The E2F-Cdc2 Cell-Cycle Pathway Specifically Mediates Activity Deprivation-Induced Apoptosis of Postmitotic Neurons

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The Journal of Neuroscience, March 1, 2003, 23(5):1649

The E2F-Cdc2 Cell-Cycle Pathway Specifically Mediates Activity Deprivation-Induced Apoptosis of Postmitotic Neurons
Yoshiyuki Konishi and Azad Bonni
Department of Pathology, Harvard Medical School, Boston, Massachusetts 02115

  ABSTRACT

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
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Neuronal apoptosis plays a critical role in the normal development of the mammalian brain and is thought to contribute tothe pathogenesis of several neurologic disorders. However, theintracellular mechanisms underlying apoptosis of neurons remainincompletely understood. In the present study, we characterizeda cell-cycle-based mechanism by which neuronal activity deprivationinduces apoptosis of postmitotic neurons. Activity deprivation,but not growth factor withdrawal, was found to induce Cdc2 expressionand consequent Cdc2-mediated apoptosis in granule neurons of thedeveloping rat cerebellum. We found that activity deprivationinduces cdc2 transcription in neurons via an E2F-binding element(EBE) within the cdc2 promoter. The transcription factor E2F1that is expressed in granule neurons was found in DNA bindingassays to bind to the EBE of the cdc2 gene. In chromatin immunoprecipitationanalysis, endogenous E2F1 forms a complex with the promoter ofthe endogenous cdc2 gene in granule neurons, indicating that endogenousE2F1 is poised to activate transcription of the endogenous cdc2gene in neurons. Consistent with this conclusion, a dominant interferingform of E2F, when expressed in granule neurons, blocked activitydeprivation-induced cdc2 transcription. In other experiments,we found that the expression of E2F1 in granule neurons inducesCdc2 expression and promotes neuronal apoptosis via the activationof Cdc2. Remarkably, in contrast to inducing the E2F-mediatedexpression and activation of Cdc2 in granule neurons, activitydeprivation fails to stimulate the expression of E2F-target genesthat trigger DNA synthesis and replication. Together, our findingsdefine a novel apoptotic mechanism whereby E2F selectively couplesan activity deprivation-induced signal to cdc2 transcription inthe absence of stimulating DNA synthesis and thus culminatingin Cdc2-mediated apoptosis of postmitoticneurons.

Key words: Cdc2; E2F; apoptosis; neuron; activity; transcription; cell cycle; promoter

  Introduction

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

During the development of the mammalian brain, the generation of neurons from their precursor cells coincides with their exitfrom the cell cycle (Caviness et al., 1995; McConnell, 1995).Although postmitotic neurons do not undergo cell division, theycontinue to express components of the cell cycle for some timeafter their terminal differentiation (Freeman et al., 1994; Vincentet al., 1997; Busser et al., 1998; Padmanabhan et al., 1999).Accumulating evidence suggests that these cell-cycle proteinsplay a key role in programmed cell death or apoptosis of postmitoticneurons that is critical to the normal development of the mammalianbrain (for review, see Liu and Greene, 2001a). However, the intracellularmechanisms that trigger reactivation of components of the cellcycle in postmitotic neurons remain to be elucidated. In addition,the mechanisms by which cell-cycle proteins induce apoptosis ofneurons remain incompletelyunderstood.

Within the developing brain, the cerebellar granule neuron population has been widely used to characterize the cellular andmolecular mechanisms of neuronal apoptosis. Proliferating granuleneuron precursors differentiate into postmitotic granule neuronswithin the external granule cell layer (EGL) of the developingcerebellum (Hatten and Heintz, 1995). Newly generated granuleneurons migrate from the EGL into the underlying internal granulecell layer (IGL) where they take on the properties of mature granuleneurons (Altman and Bayer, 1997). Granule neuron apoptosis isobserved in both the EGL and IGL, peaking in the first to secondweek of the postnatal rat cerebellum (Wood et al., 1993).

Granule neurons cultured from the rat cerebellum undergo apoptosis that is suppressed by neuronal activity and growth factors(D'Mello et al., 1993, 1997; Galli et al., 1995; Miller and Johnson,1996). Growth factors are typically provided by serum or by ahigh concentration of insulin that activates the insulin-likegrowth factor 1 (IGF1) receptor (Cohick and Clemmons, 1993; Alessiet al., 1996). Neuronal activity is mimicked by a high concentrationof extracellular KCl that triggers membrane depolarization leadingto the entry of calcium through voltage-sensitive calcium channels(VSCCs) (Catterall, 2000). Granule neurons undergo apoptosis whenthey are deprived of membrane-depolarizing concentrations of KClor when they are deprived of growth factors. The mechanisms bywhich activity deprivation or growth factor withdrawal inducesapoptosis are beginning to be characterized (Watson et al., 1998;Levkovitz and Baraban, 2001; Yamagishi et al., 2001; Putcha etal., 2002). An important question that remains to be addressedis whether there is specificity in the mechanisms that mediateactivity deprivation-induced or growth factor withdrawal-inducedneuronalapoptosis.

Recently, we reported that in newly differentiated cerebellar granule neurons, neuronal activity deprivation triggers theactivation of the protein kinase Cdc2, a cyclin-dependent kinasewith an established function in driving proliferating cells throughmitosis (Konishi et al., 2002). In granule neurons, activatedCdc2 mediates activity deprivation-induced apoptosis by directlyphosphorylating the BH3-only protein Bcl-2-associated death promoter(BAD) at a distinct site, serine 128, and thereby activating BAD-mediatedapoptosis (Konishi et al., 2002). Thus, reactivation of the cell-cyclecomponent Cdc2 by neuronal activity deprivation directly activatesthe cell death machinery. A major question that was raised bythese findings is: how is Cdc2 activity regulated in postmitoticneurons? In particular, how does neuronal activity deprivationinduce the activity of Cdc2 in postmitotic neurons, thereby triggeringapoptosis?

In this study, we characterized a specific mechanism by which activity deprivation induces neuronal apoptosis. We found thatactivity deprivation, but not growth factor withdrawal, inducesthe expression of Cdc2 in granule neurons, and that Cdc2 activityspecifically mediates activity deprivation-induced neuronal apoptosis.Activity deprivation was found to induce cdc2 transcription ingranule neurons via a regulatory site within the cdc2 promoterthat binds the transcription factor E2F1. In chromatin immunoprecipitationanalyses, we found that endogenous E2F1 in cerebellar granuleneurons forms a complex with the promoter of the endogenous cdc2gene, suggesting that the cdc2 gene is a target of endogenousE2F1 in cerebellar granule neurons. Consistent with this interpretation,the expression of a dominant interfering form of E2F was foundto inhibit activity deprivation-induced cdc2 transcription ingranule neurons. In other experiments, we found that the expressionof E2F1 in granule neurons induces the expression of endogenousCdc2 and triggers apoptosis. The E2F1-induced apoptosis was foundto be reduced significantly by coexpression of a dominant interferingform of Cdc2. Together, our findings define the E2F-Cdc2 cell-cyclepathway as a novel and specific mechanism by which activity deprivationinduces apoptosis of postmitotic neurons. In proliferating cells,E2F is believed to regulate the expression of a large set of genesthat drive these cells through the cell cycle (DeGregori et al.,1995; Dyson, 1998; Harbour and Dean, 2000; Ishida et al., 2001;Ren et al., 2002). In contrast, activity deprivation of granuleneurons fails to induce the set of E2F-regulated genes servinga role in DNA synthesis and replication. We conclude that thecdc2 gene represents a select target of E2F in activity-deprivedpostmitotic neurons, and that the activation of Cdc2 in the absenceof DNA synthesis in postmitotic neurons might signal apoptosisin a similar manner to unscheduled Cdc2 activation in proliferatingcells (Shi et al., 1994).

