this barrier and allows 60% of MARK2 transfected cells even without serum withdrawal and retinoic acid to differentiate and extend neurites (see cell at center in a and b, arrow and see histogram e). (c and d) When N2a cells are transfected with dnMARK2, only a small fraction of the cells expressing dnMARK2 (6%) form extended neurites after differentiation (Figure 3e).

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Figure 4. Inhibition of neurite outgrowth by inactive MARK2 (dnMARK2) or nonphosphorylatable Tau (KXGA). N2a cells stably transfected with htau40 can be differentiated by serum withdrawal and retinoic acid (see b and c, asterisks). However, dnMARK2 prevents neurite formation (see a, arrows). (d) Histogram showing that dnMARK2 suppresses neurites (ca. 90% of transfected cells fail to develop neurites). (a-c) Expression of a dominant negative mutant (dnMARK2) in N2a/htau40 cells. (a) Staining for dnMARK2 (antibody 12CA5). (b) Staining for tau (K9JA). (c) Staining for tubulin (DM1A). (e-g) N2a cells cotransfected transiently with GFP-MARK2 and KXGA/htau23 and then differentiated. The doubly transfected cells (arrows) show no neurites, whereas the untransfected cell has extended neurites. (h) Histogram showing the fraction of N2a with extended neurites after transfection: control N2a cells, cells transfected with htau23, MARK2, htau23-KXGA mutant, double transfection with htau23-KXGA and MARK2. The data illustrate that htau23 and MARK2 promote neurite outgrowth, htau23-KXGA abolishes this activation, and even MARK2 is not able to rescue the inhibitory effect of the KXGA-tau mutant on neurite formation after differentiation, because the phosphorylation of tau at its KXGS motifs is blocked.

To show that MARK2 indeed phosphorylates the KXGS motifs of tau in living cells we transiently transfected GFP-MARK2 (or itsdominant negative mutant) into N2a cells stably transfected withtau. Differentiated cells were analyzed by GFP fluorescence (showingMARK2; Figure 5a), immunofluorescence with the antibody p-MARKagainst active MARK2 (Figure 5b), and phospho-KXGS motifs in tau(antibody 12E8; Seubert et al., 1995; Figure 5c). The three patternswere similar, suggesting that active MARK2 localizes in the samecompartments as tau throughout the cell and would therefore beable to phosphorylate it. In contrast, transfection with dnMARK2showed no differentiation, no staining for active MARK2, and nophospho-KXGS tau (our unpublished data). To corroborate thesefindings the proteins were isolated from the N2a cells, and phosphorylationsites were determined by phospho-sensitive antibodies of knownspecificities in Western blots (Figure 5, d and e). The pan-tauantibody K9JA detects tau regardless of phosphorylation and servesas a standard for the protein concentration. Antibody 12E8 detectsthe phosphorylated KXGS motifs in the tau-repeats 1 and 4 (containingS262 and S356). Its signal is enhanced when MARK2 is transfected(Figure 5d, lane 2) but weak with no transfection or after transfectionwith dnMARK2 (Figure 5d, lanes 1 and 3). The weak reaction inlane 1 presumably reflects the residual activity of the endogenousMARK isoforms. As a control, the expression of MARK2 (active orinactive) is revealed by the antibody against the HA-tag (Figure5, d and e). Finally, the state of activation of MARK2 is shownby the rabbit polyclonal peptide antibody p-MARK (SA6941) raisedagainst a peptide of the phosphorylated activating loop of MARK2(with phosphorylated T208 and S212). This antibody was affinitypurified and characterized in detail; Figure 5g shows that recombinantMARK2 can be phosphorylated and activated 10-fold by a kinaseactivity in brain extract (Drewes et al., 1997). This phosphorylationof MARK causes a shift in the SDS gel and the reaction with p-MARKantibody (Figure 5f). The p-MARK antibody shows a pronounced signalin the blot after transfection of the cells with active MARK2,but only a weak signal without MARK2 transfection or with dnMARK2(Figure 5d, lanes 1-3). The data argue that the elaboration ofneurites is achieved by MARK2 phosphorylating the KXGS motifson tau. The effect can be demonstrated even more clearly whenthe experiment is repeated, but cells are incubated with the phosphataseinhibitor okadaic acid (0.2 µM, 30 min) before harvesting. Inthis case the phosphorylation at the KXGS motifs seen by antibody12E8 (against p-Tau) in blots is particularly pronounced aftertransfection with MARK2 (Figure 5e, lane 2), but not with dnMARK2(Figure 5e, lane 3), indicating that other kinases do not phosphorylatethe KXGS motifs in the presence of okadaic acid.

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Figure 5. Phosphorylation of tau induced by MARK2. (a-c) N2a/htau40 cells transiently transfected with GFP-MARK2, differentiated, fixed after 24 h, and analyzed by fluorescence microscopy. (a) Distribution of GFP-MARK2. (b) Immunofluorescence of p-MARK antibody against active MARK2 (phosphorylated T-loop). (c) Antibody 12E8 against phospho-KXGS motifs of tau. Note that active MARK2 and phosphorylated tau at KXGS sites colocalize (see below). (d and e) N2a/htau40 cells were transiently transfected with MARK2 or a dominant negative mutant (dnMARK2), differentiated for 6 h, and analyzed by preparing a cell lysate and probing by Western blotting with a panel of antibodies against phosphorylated MARK2 and tau. The data show that MARK2 causes the phosphorylation of the KXGS motifs of tau and dnMARK2 inhibits this. (d) Lane 1, control N2a/htau40 cell extract. Lane 2, transfection with MARK2. Lane 3, transfection with dominant negative MARK2 (T208A and S212A). Antibody K9JA ("Tau") stains tau independently of phosphorylation. The three samples contain the same amount of tau. Antibody 12E8 against the phosphorylated KXGS motifs in tau repeats 1 and 4 (phospho-S262 and -S356, "p-Tau") shows stronger staining in the case of MARK2 transfection (lane 2), but only weak staining without MARK2 transfection (lane 1), and no staining with dnMARK2 (lane 3). The antibody against hemagglutinin-tag ("MARK") reveals the expression of exogenous MARK2 or dnMARK2 (lanes 2 and 3) but is absent from untransfected cells (lane 1). The antibody SA6941 against phosphorylated T-loop peptide on MARK2 (pT208, pS212, corresponding to activated MARK2) shows pronounced staining after transfection of exogenous MARK2 (lane 2) but only weak staining in controls (lane 1), corresponding to the activity of endogenous MARK-like kinases, and no staining in the presence of dnMARK. (e) N2a/htau40 cells were transiently transfected with MARK2 or a dominant negative mutant, dnMARK2, differentiated for 6 h, and before harvesting treated for 30 min with 0.2 µM okadaic acid. Note that only the sample expressing the transfected wt MARK2, but not dnMARK2, has clearly increased phosphorylation at KXGS motifs shown by reaction with antibody 12E8 ("p-Tau", lane 2). This means that MARK2 but not other endogenous kinases such as PKA are responsible for tau phosphorylation at KXGS motifs in these conditions. (f and g) Western blot analysis demonstrating the specificity of the p-MARK antibody (polyclonal antibody SA6941) against the posphorylation sites T208 and S212 in the activating loop of kinase MARK2. Top, MARK2 protein before (lane 1) and after (lane 2) phosphorylation by brain extract kinase activity (see MATERIALS AND METHODS). Bottom, antibody p-MARK (SA6941) recognizes exclusively the phosphorylated MARK2 (lane 2) whose increased activity is demonstrated in the histogram (g). (h-j) N2a/htau40 cells transiently transfected with HA-tagged MARK2, fixed 24 h after differentiation and analyzed by confocal fluorescence microscopy. (h) Distribution of MARK2 by using fluorescent HA antibody. (i) Fluorescence of phalloidin-labeled actin. (j) Merge of h and i. Note that MARK2 and actin largely colocalize.

