Evidence for a Role of Mixed Lineage Kinases in Neuronal Apoptosis

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The Journal of Neuroscience, July 15, 2001, 21(14):4949-4957

Evidence for a Role of Mixed Lineage Kinases in Neuronal Apoptosis
Mónica Mota¹, Melissa Reeder², Jonathan Chernoff², and Chantal E. Bazenet¹
¹ Eisai London Research Laboratories, University College London, London WC1E 6BT, United Kingdom, and ² Fox Chase Cancer Center, Philadelphia, Pennsylvania 19111

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Superior cervical ganglion (SCG) sympathetic neurons die by apoptosis when deprived of nerve growth factor (NGF). It has beenshown previously that the induction of apoptosis in these neuronsat NGF withdrawal requires both the activity of the small GTP-bindingprotein Cdc42 and the activation of the c-Jun N-terminal kinase(JNK) pathway. The mixed lineage kinase 3 (MLK3) belongs to afamily of mitogen-activated protein (MAP) kinase kinase kinases.MLK3 contains a Cdc42/Rac interactive-binding (CRIB) domain andactivates both the JNK and the p38 MAP kinase pathways. In thisstudy the role of MLK3 in the induction of apoptosis in sympatheticneurons has been investigated. Overexpression of an active MLK3induces activation of the JNK pathway and apoptosis in SCG neurons.In addition, overexpression of kinase dead mutants of MLK3 blocksapoptosis as well as c-Jun phosphorylation induced by NGF deprivation.More importantly, MLK3 activity seems to increase by 5 hr afterNGF withdrawal in both differentiated PC12 cells and SCG neurons.We also show that MLK3 lies downstream of Cdc42 in the neuronaldeath pathway. Regulation of MLK3 in neurons seems to be dependenton MLK3 activity and possibly on an additional cellular component,but not on its binding to Cdc42. These results suggest that MLK3,or a closely related kinase, is a physiological element of NGFwithdrawal-induced activation of the Cdc42-c-Jun pathway and neuronaldeath. MLK3 therefore could be an interesting therapeutic targetin a number of neurodegenerative diseases involving neuronalapoptosis.

Key words: apoptosis; Cdc42; MLK3; signal transduction; sympathetic neurons; Jun kinase

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Activation of the c-Jun transcriptional pathway has been shown to be an important regulator of apoptosis of sympathetic neuronsinduced by nerve growth factor (NGF) withdrawal by both microinjectionof antibodies against c-Jun or expression of a c-Jun dominantnegative mutant (Estus et al., 1994; Ham et al., 1995). Consistentwith these observations, removal of survival factors leads tothe activation of c-Jun N-terminal kinase (JNK), either aloneor together with p38 mitogen-activated kinase, in a number ofneuronal death paradigms, including PC12 cells (Xia et al., 1995),superior cervical ganglion (SCG) neurons (Ham et al., 1995; Eilerset al., 1998), and embryonic motoneurons (Maroney et al., 1998).In addition, phosphorylation of c-Jun and activation of JNK havebeen observed after neuronal injury in the adult rat brain (Herdegenet al., 1998) (for review, see Mielke and Herdegen, 2000). Takentogether, these studies demonstrate that the pathways regulatingboth the level of c-Jun and its phosphorylation are crucial forthe induction of neuronal cell death. Therefore, we were interestedin identifying the upstream signaling pathways regulating theactivation of the JNK-c-Jun pathway inneurons.

Recently, we have shown that, in rat SCG neurons, the Rho-like GTPases, Cdc42 and Rac1, are required for NGF withdrawal-induceddeath and that they induce apoptosis via activation of the c-Juntranscriptional pathway (Bazenet et al., 1998). Despite a plethoraof complex results (for review, see Johnson, 1999), it is stillunclear how Cdc42 directly activates the JNK pathway, especiallyin neuronal systems. The small GTP-binding proteins act via various,multiple downstream mitogen-activated protein (MAP) kinase kinasekinases, depending on the cell type, which bind the active GTP-boundform of the small G-proteins and induce JNK activity and transcriptionalactivation (Lim et al., 1996; Tapon and Hall, 1997; Van Aelstand D'Souza-Schorey, 1997) (for review, see Johnson, 1999). Thereare several likely intermediates in the signaling cascades linkingCdc42 to the JNK pathway, including the p21-activated kinases(rat p65PAK/PAK1/PAK $alpha$ , PAK-2/PAK $gamma$ , PAK-3/PAK $beta$ , and PAK4; Bagrodiaet al., 1995; Knaus et al., 1995; Manser et al., 1995; Martinet al., 1995; Brown et al., 1996; Abo et al., 1998), the germinalcenter kinase (GCK; Pombo et al., 1995), the nick-interactingprotein (NIK; Su et al., 1997), MEKK1 and MEKK4 (Fanger et al.,1997; Gerwins et al., 1997), plenty of SH3 (POSH) (Tapon et al.,1998), and the mixed lineage kinase family (MLK1, MLK2, MLK3,DLK, LZK) (Dorow et al., 1993; Holzman et al., 1994; Reddy andPleasure, 1994; Fan et al., 1996; Hirai et al., 1996; Rana etal., 1996; Teramoto et al., 1996; Tibbles et al., 1996; Hiraiet al., 1997; Sakuma et al., 1997; Nagata et al., 1998).