  Materials and Methods

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Antibodies. Mouse monoclonal antibodies to Cdc2 and actin and rabbit polyclonal antibody to BAD, E2F1, proliferating cellnuclear antigen (PCNA), Cdk2, and hemagglutinin (HA) were obtainedfrom Santa Cruz Biotechnology (Santa Cruz, CA). The mouse monoclonalantibody to $beta$ -galactosidase (Promega, Madison, WI) and cleavedcaspase-3 (Cell Signaling, Beverly, MA) were also purchased. Thephospho128-BAD antibody was described previously (Konishi et al.,2002).

Cerebellar granule neuron cultures and transfections. Cerebellar granule neurons were prepared as described previously (Bonniet al., 1999). One day after preparation, cytosine arabinofuranoside(AraC) (10 µM) was added to inhibit proliferation of non-neuronalcells. Transfection of granule neuron cultures was done usinga modified calcium phosphate method as described previously (Konishiet al., 2002). In the experiments in Figure 2A, 0.1 µg of cdc2-fireflyluciferase reporter plasmid and 0.02 µg of elongation factor (EF)-renillaluciferase together with 0.5 µg of carrier plasmid were transfected.In the experiments in Figure 3A, 0.1 µg of cdc2-firefly luciferaseplasmid, 0.02 µg of EF-renilla luciferase plasmid, and 1 µg ofE2F1 expression plasmid were transfected. In the experiments inFigure 3, B and C, 1 µg of green fluorescent protein (GFP) plasmid,0.25 µg of $beta$ -galactosidase expression plasmid, and 1 µg of E2F1expression plasmid were transfected. In the experiments in Figure4A-G, 2 µg of E2F1 expression plasmid was transfected. In theexperiments in Figure 4I, 0.1 µg of cdc2-firefly luciferase plasmid,0.02 µg of EF-renilla luciferase, and 0.1 µg of E2F-Rb expressionplasmid together with 0.5 µg of carrier plasmid were transfected.In the experiments in Figure 4J, 1 µg of E2F-Rb or the vectorplasmid together with 0.25 µg of $beta$ -galactosidase expression plasmidwere transfected. In the experiments in Figure 5A-E, 0.5 µg ofE2F1 expression plasmid and 0.25 µg of $beta$ -galactosidase expressionplasmid were transfected. In the experiments in Figure 5F, 0.5µg of E2F1 expression plasmid, 0.5 µg of a dominant interferingform of Cdc2 (Cdc2-DN) expression plasmid, and 0.25 µg of $beta$ -galactosidaseexpression plasmid weretransfected.

Western blot analysis. For Western blot analysis, cerebellar granule neurons were harvested with a lysis buffer containing20 mM Tris-HCl, pH 7.5, 150 mM NaCl, 1% Triton X-100, 5 mM EGTA,25 mM $beta$ -glycerophosphate, 1 mM DTT, 1 mM PMSF, 1 mM NaVO₃, andprotease inhibitors. Protein amounts were measured by a Bradfordassay. Equal amounts of proteins were separated by SDS-PAGE andtransferred to nitrocellulose membranes. Immunoblotting was performedas described previously (Bonni et al., 1999).

Immunocytochemistry. In the experiments in Figures 3, B and C, and 4A-G, cerebellar granule neurons were fixed in 4% paraformaldehydefor 20 min at room temperature. Neurons were washed twice withPBS and permeabilized with PBS containing 0.4% Triton X-100 for20 min, followed by blocking with TBS containing 0.02% Tween 20and 10% milk for 1 hr at room temperature. Primary antibody incubationswere performed at 4°C overnight in TBS containing 0.02% Tween20 and 3% bovine serum albumin. In experiments in which bromodeoxyuridine(BrdU) incorporation was measured in Figure 6A-D, cells were fixedwith a mixture of ethanol and glycine solution at $-$ 20°C for 20min. Immunocytochemistry for BrdU was performed as described inthe Labeling and Detection Kit I (Roche Diagnostics, Indianapolis,IN).

Neuronal survival and apoptosis assays. In the experiments in Figures 4J and 5, transfected cerebellar granule neurons werefixed in 4% paraformaldehyde. Indirect immunofluorescence wasperformed using an antibody to $beta$ -galactosidase to visualize transfectedneurons. Neuronal survival and apoptosis were assessed in $beta$ -galactosidase-expressingneurons based on the integrity of neurites and integrity of thenucleus as determined by the staining with DNA dye bisbenzimide(Hoechst 33258) as described previously (Konishi et al., 2002).Cell counts were performed in a blindedmanner.

Electrophoretic mobility shift assays. Electrophoretic mobility shift assays (EMSAs) were performed as described previously(Campanero et al., 1999). Nuclear extracts from cerebellar granuleneurons were prepared as described previously (Schreiber et al.,1989). The DNA probe was prepared by annealing the following oligonucleotides:5'-TTCCTCTTTCTTTCGCGCTCTAGCCACC-3' and 5'-GGGTGGGCTAGAGCGCGAAAGAAAGAGGA-3'.Nuclear extracts of cerebellar granule neurons (5 µg) were incubatedin 10 µl of a preincubation mixture containing 20 mM HEPES/KOH,pH 7.9, 20% glycerol, 0.1 M KCl, 0.2 mM EDTA, 0.5 mM DTT, and0.2 µg of sheared herring sperm DNA for 30 min on ice. After preincubation,0.1 ng of the radiolabeled probe was added to the reaction mixtureand incubated for 30 min on ice. In competition assays, cold wild-typeE2F-binding element (EBE) probe or a mutant EBE probe in whichCG (underlined in the sequence above) was replaced by AT was addedto the preincubation mixture. For reactions including antibodies,rabbit antibody that recognizes E2F1 specifically or a controlrabbit anti-HA antibody was added to the preincubation mixture.DNA-protein complexes were analyzed on a 4% polyacrylamide-0.1%bisacrylamide nondenaturing gel in 0.5% Tris-borate-EDTA at 4°C.The gel was dried and analyzed byautoradiography.

