N-myc Promotes Survival and Induces S-Phase Entry of Postmitotic Sympathetic Neurons

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Neuroblastoma

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The Journal of Neuroscience, February 1, 2002, 22(3):815-824

N-myc Promotes Survival and Induces S-Phase Entry of Postmitotic Sympathetic Neurons
Kirmo Wartiovaara¹, Fanie Barnabé-Heider², Freda D. Miller¹^,², and David R. Kaplan¹^,²
¹ Brain Tumor Research Center and ² Center for Neuronal Survival, Montreal Neurological Institute, McGill University, Montreal, Quebec, Canada H3A 2B4

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In most postmitotic neurons, expression or activation of proteins that stimulate cell cycle progression or DNA replicationresults in apoptosis. One potential exception to this generalizationis neuroblastoma (NB), a tumor derived from the sympathoadrenallineage. NBs often express high levels of N-myc, a proto-oncogenethat can potently activate key components of the cell cycle machinery.Here, we show that in postmitotic sympathetic neurons, N-myc caninduce S-phase entry while protecting neurons from death causedby aberrant cell cycle reentry. Specifically, these experimentsdemonstrate that expression of N-myc at levels similar to thosein NBs caused sympathetic neurons to reenter S-phase, as monitoredby 5-bromo-2-deoxyuridine incorporation and expression of cellcycle regulatory proteins, and rescued them from apoptosis inducedby withdrawal of their obligate survival factor, nerve growthfactor. The N-myc-induced cell cycle entry, but not enhanced survival,was inhibited by coexpression of a constitutively hypophosphorylatedform of the retinoblastoma tumor suppressor protein, suggestingthat these two effects of N-myc are mediated by separate pathways.In contrast, N-myc did not cause S-phase entry in postmitoticcortical neurons. Thus, N-myc both selectively causes sympatheticneurons to reenter the cell cycle and protects them from apoptosis,potentially contributing to their transformation toNBs.

Key words: neuronal cell cycle; neuronal apoptosis; NGF; pRb; neuroblastoma; cortical neurons; sympathetic neurons; N-myc; S-phase

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Neuroblastoma (NB), a malignant tumor of children, is derived from the neural crest and arises in the sympathoadrenal system.Because NB is the most common extracranial tumor of children butis very rare in adults, it is likely that malignant transformationoccurs at some point during the development of the sympatheticnervous system, perhaps during the transition from a neural crestprecursor to a postmitotic sympathetic neuron. In this regard,two key questions involve the mechanisms that (1) maintain sympatheticprecursor and/or postmitotic neurons in the cell cycle and (2)allow these transformed sympathetic cells to escape the defaultapoptotic pathways that are normally triggered when progenitorsfail to appropriately exit the cell cycle (for review, see Milleret al., 2000).

Most previous work examining the cell cycle machinery involved in neuronal terminal mitosis has focused on CNS neurons. Thesestudies have demonstrated that the retinoblastoma tumor suppressor,pRb, plays an essential role in inducing terminal mitosis (Clarkeet al., 1992; Jacks et al., 1992; Lee et al., 1992, 1994; Slacket al., 1998). pRb binds to the E2F family of transcription factors,blocking transcriptional activation by E2F and of cell cycle genes,thereby preventing entry into the S-phase of the cell cycle (forreview, see Slack and Miller, 1996). When this pRb-mediated cellcycle exit is perturbed, CNS neurons apoptose, likely by a p53-mediateddefault apoptotic pathway (Macleod et al., 1996; Slack et al.,1998). It is unclear whether similar mechanisms are essentialfor the transition from a cycling sympathetic neuroblast to apostmitotic sympathetic neuron. In fact, the mechanisms appearto be fundamentally different: sympathetic neuroblasts expressa neuronal phenotype while still dividing (Rothman et al., 1978;Rohrer and Thoenen, 1987; Memberg and Hall, 1995), whereas mostCNS progenitors express a neuronal phenotype only when they undergoterminal mitosis (Lauder and Bloom, 1974; Rothman et al., 1980;Koulakoff et al., 1983; Menezes and Luskin, 1994; Gloster et al.,1999).

Significantly more is known about the mechanisms regulating sympathetic neuron survival and apoptosis. These neurons requirenerve growth factor (NGF) and activation of the TrkA/NGF receptorto survive and, in their absence, undergo apoptosis (for review,see Kaplan and Miller, 2000). Apoptosis can occur via two pathways:a p75NTR-Jun-N-terminal kinase (JNK)-dependent pathway (Majdanet al., 1997, 2001; Bamji et al., 1998) and a second pathway thatinvolves the stimulation of the cell cycle machinery (Freemanet al., 1994; Farinelli and Greene, 1996; Park et al., 1996, 1997).These pathways use p53 and its family member p73 as checkpointsto regulate apoptosis (Aloyz et al., 1998; Pozniak et al., 2000a).Thus, both the survival and terminal mitosis of sympathetic neuronsmay rely on two well known tumor suppressors, p53 and pRb. Itis therefore surprising that neither pRb nor p53 is mutated inNB, although p53 localization is sometimes altered (Vogan et al.,1993; Goldman et al., 1996). Instead, the N-myc proto-oncogeneis often found to be amplified in NB, and this amplification isone of the most important molecular markers for poor prognosisin patients with this tumor (Brodeur et al., 1984).

N-myc is a transcription factor that regulates a number of genes involved in cell proliferation and apoptosis and directlybinds to cell cycle regulators such as pRb (Rustgi et al., 1991).The N-myc homozygous null mouse dies in midgestation and has fewerneuronal cells in the peripheral ganglia (Stanton and Parada,1992; Stanton et al., 1992; Sawai et al., 1993). In the developingavian and Drosophila PNS, overexpression of N-myc stimulates G₁/S-phaseprogression, ventral migration, and neural differentiation (Wakamatsuet al., 1997). In mice, the sequestration in the cytoplasm andthus inactivation of N-myc may be required for the neurotrophin-inducedcell cycle arrest of sensory precursor cells (ElShamy et al.,1998). Consistent with their role as cell cycle regulators duringdevelopment, myc family members are highly expressed in the childhoodtumors NB, medulloblastoma, and Wilms' tumor (Nisen et al., 1986).However, the precise mechanisms whereby N-myc mediates its normalphysiological role or its pathological oncogenic role are notclear.