In this study we concentrated our efforts on mediators containing a Cdc42/Rac interactive-binding (CRIB) region (Burbelo etal., 1995) and more specifically on members of the MLK family.The MLKs have a distinctive protein kinase domain that shows structuralfeatures of both tyrosine and serine/threonine protein kinases,and they all have two leucine zipper-like motifs, located at theC terminus of the kinase domain, which are necessary for dimerizationthat then precedes the activation of MLKs (Dorow et al., 1993;Ezoe et al., 1994; Gallo et al., 1994; Ing et al., 1994; Leungand Lassam, 1998). The MLK family has been divided into two subgroups,based on their structural differences: the MLK subgroup includesMLK1, MLK2/MST, and MLK3/SPRK/PTK1; the DLK subgroup includesDLK/MUK/ZPK and LZK (which do not contain an SH3 domain or a CRIBdomain). Of the three known MLKs, MLK2 and MLK3 interact withGTP-Cdc42 and activate the JNK pathway (Nagata et al., 1998).When overexpressed in mammalian cells, MLK3 activates JNK viathe phosphorylation and activation of SEK/MKK4 (Rana et al., 1996)or MKK7 (Whitmarsh et al., 1998). Moreover, putative scaffoldproteins, JIP-1 (JNK interacting protein-1) and JIP-2 have recentlybeen identified and shown to interact in a specific manner withmembers of the MLK family and with MKK7 and JNK, but not withCdc42, thereby linking these kinase-signaling components (Dickenset al., 1997; Whitmarsh et al., 1998; Yasuda et al., 1999). MLK3has also been shown to activate the MAPK p38 kinase pathway viaMKK3/6 (Tibbles et al., 1996) and the extracellular signal-relatedprotein kinase (ERK) pathway (Hartkamp et al., 1999). In addition,expression of a dominant negative mutant of MLK3 led to a reductionin the Cdc42-dependent activation of JNK (Teramoto et al., 1996),and MLK3 CRIB domain has been shown to be required for its associationwith and activation by Cdc42 in human embryonic kidney 293 cells(Bock et al., 2000). Altogether, these studies strongly suggestthat MLK3 may be an important element within the mechanism ofstress-induced activation of the JNK pathway and of neuronaldeath.

Herein, using wild type (WT) and various MLK3 mutants [kinase dead (KD), CRIB( $-$ ), and KD CRIB( $-$ )], we showed that overexpressionof a kinase-active MLK3 is sufficient to induce apoptosis in ratsympathetic neurons and that this induction of cell death is accompaniedby an increase in the level of phosphorylated c-Jun. In addition,both kinase dead, dominant negative mutants of MLK3 could significantlyblock NGF withdrawal-induced cell death and its concomitant increasein the phosphorylation of c-Jun. Overexpression of both kinasedead mutants of MLK3 could also block death induced by Cdc42.Finally, an increase in MLK3 activity was observed 5 hr afterthe induction of apoptosis in both differentiated PC12 cells andSCG neurons. The present study strongly supports the notion thatMLK3, or a closely related kinase, plays a crucial and physiologicalrole in neuronal apoptotic celldeath.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cell culture. Sympathetic neurons were isolated from SCG of 1-d-old Sprague Dawley rats (supplied by the Biological ServicesUnit, University College London) as described previously (Hamet al., 1995). Briefly, neurons were plated on 13 mm glass coverslipscoated with poly-L-lysine and laminin (both from Sigma, Poole,UK) at a density of 8000-10,000 cells per coverslip and culturedin SCG growth medium [DMEM (Sigma), 10% heat inactivated fetalcalf serum (FCS; Globepharm, Surrey, UK), 2 mM each of glutamineand penicillin-streptomycin (both from Life Technologies, Paisley,UK), 100 ng/ml NGF, and 20 µM each of the anti-mitotic agentsfluoro-deoxyuridine and uridine (Sigma)]. Neurons were kept inculture in the presence of NGF for 5-7 d before being used forexperiments. NGF withdrawal was performed by refeeding the cellswith the SCG growth medium that lacked NGF but was supplementedwith 100 ng/ml of neutralizing anti-NGF antibody (Boehringer Mannheim,Mannheim, Germany). In some experiments, SCG neurons were pretreatedfor 2 hr with 100 µM of the broad caspase inhibitor benzyloxycarbonyl-Val-Ala-Asp(O-methyl)-fluoromethylketone (zVAD-fmk, Enzyme Systems Products,Dublin, CA) before being withdrawn from NGF. zVAD-fmk was presentin the culture medium throughout theexperiment.

PC12 cells were seeded at a density of 2 × 10⁶ cells per 9-cm-diameter dish and coated with poly-L-lysine (Sigma) and rat tailcollagen (Upstate Biotechnology, Buckingham, UK). The cells werecultured in defined medium supplemented with 10 µg/ml insulinand 2% FCS as described previously (Doherty et al., 1988). PC12cells were differentiated by culturing them with defined mediumsupplemented with 100 ng/ml 2.5S NGF (Promega, Southampton, UK).The cells were used within 7-8 d of NGF differentiation. NGF withdrawalwas performed by refeeding the cells with the defined medium containing100 ng/ml of anti-NGF antibody (BoehringerMannheim).

Jurkat cells were diluted to a density of 2.5 × 10⁴ cells/ml and cultured in DMEM supplemented with 10% FCS, 2 mM glutamine,and penicillin-streptomycin for 24hr.

Cos-7 cells were grown in DMEM supplemented with 10% FCS, 2 mM glutamine, and penicillin-streptomycin (both from LifeTechnologies).

Immunoblotting. The culture medium of differentiated PC12 cells and SCG neurons was removed and centrifuged at 2000 rpm for10 min at 4°C to collect the detached cells. The cells remainingon the dish were rinsed twice with PBS and lysed with 250 µl ofcold lysis buffer [ containing (in mM) 50 Tris-HCl, pH 7.4, 250NaCl, 5 EDTA, 50 NaF, 1 Na₃VO₄, and 1 PMSF plus 0.1% Nonidet P-40,10 µg/ml aprotinin, 1 µg/ml leupeptin, and 10 µg/ml TPCK]. Thecells were scraped, and the lysate was added to the pellet ofdetached apoptotic cells and further incubated on ice for 10 min.The Jurkat cells were centrifuged for 5 min at 2000 rpm and resuspendedin 100 µl of lysis buffer. The nuclei and cell membranes wereremoved by centrifugation at 5000 rpm for 15 min at 4°C. Proteinconcentration in the supernatants was determined by the Bradfordmethod.