Chromatin immunoprecipitation assays. Chromatin immunoprecipitation assays were performed as described previously (Takahashiet al., 2000; Rayman et al., 2002). Approximately 4.5 × 10⁷ cerebellar granule neurons were used in each reaction. Chromatinprepared from granule neurons was precipitated using 4 µg of rabbitantibody that recognizes E2F1 specifically or control anti-HAantibody together with protein A-Sepharose at 4°C overnight. Precipitatedchromatin was treated with proteinase K and RNase A at 55°C for3 hr followed by overnight incubation at 65°C to reverse cross-linking.Primers used for PCR that anneal to the rat cdc2 promoter in aregion encompassing the EBE were designed as follows: 5'-CTGAGCTCAAGAGTCAGTTGGCG-3'and 5'-CGCCAATCCGATTGCACGTAGAC-3'. PCRs were performed using 1/20thof chromatin precipitates. PCR products were labeled with [ $alpha$ ³²-P]dCTP and detected by autoradiography. Experiments were performedthree times using chromatin that was preparedindependently.

  Results

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Cdc2 specifically mediates activity deprivation-induced granule neuron apoptosis

We recently characterized the Cdc2-BAD signaling pathway as a novel apoptotic mechanism that is activated in newly generatedcerebellar granule neurons with the suppression of neuronal activity(Konishi et al., 2002). Because common signaling mechanisms typicallymediate apoptosis of neurons during trophic factor withdrawal,we tested whether the Cdc2-BAD apoptotic pathway is also activatedin neurons during growth factorwithdrawal.

Cerebellar granule neurons were prepared from postnatal day 6 (P6) rat pups and cultured in the presence of serum and highconcentrations of KCl (30 mM) that induce membrane depolarizationand consequent activation of VSCCs. We first characterized theactivation of the Cdc2-BAD pathway in activity-deprived granuleneurons. After 2 d in vitro (DIV), granule neuron cultures (P6plus 2 DIV) were placed in survival medium [Basal Medium Eagle(BME) plus 30 mM KCl plus serum] or were deprived of membrane-depolarizingconcentrations of KCl (BME plus 5 mM KCl plus serum). After 24hr, cultures were subjected to Western blot analysis using anantibody to Cdc2, an antibody that recognizes the serine 128 phosphorylatedform of BAD specifically (phospho128-BAD antibody), or an antibodythat recognizes BAD regardless of its phosphorylation state (N-20BAD antibody). Activity deprivation induced the expression ofendogenous Cdc2 protein and induced the phosphorylation of endogenousBAD at serine 128 in granule neurons (Fig. 1A, lanes 1 and 2)(Konishi et al., 2002).

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Figure 1. Cdc2 specifically mediates activity deprivation-induced apoptosis of cerebellar granule neurons. A, Lysates of granule neuron cultures (P6 plus 2 DIV) that were in survival medium [30 mM KCl plus serum, lane 1; 30 mM KCl plus insulin (Ins), lane 3)], that were deprived of KCl (5 mM KCl plus serum, lane 2), or that were deprived of growth factors (30 mM KCl, lane 4) for 24 hr were immunoblotted with a mouse monoclonal antibody that recognizes Cdc2 (top), the rabbit phospho128 (P128)-BAD antibody (middle), or an antibody that recognizes BAD regardless of its phosphorylation (bottom). Activity withdrawal significantly induced the expression of Cdc2 (1.4 ± 0.1 fold; n = 3; p < 0.001; ANOVA) and the phosphorylation of BAD at serine 128 (1.9 ± 0.1 fold; n = 3; ANOVA; p < 0.001), but insulin withdrawal failed to induce Cdc2 expression (0.8 ± 0.1 fold; n = 3) or to induce the BAD serine 128 phosphorylation (1.1 ± 0.2 fold; n = 3). B, Cerebellar granule neurons (P6 plus 2 DIV) were kept in survival medium (30 mM KCl plus serum, left; 30 mM KCl plus insulin, right) or were deprived for 48 hr of KCl (5 mM KCl plus serum, left) or insulin (30 mM KCl, right) in the presence of the Cdc2 inhibitor roscovitine (Rosc; 10 µM) or its vehicle [dimethylsulfoxide (DMSO)]. Roscovitine inhibited neuronal activity deprivation-induced apoptosis (mean ± SEM; n = 3; ANOVA; p < 0.01) but not growth factor withdrawal-induced apoptosis. C, Lysates of cerebellar granule neurons (P6 plus 2 DIV) that were treated as in B in the presence of DMSO (D) or roscovitine (R) were immunoblotted using an antibody to the cleaved form of caspase-3 (top) or an antibody that recognizes actin (bottom) to serve as control for equal protein loading. D, Lysates of cerebellar granule neurons that were placed in full medium (30 mM KCl plus serum) or deprived of KCl (5 mM KCl plus serum) for the indicated times were immunoblotted with the antibody to Cdc2 (top) or the antibody to actin (bottom). E, Northern blot analysis of total RNA from cerebellar granule neuron cultures that had either been maintained in full medium (30 mM KCl plus serum, lanes 1 and 2) or deprived of activity (5 mM KCl plus serum, lanes 3 and 4) for 24 hr. RNA was subjected to Northern blot analysis using a cdc2 probe (top) or glyceraldehyde-3-phosphate dehydrogenase (GAPDH; bottom).

We next tested whether growth factor withdrawal also induces Cdc2 expression and BAD serine 128 phosphorylation in neurons.Activation of the IGF1 receptor by a high concentration of insulin(10 µg/ml) in granule neurons provides a prototypical growth factor-inducedsurvival signal in granule neurons (D'Mello et al., 1993; Dudeket al., 1997). P6 plus 2 DIV granule neurons were placed in survivalmedium (BME plus 30 mM KCl plus insulin) or were deprived of growthfactor signaling (BME plus 30 mM KCl). Surprisingly, we foundthat growth factor withdrawal failed to induce the expressionof Cdc2 and failed to induce the phosphorylation of BAD at serine128 (Fig. 1A, lanes 3 and 4).

In assays of cell survival, inhibition of Cdc2 activity by roscovitine protected cerebellar granule neurons from activitydeprivation-induced apoptosis (Fig. 1B) (Konishi et al., 2002)but failed to protect granule neurons against growth factor withdrawal-inducedapoptosis (Fig. 1B), suggesting that Cdc2 is not required forgrowth factor withdrawal-induced neuronal apoptosis. In otherexperiments, both activity deprivation and growth factor withdrawaltriggered the accumulation of the cleaved product of the proteasecaspase-3 that reflects caspase-3 activation (Fig. 1C) (Di Cuntoet al., 2000). However, consistent with results of the cell-survivalassays, although the inhibition of Cdc2 by roscovitine inhibitedactivity deprivation-induced caspase-3 cleavage, roscovitine failedto inhibit growth factor withdrawal-induced caspase-3 cleavage(Fig. 1C). We also found that expression of Cdc2-DN that blocksactivity deprivation-induced neuronal apoptosis (van den Heuveland Harlow, 1993; Konishi et al., 2002) failed to inhibit granuleneuron apoptosis after insulin withdrawal (data not shown). Together,these results indicate that activity deprivation selectively inducesthe Cdc2-BAD apoptotic pathway and that Cdc2 promotes apoptosisspecifically after neuronal activity deprivation but does notmediate growth factor withdrawal-induced apoptosis of cerebellargranuleneurons.