As seen in Figure 5, a-c, the differentiated N2a cells showed numerous filopodia and microspikes emanating from the cell bodyand the neurites, suggesting that active MARK2 and phospho-taumight colocalize with the actin network. We therefore transfectedMARK2 transiently into N2a-htau40 cells and checked the distributionof MARK2 and actin by immunofluorescence. Figure 5, h-j, showsby confocal microscopy that the pattern of MARK2 coincides largelywith that of actin. We hypothesize that tau phosphorylated atKXGS motifs detaches from microtubules and partly translocatesto the actin network during neurite outgrowth, consistent withrecent observations with MAP2 phosphorylated at KXGS motifs (Ozerand Halpain, 2000).

MARK Is Potently Inhibited by Hymenialdisine

Tau contains multiple phosphorylation sites that could affect its function in different ways. The majority (95%) of tau'sendogenous phosphorylation in cells occurs on SP or TP motifsin the regions flanking the repeats (Illenberger et al., 1998;Biernat and Mandelkow, 1999). These sites are phosphorylated byproline-directed kinases such as cdk5 and GSK-3 $beta$ , which are knownto play a role in differentiating neurons. To analyze the roleof these kinases in process outgrowth we used two novel potentinhibitors of both cdk5 and GSK-3 $beta$ , FL and HD (Meijer et al.,2000; Leclerc et al., 2001), and applied them to N2a cells stablytransfected with htau40. Figure 6a shows that control cells developextended neurites (~25%) in differentiation medium. When the cellswere exposed to 50 µM FL, neurite outgrowth was similar or somewhatenhanced (Figure 6, b and d), consistent with our previous observationthat phosphorylation of tau at SP or TP motifs was neutral orsomewhat inhibitory (Biernat and Mandelkow, 1999). In contrast,when N2a/htau40 cells were treated with the kinase inhibitor HD(50 µM), neurite outgrowth was strongly inhibited (~3%; Figure6, c and d). How can this apparent discrepancy between the twokinase inhibitors be explained? To answer this question the affectedphosphorylation sites on tau had to be determined in more detail.This cannot be achieved with N2a or N2a/htau40 cells because theirlevel of tau is too low for biochemical analysis. We thereforeturned to the Sf9 cell system that generates sufficient quantitiesof protein for the biochemical analysis of transfected tau. Thejustification is the observation that the interplay between tauand tau kinases during process formation is qualitatively similarbetween neuronal and nonneuronal cells (Biernat and Mandelkow,1999).

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Figure 6. Effect of kinase inhibitors FL and HD on tau-induced neurite outgrowth in N2a cells stably transfected with htau40. (a) Control N2a/htau40 cells were differentiated and stained for immunofluorescence with tau antibody K9JA; ~25% of cells develop extended cell processes. (b) N2a/htau40 cells differentiated and treated with 50 µM FL, a strong inhibitor of cdk5 and GSK-3 $beta$ (Leclerc et al., 2001

). Neurite outgrowth is somewhat enhanced (~35%). (c) N2a/htau40 cells differentiated and treated with 50 µM HD, also a strong inhibitor of cdk5 and GSK-3 $beta$ (Meijer et al., 2000

). Neurite outgrowth is strongly inhibited (~3%). (d) Histogram illustrating the fraction of N2a/htau40 cells bearing extended neurites after differentiation and treatment with kinase inhibitors HD and FL. HD strongly reduces the extent of neurite formation, and FL causes a slight increase.

Figure 7 illustrates untreated Sf9 cells (diameter around 20 µm, no cell processes; Figure 7a) and cells transfected withhtau23 (Figure 7b). After 30 h of transfection, ~25% of thesecells were enlarged and developed a single cell process of uniformdiameter. Next, we exposed the cells to the drug FL (50 µM). Thisresulted in a pronounced threefold increase in cells with processes(~75%; Figure 7, c and e), arguing that proline-directed phosphorylationof tau by cdk5 and GSK-3 $beta$ is inhibitory for cell processes. However,when the cells were exposed to HD, process formation was stronglyreduced (~10%; Figure 7, d and e). The results showed that bothN2a cells and tau-transfected Sf9 cells had a similar responseto the kinase inhibitors FL and HD.

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Figure 7. Effect of kinase inhibitors FL and HD on tau-induced process outgrowth in Sf9 cells. (a) Untreated Sf9 cells (control), showing round shapes) and no cell processes. (b) Sf9 cells transfected with htau23 by baculovirus vector; ~30% grow extended cell processes up to 100 µm. They also have larger cell bodies (2- to 3-fold). (c) Sf9 cells transfected with htau23 and treated with the kinase inhibitor FL (50 µM). The number of cells with processes increases strongly (~3-fold). (d) Sf9 cells transfected with htau23 and treated with the kinase inhibitor HD (50 µM). The number of cells with processes drops to ~10%. (e) Histogram displaying the efficiency of process formation by Sf9 cells in the presence of kinase inhibitors. HD inhibits them strongly, LiCl and H89 promote modestly, and FL promotes strongly.

The phosphorylation sites on tau were determined using site-specific antibodies on Western blots, and by 2D phosphopeptidemapping (Figure 8). As shown previously (Illenberger et al., 1998;Godemann et al., 1999), major targets of GSK-3 $beta$ on tau are S404,followed by S396 (which together make up the epitope of PHF-1),and to a lesser extent S202 and T205 (antibody AT-8). The majortargets of cdk5 are S235 followed by T231 (epitope of antibodyAT-180), S202/T205 (AT-8 epitope), whereas the reaction with PHF-1is very weak because S404 is a major site but not S396. The Sf9cells contain very active kinases so that all phosphorylation-dependentantibody reactions are observed on the transfected tau (Biernatand Mandelkow, 1999). Figure 8a (lane 1) illustrates this forthe antibodies 12E8 (pS262 and pS356), AT-100 (pT212 and pS214),AT-180 (pT231 and pS235), AT-8 (pS202 and pT205), and PHF-1 (pS396and pS404). When the inhibitor FL is added to the cells (Figure8a, lane 3), the reactions of tau in Western blots with antibodiesAT-100, AT-180, AT-8, and PHF-1 are strongly suppressed. The sameis true for the inhibitor HD (Figure 8a, lane 2). However, therewas an unexpected difference with regard to antibody 12E8, diagnosticfor the KXGS motifs containing phospho-S262/S356. FL allows phosphorylationat these sites, and HD inhibits it, as seen in the Western blot(Figure 8a, lanes 2 and 3). Because neither GSK-3 $beta$ nor cdk5 phosphorylateS262 or S356 (Godemann et al., 1999), the result suggests thatHD is also an inhibitor of MARK2, the kinase phosphorylating thesesites most efficiently. This was tested directly by kinase activityassays performed with recombinant MARK2 and GSK-3 $beta$ in vitro (Figure9). In the case of GSK-3 $beta$ , we found comparably strong inhibitionby HD (IC₅₀ = 0.13 µM) and FL (IC₅₀ = 0.55 µM; Figure 9). In thecase of MARK2, only HD is a strong inhibitor (IC₅₀ = 0.67 µM).