Thirty micrograms of protein were resolved by electrophoresis, using 12.5% SDS-polyacrylamide gels. Then the proteins weretransferred to nitrocellulose. The membranes were incubated for1 hr at room temperature in blocking buffer (5% nonfat dry milk,0.1% Tween 20 in PBS) and then overnight at 4°C with 200 ng/mlof an anti-MLK3 primary antibody (C-20, Santa Cruz, Santa Cruz,CA) in blocking buffer. In peptide competition experiments thediluted antibody was incubated with a 10-fold excess (in micrograms)of the antigen peptide (Santa Cruz) for 2 hr at room temperaturebefore being used for immunoblotting. After rinsing, the membraneswere washed and incubated with a horseradish peroxidase-conjugatedgoat anti-rabbit (Amersham, Buckinghamshire, UK) diluted 1:2000in blocking buffer. The blots were developed with the ECL system(Amersham).

In vitro MLK3 kinase assay. MLK3 was immunoprecipitated from differentiated PC12 cells or SCG neurons maintained in the presenceor absence of NGF; the lysates were precleared by the additionof 15 µl of 1:1 slurry of protein A-agarose beads previously washedin lysis buffer [containing (in mM) 50 HEPES, pH 7.5, 150 NaCl,1 EGTA, 150 NaF, 1.5 MgCl₂, 1 Na₃VO₄, 10 $beta$ -glycerophosphate, and1 PMSF plus 1% Triton X-100, 10% glycerol, 1 µg/ml aprotinin,1 µg/ml leupeptin, and 1 µg/ml pepstatin]. After 15 min of incubationat 4°C, 7.5 µg of MLK3 antibody was added to the lysate of 4 ×10⁶ cells (PC12 cells) or 1.5 × 10⁵ cells (SCG neurons) together with 15 µl of 1:1 slurry of prewashedprotein A-agarose beads. Then the mixture was incubated end overend for 1 hr. The beads were spun down for 2 min at 4°C and washedtwice with lysis buffer and once with MLK3 buffer (50 mM Tris-HCl,pH 7.4, 10 mM MgCl₂, and 1 mM EGTA). Finally, the beads were resuspendedin 10 µl of kinase buffer and incubated with 20 µg/ml of myelinbasic protein (MBP) as an exogenous substrate for 10 min at 4°C,after which 10 µCi of [ $gamma$ -³²P]ATP was added to the immunoprecipitates. The reaction was allowedto proceed for 10 min at 30°C and was stopped by the additionof 20 µl of 2× sample buffer (4% SDS, 5.6 M 2-mercaptoethanol,20% glycerol, 200 mM Tris-HCl, pH 6.8, and 1% bromophenol blue)containing 20 mM EDTA. The samples were heated up at 98°C andthen separated on a 12.5% SDS-PAGE polyacrylamide gel. The gelwas stained with colloidal blue (Invitrogen, Groningen, The Netherlands)for 3 hr at room temperature, destained with water, and dried.The labeled proteins were revealed by autoradiography or by usingthe STORM PhosphorImager analysis (Molecular Dynamics, AmershamPharmacia Biotech, Buckinghamshire, UK); the intensity of eachband was determined by using ImageQuant software (Molecular Dynamics,Amersham Pharmacia Biotech). The results were plotted as agraph.

Microinjection and survival assay. Sympathetic neurons were microinjected as described previously (Bazenet et al., 1998).All plasmids were double-purified on a cesium chloride gradientand resuspended in H₂O. The injection mix comprised plasmid DNAin 0.5× PBS ( $-$ Ca²⁺ and $-$ Mg²⁺) and 5 mg/ml 70,000 kDa Texas Red-dextran (survival assay; MolecularProbes, Eugene, OR) or 2.5 mg/ml purified guinea pig IgG (immunostaininganalysis; Sigma) to identify the injected cells. Four hours afterinjection the neurons were re-fed as described above. The percentageof cell survival was assessed as described previously (Bazenetet al., 1998). Briefly, only the injected cells displaying a normalnucleus and intact neurites were counted asalive.

Immunofluorescence analysis. At 24 hr after microinjection, SCG neurons were fixed in 3% para-formaldehyde, permeabilizedwith 0.5% Triton X-100 in PBS, and blocked with 50% goat serumand 0.5% BSA in PBS. Then they were stained with a specific monoclonalphospho-c-Jun antibody (raised against a phosphopeptide, encompassingamino acids 57-68) and with phosphoserine 63 (Watson et al., 1998)or a monoclonal antibody against the FLAG epitope (Sigma) andthen with a FITC-conjugated secondary antibody and a rhodamine-conjugatedanti-guinea pig IgG antibody (Stratech Scientific, Luton, UK)to detect the injected cells. Only those cells showing a clearincrease over the background staining were scored as positive.To examine nuclear morphology, were stained with Hoechst dye (Hoechst33342, Sigma) at 10 µg/ml. Shrunken, condensed, or fragmentednuclei were consideredpyknotic.

Preparation of total RNA from SCG neurons. The growth medium of SCG neurons was transferred to a centrifuge tube and keptto collect the detached apoptotic cells. The cells remaining onthe dish were harvested by rinsing them in a small volume of ice-coldPBS. The adherent and floating cells were pooled and spun at 2000rpm for 10 min at 4°C and rinsed twice with PBS; total RNA wasprepared with the RNeasy mini kit (Qiagen, West Sussex,UK).