Activity deprivation induces cdc2 transcription in granule neurons via an E2F-binding element within the cdc2 promoter

Having identified the Cdc2-BAD pathway as a specific mediator of activity deprivation-induced neuronal apoptosis, we focusedour attention on the characterization of the mechanism by whichactivity deprivation induces the expression and consequent activationof Cdc2 in granule neurons. We performed a kinetic analysis ofactivity deprivation-induced Cdc2 protein expression in granuleneurons, and found that the induction of Cdc2 protein was notapparent in the first 12 hr but became evident 24 hr after KClwithdrawal (Fig. 1D). The elevated levels of Cdc2 were maintainedthereafter at 48 and 72 hr after the KCl withdrawal (see Fig.6) (data not shown). The kinetics of activity deprivation-inducedCdc2 expression is characteristic of a late response gene. Todistinguish between the two major possibilities that activitydeprivation induction of Cdc2 occurs via a mechanism that is predominantlyat the level of protein turnover or translation or at the levelof transcription or mRNA processing, we characterized the effectof activity deprivation on the amount of cdc2 mRNA in granuleneurons. We found that the expression of cdc2 mRNA was robustlyinduced in granule neurons 24 hr after KCl withdrawal (Fig. 1E).Together, these results suggest that activity deprivation inducesthe expression of Cdc2 via an alteration in cdc2 transcriptionor mRNAturnover.

We next determined whether activity deprivation regulates cdc2 expression at the transcriptional level. In transient transfectionexperiments in granule neurons, we tested the effect of activitydeprivation on the activity of a luciferase reporter gene thatcontains 3.2 kb of the 5' regulatory sequence of the cdc2 gene( $-$ 3200/cdc2) (Sugarman et al., 1995). We found that KCl withdrawalrobustly stimulated the expression of the $-$ 3200/cdc2-luciferasereporter gene in granule neurons (Fig. 2A). These results suggestthat activity deprivation stimulates Cdc2 expression by inducingcdc2 transcription.

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Figure 2. Activity deprivation induces cdc2 transcription via an EBE within the cdc2 promoter. A, Schematic representation of cdc2 promoter-luciferase reporter constructs and their activity in cerebellar granule neurons. Cerebellar granule neurons (P6 plus 2 DIV) were transfected with the indicated cdc2 firefly-luciferase reporter plasmid and reporter gene that is controlled by the elongation factor promoter (EF-renilla) and incubated for 4-5 hr in conditioned full medium (30 mM KCl plus serum). Transfected neurons were then placed in full medium (30 mM KCl plus serum; black bars) or deprived of neuronal activity (5 mM KCl plus serum; gray bars) for 36 hr and then subjected to dual-luciferase assay (Promega). The normalized firefly-luciferase activity of each cdc2 luciferase reporter gene is shown relative to the activity of $-$ 94/cdc2 luciferase gene in membrane-depolarized granule neuron cultures. Values shown are mean ± SEM (n = 4). Activity deprivation significantly increased the expression of the $-$ 3200/cdc2 and $-$ 245/cdc2 reporter genes (ANOVA; p < 0.05) but not of the $-$ 245mEBE/cdc2 or the $-$ 94/cdc2 reporter genes. B, Nuclear extracts prepared from cerebellar granule neuron cultures (P6 plus 2 DIV) maintained in full survival medium (30 mM KCl plus serum) or deprived of neuronal activity (5 mM KCl plus serum) for 24 hr were subjected to an EMSA. The radiolabeled probe contains the EBE within the cdc2 promoter. For competition analysis, excess amount of wild-type cold probe (lanes 4 and 5) or a probe that contains a point mutation within the EBE (lanes 6 and 7) was added to the reaction. C, A rabbit antibody to E2F1 (2 µg, lane 3; 5 µg, lane 4) or a control antibody (anti-HA antibody, 2 µg, lane 5; 5 µg, lane 6) was added to the EMSA reaction. Three protein-DNA complexes that are shown as specific EBE-protein complexes in B (arrowheads) were blocked or super-shifted (bracket) by the addition of E2F1 antibody but not by control antibody.

Deletion analysis of the cdc2 promoter in granule neurons revealed that the region of the promoter between nucleotide $-$ 245and nucleotide $-$ 94 relative to the transcriptional start siteof the cdc2 gene plays a critical role in activity withdrawal-inducedcdc2 transcription. The basal level of cdc2 promoter-mediatedtranscription in membrane-depolarized granule neurons was notaffected by the 5' deletion mutants (Fig. 2A). These results argueagainst the interpretation that activity deprivation in granuleneurons triggers the derepression of the cdc2 promoter. Rather,these results suggest that activity deprivation induces the activityof a transcription factor that stimulates cdc2 transcription ingranuleneurons.

We next focused our effort on identifying the site within the $-$ 245 to $-$ 94 region of the cdc2 promoter that mediates activitydeprivation-induced cdc2 transcription. This region of the cdc2promoter contains an EBE at $-$ 128 that is conserved in the ratand human cdc2 genes. The EBE plays an important role in mediatingcdc2 transcription in proliferating cells (Dalton, 1992; Shimizuet al., 1995). We therefore asked whether the EBE might mediatecdc2 transcription in the postmitotic granule neurons after KClwithdrawal. We found that mutation of the EBE within the contextof the $-$ 245/cdc2 reporter gene reduced significantly the abilityof KCl withdrawal to induce cdc2 promoter-mediated transcription(Fig. 2A). These results suggest that the EBE within the cdc2promoter plays a critical role in mediating activity deprivation-inducedcdc2transcription.

Members of the E2F family of transcription factors bind the EBE in proliferating cells (Tommasi and Pfeifer, 1995; Takahashiet al., 2000; Rayman et al., 2002). We therefore tested whetherthe EBE within the cdc2 promoter binds to an E2F family memberin granule neurons. In EMSAs, the EBE formed protein-DNA complexeswhen incubated with nuclear extracts of cerebellar granule neurons(Fig. 2B). The incubation of excess cold wild-type EBE in theDNA binding reaction, but not of mutant EBE known to disrupt itsbinding to E2Fs, reduced partly or completely the formation ofthree protein-DNA complexes (Fig. 2B, arrowheads). These resultssuggest that the EBE within the cdc2 promoter binds E2F transcriptionfactors that are present in nuclear extracts of granule neurons.The three EBE-protein complexes were disrupted or supershiftedwith the addition of an antibody that recognizes E2F1 specifically(Fig. 2C, bracket), but not by a control antibody. There was anincreased amount of EBE-binding activity in nuclear extracts ofactivity-deprived granule neurons (Fig. 2B), suggesting that activitydeprivation stimulates the activity of endogenous E2F1 in neurons.These data suggest that granule neurons express E2F1 that bindsto the EBE within the cdc2 promoter and raised the possibilitythat E2F1 might mediate activity deprivation-induced cdc2 transcriptionin cerebellar granuleneurons.