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Figure 8. Effect of kinase inhibitors on phosphorylation of htau23 in Sf9 cells. (a and b) Antibody blots. (c and f) 2D phosphopeptide maps. (a) Lane 1, no inhibitor (control). Lane 2, 50 µM HD. Lane 3, 50 µM FL. From top to bottom: Coomassie-stained gel (control) showing roughly equal amounts of tau; Western blot with antibody K9JA that recognizes tau independently of phosphorylation; antibody 12E8 (against phosphorylated KXGS motifs). The inhibitor HD prevents phosphorylation (lane 2) because it inhibits MARK and related kinases, and not because of its inhibition of GSK-3 $beta$ (see below). LiCl and PKA inhibitors have no pronounced effect (Figure 8b, lanes 1 and 2). Antibody AT-100 (against phospho-T212 and S214). This epitope requires the activity of GSK-3 $beta$ (to phosphorylate T212), and PKA (to phosphorylate S214; Zheng-Fischhofer et al., 1998

). Therefore, the epitope is blocked by both HD and FL (lanes 2 and 3). Antibody AT-180 (against phospho-T231 and S235). This is an epitope induced by cdk5 and GSK-3 $beta$ , and thus the signal is blocked by both HD and FL (lanes 2 and 3). Antibody AT-8 (against phospho-S202 and T205). This is an epitope induced mainly by cdk5, and therefore the signal is blocked by both HD and FL (lanes 2 and 3). Antibody PHF-1 (against phospho-S396 and S404). This epitope is phophorylated mainly by GSK-3 $beta$ , and therefore the signal is inhibited by HD, but less by FL. (b) Lane 1, 50 mM LiCl. Lane 2, 50 µM H89, a PKA inhibitor. (c-f) Two-dimensional phosphopeptide maps of htau23 protein expressed in Sf9 cells and phosphorylated by endogenous kinases without (c), or in the presence of kinase inhibitors (d-f). (c) Control, tau expressed in Sf9 cells. (d) Inhibition by 50 µM HD to inhibit cdk5, GSK-3 $beta$ , and MARK. (e) Inhibition by 50 mM LiCl to inhibit GSK-3 $beta$ . (f) Inhibition by 50 µM FL to inhibit cdk5 and GSK3 $beta$ ; note that c, e, and f show spots for phosphorylated S262 (circle, also see insert in e at higher exposure), d does not because HD inhibits MARK activity.

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Figure 9. In vitro inhibition assay of kinases of tau by inhibitors HD and FL. (a) MARK2. (b) GSK3 $beta$ . Note that GSK-3 $beta$ is inhibited by HD (IC₅₀ = 0.13 µM) and FL (IC₅₀ = 0.55 µM), but MARK2 is inhibited mainly by HD (IC₅₀ = 0.67 µM), whereas FL is only a weak inhibitor (IC₅₀ = 38 µM).

Additional control experiments on Sf9 cells were done with LiCl, a specific inhibitor of GSK-3 $beta$ (Stambolic et al., 1996),and H89, an inhibitor of PKA (Chijiwa et al., 1990). These experimentswere prompted by our previous observations that PKA can phosphorylatethe KXGS motifs of tau in vitro, albeit with low efficiency (Schneideret al., 1999), and by conflicting reports that GSK-3 $beta$ could alsophosphorylate KXGS motifs (Moreno et al., 1995; Godemann et al.,1999). We tested these two kinases with their inhibitors (LiClfor GSK-3 $beta$ , H89 for PKA) and found that the reaction with theantibody 12E8 against pSer262 was not affected (Figure 8b, lanes1 and 2, compare with control in Figure 8a, lane 1); in contrast,50 µM HD suppressed the reaction with antibody 12E8 (Figure 8a,lane 2). This was confirmed by phosphopeptide mapping of tau inSf9 cells after treatment with 50 mM LiCl to inhibit GSK-3 $beta$ (seebelow, Figure 8e, circled spot). Furthermore, the quantificationof tau-induced cell processes of Sf9 cells after treatment withinhibitors LiCl or H89 showed a slight increase, rather than thepronounced decrease observed with the MARK inhibitor HD (Figure7e). This suggests that GSK-3 $beta$ and PKA are not responsible forthe phosphorylation of KXGS motifs in tau during cell processformation.

Finally, we performed metabolic labeling of Sf9 cells with ³²P and analyzed the phosphorylation state of tau by phosphopeptidemapping (Figure 8, c-f). The reference map of tryptic phosphopeptidesof tau expressed in Sf9 cells is shown in Figure 8c; the identificationof the spots is described in detail elsewhere (Illenberger etal., 1998; Biernat and Mandelkow, 1999). The spots of pS262 andpS356 are rather weak compared with those of the SP or TP motifs.Nevertheless, the spot of pS262 is clearly visible in the mapsobtained with LiCl or FL (Figure 8, e and f, circles, see inset),but not with HD (Figure 8d, circle). This confirms that HD isalso an inhibitor of MARK2, and that GSK-3 $beta$ or cdk5 are not responsiblefor the phosphorylation of tau at S262 in Sf9cells.

The results with kinase inhibitors explain the antibody reactions (disappearance of 12E8 staining in the presence of inhibitorHD), but more importantly they explain the response of the cellsto inhibitor treatment. As noted above, phosphorylation at KXGSmotifs is essential for process formation. Because this is achievedby MARK2, the inhibitor HD (but not FL) suppresses the cell processes(Figure 7, d and e) because it is also an inhibitor of MARK2 andnot because it is also an inhibitor of GSK-3 $beta$ andcdk5.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

In this study, we asked how the function of tau, a protein known to initiate axonal outgrowth, is regulated by phosphorylation,and what kinases are responsible for it. We argue that the phosphorylationof tau at its KXGS motifs by the kinase MARK is critical in neuronsand nonneuronal cell models (N2a and Sf9 cells). Because thesecell types contain little or no endogenous tau, cell processescan be strongly enhanced by transfection with exogenous tau. Theevidence for the importance of MARK is based on experiments wherewe changed either the activity of the regulator kinase MARK orthe sites on its effector protein tau. The function of tau waschanged by point mutations at the target sites of MARK by replacingthe KXGS motifs with nonphosphorylatable KXGA motifs. KXGA-tauwas not able to stimulate neurite outgrowth in N2a cells. Theactivity of MARK was changed in three ways: 1) transient transfectionof cells with MARK2, one of the MARK isoforms, which can be activatedby phosphorylation at the activating loop (Drewes et al., 1997);2) transfection with a dominant negative MARK lacking the regulatoryphosphorylation sites (T208A and S212A); and 3) inactivation ofMARK by hymenialdisine, a new kinase inhibitor (Meijer et al.,2000). When MARK was inactivated, no stimulation of neurite outgrowthoccurred.

Because tau contains many phosphorylation sites, an obvious issue is to distinguish their effects on the functions of tau.This is a common problem in the field because tau's phosphorylationin cells is often detected by antibodies that may vary in affinityand specificity. Many of the "Alzheimer-diagnostic" antibodiesare directed against phospho-SP or -TP motifs, suggesting theactivity of proline-directed kinases (e.g., MAP kinase, GSK-3 $beta$ ,or cdk5). In our case, we can rule out a major role of these kinasesfor tau-induced neurite outgrowth because the AP-tau mutant (whereall SP or TP motifs were turned into AP) shows a similar or greaterstimulation of neurites than normal tau, contrary to the KXGA-mutantof tau. This agrees with previous observations on Sf9 cells (Biernatand Mandelkow, 1999). Other, non-KXGS or non-SP/TP phosphorylationsites are also of minor importance because they represent a minorfraction of cellular phosphorylation sites (Watanabe et al., 1993,Illenberger et al., 1998), and they are not phosphorylated byMARK so that they cannot explain the effects of MARK inhibition(Drewes et al., 1995). A special issue is the possible phosphorylationof KXGS motifs by two other kinases, GSK-3 $beta$ or PKA. In one studyGKS-3 $beta$ was thought to phosphorylate tau at S262 (Moreno et al.,1995), but our subsequent analysis showed that this was due toother activities in the kinase preparation (Godemann et al., 1999).This is confirmed herein by the LiCl experiment that inhibitsthe GKS-3 $beta$ targets on tau (SP or TP motifs; Figure 8b, lane 1,PHF1 staining) without affecting the KXGS sites (Figure 8b, lane1, staining with 12E8, and Figure 8e, spot of phospho-S262 ininset). PKA remains another possibility; it indeed phosphorylatestau at several sites, including the KXGS motifs (albeit much lessefficiently than MARK; Drewes et al., 1995; Schneider et al.,1999). However, inhibition of PKA by H89 did not inhibit processformation (Figure 7e), contrary to inhibition of MARK by HD anddid not inhibit the phosphorylation of KXGS motifs (Figure 8b,lane 2, staining with 12E8). We also showed in an in vitro activityassay (Figure 9) that hymenialdisine is able to inhibit MARK,but not PKA. Furthermore, the treatment of N2a/htau40 cells withokadaic acid led to the increase in phosphorylation at KXGS motifsonly after transfecting the cells with MARK2 (but not with dnMARK2),nor in cells without transfected MARK2 (Figure 5e, lanes 1-3).This suggests that no other kinase phosphorylates the KXGS-motifsof tau in differentiating N2a cells even under the conditionsof okadaic acid, pointing to MARK2 as the responsible kinase.Finally, in living cells GFP-MARK2 (but not dnMARK2) colocalizeswith MARK2 activity (as shown by the p-MARK antibody) and phospho-KXGStau (Figure 5, a-c). Collectively, the biochemical and immunofluorescenceevidence suggests that MARK2 or a kinase of the MARK family isthe kinase phosphorylating tau at KXGS motifs in differentiatingN2acells.