Reverse transcription-PCR. First-strand cDNA was prepared from the total RNA extracts from SCG neurons with Superscript IIRNase H Reverse Transcriptase (Life Technologies, Paisley, UK).Briefly, 2 µg of total SCG RNA was incubated with 0.5 µg of Oligo-dT_12-18primer (Life Technologies) and 3 µg of random primers (Life Technologies)in a total volume of 20 µl for 10 min at 70°C. The reaction mixwas placed on ice for 1-2 min before the addition of 4 µl of First-StrandBuffer, 2 µl 0.1 M DTT (all from Life Technologies), and 1 µlof 10 mM dNTP mix. The contents of the tube were mixed gentlyand incubated at 42°C for 2 min. Two hundred units of SuperScriptII were added, and the reaction mix was incubated for 50 min at42°C. The reaction was inactivated by heating to 70°C for 15 min.The PCR reactions were performed with the Elongase Enzyme Mixkit (Life Technologies) by following the manufacturer's recommendations.The following primers were used: forward primer, 5'-GTCATGGAATGGCAGTGG-3';reverse primer, 5'-GGCTGTAGTCGAACAGG-3'. The PCR products wereanalyzed on a 1% agarosegel.

Plasmids. pcDNA-FLAG MLK3 and MLK3 KD were obtained from Jim Woodgett (Ontario Cancer Institute, Toronto, Canada) (Tibbleset al., 1996). The CRIB( $-$ ) mutants MLK3 S493P, P495A, and H500Lwere made by using the Gene Editor in vitro site-directed mutagenesissystem (Promega). V12Cdc42 was a gift from Alan Hall (UniversityCollege London, London,UK).

In vivo binding of MLK3 proteins to Cdc42. Cos-7 cells were transiently transfected with 0.5 mg of myc-tagged Cdc42 (pRK5)or vector control along with 2 mg of the various FLAG-tagged MLK3constructs by the Lipofectamine method (Life Technologies). Cellswere harvested 48 hr after transfection in a Nonidet P-40 lysisbuffer [1% Nonidet P-40, 10% glycerol, and (in mM) 20 Tris, pH8.0, 137 NaCl, 50 NaF, 10 $beta$ -glycerophosphate, 1 PMSF, and 10 sodiumorthovanadate plus 10 µg/ml aprotinin]. The lysates were adjustedfor equal protein, and each sample was divided so that two-thirdsof the lysate was incubated with anti-myc antibodies (A-14, SantaCruz, Santa Cruz, CA) to immunoprecipitate Cdc42 along with boundMLK3 proteins; one-third of the lysate was incubated with anti-FLAGantibodies (M2, Scientific Imaging Systems, Kodak, Rochester,NY) to immunoprecipitate MLK3 protein. The immune complexes werecollected with protein A-agarose beads (Pierce, Rockford, IL),washed with the above lysis buffer without protease inhibitors,and analyzed by Western blotting to detect MLK3 protein with anti-FLAGantibodies.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

MLK3 is expressed in neuronal cells

MLK3 expression in rat neurons was determined at both mRNA and protein levels. Primers, based on the human MLK3 sequence fora 120 base pair glycine-rich region that is highly specific forMLK3 (amino acids 15-54; Sakuma et al., 1997), were designed andRNA-extracted from either PC12 cells or purified cultures of SCGneurons and then amplified by RT-PCR. A single PCR product of120 bases from both PC12 cells and SCG neurons, as predicted forMLK3, was obtained (Fig. 1A). Sequencing of these products confirmedthat they were derived from MLK3. The identified rat sequenceshares >83% homology with the human sequence at the amino acidlevel. Our second approach was to analyze cell extracts for thepresence of MLK3 protein. Extracts from Jurkat cells (positivecontrol for the antibody), PC12 cells, and SCG neurons were prepared.Western blotting that used the MLK3 antibody detected a 95 kDaband in the Jurkat cells, PC12 cells, and SCG extracts (Fig. 1B),confirming that MLK3 indeed is expressed in neurons. The immunodetectionof MLK3 could be competed by a 10-fold excess by weight of thepeptide antigen, confirming the specificity of this antibody.

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Figure 1. MLK3 is expressed in sympathetic neurons. A, MLK3 RNA is expressed in sympathetic neurons. Sympathetic neurons cultured for 6 d in the presence of NGF were lysed in RNA lysis buffer, and total RNA was extracted. RT-PCR was performed on the total RNA, and the products were analyzed on a 1.0% agarose gel. The amplified 120 bp fragment was sequenced and is consistent with MLK3. B, MLK3 protein is expressed in sympathetic neurons and PC12 cells. Cell extracts were prepared from SCG neurons, cultured for 6 d in the presence of NGF, 7-d-differentiated PC12 cells, and Jurkat cells. Then 30 µg of protein was resolved on a 12.5% SDS-PAGE polyacrylamide gel, transferred onto nitrocellulose, and probed with a polyclonal antibody to MLK3. The 95 kDa MLK3 band is competed away by the addition of the peptide antigen.

Characterization of MLK3 mutants and expression in SCG neurons

To investigate the role of MLK3 in neuronal death induced either by NGF withdrawal or the expression of Cdc42, we examinedthe effect of different MLK3 mutants [K144E, CRIB( $-$ ), and CRIB( $-$ )K144E].The K144E mutation in the ATP-binding site inactivates MLK3, therebyacting as a kinase dead (KD), dominant negative mutant (Tibbleset al., 1996). To abrogate the binding of MLK3 to the small GTP-bindingproteins, we introduced additional mutations, S493P, P495A, andH500L (three of five crucial amino acids in the consensus CRIBsequence; Burbelo et al., 1995). These amino acids were replacedin both wild type (WT) and KD MLK3 to generate the correspondingCRIB( $-$ ) mutants. To verify the binding properties of these mutants,we transiently transfected Cos-7 cells with myc-tagged Cdc42,along with the various FLAG-tagged MLK3 constructs. Then 2 d laterthe immunoprecipitates of the myc-tagged Cdc42 were analyzed byWestern blotting for the presence of bound MLK3. In addition,the FLAG-tagged MLK3 proteins were immunoprecipitated to checktheir level of expression. WT and KD MLK3, but not WT CRIB( $-$ )or KD CRIB( $-$ ), coimmunoprecipitated with Cdc42, demonstratingthat the CRIB( $-$ ) mutants fail to bind the activated Cdc42 andfunction as expected (Fig. 2A).