E2F mediates activity deprivation-induced cdc2 transcription in postmitotic granule neurons

The finding that the EBE of the cdc2 promoter binds to E2F1 and mediates activity deprivation-induced cdc2 transcription ledus next to address the question of whether E2F mediates activitydeprivation-induced cdc2 transcription in cerebellar granule neurons.First, we asked whether E2F1 has the capacity to induce cdc2 transcriptionin granule neurons, which are in a postmitotic state. We imaginedthat E2F1 that is expressed in membrane-depolarized granule neuronsis maintained in a repressed state to prevent the induction ofcdc2 and of genes that might trigger reentry of neurons into thecell cycle. Therefore, to investigate the ability of E2F1 to inducetranscription of the cdc2 gene in granule neurons, we overexpressedE2F1 in granule neurons together with the cdc2-luciferase ( $-$ 245/cdc2)reporter plasmid. We found that overexpressed E2F1 strongly enhancedcdc2 promoter-mediated transcription (Fig. 3A). In contrast towild-type E2F1, a mutant E2F1 that is unable to bind to the EBEbecause of an amino acid substitution within the DNA binding domainof E2F1 [E2F1(132E)] (Johnson et al., 1993) failed to induce thecdc2 promoter effectively (Fig. 3A). In addition, mutation ofthe EBE within the cdc2 promoter ( $-$ 245mEBE/cdc2) significantlyinhibited E2F1-dependent transcriptional activation of the cdc2promoter, arguing against the interpretation that E2F1-inducedcdc2 transcription occurs via the squelching of transcriptionalcorepressors or through a mechanism that is independent of E2Fbinding to the cdc2 promoter. Together, these results demonstratethe ability of E2F1 to induce cdc2 transcription in granule neuroncultures.

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Figure 3. E2F1 activates cdc2 promoter-mediated transcription in postmitotic cerebellar granule neurons. A, Cerebellar neuron cultures (P6 plus 2 DIV) were transfected with the $-$ 245/cdc2 or $-$ 245/mEBE/cdc2 luciferase reporter plasmids together with the EF-renilla reporter gene and an expression plasmid encoding E2F1, an E2F1 mutant in which the DNA-binding domain is mutated [E2F1(132E)], or their control vector. One day after transfection, transfected cells were harvested and subjected to a dual-luciferase assay. Normalized reporter activities are shown relative to the reporter activity of the $-$ 245/cdc2 luciferase gene that was cotransfected with the vector control plasmid. Values shown are mean ± SEM (n = 4). The activity of the $-$ 245/cdc2 reporter gene was significantly increased by E2F1 (ANOVA; p < 0.001) but not by E2F1(132E). Mutation within the EBE ( $-$ 245/mEBE/cdc2) significantly decreased E2F1 induction of cdc2 transcription (ANOVA; p < 0.001). B, Cerebellar granule neurons were transfected with the control GFP, cdc2/GFP reporter gene, or CMV/GFP reporter gene together with an expression plasmid encoding E2F1 or its control vector and an expression plasmid encoding $beta$ -galactosidase ( $beta$ -gal). Two days after transfection, cells were subjected to indirect immunofluorescence with an antibody to $beta$ -galactosidase, and GFP reporter gene activity was monitored by visualizing GFP in transfected cells. E2F1 induced the cdc2/GFP reporter. C, Cerebellar granule neuron cultures were transfected with the E2F1-expression vector together with the cdc2/GFP reporter gene. Transfected cultures were subjected to indirect immunofluorescence with an antibody to $beta$ -tubulin type III (Tuj1) that is expressed in postmitotic neurons, and GFP visualization was used to monitor the cdc2/GFP reporter activity. Cell bodies (arrowheads) and neurites (open arrows) of all GFP-positive cells also stained with the Tuj1 antibody.

Granule neuron cultures contain >95% granule neurons, and the introduction of plasmids into these cultures in our transfectionstargets granule neurons selectively, because 99% of transfectedcells are granule neurons (Konishi et al., 2002). Nevertheless,because E2F-mediated transcription might be much more effectivein non-neuronal cells, we investigated the possibility that E2F1induction of cdc2 transcription in our experiments might arisepredominantly from cdc2 promoter activity in the non-neuronalcells. We therefore generated a construct in which the GFP reportergene is driven by the cdc2 promoter (cdc2/GFP) (Fig. 3B). We transfectedcerebellar granule neuron cultures with a GFP, cdc2/GFP, or cytomegalovirus(CMV)/GFP reporter gene together with an expression plasmid encoding $beta$ -galactosidase. Cultures were fixed 2 d after transfection andsubjected to indirect immunofluorescence using a mouse monoclonalantibody to $beta$ -galactosidase. The activity of the cdc2 promoterwas monitored by visualizing GFP fluorescence. In the absenceof E2F1, the activity of GFP was very weak and near backgroundfluorescence levels. In contrast, the expression of E2F1 stronglyinduced the cdc2/GFP reporter gene but had little effect on thecontrol GFP reporter or CMV/GFP reporter gene (Fig. 3B). In otherexperiments, we found that the cells that expressed the E2F1-inducedcdc2 promoter-mediated GFP also expressed the neuron specific $beta$ -tubulin type III (Fig. 3C). Together, these results establishthat E2F1 possesses the capacity to activate cdc2 promoter-mediatedtranscription in postmitotic cerebellar granuleneurons.

We next examined whether E2F1 has the ability to induce transcription of the endogenous cdc2 gene in cerebellar granule neurons.We transfected cerebellar granule neurons with an expression plasmidencoding HA-tagged E2F1 or HA-tagged E2F1(132E). Two days aftertransfection, granule neurons were subjected to indirect immunofluorescenceusing a rabbit antibody to HA and a mouse monoclonal antibodyto Cdc2. Robust endogenous Cdc2 immunoreactivity was detectedin granule neurons in which wild-type E2F1 was expressed (Fig.4A-C). In contrast, we detected weak endogenous Cdc2 immunoreactivityin E2F1(132E)-expressing granule neurons (Fig. 4D-F). The percentageof strong Cdc2-positive granule neurons was quantified and revealedthat strong endogenous Cdc2 was detected in a large fraction (82%)of E2F1-expressing granule neurons but only in 10% of E2F1(132E)-expressinggranule neurons (Fig. 4G). These results suggest that the expressionof E2F1 stimulates endogenous Cdc2 expression in cerebellar granuleneurons.