Microtubule stability is considered to be necessary for neurites because they provide mechanical strength and tracks for theintracellular transport. The phosphorylation of the KXGS motifsof tau during neurite outgrowth tends to detach tau from microtubulesand thus renders microtubules less stable. This is the oppositeof what one would expect intuitively, and therefore the questionarises why this should be important for neurite outgrowth. Theanswer may lie in a more subtle role of microtubules: As the growthcone advances, actin filaments prepare the ground in the formof transient lamellipodia and filopodia. This ground is probedby pioneering microtubules that make temporary excursions intothe actin meshwork and retract again, until finally a decisionis made to stabilize them, form bundles, and allow the growthcone to advance (reviewed in Borisy and Svitkina, 2000; Bradkeand Dotti, 2000; Goode et al., 2000). Thus, microtubules mustbe dynamically instable before neurites can extend. This explainswhy the suppression of dynamic instability suffices to block thegrowth of neurites, even when the polymer mass is not changed(Baas and Ahmad, 1993; Liao et al., 1995; Tanaka et al., 1995;Rochlin et al., 1996; Kaverina et al., 1998). The cell seems touse tau or related MAPs for this regulation (Drubin and Kirschner,1986; Panda et al., 1999). Tau is present in the growth cone,but it is largely detached from microtubules (Black et al., 1996).Why should this pool of tau not stabilize microtubules so thatthey can advance out of the shaft of the neurite? We suggest thattau is locally phosphorylated at the KXGS motifs, is thereforeunable to bind to microtubules (thus rendering them unstable),and relocates to the actin network (Figure 5c; Ozer and Halpain,2000, for the analogous case of MAP2). Only a small fraction ofmicrotubules are highly dynamic (Waterman-Storer and Salmon, 1997;Kabir et al., 2001); this explains why the overall extent of KXGS-phosphorylationis low in normal cells, in spite of its crucial role (Biernatand Mandelkow, 1999).

It is interesting to compare our results with two other studies on the phosphorylation of tau in neurons. Mandell and Banker(1996) argued that tau phosphorylation was lowest at the distalend of the neurite where microtubules are most dynamic. This seemedpuzzling because unphosphorylated tau is often considered tantamountto stable microtubules. The finding can be explained by notingthat the authors had used the antibody AT-8, which senses twophosphorylated SP and TP motifs outside the repeat domain (S202and T205), but does not recognize the phosphorylation at KXGSmotifs. We have shown elsewhere that the phosphorylation at theSP or TP motifs sites has only a modest effect on the tau-microtubulebinding (Biernat et al., 1993), and indeed all proline-directedsites combined have no major influence on neurite outgrowth (Figure2f), in contrast to the KXGS motifs. Overall, the role of proline-directedphosphorylation of tau is poorly understood and may be importantin other contexts, for example, protection against degradation(Litersky and Johnson, 1995), cell division (Ookata et al., 1997;Illenberger et al., 1998), and compartmentalization in neurons(Binder et al., 1985; Hirokawa et al., 1996).

In a related study, Ozer and Halpain (2000) investigated the phosphorylation of MAP2 in HeLa cells. This MAP is similar totau and the endogenous HeLa MAP4 by having homologous repeats,including KXGS motifs, and is sorted into the somatodendriticcompartment of neurons (in contrast to axonal tau). The authorsfound that the KXGS motifs of MAP2 could be phosphorylated byPKA, resulting in the dissociation of MAP2 from microtubules andtranslocation to the actin network. This would be consistent withthe fact that PKA binds to MAP2 through its regulatory RII subunit(Obar et al., 1989), which is not the case for tau. The commondenominator for their results and ours would be that the cellneeds to control the dynamics of microtubules by phosphorylatingthe locally available MAPs at their KXGS motifs. This could betau in axons, MAP2 in dendrites, and presumably MAP4 in othercell types. The phosphorylation could be achieved by differentkinases (e.g., MARK or PKA), with the same result of detachingthe MAPs from the microtubules. Alternatively, it is possiblethat there is a more complex mechanism involving activating kinasesand/or phosphatases. In our experimental system we found no evidencefor a major role of PKA in initiating neurite outgrowth, consistentwith a role of kinases of the MARK/PAR-1 family in establishingcell polarity (Drewes et al., 1998; Kemphues, 2000, Shulman etal., 2000; Tomancak et al., 2000).

Neurons contain several MAPs with different distributions and partially overlapping functions. For example, tau and MAP1bcan substitute for one another during axonal growth in differentextracellular environments (DiTella et al., 1996). A transgenicmouse lacking only tau is viable, but a mouse model lacking bothtau and MAP1b shows severe defects in axonogenesis (Harada etal., 1994; Takei et al., 2000). The complementarity extends evento molecular properties: Phosphorylation of tau at certain sitesdetaches tau from microtubules and makes them more dynamic, whereascertain phosphorylations of MAP1b promote the binding to microtubules,and in both cases there is a gradient along axons, with the loweraffinity species near the growth cone (Ulloa et al., 1994). Down-regulationof GSK-3 $beta$ by the WNT signaling pathway or inhibition by lithiuminduces the dephosphorylation of MAP1b, its detachment from microtubules,and hence axonal remodeling such as increased growth cone sizeand branching (Lucas et al., 1998). Because hymenialdisine isan inhibitor not only of MARK but also of GSK-3 $beta$ (Meijer et al.,2000), one could argue that its effect on neurite outgrowth mightbe mediated by GSK-3 $beta$ and possibly MAP1b. This can however beruled out because two other inhibitors of GSK-3 $beta$ , lithium andflavopiridol, do not reproduce the effects of HD. Furthermore,the effects of MARK inhibition mediated by tau (i.e., inhibitionof neurite outgrowth) are opposite from the effects of GSK-3 $beta$ inhibition mediated by MAP1b (growth cone remodeling). In otherwords, the inhibition of MARK reduces microtubule dynamics, whereasthe inhibition of GSK-3 $beta$ enhancesdynamics.