Here, we have asked whether N-myc is capable of inducing postmitotic sympathetic neurons to reenter the cell cycle. We showthat N-myc overexpression stimulated both cell cycle progressionand survival of sympathetic neurons but had no effect on S-phaseprogression in postmitotic cortical neurons. Thus, sympatheticneurons are not completely locked out of the cell cycle, and N-myccan protect cycling neurons from apoptosis, thereby potentiallycontributing to malignanttransformation.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Sympathetic neuron cultures. Primary neuronal cultures were prepared from postnatal day 1 Sprague Dawley rat sympathetic superiorcervical ganglia essentially as described previously (Ma et al.,1992). For immunocytochemistry and nuclear staining, MTT assays,or Western blot analysis, 6,000-10,000 cells per well were platedin 8-well chamber slides, 3000-5000 cells per well were platedin 96-well chamber slides, or 0.5-1 × 10⁵ cells per well were plated in 6-well plates, respectively. Allthe plates were rat tail collagen-coated, and the cells were maintainedin Ultraculture medium containing 2 mM glutamine, 100 U/ml penicillin,100 µg/ml streptomycin (all from BioWhittaker, Walkersville, MD),and 3% rat serum (Harlan Bioproducts, Madison, WI). Neurons wereinitially cultured for 5 d in the presence of 50 ng/ml NGF (Cedarlane,Hornby, Ontario, Canada) and 7 µM cytosine arabinoside (CA). LAN-1-15Nhuman neuroblastoma cells were the kind gift of Dr. C. Thiele(National Institutes of Health, Bethesda,MD).

Cortical neuron cultures. Primary cortical neuron cultures were obtained from embryonic day (E) 16-E17 mice. The meningeswere removed, and cortical tissue was transferred into Neurobasalmedia (Invitrogen) containing 500 µM glutamine, 2% B27 supplement,and 1% penicillin-streptomycin (Invitrogen). The tissue was trituratedinto a single-cell suspension, and cells were plated in four-wellchamber slides precoated with laminin and poly-D-lysine (CollaborativeResearch) at a density of 10⁵ per well. Three days after plating, half of the media was changedwith fresh media supplemented with 7 µM CA (final concentration).Three days later, all media was replaced with fresh media withoutCA. Infection with recombinant adenovirus was at 6 d afterplating.

Recombinant adenovirus infections. The adenovirus coding for human N-myc was constructed as described (He et al., 1998). Briefly,the N-myc cDNA was cloned into the pAdTrack shuttle vector, recombinedwith the pAdEasy adenoviral vector in bacteria, transfected, andamplified in human embryonic kidney (HEK)293 cells. The viruseswere purified on CsCl gradients and titered in HEK293 cells, aswe have described previously (Slack et al., 1996). The other adenoviruseshave been described previously and encode a constitutively hypophosphorylatedform of pRb (Chang et al., 1995; Toma et al., 2000), p53 (Slacket al., 1996; Pozniak et al., 2000a), kinase-inactive TrkA (Vaillantet al., 1999), green fluorescent protein (GFP) (Pozniak et al.,2000a; Toma et al., 2000) (Quantum Biotechnologies), and Escherichiacoli $beta$ -galactosidase (Slack et al., 1996) (gift of Dr. Frank Graham,McMaster University, Canada). The adenoviruses were used to infectcultured sympathetic neurons at various concentrations of infectivevirus particles added per cell (multiplicity of infection; MOI).Infections of sympathetic neurons were performed by replacingthe culture media with viruses diluted in Ultraculture containingno serum or CA and with glutamine, penicillin, streptomycin, andNGF as described above. Infections of cortical neurons were similarexcept that viruses were diluted in Neurobasal medium containingglutamine, B27, penicillin, and streptomycin. After 24 hr themedia was replaced with the same media withoutvirus.

Survival experiments. Neurons were cultured for 5 d and infected as described above. To measure potential virus-induced celldeath, the neurons were maintained for an additional 4 d afterinfection and analyzed. The MTT assays, which measure mitochondrialfunction and reflect cell viability and survival, were performedin 96-well plates, each condition as a triplicate as describedpreviously (Bamji et al., 1998). Data from these assays were expressedas a percentage of MTT signal obtained in 10 ng/ml NGF (100% survival)versus zero NGF (0% survival). For the neurotrophin withdrawalexperiments, neurons were infected with recombinant adenovirus,and 2 d after infection, NGF was washed out by four 1 hr washesof Ultraculture alone. Neurons were then maintained in Ultraculturecontaining penicillin, streptomycin, and glutamine, with or withoutNGF, for 24-48 hr before analysis. MTT assays were performed 2d after NGF withdrawal as indicated above. For the assessmentof live/dead cells using Trypan blue, neurons were withdrawn fromNGF for 2 d and stained with 20% Trypan blue, and the percentageof white (live) and blue (dead) of 300 or more cells in threerandom microscope fields was quantitated. For analysis of apoptoticnuclei with Hoechst, neurons were withdrawn from NGF for 48 hr,fixed with 4% paraformaldehyde (PFA), and then stained with Hoechst33258 (Sigma, St. Louis, MO) diluted 1:3000 in PBS. Quantitationwas as for Trypan blue analysis. Terminal deoxynucleotidyl transferase-mediatedbiotinylated UTP nick end labeling (TUNEL) was performed at 24-48hr after NGF withdrawal, essentially as described previously (Vaillantet al., 1999; Pozniak et al., 2000a). Briefly, neurons were fixedfor 15 min at room temperature with 4% PFA, 0.25% glutaraldehyde(Fluka AG), and 0.2% Triton X-100 (Sigma) in 40 mM PIPES, 2.5mM EGTA, 1 mM MgCl₂, and washed with PBS. The cells were thenincubated for 1 hr at 37°C in the TUNEL reaction mix of 20 µlTdT buffer/1.5 µl terminal deoxynucleotidyl transferase (TdT)enzyme (both from Promega Corporation) and 1 µl of biotin-16-dUTP(Boehringer Mannheim). After the TUNEL reaction, cells were washed,incubated for 1 hr with streptavidin-conjugated Cy₃ secondaryantibody (1:500; Jackson ImmunoResearch Laboratories) in PBS atroom temperature, washed, Hoechst-labeled, and mounted. Digitalimage acquisition and analysis were performed with the NorthernEclipse software (Empix Inc.) using a Sony XC-75CE charge-coupleddevice videocamera.