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Figure 2. Characterization of the MLK3 mutants and expression in SCG neurons. A, In vivo binding of MLK3 proteins with Cdc42. Cos-7 cells were transiently transfected with 2 µg of various FLAG-tagged MLK3 constructs along with 0.5 µg of myc-tagged Cdc42. Cells were harvested and lysed 48 hr after transfection. Cdc42 and MLK3 were immunoprecipitated with anti-myc and anti-FLAG antibodies, respectively. Then the immune complexes were analyzed by Western blotting, using the FLAG antibody to detect MLK3 protein. B, Subcellular localization of the different MLK3 mutants in SCG neurons. Sympathetic neurons, cultured for 5-7 d in the presence of NGF, were microinjected with 0.3 mg/ml plasmid DNA and 5 mg/ml guinea pig IgG to mark the injected cells. At 24 hr after injection the cells were stained with an anti-FLAG antibody to detect MLK3 expression, an anti-guinea pig IgG antibody (anti-GPIgG) to follow the injected cells, and with Hoechst to visualize the nuclei. Scale bar, 30 µm. The arrows point to cells displaying pyknotic nuclei.

Next, we microinjected rat sympathetic neurons, cultured for 5-7 d in the presence of NGF, with 0.3 mg/ml of an empty expressionvector or the various MLK3 mutants. At 24 hr after injection thecells were stained with an anti-FLAG antibody to check the levelof expression. We consistently found that in all cases 80-100%of the injected cells expressed the MLK3 construct. Interestingly,we noticed that the kinase-active forms [WT and CRIB( $-$ )] of MLK3were expressed mainly at the plasma membrane, whereas the kinasedead mutants [KD and KD CRIB( $-$ )] were seen throughout the cytoplasmof the neurons (Fig. 2B). The leucine zipper motifs of MLK3 arenecessary and sufficient for the dimerization of the protein,which in turn is a prerequisite for the transphosphorylation andautoactivation of MLK3 (Leung and Lassam, 1998). It appears thatoverexpression of MLK3 mutants is sufficient to drive dimerizationas long as they contain the leucine zipper motifs. However, translocationof MLK3 from the cytoplasm to the plasma membrane occurred onlywith a kinase-active mutant. Surprisingly, the mutations in theCRIB domain had no effect on the subcellular localization of MLK3.This suggests that transphosphorylation recruits MLK3 to a membranecomponent other than or in addition toCdc42.

MLK3 induces neuronal cell death

We then examined the effect of these mutants on the survival of SCG neurons cultured in the presence of NGF. SCG neurons weremicroinjected with 0.3 mg/ml of an empty expression vector orof the different MLK3 mutants. The percentage of survival wasassessed 48 hr after injection. Expression of the kinase-activeforms [WT and CRIB( $-$ )] of MLK3 significantly decreased the survivalof SCG neurons in a dose-dependent manner (Fig. 3A; data not shown),whereas the empty vector and the kinase dead mutants [KD and KDCRIB( $-$ )] had no effect (Fig. 3A). The nuclear morphology of theinjected neurons was characterized by Hoechst staining. At 24hr after injection the cells expressing WT and WT CRIB( $-$ ) clearlydisplayed pyknotic nuclei, a hallmark of apoptotic cells (Figs.2B, 3B), whereas neither of the KD mutants had an effect on thenuclear morphology of the injected cells. These results demonstratethat MLK3 can induce neuronal apoptosis in the presence of NGFand that its kinase activity is required for its proapoptoticeffect.

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Figure 3. MLK3 induces neuronal apoptosis. A, Induction of neuronal cell death by MLK3 in SCG neurons. Rat sympathetic neurons, cultured for 5-7 d in the presence of NGF, were microinjected with 0.3 mg/ml empty expression vector (E) or the different MLK3 constructs [WT, KD, CRIB( $-$ ), and KD CRIB( $-$ )] along with 70 kDa Texas Red-dextran to mark the injected cells. Then 48 hr later the percentage of surviving cells was assessed. In each experiment 200 cells were injected. The results are the mean of three independent experiments ± SEM. B, MLK3 increases the number of pyknotic nuclei in SCG neurons. SCG neurons were injected with 0.3 mg/ml control empty expression vector or the various constructs of MLK3. After 24 hr the nuclear morphology was visualized by Hoechst staining. The results are the mean of three independent experiments ± SEM. C, zVAD-fmk protects SCG neurons from MLK3-induced death. The 5- to 7-d-old sympathetic neurons were pretreated with 100 µM zVAD-fmk for 2 hr or were left untreated before microinjection with 0.3 mg/ml WT MLK3. The percentage of surviving cells was assessed 48 hr later. The results are the mean of three independent experiments ± SEM.

To confirm further the apoptotic nature of this death, we examined whether an inhibitor of caspases could protect SCG neuronsfrom MLK3-induced death. Sympathetic neurons were pretreated with100 µM of zVAD-fmk for 2 hr or maintained in their culture mediumbefore microinjection with WT MLK3. The percentage of survivingcells was assessed 48 hr later. As a control, we treated SCG neuronswith zVAD-fmk and maintained them in the presence of NGF or deprivedthem of NGF. zVAD-fmk had no toxic effect and rescued SCG neuronsfrom NGF withdrawal (data not shown). We also found that zVAD-fmkcould rescue neurons from MLK3-induced death to levels almostsimilar to +NGF control, suggesting that MLK3 can activate a caspase-dependentapoptotic pathway in SCG neurons (Fig. 3C).