Finally, we note that there is growing evidence for an interplay between microtubule and actin dynamics mediated by phosphorylationof accessory components during neurite outgrowth. Several kinaseshave been described that are docked on one or both of these fibersystems and promote their organization, e.g., c-Abl, PAK5, orprotein kinase C (Kabir et al., 2001; Dan et al., 2002; Woodringet al., 2002), and MARK would be another case in point. Usually,this takes place in tight coordination with small G proteins ofthe rho family (Daub et al., 2001; Palazzo et al., 2001). Thephosphorylation of MAPs could regulate different subaspects ofmicrotubule behavior in the growth cone, such as microtubule bundlingin the shaft, dynamic instability of the pioneer microtubules,activation of tubulin scavengers such as stathmin, and anchoringat focal contacts. Furthermore, MAPs can interact with componentsother than microtubules; such as the actin cytoskeleton (Griffithand Pollard, 1982; DiTella et al., 1994; Cunningham et al., 1997;Ozer and Halpain, 2000). This may explain why different kinaseshave overlapping effects on growth cone behavior, presumably inresponse to different external signals whose nature remains tobeelucidated.

	ACKNOWLEDGMENTS

We thank Kerstin Neumann and Natalie Habbe for excellent technical assistance, Guangxun Meng for help with transfection experiments,Peter Davies (Albert Einstein College) for antibody PHF-1, PeterSeubert (Elan Pharma) for antibody 12E8, and George Pettit (Universityof Arizona) for the kinase inhibitor hymenialdisine. This workwas supported by the DeutscheForschungsgemeinschaft.

	FOOTNOTES

^* These authors contributed equally to thiswork.

^§ Corresponding author. E-mail address: mand{at}mpasmb.desy.de.

Article published online ahead of print. Mol. Biol. Cell 10.1091/mbc.02-03-0046. Article and publication date are at www.molbiolcell.org/cgi/doi/10.1091/mbc.02-03-0046.

ABBREVIATIONS

Abbreviations used: Cdk5, cdc2-like protein kinase-5; HD, hymenialdisine; FL, flavopiridol; MAPK, mitogen-activated protein kinase; MARK, microtubule affinity-regulating kinase; MOI, multiplicity of infection; PKA, protein kinase A.