5-Bromo-2-deoxyuridine incorporation and immunocytochemistry. For immunocytochemistry and 5-bromo-2-deoxyuridine (BrdU) incorporationanalysis, sympathetic neurons were plated in collagen-coated eight-wellchamber slides and cultured for 5 d as described above, and corticalneurons were plated in four-well chamber slides and cultured asdescribed. On the fifth and sixth days, for sympathetic and corticalneurons, respectively, cells were infected with the indicatedvirus or virus combination. For N-myc immunostaining, the cellswere fixed in 4% paraformaldehyde, permeabilized in 0.5% TritonX-100 in PBS, rinsed, and incubated overnight with 1 µg/ml anti-humanN-myc monoclonal antibody (Oncogene Research Products). Afterthe fixed cells were washed with PBS, the secondary anti-mouse-Cy3antibody was added for 1 hr, the cells were again washed, andthe nuclei were labeled with Hoechst dye. For the analysis ofDNA synthesis, 10 µM BrdU (Boehringer Mannheim) in fresh mediawas added for 24-48 hr. Neurons were fixed with ethanol, treatedwith 2N HCl for 10 min, 0.1 M Na₂B₄O₇, pH 8.5, for 10 min, washedwith PBS, and incubated either with monoclonal anti-BrdU (1:100;Chemicon) and polyclonal anti-neurofilament M (1:200; Chemicon)or with polyclonal sheep anti-BrdU (1:150; Research DiagnosticsInc.) and monoclonal anti-microtubule-associated protein 2 (MAP2)(1:400; Sigma) in PBS overnight at 4°C. After they were washedin PBS, the cells were incubated with secondary FITC or Cy3-conjugatedanti-sheep antibody (1:300; Jackson ImmunoResearch) for 1 hr atroom temperature, washed, and labeled with Hoechst (1:3000) tostain nuclei. In some experiments, 4, 8, or 16 µM cytosine arabinoside(a DNA polymerase inhibitor) was added at the same time as BrdU.Data acquisition and image analysis were performed as describedabove; for each treatment, at least 300 cells in each of threeto six random fields were analyzed. For double labeling of neuronsand astrocytes in cortical neuron cultures, cells were incubatedwith a monoclonal antibody to MAP2 (1:400; Sigma) and a polyclonalantibody to GFAP (1:800; Sigma). X-gal staining for $beta$ -galactosidasewas performed essentially as described (Slack et al., 1996).

Immunoprecipitations and Western blot analysis. Cells were cultured and infected, and where indicated, NGF was withdrawn asdescribed above. The cultured cells were rinsed briefly in coldTBS and then lysed in TBS lysis buffer (137 mM NaCl, 20 mM Tris,pH 8, 1% v/v NP-40, and 10% glycerol) or in urea extraction buffer(8 M urea, 4% 3-[(3-deoxycholic acid (cholamidopropyl)dimethylammonio]-1-propanesulfonate),40 mM Tris, pH 8.0) supplemented with Mini Complete protease inhibitormixture (Boehringer Mannheim) and 1.5 mM sodium vanadate. Lysateswere scraped into Eppendorf tubes and rocked for 10 min at 4°C.Samples were cleared by centrifugation, and the protein concentrationwas determined by the BCA assay (Pierce Chemical) using BSA asa standard. For SDS-PAGE, samples were boiled in sample buffer,separated by 7.5-15% SDS-PAGE gradient gels, and transferred tonitrocellulose membranes. The filters were blocked with 5% skimmilk powder in TBS-T (TBS + 1% Tween 20) for 1-2 hr and incubatedwith primary antibodies against p75NTR (1:1000; Promega), phospho-JNK(1:5000; Promega), MAPK (1:500; Santa Cruz Biotechnology), N-myc(1:1000; Oncogene Research Products), $alpha$ -tubulin (1:5000; OncogeneSciences), cyclin-dependent kinase 2 (cdk2) (1:1000, Santa CruzBiotechnology), or cyclin E (2 µg/ml; UpstateBiotechnology).

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Posmitotic sympathetic neurons enter S-phase of the cell cycle in response to overexpression of N-myc

To determine whether overexpression of N-myc is sufficient to perturb the cell cycle status and/or survival of postmitoticsympathetic neurons, we constructed a recombinant adenovirus expressinghuman N-myc and GFP under the control of separate but identicalcytomegalovirus promoters (Fig. 1A). We then used this virus totransduce neonatal, postmitotic sympathetic neurons that had beencultured for 5 d in the presence of 50 ng/ml NGF. A substantialnumber of neurons were transduced by infection with this virusat MOIs as low as 50, and this number increased with increasingviral MOIs so that as many as 95% of the neurons were detectablyinfected at an MOI of 300, as indicated by expression of GFP (Fig.1B). Confirmation that the GFP-positive neurons also expressedincreased levels of N-myc was obtained by performing immunocytochemistryfor N-myc on the infected neurons (Fig. 1D). All cells that expressedGFP also expressed high levels of N-myc, and much of this N-mycwas localized to the nucleus, as would be predicted. Western blotanalysis for N-myc confirmed this morphological data and demonstratedthat the virus expressed a recombinant protein of the appropriatemolecular weight of 64 kDa (Fig. 1C). Importantly, these Westernblots also demonstrated that N-myc is endogenously expressed incultured postmitotic sympathetic neurons. Moreover, the levelsof human N-myc expression in cultures obtained at MOIs of 100-300were similar to those seen in the human neuroblastoma cell lineLAN-1-15N (Ciccarone et al., 1989), where the N-myc gene is amplified(Fig. 1C). No conclusions, however, can be drawn regarding therelative level of human N-myc overexpression in sympathetic neurons,because the antibody may not cross-react equally well with thehuman (adenoviral) and rodent (endogenous) proteins.

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Figure 1. Characterization of a recombinant adenovirus expressing human N-myc. A, Adenovirus construct encoding human N-myc and green fluorescent protein under separate but identical CMV promoters. B, Adenovirus N-myc (AdN)-myc is expressed in sympathetic neurons. Fluorescent micrograph of GFP expression in postmitotic sympathetic neurons 72 hr after infection with 300 MOI of AdN-myc. C, Western blot of equal amounts of protein isolated from LAN-1-15N neuroblastoma cells and from sympathetic neurons infected for 48 hr with 0-300 MOI of N-myc adenovirus and probed with an antibody for N-myc. Note that uninfected sympathetic neurons express N-myc and that LAN-1-15N cells express levels of N-myc similar to sympathetic neurons infected with 100-300 MOI of the N-myc adenovirus. D, Photomicrographs of sympathetic neurons infected with AdN-myc and then analyzed for expression of GFP and immunocytochemically for expression of N-myc ( $alpha$ -N-myc). Cells were also stained with the nuclear dye Hoechst 33258 to identify all of the cells in the field. Note that cells that are GFP positive are also overexpressing N-myc and that the overexpressed N-myc is primarily nuclear. Scale bar, 50 µm.