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Figure 4. E2F1 mediates activity deprivation-induced cdc2 transcription and apoptosis in cerebellar granule neurons. A-F, Cerebellar granule neurons (P6 plus 2 DIV) were transfected with an expression plasmid encoding HA-tagged E2F1 or HA-tagged E2F1(132E). Two days after transfection, cultures were subjected to indirect immunofluorescence using a rabbit anti-HA antibody and the mouse monoclonal antibody to Cdc2 together with the DNA dye bisbenzimide (Hoechst 33258) to reveal cell nuclei. Arrowheads indicate HA-E2F1- or HA-E2F1(132E)-expressing neurons. G, Quantification of experiments in A-F showing the percentages of E2F1- or E2F1(132E)-expressing neurons that exhibit high endogenous Cdc2 immunoreactivity. The percentage of transfected neurons with high Cdc2 immunoreactivity was significantly higher in E2F1-expressing neurons than in E2F1(132E)-expressing neurons (mean ± SEM; n = 3; p < 0.001; t test). H, Chromatin immunoprecipitation from cerebellar granule neuron cultures using no antibody (lane 1), a rabbit antibody to HA to serve as a control (lane 2), and an antibody against E2F1 (lane 3). Precipitated chromatin was subjected to PCR analysis using a set of primers encompassing the EBE within the cdc2 promoter (as shown in the figure). Endogenous cdc2 promoter was specifically coprecipitated with immunoprecipitated E2F1 (lane 3). I, Cerebellar granule neurons (P6 plus 2 DIV) were transfected with the $-$ 3200/cdc2-luciferase reporter plasmid together with a control vector or an expression plasmid encoding the dominant interfering form of E2F (E2F-Rb), in which the E2F1 DNA-binding region (1-368) was fused to Rb (379-972). Transfected cultures were processed as in Figure 2A. Activity deprivation induced cdc2 promoter-mediated transcription in vector-transfected (mean ± SEM; n = 4; ANOVA; p < 0.0001) but not in E2F-Rb-expressing granule neurons. J, Cerebellar granule neurons (P6 plus 2 DIV) were transfected with the E2F-Rb expression plasmid or the control vector together with an expression plasmid encoding $beta$ -galactosidase. One day after transfection, granule neurons were placed in full medium (30 mM KCl plus serum) or deprived of neuronal activity (5 mM KCl plus serum) for 2 d. Transfected neurons were subjected to indirect immunofluorescence using the monoclonal antibody to $beta$ -galactosidase and the DNA dye bisbenzimide (Hoechst 33258). Cell survival and death were measured in $beta$ -galactosidase-expressing neurons based on the integrity of neurites and nucleus. KCl withdrawal significantly reduced the survival of vector-transfected granule neurons (n = 3; ANOVA; p < 0.05) but not of E2F-Rb-expressing granule neurons.

We next characterized the role of endogenous E2F in mediating cdc2 expression in activity-deprived cerebellar granule neurons.To examine whether endogenous E2F might mediate transcriptionof the endogenous cdc2 gene, we performed chromatin immunoprecipitationanalysis. Chromatin was prepared from cerebellar granule neuronsand was immunoprecipitated using no antibody, a control antibody,or an anti-E2F1 antibody together with protein A-Sepharose beads.Immunoprecipitated chromatin was subjected to PCR using primersdesigned to anneal to the cdc2 promoter in a region encompassingthe EBE (Fig. 4H). We found that the endogenous cdc2 promoterwas coprecipitated with endogenous E2F1 (Fig. 4H). The resultsof control experiments using no antibody or control antibody supportedthe interpretation that the endogenous cdc2 promoter and endogenousE2F1 coprecipitated specifically (Fig. 4H). These results suggestthat the endogenous cdc2 gene is a target of endogenous E2F1 inpostmitotic neurons. Next, we tested the effect of a dominantinterfering form of E2F, in which the DNA-binding domain of E2F1was fused to the repressor Rb (E2F-Rb) (Sellers et al., 1995,1998), on the ability of KCl withdrawal to induce the cdc2 promoterin cerebellar granule neurons. E2F-Rb is expected to inhibit endogenousE2F proteins by blocking their ability to induce transcription(Sellers et al., 1995, 1998). We found that E2F-Rb, when coexpressedwith the $-$ 3200/cdc2-luciferase reporter gene, abolished KCl withdrawalinduction of the cdc2 promoter (Fig. 4I). Together with the findingof chromatin immunoprecipitation experiments, these results suggestthat endogenous E2F mediates neuronal activity deprivation-dependentcdc2transcription.

The E2F-cdc2 cell-cycle pathway promotes granule neuron apoptosis

Our results suggesting that E2F1 mediates activity deprivation-induced cdc2 transcription raised the question of whether E2F1and Cdc2 lie on a biochemical pathway that mediates activity deprivation-inducedapoptosis of neurons. E2F1 has been demonstrated to promote apoptosisin postmitotic neurons including cerebellar granule neurons (O'Hareet al., 2000; Gendron et al., 2001; Liu and Greene, 2001b). Consistentwith these observations, we found that the dominant interferingform of E2F (E2F-Rb), when expressed in granule neurons, blockedthe ability of KCl withdrawal to induce apoptosis (Fig. 4J), suggestingthat endogenous E2F proteins mediate activity deprivation-inducedapoptosis ofneurons.

The molecular mechanisms by which E2F1 promotes apoptosis remain to be elucidated. Because activity deprivation induces E2F-mediatedcdc2 transcription (this study) and because the activity of Cdc2promotes granule neuron apoptosis (Konishi et al., 2002), we askedwhether the proapoptotic function of E2F1 in cerebellar granuleneurons is mediated via the induction and activation of Cdc2.We first established that the expression of E2F1 induces granuleneuron apoptosis in our cultures. Granule neurons were transfectedwith an E2F1 expression plasmid or the control vector and werethen maintained in full medium or deprived of membrane-depolarizingconcentrations of KCl for just 24 hr to obtain a negligible amountof activity withdrawal-induced apoptosis in vector-transfectedcultures to allow the detection of apoptosis on E2F1 overexpression(Fig. 5A). Although the expression of E2F1 induced apoptosis inmembrane-depolarized cultures, E2F1-mediated apoptosis was moremarked in cultures that were deprived of depolarizing concentrationsof KCl (Fig. 5A-E), suggesting that activity deprivation furtheractivates the ability of E2F1 to induce apoptosis or that additionalactivity deprivation-induced mechanisms cooperate with E2F1 toinduce apoptosis. The expression of the mutant E2F1 protein [E2F1(132E)],that poorly binds to the EBE, failed to effectively induce neuronalapoptosis, suggesting that the binding of E2F1 to the promoterof responsive genes is necessary for E2F1 to stimulate transcriptionof apoptotic genes and thereby trigger apoptosis. We next askedwhether Cdc2 might constitute an apoptotic gene target of E2F1in granule neurons. We determined whether the inhibition of Cdc2activity rescues granule neurons from E2F1-induced apoptosis.We found that a dominant interfering form of Cdc2 in which anamino acid is mutated in the catalytic region (Cdc2-DN), whencoexpressed with E2F1 in granule neurons, significantly reducedE2F1-induced apoptosis (Fig. 5F). These results indicate thatCdc2 is functionally downstream of E2F1, and that the E2F-Cdc2cell-cycle pathway thus provides an apoptotic signal in postmitoticneurons.