	REFERENCES

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Ackmann, M., Wiech, H., and Mandelkow, E. (2000). Non-saturable binding indicates clustering of tau on the microtubule surface in a paired helical filament-like conformation. J. Biol. Chem. 275, 30335-30343[Abstract/Free Full Text].
Baas, P., and Ahmad, F. (1993). The transport properties of axonal microtubules establish their polarity orientation. J. Cell Biol. 111, 495-509[Abstract/Free Full Text].
Baas, P.W., Pienkowski, T.P., and Kosik, K.S. (1991). Processes induced by tau expression in Sf9-cells have an axon-like microtubule organization. J. Cell Biol. 115, 1333-1344[Abstract/Free Full Text].
Barlow, S., Gonzalez-Garay, M.L., West, R., Olmsted, J.B., and Cabral, F. (1994). Stable expression of heterologous microtubule-associated proteins (MAPs) in Chinese hamster ovary cells: evidence for differing roles of MAPs in microtubule organization. J. Cell Biol. 126, 1017-1029[Abstract/Free Full Text].
Biernat, J., Gustke, N., Drewes, G., Mandelkow, E.-M., and Mandelkow, E. (1993). Phosphorylation of serine 262 strongly reduces the binding of tau protein to microtubules: distinction between PHF-like immunoreactivity and microtubule binding. Neuron 11, 153-163[CrossRef][Medline].
Biernat, J., and Mandelkow, E.-M. (1999). The development of cell processes induced by tau protein requires phosphorylation of serine 262 and 356 in the repeat domain and is inhibited by phosphorylation in the proline-rich domains. Mol. Biol. Cell 10, 727-740[Abstract/Free Full Text].
Binder, L.I., Frankfurter, A., and Rebhun, L. (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].
Böhm, H., Brinkmann, V., Drab, M., Henske, A., and Kurzchalia, T.V. (1997). Mammalian homologues of C. elegans PAR-1 are asymmetrically localized in epithelial cells and may influence their polarity. Curr. Biol. 7, 603-606[CrossRef][Medline].
Borisy, G.G., and Svitkina, T.M. (2000). Actin machinery: pushing the envelope. Curr. Opin. Cell Biol. 12, 104-112[CrossRef][Medline].
Boyle, W.J., van der Geer, P., and Hunter, T. (1991). Phosphopeptide mapping and phosphoamino acid analysis by two-dimensional separation on thin layer cellulose plates. Methods Enzymol. 201, 110-149[Medline].
Bradke, F., and Dotti, C.G. (1999). The role of local actin instability in axon formation. Science 283, 1931-1934[Abstract/Free Full Text].
Bradke, F., and Dotti, C.G. (2000). Establishment of neuronal polarity: lessons from cultured hippocampal neurons. Curr. Opin. Neurobiol. 10, 574-581[CrossRef][Medline].
Brandt, R., Leger, J., and Lee, G. (1995). Interaction of tau with the neural plasma membrane mediated by tau's amino-terminal projection domain. J. Cell Biol. 131, 1327-1340[Abstract/Free Full Text].
Brown, A.J., Hutchings, C., Burke, J.F., and Mayne, L.V. (1999). Application of a rapid method (targeted display) for the identification of differentially expressed mRNAs following NGF-induced neuronal differentiation in PC12 cells. Mol. Cell. Neurosci. 13, 119-130[CrossRef][Medline].
Butner, K.A., and Kirschner, M.W. (1991). Tau-protein binds to microtubules through a flexible array of distributed weak sites. J. Cell Biol. 115, 717-730[Abstract/Free Full Text].
Caceres, A., and Kosik, K.S. (1990). Inhibition of neurite polarity by tau antisense oligonucleotide in primary cerebellar neurons. Nature 343, 461-463[CrossRef][Medline].
Chijiwa, T., Mishima, A., Hagiwara, M., Sano, M., Hayashi, K., Inoue, T., Naito, K., Toshioka, T., and Hidaka, H. (1990). Inhibition of forskolin-induced neurite outgrowth and protein phosphorylation by a newly synthesized selective inhibitor of cyclic AMP-dependent protein kinase, N-[2-(p-bromocinnamylamino)ethyl]-5-isoquinolinesulfonamide (H-89), of PC12D pheochromocytoma cells. J. Biol. Chem. 265, 5267-5272[Abstract/Free Full Text].
Cleveland, D.W., Hwo, S.-Y., and Kirschner, M.W. (1977). Physical and chemical properties of purified tau factor and the role of tau in microtubule assembly. J. Mol. Biol. 116, 227-247[CrossRef][Medline].
Cunningham, C., Leclerc, N., Flanagan, L., Lu, M., Janmey, P., and Kosik, K. (1997). Microtubule-associated protein 2c reorganizes both microtubules and microfilaments into distinct cytological structures in an actin-binding protein-280-deficient melanoma cell line. J. Cell Biol. 136, 845-857[Abstract/Free Full Text].
Dan, C., Nath, N., Liberto, M., and Minden, A. (2002). PAK5, a brain-specific kinase, promotes neurite outgrowth in N1E-115 cells. Mol. Cell. Biol. 22, 567-577[Abstract/Free Full Text].
Daub, H., Gevaert, K., Vandekerckhove, J., Sobel, A., and Hall, A. (2001). Rac/cdc42 and p65PAK regulated the microtubule-destablizing protein stathmin through phosphorylation at serine 16. J. Biol. Chem. 276, 1677-1680[Abstract/Free Full Text].
Delacourte, A., and Buee, L. (2000). Tau pathology: a marker of neurodegenerative disorders. Curr. Opin. Neurol. 13, 371-376[CrossRef][Medline].
DiTella, M.C., Feiguin, F., Carri, N., Kosik, K.S., and Caceres, A. (1996). MAP-1B/TAU functional redundancy during laminin-enhanced axonal growth. J. Cell Sci. 109, 467-477[Abstract].
DiTella, M., Feiguin, F., Morfini, G., and Caceres, A. (1994). Microfilament-associated growth cone component depends upon Tau for its intracellular localization. Cell Motil. Cytoskeleton 29, 117-130[CrossRef][Medline].
Drewes, G., Trinczek, B., Illenberger, S., Biernat, J., Schmitt-Ulms, G., Meyer, H.E., Mandelkow, E.-M., and Mandelkow, E. (1995). MAP/microtubule affinity regulating kinase (P110/mark): a novel protein kinase that regulates tau-microtubule interactions and dynamic instability by phosphorylation at the Alzheimer-specific site Serine 262. J. Biol. Chem. 270, 7679-7688[Abstract/Free Full Text].
Drewes, G., Ebneth, A., and Mandelkow, E.-M. (1998). MAPs, MARKs, and microtubule dynamics. Trends Biochem. Sci. 23, 307-311[CrossRef][Medline].
Drewes, G., Ebneth, A., Preuss, U., Mandelkow, E.-M., and Mandelkow, E. (1997). MARK: a novel family of protein kinases that phosphorylate microtubule-associated proteins and trigger microtubule disruption. Cell 89, 297-308[CrossRef][Medline].
Drubin, D., and Kirschner, M. (1986). Tau protein function in living cells. J. Cell Biol. 103, 2739-2746[Abstract/Free Full Text].
Ebneth, A., Drewes, G., Mandelkow, E.-M., and Mandelkow, E. (1999). Phosphorylation of MAP2c and MAP4 by MARK kinases leads to the destabilization of microtubules in cells. Cell Motil. Cytoskeleton 44, 209-224[CrossRef][Medline].
Ebneth, A., Godemann, R., Stamer, K., Illenberger, S., Trinczek, B., Mandelkow, E.-M., and Mandelkow, E. (1998). Overexpression of tau protein alters kinesin-dependent trafficking of vesicles, mitochondria, and endoplasmic reticulum: implications for Alzheimer's disease. J. Cell Biol. 143, 777-794[Abstract/Free Full Text].
Edson, K., Weisshaar, B., and Matus, A. (1993). Actin depolymerization induces process formation on MAP2-transfected nonneuronal cells. Development 117, 689-700[Abstract].
Esmaeli-Azad, B., Mccarty, J.H., and Feinstein, S.C. (1994). Sense and antisense transfection analysis of tau-function: tau influences net microtubule assembly, neurite outgrowth and neuritic stability. J. Cell Sci. 107, 869-879[Abstract].
Godemann, R., Biernat, J., Mandelkow, E., and Mandelkow, E.-M. (1999). Phosphorylation of tau protein by recombinant GSK-3 $beta$ : pronounced phosphorylation at select Ser/Thr-Pro motifs but no phosphorylation at Ser262 in the repeat domain. FEBS Lett. 454, 157-164[CrossRef][Medline].
Goedert, M., Spillantini, M., Jakes, R., Rutherford, D., and Crowther, R.A. (1989). Multiple isoforms of human microtubule-associated protein-tau: sequences and localization in neurofibrillary tangles of Alzheimers-disease. Neuron 3, 519-526[CrossRef][Medline].
Goode, B.L., Drubin, D.G., and Barnes, G. (2000). Functional cooperation between the microtubule and actin cytoskeletons. Curr. Opin. Cell Biol. 12, 63-71[CrossRef][Medline].
Griffith, L.M., and Pollard, T.M. (1982). The interaction of actin filaments with microtubules and microtubule-associated proteins. J. Biol. Chem. 257, 9143-9151[Abstract/Free Full Text].
Guo, S., and Kemphues, K.J. (1995). par-1, a gene required for establishing polarity in C. elegans embryos, encodes a putative Ser/Thr kinase that is asymmetrically distributed. Cell 81, 611-620[CrossRef][Medline].
Gustke, N., Trinczek, B., Biernat, J., Mandelkow, E.-M., and Mandelkow, E. (1994). Domains of tau protein and interactions with microtubules. Biochemistry 33, 9511-9522[CrossRef][Medline].
Hanks, S.K., and Hunter, T. (1995). Protein kinases 6. The eukaryotic protein kinase superfamily: kinase catalytic domain structure and classification. FASEB J. 9, 576-596[Abstract].
Harada, A., Oguchi, K., Okabe, S., Kuno, J., Terada, S., Ohshima, T., Sato-Yoshitake, R., Takei, Y., Noda, T., and Hirokawa, N. (1994). Altered microtubule organization in small-caliber axons of mice lacking tau protein. Nature 369, 488-491[CrossRef][Medline].
Hirokawa, N., Funakoshi, T., Satoharada, R., and Kanai, Y. (1996). Selective stabilization of tau in axons and microtubule-associated protein 2c in cell-bodies and dendrites contributes to polarized localization of cytoskeletal proteins in mature neurons. J. Cell Biol. 132, 667-679[Abstract/Free Full Text].
Illenberger, S., Drewes, G., Trinczek, B., Biernat, J., Meyer, H.E., Olmsted, J.B., Mandelkow, E.-M., and Mandelkow, E. (1996). Phosphorylation of microtubule-associated proteins MAP2 and MAP4 by the protein kinase p110-MARK: phosphorylation sites and regulation of microtubule dynamics. J. Biol. Chem. 271, 10834-10843[Abstract/Free Full Text].
Illenberger, S., Zheng-Fischhofer, Q., Preuss, U., Stamer, K., Baumann, K., Trinczek, B., Biernat, J., Godemann, R., Mandelkow, E.-M., and Mandelkow, E. (1998). The endogenous and cell-cycle dependent phosphorylation of tau protein in living cells: implications for Alzheimer's disease. Mol. Biol. Cell, 9, 1495-1512[Abstract/Free Full Text].