Using this recombinant adenovirus, we determined whether expression of N-myc at levels similar to those seen in NBs was sufficientto cause cell cycle entry in postmitotic sympathetic neurons.To ask this question, we infected neurons with the N-myc adenovirusand then added BrdU to the NGF-containing media 1 d later to labelnewly synthesized DNA. We then performed double-label immunocytochemistry48 hr later for BrdU and for neurofilament-M, which is specificfor neurons. As predicted, when neurons were mock infected orwere infected with 200 MOI of control adenoviruses expressing $beta$ -galactosidase (Fig. 2A) or GFP (data not shown), we detectedno or very few neurons that were positive for BrdU, although someof the small percentage of non-neuronal cells present in thesecultures were positive (Fig. 2A). Confirmation that most of thesympathetic neurons were transduced with 200 MOI of the $beta$ -galactosidaseadenovirus, as we have reported previously (Slack et al., 1996),was obtained by staining the infected cultures with X-gal (Fig.2E).

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Figure 2. Overexpression of N-myc in postmitotic sympathetic neurons leads to S-phase entry. A-C, Photomicrographs of sympathetic neurons infected with recombinant adenovirus, pulse-labeled with BrdU, and then immunocytochemically analyzed for expression of neurofilament-M (green) and BrdU (red). In some cases, cells were also labeled with Hoechst to label all nuclei (blue). A, AdLacZ-expressing neurons do not incorporate BrdU. Neurons were infected with 200 MOI of a $beta$ -galactosidase adenovirus and maintained in 10 ng/ml NGF for 3 d. Note that none of the neurofilament-positive neurons are BrdU positive (arrows) and that the only BrdU-positive cells are neurofilament-negative non-neuronal cells (arrowheads). B, Uninfected neurons that were withdrawn from NGF in the presence of BrdU for 30 hr and then analyzed immunocytochemically. Note that a neurofilament-negative non-neuronal cell with an intact nucleus has incorporated BrdU (arrowhead) but that neurons in different phases of apoptosis are not BrdU positive (arrows). C, AdN-myc-expressing neurons incorporate BrdU. Neurons were infected with 200 MOI of N-myc adenovirus and maintained in the presence of NGF. One day later BrdU was added, and cells were analyzed immunocytochemically 48 hr later. Note that under these conditions, many of the neurofilament-positive neurons are BrdU positive (arrows). Scale bar: A, C, 100 µm; B, 50 µm. D, Quantitation of the percentage of cells positive for both BrdU and neurofilament after infection with various MOIs of recombinant adenovirus in the presence of NGF for 1 d, followed by the addition of BrdU for an additional 48 hr. Neurons were infected with recombinant adenoviruses expressing N-myc, constitutively hypophosphorylated pRb (Rb) (Toma et al., 2000), p53 (Slack et al., 1996), $beta$ -galactosidase (LacZ), or a kinase-inactive mutant of TrkA (KDTrkA) (Vaillant et al., 1999). Values derive from counts of at least 300 cells in four or more random microscope fields per condition, and error bars represent the SD of the mean. Similar results were obtained in four independent experiments. **p < 0.01; Student's t test. Note that only N-myc led to BrdU incorporation in sympathetic neurons. E, Staining for $beta$ -galactosidase (LacZ) in cultures of sympathetic neurons transduced with 200 MOI of the $beta$ -galactosidase adenovirus. Note that most of the sympathetic neurons are positively stained. F, Inhibition of N-myc stimulated cell cycle entry by DNA polymerase inhibition. Percentage of BrdU-positive neurons 48 hr after infection with 50 or 200 MOI AdN-myc, cultured in the presence of BrdU with or without 4, 8, or 16 µM cytosine arabinoside for the final 24 hr. Quantitation was performed as in D. Similar results were obtained in three independent experiments. Concentrations of CA shown here did not increase apoptotic cell morphology over the time of the experiment. **p < 0.05; ***p < 0.001. G, AdN-myc expression increases the levels of the S-phase markers cyclin E and cdk2. Western blot analysis of equal amounts of protein from sympathetic neurons that were uninfected (0) or infected with 200 MOI of adenoviruses expressing either $beta$ -galactosidase (LacZ) or N-myc for 2 d. Blots were reprobed for total $alpha$ -tubulin as a loading control. Similar results were obtained in two independent experiments.

In contrast, when neurons cultured in the presence of NGF were infected with 200 MOI of the N-myc adenovirus, most of theneurofilament-positive neurons were also BrdU positive (Fig. 2C).Quantitation of this result in four independent experiments revealedthat up to 58% of the neurons were positive after a 48 hr pulseof BrdU (Fig. 2D). In contrast, no increase in neuronal BrdU incorporationwas observed in neurons infected with up to 800 MOI of the $beta$ -galactosidaseadenovirus (Fig. 2D). To confirm that this enhanced BrdU incorporationwas not caused simply by DNA damage or fragmentation, we performedsimilar experiments with sympathetic neurons that were withdrawnfrom NGF, a treatment that causes DNA fragmentation coincidentwith cellular apoptosis. NGF withdrawal never led to BrdU incorporationin sympathetic neurons (Fig. 2B). Similarly, no BrdU incorporationwas observed after infection with adenoviruses expressing p53(Aloyz et al., 1998) or a kinase-inactive form of TrkA (Vaillantet al., 1999) (Fig. 2D), both of which cause sympathetic neuronapoptosis in the presence ofNGF.

As an additional control for the specificity of BrdU incorporation, we determined whether we could rescue this effect by inhibitingDNA polymerase activity. To perform these experiments, neuronswere infected with 50 or 200 MOI of N-myc adenovirus, and 4-16µM DNA polymerase inhibitor CA was added at the same time as theBrdU. Twenty-four hours later, neurons were immunocytochemicallydouble labeled for neurofilament and BrdU. Quantitation of theseexperiments (Fig. 2F) revealed that 50 and 200 MOI of N-myc caused~17 and 35%, respectively, of the neurons to incorporate BrdUand that CA inhibited this effect in a concentration-dependentmanner.