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Figure 5. Cdc2 mediates E2F1-induced neuronal apoptosis. A, Cerebellar granule neurons (P6 plus 2 DIV) were transfected with the expression plasmid encoding E2F1, E2F1(132E), or their control vector together with an expression plasmid encoding $beta$ -galactosidase. One day after transfection, granule neurons were placed in full medium (30 mM KCl plus serum) or deprived of neuronal activity (5 mM KCl plus serum) for 24 hr. Transfected neurons were subjected to indirect immunofluorescence and cell survival assays as in Figure 4J. The expression of E2F1 significantly reduced the survival of cerebellar granule neurons [mean ± SEM; n = 3; ANOVA; p < 0.05 (30 mM KCl), p < 0.005 (5 mM KCl)]. However, E2F1(132E) had little effect on the survival of cerebellar granule neurons. B-E, Representative images of cerebellar granule neurons transfected with the control vector (B, C) or the E2F1 expression plasmid (D, E). In the vector control, several healthy neurons appear (closed arrowheads), whereas several E2F1-transfected neurons are undergoing apoptosis (open arrowheads). F, Cerebellar granule neurons were transfected with the E2F1 expression plasmid together with Cdc2-DN or its vector control together with the $beta$ -galactosidase expression plasmid. Transfected neurons were deprived of neuronal activity (5 mM KCl plus serum) for 24 hr and subjected to indirect immunofluorescence and cell survival assay as in Figure 4J. Cdc2-DN significantly reduced E2F1-induced apoptosis (mean ± SEM; n = 4; ANOVA; p < 0.01).

The similarity in the ability of E2F1 to induce cdc2 in both postmitotic and proliferating cells raised the question of theextent of similarity in the regulation of E2F1 function in twocell types. In proliferating cells, E2F1 regulates the expressionof a large set of genes that promote DNA synthesis and replication(DeGregori et al., 1995; Dyson, 1998; Harbour and Dean, 2000;Ishida et al., 2001; Ren et al., 2002). We therefore asked whetherthe activation of the E2F-Cdc2 cell-cycle pathway in activity-deprivedgranule neurons also leads to the induction of genes that servea role in DNA synthesis. We determined whether activity deprivationstimulates DNA synthesis in granule neurons. Cerebellar granuleneuron cultures were incubated with bromodeoxyuridine for 24 hr.As expected, non-neuronal cells incorporated BrdU. However, wefailed to detect BrdU-positive neurons in these cultures. Theseresults indicate that despite the activation of the E2F-Cdc2 cell-cyclepathway in neurons on activity deprivation, the DNA synthesismachinery is not activated in granule neurons (Fig. 6A-D). Consistentwith this conclusion, we found that although activity deprivationinduced Cdc2 expression, activity deprivation failed to inducethe expression of the DNA-synthesis related factors PCNA and Cdk2in granule neurons (Fig. 6E). Together, our results suggest thatactivity deprivation induces the E2F-mediated expression of Cdc2in neurons but fails to induce E2F-regulated genes that turn onthe DNA synthesis machinery. The activation of the mitotic kinaseCdc2 in postmitotic neurons in the absence of DNA synthesis maythus comprise the trigger for apoptosis.

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Figure 6. Activity deprivation does not stimulate DNA synthesis in cerebellar granule neurons. A-D, Cerebellar granule neuron cultures (P6 plus 2 DIV) were labeled with BrdU for 24 hr in cultures that were in full medium (30 mM KCl plus serum) or that were deprived of activity (5 mM KCl plus serum) in the presence or absence of the antimitotic agent AraC. Incorporated BrdU was detected by immunofluorescence using a mouse monoclonal antibody that recognizes BrdU. Postmitotic granule neurons in culture were identified using a rabbit antibody that recognizes microtubule-associated protein 2 (MAP2). MAP2-negative non-neuronal cells incorporated BrdU in the absence of AraC, whereas postmitotic granule neurons did not incorporate BrdU in the presence or absence of AraC. E, Lysates of cerebellar granule neurons (P6 plus 2 DIV) that were placed in full medium or deprived of activity for 24 or 48 hr were subjected to immunoblotting using an antibody to PCNA, Cdk2, Cdc2, or actin. Activity deprivation induced the level of Cdc2 protein but failed to induce the expression of PCNA or Cdk2.

  Discussion

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

In this study, we have characterized a cell-cycle mechanism that specifically mediates activity deprivation-induced apoptosisof postmitotic neurons. We have found that the mitotic kinaseCdc2 mediates apoptosis of cerebellar granule neurons with thedeprivation of neuronal activity but not with growth factor withdrawal.Activity deprivation induces the expression of Cdc2, leading toCdc2-mediated neuronal apoptosis, by stimulating transcriptionof the cdc2 gene in granule neurons. An EBE within the cdc2 promoterwas found to bind to E2F1 and mediate activity deprivation-inducedcdc2 transcription in granule neurons. We found that endogenousE2F1 in granule neurons occupies the promoter of the endogenouscdc2 gene in chromatin-immunoprecipitation analysis. Consistentwith these results, we also found that inhibition of E2F proteinby a dominant interfering form of E2F blocks activity deprivation-inducedcdc2 transcription. In other experiments, we found that the expressionof E2F1 in granule neurons induces the expression of Cdc2, whichin turn mediates E2F1-induced apoptosis. Finally, although activitydeprivation induces the E2F-mediated expression of Cdc2 in granuleneurons, activity deprivation in neurons fails to induce the expressionof genes that drive DNA synthesis and replication. Together, ourfindings define E2F-Cdc2 as a novel cell-cycle pathway in postmitoticneurons that selectively propagates an apoptotic signal duringneuronal activitydeprivation.

A role for reactivation of the cell-cycle machinery in apoptosis of postmitotic neurons was suggested nearly a decade ago(for review, see Liu and Greene, 2001a). However, the regulationof the cell-cycle machinery in postmitotic neurons and the mechanismsby which cell-cycle activation mediates neuronal apoptosis arejust beginning to be elucidated. One of the early observationsin this field was the finding that the withdrawal of nerve growthfactor (NGF) from sympathetic neurons induces the expression ofcyclin D1 expression in these neurons (Freeman et al., 1994).This observation was extended to a number of paradigms of neuronalapoptosis, including activity deprivation of cerebellar granuleneurons and the exposure of neurons to DNA-damaging agents andother pathogenic stimuli (Park et al., 1997, 1998; Padmanabhanet al., 1999). In these studies, the induction of cyclin D1 wasfound to lead to the activation of D1-associated cdk4/6, and inhibitionof these kinases protected neurons against apoptosis (Park etal., 1997, 1998; Padmanabhan et al., 1999).