Imahori, K., and Uchida, T. (1997). Physiology and pathology of tau protein kinases in relation to Alzheimer's disease. J. Biochem. 121, 179-188.
Jenkins, S.M., and Johnson, G.V.W. (1997). Phosphorylation of microtubule-associated protein tau on Ser 262 by an embryonic 100 kDa protein kinase. Brain Res. 767, 305-313[CrossRef][Medline].
Jordan, M.A., and Wilson, L. (1998). Use of drugs to study role of microtubule assembly dynamics in living cells. Methods Enzymol. 298, 252-76[Medline].
Kabir, N., Schaefer, A.W., Nakhost, A., Sossin, W.S., and Forscher, P. (2001). Protein kinase C activation promotes microtubule advance in neuronal growth cones by increasing average microtubule growth lifetimes. J. Cell Biol. 152, 1033-1044[Abstract/Free Full Text].
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].
Kaverina, I., Rottner, K., and Small, J.V. (1998). Targeting, capture, and stabilization of microtubules in early focal adhesions. J. Cell Biol. 142, 181-190[Abstract/Free Full Text].
Kemphues, K. (2000). PARsing embryonic polarity. Cell 101, 345-348[CrossRef][Medline].
Knops, J., Kosik, K., Lee, G., Pardee, J., Cohen-Gould, L., and McConlogue, L. (1991). Overexpression of tau in a nonneuronal cell induces long cellular processes. J. Cell Biol. 114, 725-733[Abstract/Free Full Text].
Knowles, R., Leclerc, N., and Kosik, K.S. (1994). Organization of actin and microtubules during process formation in tau-expressing Sf9 cells. Cell Motil. Cytoskeleton 28, 256-264[CrossRef][Medline].
Leclerc, S., et al. (2001). Indirubins inhibit glycogen synthase kinase-3b and CDK5/p25, two protein kinases involved in abnormal tau phosphorylation in Alzheimer's disease: a property common to most CDK inhibitors? J. Biol. Chem. 276, 251-260[Abstract/Free Full Text].
Lee, V.M.Y., Balin, B.J., Otvos, L., 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].
Lee, G., Cowan, N., and Kirschner, M. (1988). The primary structure and heterogeneity of tau protein from mouse brain. Science 239, 285-288[Abstract/Free Full Text].
Lee, G., Newman, S.T., Gard, D.L., Band, H., and Panchamoorthy, G. (1998). Tau interacts with src-family non-receptor tyrosine kinases. J. Cell Sci. 111, 3167-3177[Abstract].
Leger, J.G., Brandt, R., and Lee, G. (1994). Identification of tau protein regions required for process formation in PC12 cells. J. Cell Sci. 107, 3403-3412[Abstract].
Levin, D.E., and Bishop, J.M. (1990). A putative protein-kinase gene (kin1+) is important for growth polarity in Schizosaccharomyces pombe. Proc. Natl. Acad. Sci. USA 87, 8272-8276[Abstract/Free Full Text].
Liao, H., Li, Y., Brautigan, D.L., and Gundersen, G.G. (1998). Protein phosphatase 1 is targeted to microtubules by the microtubule-associated protein tau. J. Biol. Chem. 273, 21901-21908[Abstract/Free Full Text].
Liao, G., Nagasaki, T., and Gundersen, G.G. (1995). Low concentrations of nocodazole interfere with fibroblast locomotion without significantly affecting microtubule level: implications for the role of dynamic microtubules in cell locomotion. J. Cell Sci. 108, 3473-3483[Abstract].
Litersky, J.M., and Johnson, G.V.W. (1995). Phosphorylation of tau in-situ: inhibition of calcium-dependent proteolysis. J. Neurochem. 65, 903-911[Medline].
Lopez, L.A., and Sheetz, M.P. (1995). A microtubule-associated protein (MAP2) kinase restores microtubule motility in embryonic brain. J. Biol. Chem. 270, 12511-12517[Abstract/Free Full Text].
Lucas, F., Goold, R., Gordon-Weeks, P., and Salinas, P. (1998). Inhibition of GSK-3 $beta$ leading to the loss of phosphorylated MAP-1B is an early event in axonal remodelling induced by WNT-7a or lithium. J. Cell Sci. 111, 1351-1361[Abstract].
Mandell, J.W., and Banker, G.A. (1996). A spatial gradient of tau-protein phosphorylation in nascent axons. J. Neurosci. 16, 5727-5740[Abstract/Free Full Text].
Mandelkow, E.-M., and Mandelkow, E. (1998). Tau in Alzheimer's disease. Trends Cell Biol. 8, 425-427[CrossRef][Medline].
Meijer, L., et al. (2000). Inhibition of cyclin-dependent kinases, G.S.K-3b and casein kinase 1 by hymenialdisine, a marine sponge constituent. Chem. Biol. 7, 51-63[CrossRef][Medline].
Moreno, F.J., Medina, M., Perez, M., Degarcini, E.M., and Avila, J. (1995). Glycogen-synthase kinase-3 phosphorylates recombinant human tau protein at Serine-262 in the presence of heparin (or tubulin). FEBS Lett. 372, 65-68[CrossRef][Medline].
Morishima-Kawashima, M., Hasegawa, M., Takio, K., Suzuki, M., Yoshida, H., Titani, K., and Ihara, Y. (1995). Proline-directed and non-proline-directed phosphorylation of PHF-tau. J. Biol. Chem. 270, 823-829[Abstract/Free Full Text].
Nelson, W.J., and Grindstaff, K.K. (1997). Cell polarity: par for the polar course. Curr. Biol. 7, R562-R564[CrossRef][Medline].
Obar, R.A., Dingus, J., Bayley, H., and Vallee, R.B. (1989). The RII subunit of cAMP-dependent protein-kinase binds to a common amino-terminal domain in microtubule-associated proteins 2a, 2b, and 2c. Neuron 3, 639-645[CrossRef][Medline].
Ookata, K., Hisanaga, S., Sugita, M., Okuyama, A., Murofushi, H., Kitazawa, H., Chari, S., Bulinski, J.C., and Kishimoto, T. (1997). MAP4 is the in-vivo substrate for cdc2 kinase in HeLa cells: identification of an M-phase specific and a cell cycle-independent phosphorylation site in MAP4. Biochemistry 36, 15873-15883[CrossRef][Medline].
Ozer, R., and Halpain, S. (2000). Phosphorylation-dependent localization of microtubule-associated protein MAP2c to the actin cytoskeleton. Mol. Biol. Cell 11, 3573-3587[Abstract/Free Full Text].
Palazzo, A., Cook, T., Alberts, A., and Gundersen, G.G. (2001). m-Dia mediates Rho-regulated formation, and orientation of stable microtubules. Nat. Cell Biol. 3, 723-729[CrossRef][Medline].
Panda, D., Miller, H.P., and Wilson, L. (1999). Rapid treadmilling of brain microtubules free of microtubule-associated proteins in vitro and its suppression by tau. Proc. Natl. Acad. Sci. USA 96, 12459-12464[Abstract/Free Full Text].
Rochlin, M.W., Wickline, K., and Bridgman, P. (1996). Microtubule stability decreases axon elongation but not axoplasm production. J. Neurosci. 16, 3236-3246[Abstract/Free Full Text].
Schneider, A., Biernat, J., von Bergen, M., Mandelkow, E., and Mandelkow, E.-M. (1999). Phosphorylation that detaches tau protein from microtubules (Ser262, Ser214) also protects it against aggregation into Alzheimer paired helical filaments. Biochemistry 38, 3549-3558[CrossRef][Medline].
Seubert, P., et al. (1995). Detection of phosphorylated Ser(262) in fetal tau, adult tau, and paired helical filament tau. J. Biol. Chem. 270, 18917-18922[Abstract/Free Full Text].
Shulman, J., Benton, R., and St. Johnston, D. (2000). The Drosophila homolog of C. elegans PAR-1 organizes the oocyte cytoskeleton and directs oskar mRNA localization to the posterior pole. Cell 101, 377-388[CrossRef][Medline].
Sontag, E., Nunbhakdi-Craig, V., Lee, G., Brandt, R., Kamibayashi, C., Kuret, J., White, C., Mumby, M., and Bloom, G. (1999). Molecular interactions among protein phosphatase 2A, tau, and microtubules. Implications for the regulation of tau phosphorylation and the development of tauopathies. J. Biol. Chem. 274, 25490-25498[Abstract/Free Full Text].
Stambolic, V., Ruel, L., and Woodgett, J.R. (1996). Lithium inhibits glycogen-synthase kinase-3 activity and mimics wingless signaling in intact cells. Curr. Biol. 6, 1664-1668[CrossRef][Medline].
Stamer, K., Vogel, R., Thies, E., Mandelkow, E., and Mandelkow, E.-M. (2002). Tau blocks traffic of organelles, neurofilaments, and APP-vesicles in neurons and enhances oxidative stress. J. Cell Biol. 156, 1051-1063[Abstract/Free Full Text].
Tanaka, E., Ho, T., and Kirschner, M.W. (1995). Microtubule behavior in the growth cones of living neurons during axon elongation. J. Cell Biol. 115, 345-363[Abstract/Free Full Text].
Tomancak, P., Piano, F., Riechmann, V., Gunsalus, K.C., Kemphues, K.J., and Ephrussi, A. (2000). A Drosophila melanogaster homologue of Caenorhabditis elegans par-1 acts at an early step in embryonic-axis formation. Nat. Cell Biol. 2, 458-460[CrossRef][Medline].
Takei, Y., Teng, J., Harada, A., and Hirokawa, N. (2000). Defects in axonal elongation and neuronal migration in mice with disrupted tau and MAP1b genes. J. Cell Biol. 150, 989-1000[Abstract/Free Full Text].
Ulloa, L., Montejo de Garcini, E., Gomez-Ramos, P., Moran, M.A., and Avila, J. (1994). Microtubule-associated protein MAP1B showing a fetal phosphorylation pattern is present in sites of neurofibrillary degeneration in brains of Alzheimer's disease patients. Brain Res. Mol. Brain Res. 26, 113-122[Medline].
Waterman-Storer, C.M., and Salmon, E.D. (1997). Actomyosin-based retrograde flow of microtubules in the lamella of migrating epithelial cells influences microtubule dynamic instability and turnover and is associated with microtubule breakage and treadmilling. J. Cell Biol. 139, 417-434[Abstract/Free Full Text].
Waterman-Storer, C., and Salmon, E.D. (1999). Positive feedback interactions between microtubule and actin dynamics during cell motility. Curr. Opin. Cell Biol. 11, 61-67[CrossRef][Medline].
Watanabe, A., Hasegawa, M., Suzuki, M., Takio, K., Morishima-Kawashima, M., Titani, K., Arai, T., Kosik, K.S., and Ihara, Y. (1993). In vivo phosphorylation sites in fetal and adult rat tau. J. Biol. Chem. 268, 25712-25717[Abstract/Free Full Text].
Woodring, P.J., Litwack, E.D., O'Leary, D.D., Lucero, G.R., Wang, J.Y., and Hunter, T. (2002). Modulation of the F-actin cytoskeleton by c-Abl tyrosine kinase in cell spreading and neurite extension. J. Cell Biol. 156, 879-892[Abstract/Free Full Text].
Zheng-Fischhofer, Q., Biernat, J., Mandelkow, E.-M., Illenberger, S., Godemann, R., and Mandelkow, E. (1998). Sequential phosphorylation of tau-protein by GSK-3b and protein kinase A at Thr212 and Ser214 generates the Alzheimer-specific epitope of antibody AT100 and requires a paired helical filament-like conformation. Eur. J. Biochem. 252, 542-552[Medline].