To confirm that the enhanced BrdU incorporation reflected S-phase entry, we analyzed expression of two proteins known to beinduced during S-phase of the cell cycle: cyclin-dependent kinase2 (cdk2) and cyclin E (for review, see Ekholm and Reed, 2000).Specifically, sympathetic neurons were infected with 200 MOI ofadenoviruses encoding either $beta$ -galactosidase or N-myc and werelysed 2 d later. Western blot analysis of equal amounts of proteinrevealed that levels of both of these proteins were increasedin neurons overexpressing N-myc (Fig. 2G).

Finally, we determined whether N-myc overexpression caused sympathetic neurons to divide. Mitotic figures were never observedduring extensive time-lapse analysis of multiple cultures, norwere dividing neuronal cell bodies observed. Because these analyseswere performed at MOIs of N-myc adenovirus where >50% of neuronsincorporated BrdU, we conclude that N-myc overexpression promotesS-phase entry but is insufficient to cause postmitotic neuronsto proceed into mitosisitself.

Overexpression of N-myc inhibits sympathetic neuron apoptosis after NGF withdrawal

One hypothesis postulates that postmitotic neurons inevitably undergo apoptosis when they are forced to reenter the cell cycle.We therefore asked whether N-myc caused sympathetic neuron apoptosiscoincident with cell cycle entry. Sympathetic neurons were infectedwith the N-myc adenovirus in the presence of NGF, and 4 d laterwe performed MTT assays, which measure mitochondrial function.Results of this experiment demonstrated that overexpression ofN-myc had no adverse effects on sympathetic neuron survival (Fig.3A), despite the fact that it caused S-phase entry. Similar resultswere obtained when neurons were infected with a control GFP adenovirusat the same MOIs (Fig. 3A). Thus, in sympathetic neurons, cellcycle reentry is not obligately coupled to apoptosis.

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Figure 3. N-myc promotes sympathetic neuron survival after NGF withdrawal. A, AdN-myc does not decrease the survival of sympathetic neurons in the presence of NGF. MTT survival assays of sympathetic neurons selected in NGF, infected with 100-400 MOI of N-myc, GFP, or hypophosphorylated pRb adenovirus, maintained in NGF, and assayed 4 d after infection are shown. All conditions were performed in triplicate, and error bars represent the SD of the mean. Values derive from one representative experiment of three and are normalized to those obtained for uninfected neurons maintained in 10 ng/ml NGF, which are considered to be 100% survival. No significant alterations are seen in any of the conditions. B-D, Adenovirus-mediated expression of N-myc rescues sympathetic neurons from apoptosis induced by NGF withdrawal, as monitored by MTT assays (B), nuclear morphology (C), and Trypan blue exclusion (D). In all experiments, neurons were infected with adenovirus, withdrawn from NGF 2 d later, and analyzed after an additional 2 d. B, MTT assays of neurons infected with 80-320 MOI N-myc, GFP, or hypophosphorylated pRb adenovirus. Values were normalized to those obtained for uninfected neurons either maintained in NGF (100%) or withdrawn from NGF (1%). Values represent the average of three independent experiments, each of which was performed in triplicate. *p < 0.05; Student's t test comparing results obtained with the N-myc versus control GFP adenovirus. C, D, Percentage of living cells or nonapoptotic cells counted by Hoechst-labeled intact nuclei (C) or Trypan blue exclusion (D) after virus infection and NGF withdrawal. For both methods, values were obtained by counting three randomly selected microscope fields in each condition, and the error bars represent the SD of the mean. Values are representative results of one of two independent experiments. **p < 0.01; Student's t test comparing results obtained using the N-myc versus control $beta$ -galactosidase (LacZ) adenovirus.

We then asked whether overexpression of N-myc might provide a survival advantage to sympathetic neurons, as might be predictedby its role in promoting neuroblastoma. To perform these experiments,neurons were infected with 80-320 MOI of N-myc adenovirus; 2 dlater they were withdrawn from NGF, and MTT assays were performedafter an additional 2 d. This analysis revealed that N-myc significantlyinhibited NGF withdrawal-induced apoptosis in a concentration-dependentmanner (Fig. 3B). Such a rescue was never observed with adenovirusesexpressing either GFP (Fig. 3B) or $beta$ -galactosidase (data not shown).The rescue observed with N-myc overexpression was similar to orbetter than that observed with pro-survival proteins such as activatedRas (Mazzoni et al., 1999).

To confirm that the MTT assay was measuring neuronal survival and to determine the percentage of neurons that were rescuedfrom apoptosis, we performed two additional assays. Neurons wereinfected with 50 or 200 MOI N-myc adenovirus, were withdrawn fromNGF after 2 d, and then the percentage of live cells was determined48 hr later by counting neurons with intact, Hoechst-positivenuclei (Fig. 3C) or by Trypan blue exclusion (Fig. 3D). Both assaysdemonstrated a dose-dependent rescue of 65-85% of the neuronsby overexpression of N-myc (Fig. 3C,D). As predicted, no suchrescue was observed with similar MOIs of the $beta$ -galactosidase adenovirus.Finally, to demonstrate that N-myc was actually rescuing neuronsfrom apoptosis, we performed TUNEL. Neurons were infected withadenoviruses expressing either N-myc and GFP or GFP alone, werewithdrawn from NGF, and assayed 24 hr later. This analysis demonstratedthat for neurons infected with the GFP virus, many of the GFP-positivecells were also TUNEL positive (Fig. 4A-C). In contrast, for neuronsinfected with the N-myc/GFP virus, few of the GFP-positive cellswere TUNEL positive (Fig. 4D-F). Quantitation of the total numberof TUNEL-positive cells confirmed that overexpression of N-mycsignificantly rescued sympathetic neurons from apoptosis afterNGF withdrawal (Fig. 4G).

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Figure 4. N-myc overexpression inhibits sympathetic neuron apoptosis after NGF withdrawal. A-F, TUNEL of sympathetic neurons infected with adenoviruses expressing GFP (AdGFP; A-C) or N-myc (this virus also expresses GFP) (AdN-myc; D-F) and withdrawn from NGF for 48 hr. Photomicrographs show TUNEL-positive nuclei (A, D), GFP-expressing cells (B, E), and Hoechst-positive nuclei (C, F) in the same fields (A-C and D-F). Arrows indicate the same neurons in each field. Note that neurons infected with the adenovirus expressing only GFP (A-C) are TUNEL positive and display shrunken, apoptotic nuclei, but that those infected with the virus expressing both GFP and N-myc (D-F) are not TUNEL positive. Scale bar, 100 µm. G, Percentage of TUNEL-positive cells 24 hr after NGF withdrawal. Neurons were infected with various MOIs of the N-myc or GFP adenoviruses, and the total number of TUNEL-positive nuclei in three randomly selected fields was counted. The values represent the average of two independent experiments, and error bars represent the SD of the mean. **p < 0.01 in Student's t test comparing apoptotic (TUNEL-positive) cell percentage after infection with AdN-myc versus AdGFP.