MLK3 activity is increased after NGF deprivation in differentiated PC12 cells and in SCG neurons

More importantly, we wanted to examine whether the induction of neuronal apoptosis by NGF deprivation had any effect on theendogenous MLK3. To address this issue, we determined MLK3 activityin both differentiated PC12 cells and SCG neurons. PC12 cellswere differentiated for 7 d and either maintained in the presenceof NGF or withdrawn from NGF, as described in Materials and Methods.After 3, 5, and 7 hr the cells were lysed, and MLK3 was immunoprecipitatedwith a specific antibody raised against the C-terminal regionof MLK3. The kinase activity of the resulting immunoprecipitateswas assayed against the myelin basic protein. A 2.5-fold increasein MLK3 activity above basal level was observed and peaked at~5 hr after NGF withdrawal, whereas no significant variationswere seen when the cells were maintained in the presence of NGF(Fig. 4A,B).

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Figure 4. MLK3 activity is increased after NGF withdrawal in PC12 cells and in SCG neurons. MLK3 kinase assays were performed in differentiated PC12 cells (A, B) and in SCG neurons (5 DIV; C) that had been maintained in the presence of NGF or withdrawn from NGF for 3, 5, and 7 hr, as described in Materials and Methods. Fold activation of MLK3 activity was obtained by scanning the gels on a STORM PhosphorImager. A representative autoradiograph of a MLK3 kinase assay in PC12 cells is shown in A. The level of MLK3 activity at time 0 was set at 1. The results are the mean of three independent experiments ± SEM.

We next measured MLK3 activity in SCG neurons [5 d in vitro (5 DIV)] either maintained in the presence of NGF or withdrawnfrom NGF for 3, 5, and 7 hr. A comparable increase in the basallevel of MLK3 activity was observed in apoptotic SCG neurons (Fig.4C). Our results suggest that NGF withdrawal leads to the activationof MLK3 in both differentiated PC12 cells and SCG neurons, implicatinga role for MLK3 as a physiological mediator of neuronalapoptosis.

MLK3 activity is required for NGF withdrawal- and Cdc42-induced neuronal death

To confirm that MLK3 plays a role in NGF withdrawal-induced death, we microinjected each of the MLK3 constructs as well asan empty expression vector control (negative control) and Bcl-2(positive control) into SCG neurons. The cells were withdrawnfrom NGF, and the percentage of surviving cells was assessed 48hr later. Both dominant negative mutants [KD and KD CRIB( $-$ )] protectedthe neurons from NGF withdrawal-induced death to levels similarto those obtained with Bcl-2 (Fig. 5A). Neither WT forms of MLK3[WT and WT CRIB( $-$ )] rescued the sympathetic neurons (Fig. 5A).In addition, we looked at the effect of these mutants on the nuclearmorphology of the injected neurons by Hoechst staining at 24 hrafter injection. The cells injected with the empty vector controlhad clearly started to display pyknotic nuclei, whereas the cellsinjected with the kinase dead mutants of MLK3 had a much lowerpercentage of condensed or fragmented nuclei (Fig. 5B). Theseresults confirm that MLK3 is involved in the mediation of apoptosisin SCG neurons and that its kinase activity seems to be an importantrequirement for the execution of neuronal cell death.

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Figure 5. MLK3 is required for NGF withdrawal- and Cdc42-induced deaths. A, MLK3-KD mutants prevent NGF withdrawal-induced cell death in SCG neurons. SCG neurons, cultured for 5-7 d in the presence of NGF, were microinjected with 70 kDa Texas Red-dextran and 0.3 mg/ml of the various MLK3 mutants, an empty vector, or 0.05 mg/ml Bcl-2. Then 4 hr later the cells were withdrawn from NGF, and the number of injected cells was scored (100% value). The percentage of surviving cells was assessed after 48 hr, as described in Materials and Methods. The results are the mean of three independent experiments ± SEM. B, MLK3-KD mutants decrease the number of pyknotic nuclei after NGF withdrawal from SCG neurons. Neurons were injected with 0.3 mg/ml control empty expression vector or the different MLK3 mutants and withdrawn from NGF. After 24 hr the nuclear morphology was visualized by Hoechst staining. The results are the mean of three independent experiments ± SEM. C, Cdc42-induced apoptosis requires MLK3 activity. We coinjected 0.3 and 0.5 mg/ml KD MLK3 along with 0.1 mg/ml V12Cdc42 and 70 kDa Texas Red-dextran into SCG neurons. The cells were maintained in the presence of NGF, and the percentage of surviving cells was assessed 48 hr after injection as described previously. The results are the mean of three independent experiments ± SEM. D, Cdc42-induced apoptosis does not require binding to MLK3. KD CRIB( $-$ )MLK3, at the indicated concentrations (in mg/ml), and 0.1 mg/ml V12Cdc42 were microinjected into 5- to 7-d-old SCG neurons maintained in the presence of NGF. The percentage of surviving cells was assessed 48 hr later. The results are the mean of three independent experiments ± SEM.

We have recently shown that constitutively activated forms of the Rho family of GTPases, Cdc42 and Rac1, could induce apoptosisof SCG neurons via the activation of the c-Jun transcriptionalpathway (Bazenet et al., 1998). To examine whether MLK3 and Cdc42were on the same death-signaling pathway, we coinjected an activatedmutant of Cdc42 (V12Cdc42) with both the CRIB(+) or CRIB( $-$ ) kinasedead mutants of MLK3 into SCG neurons. The percentage of survivingcells was assessed 48 hr after injection. Regardless of its abilityto bind Cdc42, a kinase-inactive mutant of MLK3 efficiently blocksV12Cdc42-induced death (Fig. 5C,D), suggesting that the kinaseactivity of MLK3, but not its binding to Cdc42, is crucial forthe induction of apoptosis by Cdc42 and that MLK3 is a downstreammediator of Cdc42 signaling in sympathetic neurons. These resultsdemonstrate that blocking MLK3 activity is sufficient to inhibitboth NGF withdrawal- and Cdc42-induceddeath.