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I. Khlistunova, J. Biernat, Y. Wang, M. Pickhardt, M. von Bergen, Z. Gazova, E. Mandelkow, and E.-M. Mandelkow
Inducible Expression of Tau Repeat Domain in Cell Models of Tauopathy: AGGREGATION IS TOXIC TO CELLS BUT CAN BE REVERSED BY INHIBITOR DRUGS
J. Biol. Chem., January 13, 2006; 281(2): 1205 - 1214.
[Abstract] [Full Text] [PDF]

S. Kosuga, E. Tashiro, T. Kajioka, M. Ueki, Y. Shimizu, and M. Imoto
GSK-3beta Directly Phosphorylates and Activates MARK2/PAR-1
J. Biol. Chem., December 30, 2005; 280(52): 42715 - 42722.
[Abstract] [Full Text] [PDF]

B. Margolis and J.-P. Borg
Apicobasal polarity complexes
J. Cell Sci., November 15, 2005; 118(22): 5157 - 5159.
[Full Text] [PDF]

D. Matenia, B. Griesshaber, X.-y. Li, A. Thiessen, C. Johne, J. Jiao, E. Mandelkow, and E.-M. Mandelkow
PAK5 Kinase Is an Inhibitor of MARK/Par-1, Which Leads to Stable Microtubules and Dynamic Actin
Mol. Biol. Cell, September 1, 2005; 16(9): 4410 - 4422.
[Abstract] [Full Text] [PDF]

F. Darios, M.-P. Muriel, M. E. Khondiker, A. Brice, and M. Ruberg
Neurotoxic Calcium Transfer from Endoplasmic Reticulum to Mitochondria Is Regulated by Cyclin-Dependent Kinase 5-Dependent Phosphorylation of Tau
J. Neurosci., April 20, 2005; 25(16): 4159 - 4168.
[Abstract] [Full Text] [PDF]

M. Kishi, Y. A. Pan, J. G. Crump, and J. R. Sanes
Mammalian SAD Kinases Are Required for Neuronal Polarization
Science, February 11, 2005; 307(5711): 929 - 932.
[Abstract] [Full Text] [PDF]

J. Boudeau, J. W. Scott, N. Resta, M. Deak, A. Kieloch, D. Komander, D. G. Hardie, A. R. Prescott, D. M. F. van Aalten, and D. R. Alessi
Analysis of the LKB1-STRAD-MO25 complex
J. Cell Sci., December 15, 2004; 117(26): 6365 - 6375.
[Abstract] [Full Text] [PDF]

G. V. W. Johnson and W. H. Stoothoff
Tau phosphorylation in neuronal cell function and dysfunction
J. Cell Sci., November 15, 2004; 117(24): 5721 - 5729.
[Abstract] [Full Text] [PDF]

E.-M. Mandelkow, E. Thies, B. Trinczek, J. Biernat, and E. Mandelkow
MARK/PAR1 kinase is a regulator of microtubule-dependent transport in axons
J. Cell Biol., October 11, 2004; 167(1): 99 - 110.
[Abstract] [Full Text] [PDF]

S. Caenepeel, G. Charydczak, S. Sudarsanam, T. Hunter, and G. Manning
The mouse kinome: Discovery and comparative genomics of all mouse protein kinases
PNAS, August 10, 2004; 101(32): 11707 - 11712.
[Abstract] [Full Text] [PDF]

D. Cohen, P. J. Brennwald, E. Rodriguez-Boulan, and A. Musch
Mammalian PAR-1 determines epithelial lumen polarity by organizing the microtubule cytoskeleton
J. Cell Biol., March 1, 2004; 164(5): 717 - 727.
[Abstract] [Full Text] [PDF]

B. Trinczek, M. Brajenovic, A. Ebneth, and G. Drewes
MARK4 Is a Novel Microtubule-associated Proteins/Microtubule Affinity-regulating Kinase That Binds to the Cellular Microtubule Network and to Centrosomes
J. Biol. Chem., February 13, 2004; 279(7): 5915 - 5923.
[Abstract] [Full Text] [PDF]

J. L. Goldberg
How does an axon grow?
Genes & Dev., April 15, 2003; 17(8): 941 - 958.
[Full Text] [PDF]

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				J. Boudeau, J. W. Scott, N. Resta, M. Deak, A. Kieloch, D. Komander, D. G. Hardie, A. R. Prescott, D. M. F. van Aalten, and D. R. Alessi Analysis of the LKB1-STRAD-MO25 complex J. Cell Sci., December 15, 2004; 117(26): 6365 - 6375. [Abstract] [Full Text] [PDF]

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				E.-M. Mandelkow, E. Thies, B. Trinczek, J. Biernat, and E. Mandelkow MARK/PAR1 kinase is a regulator of microtubule-dependent transport in axons J. Cell Biol., October 11, 2004; 167(1): 99 - 110. [Abstract] [Full Text] [PDF]

				S. Caenepeel, G. Charydczak, S. Sudarsanam, T. Hunter, and G. Manning The mouse kinome: Discovery and comparative genomics of all mouse protein kinases PNAS, August 10, 2004; 101(32): 11707 - 11712. [Abstract] [Full Text] [PDF]

				D. Cohen, P. J. Brennwald, E. Rodriguez-Boulan, and A. Musch Mammalian PAR-1 determines epithelial lumen polarity by organizing the microtubule cytoskeleton J. Cell Biol., March 1, 2004; 164(5): 717 - 727. [Abstract] [Full Text] [PDF]

				B. Trinczek, M. Brajenovic, A. Ebneth, and G. Drewes MARK4 Is a Novel Microtubule-associated Proteins/Microtubule Affinity-regulating Kinase That Binds to the Cellular Microtubule Network and to Centrosomes J. Biol. Chem., February 13, 2004; 279(7): 5915 - 5923. [Abstract] [Full Text] [PDF]

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