Expression of constitutively hypophosphorylated pRb inhibits the S-phase entry caused by N-myc but has no effect on neuronal survival

One mechanism whereby N-myc is thought to regulate S-phase entry involves the retinoblastoma tumor suppressor protein (Rustgiet al., 1991; Lasorella et al., 2000). pRb is a key neuronal cellcycle regulator (Clarke et al., 1992; Jacks et al., 1992; Leeet al., 1992, 1994; Slack et al., 1998; Toma et al., 2000). HypophosphorylatedpRb binds to and inhibits proteins that promote S-phase entry,such as the E2F family (for review, see Slack and Miller, 1996).On this basis, we predicted that if in these experiments N-mycpromotes S-phase entry via a mechanism involving pRb, then thisS-phase entry should be inhibited by coincident overexpressionof a mutant pRb that is constitutively hypophosphorylated. Totest this prediction, sympathetic neurons were coinfected withthe N-myc adenovirus and with increasing MOIs of a recombinantadenovirus expressing constitutively hypophosphorylated pRb (Changet al., 1995; Toma et al., 2000).

To perform these experiments, we first asked whether expression of constitutively hypophosphorylated pRb on its own had anyeffect on sympathetic neuron S-phase entry. Neurons were infectedwith 50 or 200 MOI of pRb adenovirus, and then 1 d later BrdUwas added for an additional 48 hr. Double-label immunocytochemistryrevealed that few or none of the neurofilament-positive neuronswere BrdU positive (Fig. 2D). Having established that hypophosphorylatedpRb had no effects on its own, we then determined whether it couldrescue N-myc-mediated S-phase entry. Neurons were coinfected with50 MOI N-myc and 200 MOI pRb adenoviruses for 1 d and then wereincubated with BrdU for an additional 2 d. Double-label immunocytochemistryrevealed that 50 MOI N-myc adenovirus caused ~15% of sympatheticneurons to incorporate BrdU and that the pRb virus decreased thisnumber in a concentration-dependent manner so that at 200 MOIpRb, <4% of neurons were BrdU positive (Fig. 5A). In contrast,coinfection with 200 MOI of the $beta$ -galactosidase adenovirus hadno significant effect (Fig. 5A). Thus, hypophosphorylated pRbrescued the N-myc-mediated S-phase entry.

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Figure 5. Constitutively hypophosphorylated pRb inhibits the S-phase entry, but not the survival, caused by N-myc. A, Constitutively hypophosphorylated pRb rescues the N-myc-induced BrdU incorporation. Neurons were coinfected with 50 MOI N-myc adenovirus and 50-200 MOI pRb adenovirus, incubated with BrdU 1 d later, and then analyzed immunocytochemically for BrdU and neurofilament-M after an additional 2 d. As a control, neurons were coinfected with 200 MOI of a $beta$ -galactosidase adenovirus (LacZ). Quantitation was performed as described in Figure 2D. *p < 0.05; Student's t test, comparing N-myc plus pRb versus N-myc plus $beta$ -galactosidase. B, pRb has no effect on N-myc-induced survival after NGF withdrawal. Neurons were infected with 200 MOI N-myc in the presence or absence of 100 or 200 MOI hypophosphorylated pRb adenovirus, and 2 d later NGF was withdrawn. Neurons were stained with Hoechst, and intact, nonapoptotic nuclei were quantitated by counting at least 300 cells in each of three random fields. C, AdN-myc decreases p75NTR expression and inhibits the activation of JNK. Immunoblots of sympathetic neurons infected with 100 or 400 MOI of N-myc adenovirus in the presence (right panel) or absence (left panel) of NGF. Left panel, Neurons were infected with N-myc adenovirus for 48 hr and then withdrawn from NGF for an additional 24 hr. Equal amounts of protein were analyzed for expression of the p75NTR ( $alpha$ -p75), the activated, phosphorylated form of JNK ( $alpha$ -P-JNK), or for total MAP kinase protein levels ( $alpha$ -MAPK). Note that although p75NTR and phospho-JNK levels were reduced on infection with N-myc, total MAP kinase levels remained the same. Right panel, Neurons were infected with N-myc adenovirus and maintained in NGF for 72 hr before Western blot analysis. Immunoblots were first probed with an antibody to p75NTR and then reprobed with an antibody for total $alpha$ -tubulin to demonstrate that similar amounts of protein were present in each lane. Note the concentration-dependent decrease in p75NTR levels in neurons infected with the N-myc adenovirus. Similar results were obtained in four independent experiments.

We then asked whether the survival effects seen with N-myc overexpression also involved pRb. Initially, we determined whetherhypophosphorylated pRb itself had effects on sympathetic neuronsurvival. Neurons were infected with MOIs of the pRb adenovirusranging from 80 to 400 and were then either maintained in NGFor withdrawn from NGF for 2 d before MTT assays. These experimentsdemonstrated that expression of hypophosphorylated pRb on itsown had no effect on neuronal survival in either the presenceor absence of NGF (Fig. 3A,B). We then asked whether the N-myc-mediatedsurvival was affected by constitutively hypophosphorylated pRb.To perform these experiments, sympathetic neurons were coinfectedwith 200 MOI N-myc and 100 or 200 MOI constitutively hypophosphorylatedpRb virus for 2 d and were then withdrawn from NGF for an additional24-48 hr. Staining of the neurons with Hoechst and quantitationof apoptotic nuclei revealed that coexpression of hypophosphorylatedpRb had no effect on the decrease in apoptosis observed when N-mycwas overexpressed (Fig. 5B). Thus, at a ratio of N-myc to pRbvirus of 1:1, hypophosphorylated pRb rescued the N-myc-mediatedS-phase entry but not its effects on neuronal survival, suggestingthat the pathways used by N-myc to promote S-phase entry versusenhanced survival aredistinct.