Overexpression of MLK3 induces an increase in the level of phosphorylated c-Jun

MLK3 has been shown previously to activate the JNK pathway in non-neuronal cells (Teramoto et al., 1996; Tibbles et al., 1996).To investigate whether this is the case in sympathetic neurons,we examined the effect of MLK3 on the phosphorylation of c-Junin both the presence and the absence of NGF. The 5- to 7-d-oldSCG neurons were microinjected with an empty vector or with eachof the different MLK3 mutants. The cells were fixed, permeabilized,and stained with a specific phospho-c-Jun antibody. Cells injectedwith either the empty vector control or the kinase dead mutantsof MLK3 did not show any increase in the level of phosphorylatedc-Jun compared with the noninjected cells (Fig. 6A,B). However,overexpression of the kinase-active forms of MLK3 induced a clearincrease in the levels of nuclear phosphorylated c-Jun (Fig. 6A,B).Moreover, we examined whether dominant negative mutants of MLK3could prevent the increase in phosphorylated c-Jun levels thatoccurs after NGF withdrawal. Overexpression of both kinase deadmutants in sympathetic neurons blocked the increase in the levelof phosphorylated c-Jun induced by NGF withdrawal, whereas theempty vector and the kinase-active forms of MLK3 did not (Fig.6B).

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Figure 6. MLK3 activates the JNK pathway in neurons. Shown is the MLK3-dependent phosphorylation of c-Jun in SCG neurons. SCG neurons were microinjected either with 0.3 mg/ml of an empty expression vector or the different MLK3 mutants, together with 5 mg/ml guinea pig IgG to detect the injected cells, and maintained in the presence of NGF or withdrawn from NGF as indicated. After 24 hr the cells were fixed, permeabilized, and stained with an anti-guinea pig IgG antibody (A, top) and with a specific anti-phospho-c-Jun antibody (A, bottom). Only the cells in which phospho-c-Jun staining was clearly above background were scored as positive. Arrows indicate injected cells. Scale bar, 30 µm. The results were quantified and represented as a bar graph (B). They are the mean of three independent experiments ± SEM. C, FLAG- $Delta$ 169 blocks MLK3-induced apoptosis. FLAG- $Delta$ 169 at the indicated concentrations (in mg/ml) and 0.1 mg/ml of WT MLK3 were microinjected into 5- to 7-d-old SCG neurons and maintained in the presence of NGF. The percentage of surviving cells was assessed 48 hr later. The results are the mean of three independent experiments ± SEM.

An accumulation of phosphorylated c-Jun in the nucleus should lead to the activation of the c-Jun transcriptional pathway.To investigate whether MLK3-induced apoptosis requires the activationof the c-Jun transcriptional pathway, we coinjected sympatheticneurons with WT MLK3 and FLAG- $Delta$ 169, a dominant negative mutantof c-Jun that lacks the N-terminal transactivation domain andacts as a dominant inhibitor of AP-1 activity (Ham et al., 1995).Coexpression of FLAG- $Delta$ 169 completely blocked MLK3-induced death(Fig. 6C). Taken together, these results demonstrate that theMLK3 activity is important for the induction of c-Jun phosphorylationin sympathetic neurons deprived of NGF and that the death signalinduced by MLK3 is mediated by the JNK-c-Jun transcriptionalpathway.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The Cdc42-JNK-c-Jun pathway is a crucial component of the induction of apoptosis of sympathetic neurons by growth factor deprivation(Estus et al., 1994; Ham et al., 1995; Bazenet et al., 1998).Here, we investigated the relationship between MLK3 and the activationof the Cdc42-JNK-c-Jun pathway in this paradigm. In contrast toMerritt et al. (1999), who could not detect MLK3 in neurons ofrat brain slices by immunofluorescence with the same MLK3 antibody,we found that MLK3 is expressed endogenously in rat pheochromocytomacells and SCG neurons at both mRNA (Fig. 1A) and protein levels(Fig. 1B) as well as by immunocytochemistry (data notshown).

Recently, Leung and Lassam (1998) have shown that the leucine zipper-like motifs of MLK3 are sufficient for its dimerization.In addition, they demonstrated that dimerization of MLK3 is aprerequisite for its autophosphorylation and, thereby, activation.Furthermore, Leung and Lassam (1998) found that Cdc42 led to anincrease in MLK3 dimerization, suggesting that recruitment ofMLK3 to the plasma membrane by Cdc42 might increase the localconcentration of MLK3 and therefore the chances of dimerization.To study the regulation by Cdc42 and the role of MLK3 in neurons,we constructed a series of mutants. The KD mutants have an inactivekinase domain, thereby acting as dominant negatives (Tibbles etal., 1996), and the CRIB( $-$ ) mutants can no longer bind to activatedCdc42, as shown by our immunoprecipitation studies (Fig. 2A).In the light of the above findings, dimerization should stilloccur in the kinase dead mutants, and the translocation of theCRIB-containing mutants to the membrane would be increased comparedwith the CRIB( $-$ ) ones. However, we found that neither of the KDmutants locates to the plasma membrane, whereas the mutants withan intact kinase domain [CRIB(+) and CRIB( $-$ )] do (Fig. 2B), suggestingthat autophosphorylation, but not interaction with Cdc42, is requiredfor the translocation of MLK3. We cannot exclude, however, thatoverexpression of MLK3 may override the necessity for upstreamactivators ofdimerization.