As in proliferating cells, an important target of CDK4/6 in neurons is the protein Rb. The CDK4/6-induced phosphorylationof Rb is thought to control the G₁-S transition in proliferatingcells (Weinberg, 1995). During the early G₁ phase of the cellcycle, hypophosphorylated Rb binds to the transcription factorE2F and thereby represses E2F-mediated transcription (Chellappanet al., 1991; Dyson, 1998). However, the CDK-induced phosphorylationof Rb induces the derepression and transactivation of E2F-regulatedgenes leading to cell-cycle progression (Harbour et al., 1999).In postmitotic neurons, the CDK4/6-induced phosphorylation ofRb and consequent disinhibition of E2F have been linked to neuronalapoptosis in a number of settings including activity withdrawal-inducedapoptosis of granule neurons (Padmanabhan et al., 1999; O'Hareet al., 2000).

The mechanisms by which E2F mediates apoptosis of postmitotic neurons are beginning to be characterized. In a recent studyby Liu and Greene (2001b), the repression of E2F-responsive geneswas demonstrated to be required for neuronal survival. In thisstudy, NGF withdrawal in sympathetic neurons and chemotoxin stimulationof cortical neurons was demonstrated to trigger the derepressionof E2F-regulated genes leading to apoptosis (Liu and Greene, 2001b).It was also suggested in this study that transactivation of E2F-responsivegenes is not required for neuronal apoptosis (Liu and Greene,2001b).

In our study, we show that the transactivation function of E2F leads to the induction of Cdc2 expression and apoptosis incerebellar granule neurons with activity deprivation. Our findingsprovide a novel link in neurons between the activity deprivation-inducedG₁ CDK-Rb-E2F1 pathway and the mitotic kinase Cdc2 culminatingin the direct activation of the cell-death machinery via phosphorylationof the BH3-only protein BAD. We have found that activity deprivationbut not growth factor withdrawal induces the expression of Cdc2.Consistent with this result, we found that Cdc2 mediates activitydeprivation-induced but not growth factor withdrawal-induced neuronalapoptosis. We also found that E2F1 triggers apoptosis of cerebellargranule neurons, and that E2F1-induced Cdc2 mediates the abilityof E2F1 to promote apoptosis. Together, these findings suggestthat the E2F-Cdc2 cell-cycle pathway specifically mediates theactivity deprivation-induced neuronal apoptoticresponse.

In future studies, it will be important to address the question of whether in other neurons Cdc2 might be activated with apoptoticstimuli in addition to activity withdrawal. If Cdc2 but not E2F1is the specificity determinant of activity deprivation-inducedapoptosis, the cdc2 promoter may provide a valuable biochemicalendpoint in future studies for the identification and characterizationof transcription factors that cooperate with E2F1 to specificallyinduce Cdc2 in activity-deprived postmitotic neurons. However,distinct E2F1-mediated mechanisms may mediate activity deprivation-inducedapoptosis of granule neurons (this study) and apoptosis of sympatheticneurons with growth factor withdrawal or chemotoxin-induced apoptosisof cortical neurons (Liu and Greene, 2001b). The characterizationof the distinct mechanisms regulating E2F function in postmitoticneurons in the different paradigms of neuronal apoptosis in thesetwo studies may reveal additional specific signals that mediateactivity deprivation-induced neuronalapoptosis.

The observation that neuronal activity deprivation induces E2F1-mediated cdc2 transcription points to the similarity in therole of E2F1 in inducing Cdc2 in postmitotic neurons and proliferatingcells. However, we found that much of the function of E2Fs, andE2F1 in particular, to stimulate S phase genes in proliferatingcells is not recapitulated in postmitotic neurons. These observationscarry a number of implications. First, they suggest that Cdc2represents a select target of E2F in postmitotic neurons and pointto specificity mechanisms that exist in postmitotic CNS neuronsthat confer E2F with the selective ability to induce cdc2 transcriptionor that silence the majority of E2F-regulated genes. Investigationof these mechanisms might shed light on the postmitotic neuronalstate. Second, our observation of Cdc2 triggering apoptosis ofpostmitotic neurons in the absence of DNA synthesis points toa similarity of Cdc2-mediated neuronal apoptosis and the roleof premature Cdc2 activation in cycling cells culminating in apoptosis(Shi et al., 1994). It will be important to determine whetherlessons from one situation might be applied to the other. Finally,it is interesting to compare the role of the cell-cycle machineryin apoptosis of neurons in the CNS and peripheral nervous system(PNS). A recent study revealed distinct responses of CNS and PNSneurons to expression of the transcription factor N-myc that promotescell-cycle progression in dividing cells (Wartiovaara et al.,2002). Whereas N-myc induced successful re-entry of sympatheticneurons into the cell cycle, N-myc induced apoptosis of corticalneurons (Wartiovaara et al., 2002). It will be interesting tocompare the cell-cycle protein responses of PNS and CNS neuronsto activitydeprivation.

In conclusion, our findings suggest that the E2F-Cdc2 cell-cycle pathway plays a critical role in neuronal apoptosis. Ourstudy raises several questions. It will be important in futurestudies to determine the role of the E2F-Cdc2 cell-cycle pathwayin the normal development of the mammalian brain. In addition,it will be important to determine how the E2F-Cdc2 cell-cyclepathway interacts with other signals that mediate activity deprivation-inducedneuronal apoptosis. In this regard, the Jun-N-terminal kinase(JNK) signaling pathway is thought to play a critical role inapoptosis of granule neurons with the suppression of neuronalactivity (Watson et al., 1998; Le-Niculescu et al., 1999). Interestingly,we found recently that JNK induces the phosphorylation of BADat serine 128 and thereby activates BAD-mediated apoptosis (Donovanet al., 2002), raising the possibility that Cdc2 and JNK may convergeon BAD to effectively induce the cell-death machinery in neurons,or that these kinases target BAD in a temporally specific mannerin granule neurons (Donovan et al., 2002). Whether the regulationof the Cdc2 and JNK signaling pathways in activity-deprived neuronsis coordinated remains to be determined. Finally, because neuronaldeath is thought to be a major pathophysiologic feature of severalcommon neurologic disorders, including neurodegenerative diseasesand stroke (Cotman, 1998; Pettmann and Henderson, 1998; Snideret al., 1999), it will also be interesting to determine whetherthe E2F-Cdc2 cell-cycle pathway contributes to neuronal apoptosisin these neurologicaldiseases.

  FOOTNOTES

Received Aug. 16, 2002; revised Nov. 14, 2002; accepted Dec. 6, 2002.

This work was supported by a Burroughs Wellcome Career Development Award (A.B.) and by National Institutes of Health GrantR01-NS41021-01 (A.B.). A.B. is the recipient of an Alfred P. SloanFoundation Fellowship, a Robert H. Ebert Clinical Scholar Awardfrom the Esther A. and Joseph Klingenstein Fund, an EJLB FoundationAward, and a Sidney Kimmel Foundation Award. We thank B. Gaudillierefor critical reading of this manuscript, P. Hinds for helpfuldiscussions, C. K. Glass for providing the cdc2-luciferase plasmids,W. Sellers for providing the E2F1 expression plasmids, and S.Vasquez for technicalassistance.

Correspondence should be addressed to Azad Bonni, Department of Pathology, Harvard Medical School, 200 Longwood Avenue, Boston,MA 02115. E-mail: azad_bonni{at}hms.harvard.edu.

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