The apoptotic death of sympathetic neurons after NGF withdrawal requires the p75 neurotrophin receptor (Bamji et al., 1998),which directly activates a JNK-p53 apoptotic pathway (Aloyz etal., 1998). Moreover, the absolute cellular levels of p75NTR area key determinant of its ability to cause neuronal apoptosis (Barrettet al., 1998; Majdan et al., 2001). Because N-myc is a transcriptionfactor, it could potentially regulate sympathetic neuron apoptosisby regulating levels of this apoptotic receptor. To test thispossibility, sympathetic neurons were cultured in 50 ng/ml NGFand then infected with 100 or 400 MOI of the N-myc adenovirusfor 2 d. Western blot analysis revealed that N-myc overexpressionled to a substantial decrease in the levels of p75NTR (Fig. 5C).Reprobing of the same blots for proteins such as $alpha$ -tubulin orthe MAP kinases revealed that this decrease was specific to p75NTR(Fig. 5C). Similar results were obtained for neurons that werewithdrawn from NGF for 24 hr. p75NTR levels were significantlylower in neurons overexpressing N-myc, whereas levels of the MAPkinases were unchanged (Fig. 5C). Interestingly, concomitant withthis decrease in p75NTR, levels of phosphorylated JNK, a key mediatorof sympathetic neuron apoptosis after NGF withdrawal (Pozniaket al., 2000b; Harding et al., 2001), were also reduced (Fig.5C). In contrast, levels of p75NTR or phospho-JNK were unalteredby infection with a control, GFP-expressing adenovirus (data notshown). Thus, one pRb-independent mechanism that could accountfor the enhanced survival observed when N-myc was overexpressedinvolves downregulation of the p75NTR-JNK apoptoticpathway.

N-myc does not cause S-phase entry in postmitotic cortical neurons

We next focused on postmitotic cortical neurons to ask whether N-myc could induce S-phase entry in CNS neurons. To performthese experiments, we used cultures of cortical neurons that wereprimarily free of glia. Specifically, cortical neurons were culturedat E16-17 and then maintained for 6 d to ensure that all neuronsin the culture were postmitotic. To characterize the cultures,we immunostained them for MAP2, a neuron-specific protein, andfor GFAP, an astrocyte-specific protein. This analysis revealedthat >95% of the cells in these cultures were neurons, with onlya small number of astrocytes present (Fig. 6A-C). To ensure thatthe neurons were truly postmitotic, we also pulsed the cultureswith BrdU for 48 hr; virtually none of the MAP2-positive neuronswere BrdU positive (data not shown).

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Figure 6. N-myc does not cause BrdU incorporation in postmitotic cortical neurons. A-C, Immunocytochemical analysis of postmitotic cortical neuron cultures. Neurons were cultured as described in Results and double labeled with antibodies for neuron-specific MAP2 (A) and astrocyte-specific GFAP (B). Cells were also stained with Hoechst to show cell nuclei (C). The same field is shown in all three panels, and arrows indicate the occasional astrocyte present in the cultures. Note that most fields did not contain any GFAP-positive cells. D-F, Cortical neurons were infected with 100 MOI N-myc adenovirus (which also expresses GFP) and then immunostained for MAP2. Visualization of GFP (D) revealed those cells that were transduced with the N-myc adenovirus, whereas immunostaining for MAP2 (E) indicated that the infected cells were neurons. F is the merged image resulting from D and E. Arrows indicate cells that were positive for both GFP and MAP2. G-I, Cortical neurons were infected with 100 MOI N-myc adenovirus and then incubated in the presence of BrdU for 24 hr before double-label immunocytochemical analysis for MAP2 (G) and BrdU (H). The cells were also stained with Hoechst (I). The same field is shown in all three panels, and the arrow indicates a non-MAP2-positive non-neuronal cell that is BrdU positive. J, Left two bars, Quantitation of data showing that N-myc fails to promote S-phase entry in postmitotic cortical neurons. Quantitation is of data similar to those shown in D-F and indicates the percentage of MAP2-positive neurons that were GFP positive after infection with 100 MOI of N-Myc/GFP (100N-myc) or control GFP (100GFP) adenovirus. Right two bars, The percentage of MAP2-positive cells that were BrdU positive after infection with 100 MOI of either the N-myc or GFP adenoviruses. Similar results were obtained in three independent experiments.

We then used this culture system to determine whether overexpression of N-myc was sufficient to cause postmitotic corticalneurons to enter S-phase. Neurons were infected with 100 MOI N-mycor control, GFP adenovirus for 2 d and were then incubated withBrdU for 24 hr. Double-label immunocytochemical analysis for N-mycand MAP2 confirmed that ~40-50% of the cortical neurons were infectedunder these conditions (Fig. 6D-F,J). Similar numbers were infectedwith 100 MOI of the control GFP adenovirus (Fig. 6J). We thenasked whether any of the cortical neurons incorporated BrdU byperforming immunocytochemistry for MAP2 and BrdU (Fig. 6G-I).Virtually none of the MAP2-positive neurons were positive forBrdU, although the occasional MAP2-negative non-neuronal celldid show BrdU immunoreactivity (Fig. 6G-I). Quantitation of thesedata revealed that the percentage of BrdU-positive, MAP2-positivecells was similar in neurons infected with either the N-myc orcontrol GFP adenoviruses (Fig. 6J). Thus, unlike sympathetic neurons,overexpression of N-myc did not cause postmitotic cortical neuronsto enter S-phase, indicating that there is a fundamental differencein the control of S-phase entry in postmitotic cortical versussympatheticneurons.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The experiments reported in this paper support a number of major conclusions, which together provide a molecular mechanismwhereby the N-myc proto-oncogene could play a major role in thegenesis and promotion of neuroblastoma. First, data presentedhere indicate that overexpression of N-myc at levels similar tothose observed in NB promotes the survival and S-phase entry ofpostmitotic sympathetic neurons. These findings not only provideinformation about the mechanisms whereby N-myc might promote oncogenesis,but they also argue against the hypothesis that aberrant cellcycle entry inevitably causes neuronal apoptosis, at least insympathetic neurons. Second, the N-myc-induced S-phase entry canbe reversed by concomitant expression of constitutively hypophosphorylatedpRb. In contrast, hypophosphorylated pRb had no effect on N-myc-mediatedsurvival, indicating that these effects likely occur via separatedownstream pathways, only one of which (the S-phase entry) involvespRb. Finally, our data demonstrate that N-myc does not cause S-phaseentry in postmitotic cortical neurons, indicating that sympatheticand CNS neurons are "locked out" of the cell cycle by differentmechanisms and suggesting that sympathetic neurons are preferentiallysusceptible to the oncogenic actions of N-myc. Thus, N-myc selectivelycauses postmitotic sympathetic neurons to reenter the cell cycleand allows them to survive under conditions in which they wouldnormally undergo apoptosis, thereby potentially contributing totheir transformation toNB.