When we looked at the functional effect of these mutants on the survival of SCG neurons in the presence of NGF, we found thatoverexpression of both WT and WT CRIB( $-$ ) MLK3 dramatically increasedthe death of the neurons, whereas both the kinase dead mutantshad no effect (Fig. 3A). The MLK3-injected [WT and WT CRIB( $-$ )]neurons clearly displayed pyknotic nuclei (Figs. 2B, 3B), a hallmarkof apoptosis. In addition, zVAD-fmk, a broad caspase inhibitorthat has been shown to protect SCG neurons from NGF withdrawal(McCarthy et al., 1997), protected sympathetic neurons from MLK3-induceddeath (Fig. 3C). This supports the notion that MLK3 has a rolein the induction of apoptosis in SCG neurons. More importantly,a rapid increase in MLK3 activity was observed in both differentiatedPC12 cells and SCG neurons after NGF deprivation (Fig. 4A-C),suggesting that MLK3 may act as a physiological activator of thedeath pathway in neuronalcells.

Blocking MLK3 activity by overexpression of both MLK3 kinase dead mutants is sufficient to prevent neuronal apoptosis (Fig.5A,B), confirming the apoptotic effect of MLK3. Although it ispossible that the KD MLK3 interferes with a related kinase, becauseMLK3 can form complexes with coexpressed MLK2 or DLK (Leung andLassam, 1998; Tanaka and Hanafusa, 1998), our observations stronglysuggest a role of MLK3 in the induction of neuronalapoptosis.

Because overexpression of MLK3 has been shown to specifically activate JNK in non-neuronal cells (Teramoto et al., 1996; Tibbleset al., 1996), we investigated the effect of the MLK3 mutantson the phosphorylation of c-Jun in both the presence and absenceof NGF. We showed that overexpression of MLK3 [WT and CRIB( $-$ )]induced an increase in the phosphorylation of c-Jun and that kinasedead mutants of MLK3 [KD and KD CRIB( $-$ )] significantly blockedthe increase in the level of phosphorylated c-Jun induced by NGFwithdrawal (Fig. 6A,B). In addition, we showed that AP-1 activityis necessary for MLK3-induced apoptosis, because expression ofFLAG- $Delta$ 169, a c-Jun dominant negative mutant that inhibits AP-1activity (Ham et al., 1995), efficiently blocked MLK3-induceddeath (Fig. 6C). These results demonstrate that not only doesMLK3 mediate activation of the JNK-c-Jun transcriptional pathwaybut also, in dying SCG neurons, MLK3 activity is required forthe activation of thatpathway.

A hypothetical model, consistent with the above observations, is presented in Figure 7. We propose that NGF withdrawal leadsto the activation of Cdc42, which then activates MLK3, therebyturning on the JNK-c-Jun pathway. To test our model, we coinjectedKD and KD CRIB( $-$ ) MLK3 mutants and V12Cdc42 into SCG neurons andassessed the percentage of survival 48 hr later. Figure 5, C andD, shows that kinase dead mutants of MLK3 block apoptosis inducedby overexpression of Cdc42, suggesting that MLK3 activity is importantfor the induction of cell death by Cdc42 and acts as a downstreammediator of Cdc42 in SCG neurons. The inhibitory activity of thekinase dead MLK3 mutants is not related to sequestration of Cdc42in neurons. Consistent with this, Bock and coworkers (2000) showedthat, although Cdc42 activates MLK3, it is not necessary to maintainMLK3 in an activated state and that activation of MLK3 by Cdc42requires an additional cellular component.

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Figure 7. A model for the apoptotic signaling pathway mediated by NGF withdrawal. Removal of the survival agent, NGF, activates the small GTPase Cdc42. Activated Cdc42 leads to the activation of ASK1 and MLK3. Activation of MLK3 requires two steps: dimerization (1) and autophosphorylation (2); then it translocates to the plasma membrane. Activation of ASK1 and/or MLK3 leads to an increase in JNK activity via the formation of a multiprotein complex. Phosphorylation of c-Jun activates its transcriptional activity, which then turns on the transcription of genes that are necessary for neuronal apoptosis to proceed.

Recently, we have demonstrated that the apoptosis signal-regulating kinase (ASK1) is a crucial element of NGF withdrawal-inducedactivation of the Cdc42-c-Jun pathway and neuronal apoptosis (Kanamotoet al., 2000). ASK1 has also been found in complexes includingthe JIPs (JNK-interacting proteins) but to a much lower extentthan MLK3 (Dickens et al., 1997; Yasuda et al., 1999). The formationof such multiprotein complexes might be a convergence point ofvarious pathways mediated by ASK1 and by MLK3. This hypothesiscould explain the fact that expression of dominant negative mutantsof either kinase blocks the death pathway in neurons as they maycompete for common downstream partners. The relationship betweenASK1 and MLK3 and a mechanism of how these kinases are activatedremain to be elucidated. So we completed our model (Fig. 7) bysuggesting that both ASK1 and MLK3, or a related MLK protein,are activated after NGF withdrawal downstream of Cdc42, therebyinducing apoptosis of SCG neurons via the common activation ofthe JNKK1/2-JNK-c-Jun pathway. Blocking the activity of thesekinases could then be of therapeutic benefit in a number of neurodegenerativedisorders thought to involve neuronalapoptosis.

  FOOTNOTES

Received Dec. 29, 2000; revised April 5, 2001; accepted April 18, 2001.

We thank J. Woodgett for providing the MLK3 constructs and A. Hall for the Cdc42 plasmid. We also thank Cesare Spadoni andJonathan Whitfield for technical advice and Joanne Taylor, JimStaddon, and Stephen Neame for a critical reading of this manuscriptand helpfuldiscussions.
Correspondence should be addressed to Dr. Chantal Bazenet, Eisai London Research Laboratories, Bernard Katz Building, UniversityCollege London, Gower Street, London WC1E 6BT, UK. E-mail: Chantal_Bazenet{at}eisai.net.

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