Perhaps the most striking result reported here is the ability of N-myc to selectively cause postmitotic sympathetic neuronsto reenter S-phase, as monitored by BrdU incorporation and increasedexpression of cyclin E and cdk2, both of which are normally increasedduring S-phase (Ekholm and Reed, 2000). However, although ourdata strongly support the conclusion that N-myc can cause S-phaseentry, they also argue that N-myc is not sufficient to mediatefurther cell cycle progression, because we never observed mitoticfigures or cell division. Similar results have been reported intransgenic skin cells that overexpressed c-myc: the cells enteredS-phase but did not undergo cell division (Pelengaris et al.,1999). Why do only half of the neurons reenter S-phase in theseexperiments? One potential explanation involves neuronal maturity.Sympathetic neurons exit the cell cycle at time points rangingfrom E13 to postnatal day 1 (Hall and Landis, 1991), and henceafter 5 d of culturing they range from being 4 to 12 d postmitotic.It may be that the more immature sympathetic neurons are preferentiallysensitive to the cell cycle effects of N-myc. Alternatively, theexplanation may be a technical one. BrdU labeling was performedfor only 48 hr, and the length of time required for N-myc to inducea G_o to S-phase transition may bevariable.

How does N-myc mediate this S-phase entry? The results demonstrating that coexpression of hypophosphorylated pRb rescues theBrdU incorporation argues that N-myc mediates this effect viapRb. Such an effect could be mediated by direct interactions betweenN-myc and pRb (Rustgi et al., 1991), and it could also be indirectlymediated via an N-myc-induced increase in levels of the inhibitorybasic helix-loop-helix protein, Id2, which binds to hypophosphorylatedpRb and inhibits its ability to lock cells out of S-phase (Iavaroneet al., 1994; Lasorella et al., 1996; 2000). An additional, potentiallyrelated mechanism involves N-myc-mediated downregulation of thecyclin-dependent kinase inhibitor p27 (Bouchard et al., 1999;Perez-Roger et al., 1999; Yang et al., 2001), which in fibroblastsis essential for induction of cyclin E-cdk2 kinase activity, butnot for S-phase entry (Beier et al., 2000). Although the datapresented here do not distinguish between these alternative explanations,we have observed that p27 levels are decreased and Id2 levelsincreased in sympathetic neurons overexpressing N-myc (our unpublishedobservations), suggesting that decreased p27 may collaborate withincreased Id2 to trigger S-phaseentry.

Results reported here also indicate that N-myc overexpression does not induce S-phase entry in cortical neurons, suggestingthat sympathetic and cortical neurons are locked out of the cellcycle via distinct mechanisms. Such a difference could be predictedby considering the development of these two populations of neurons.Cortical neurons, like most CNS neurons, induce neuronal geneexpression and undergo terminal mitosis at the same time (Glosteret al., 1999). Perturbation of this progenitor-to-postmitoticneuron transition, for example, via functional inhibition of thepRb family (Slack et al., 1998) or via overexpression of Id2 (Tomaet al., 2000), leads to cellular apoptosis; in no conditions yetreported do cortical cells divide while expressing a neuronalphenotype. In contrast, sympathetic neuroblasts transition througha stage in which they express a neuronal phenotype while stilldividing (Rothman et al., 1978; Rohrer and Thoenen, 1987; Membergand Hall, 1995), suggesting that the nature of terminal mitosisdiffers in sympathetic versus CNS neurons. In that regard, ourfindings may indicate that the mechanisms locking most CNS neuronsout of the cell cycle are much more stringent than for sympatheticneurons.

A somewhat surprising finding reported here is that, coincident with S-phase entry, N-myc promotes enhanced survival of sympatheticneurons in the absence of NGF. This is particularly surprisingin light of findings indicating that aberrant cell cycle entryis one of the major mechanisms whereby NGF withdrawal causes sympatheticneuron apoptosis. In particular, NGF withdrawal causes increasedcyclin D1 expression (Freeman et al., 1994), and inhibition ofcdk4 and -6, both of which phosphorylate and activate pRb, issufficient to delay NGF withdrawal-induced apoptosis (Park etal., 1997). However, in this regard, data presented here showthat NGF withdrawal does not cause enhanced BrdU incorporationand that hypophosphorylated pRb is not, by itself, sufficientto rescue sympathetic neurons from apoptosis. Of themselves, ourfindings do not necessarily argue against a role for cell cycledysregulation in NGF withdrawal-induced apoptosis, although theydo demonstrate that this dysregulation does not actually leadto S-phase reentry. Instead, our data suggest that N-myc-inducedsurvival mechanisms may be "dominant" to any apoptotic signalsderiving from the coincident aberrant reentry into S-phase. Interestingly,data presented here suggest (but do not definitively establish)that one such N-myc-mediated mechanism may involve downregulationof p75NTR (Bamji et al., 1998).

N-myc is a true oncogene with overexpression in the sympathetic chain and adrenal medulla of transgenic mice that results,via unknown mechanisms, in malignant neuroblastoma (Weiss et al.,1997). The experimental and clinical data showing a strong correlationbetween N-myc gene amplification and poor outcome in neuroblastomasuggest that N-myc is involved in the malignant transformationof developing sympathetic precursors or neurons, or both. On thebasis of our data showing that N-myc can promote S-phase entryand survival of "postmitotic" sympathetic neurons, we suggesta model in which N-myc contributes to malignant neuroblastomaby either stopping sympathetic neuroblasts from exiting the cellcycle or by collaborating with other risk factors to actuallytransform postmitotic neurons and cause them to reenter the cellcycle.

  FOOTNOTES

Received May 30, 2001; revised Nov. 7, 2001; accepted Nov. 20, 2001.

This work was supported by research grants from the National Cancer Institute of Canada and Canadian Institutes of HealthResearch (CIHR) to D.R.K. and F.D.M., respectively. D.R.K. isa recipient of the Harold Johns and Canadian Cancer Society ResearchScientist Award, and F.D.M. is a CIHR Senior Scientist and a KillamScholar. K.W. was supported by funds from the Finnish Academy,Yrjö Jahnsson Foundation, and the Finnish Medical Society Duodecim;F.B.H. was supported by a National Science and Engineering ResearchCouncilstudentship.
Correspondence should be addressed to Dr. Freda Miller, Center for Neuronal Survival and Brain Tumor Research Center, MontrealNeurological Institute, McGill University, 3801 rue University,Montreal, Quebec, Canada H3A 2B4. E-mail: freda.miller{at}mcgill.ca.

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DISCUSSION
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