Ras Regulates Sympathetic Neuron Survival by Suppressing the p53-Mediated Cell Death Pathway

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The Journal of Neuroscience, November 15, 1999, 19(22):9716-9727

Ras Regulates Sympathetic Neuron Survival by Suppressing the p53-Mediated Cell Death Pathway
Irene E. Mazzoni¹^,², Farid A. Saïd³, Raquel Aloyz¹, Freda D. Miller¹, and David Kaplan¹^,²
¹ Center for Neuronal Survival and ² Brain Tumor Research Center, Montreal Neurological Institute, McGill University, Montreal, Quebec, Canada H3A 2B4, and ³ Exogen Neurosciences, Montreal, Quebec, Canada H2W 2P2

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In this report, we examine how the Ras protein regulates neuronal survival, focusing on sympathetic neurons. Adenovirus-expressedconstitutively activated Ras (RasV12) enhanced survival and thephosphorylation of Akt (protein kinase B) and MAP kinase (MAPK),two targets of Ras activity. Functional inhibition of endogenousRas by adenovirus-expressed dominant-inhibitory Ras (N17Ras) decreasednerve growth factor (NGF)-dependent survival and both Akt andMAPK phosphorylation as well. To determine the signaling pathwaysthrough which Ras mediates survival, we used Ras effector mutantsand pharmacological inhibitors that selectively suppress phosphatidylinositol3-kinase (PI3-K)/Akt or MAP kinase kinase (MEK)/MAPK pathways.The Ras effector mutant Ras^V12Y40C, which selectively stimulates PI3-K and Akt, rescued survivalin the absence of NGF, and the PI3-K inhibitor LY 294002 inhibitedboth Ras- and NGF-dependent survival. Ras^V12T³⁵S, which activates MEK/MAPK but not PI3-K/Akt, was less effectiveat rescuing survival, whereas the MEK inhibitor PD 098059 alsopartially suppressed Ras-dependent survival. To investigate themechanisms by which Ras suppresses neuronal death, we examinedwhether Ras functions by inhibiting the proapoptotic p53 pathway(Jun-N-terminal kinase/p53/BAX) that is necessary for neuronaldeath after NGF withdrawal and p75NTR activation. We found thatRasV12 suppressed c-jun, BAX, and p53 levels, whereas inhibitionof NGF-induced Ras-survival activity via N17Ras increased thelevels of these proteins. Furthermore, the E1B55K protein, whichsuppresses p53 activity, blocked N17Ras-induced neuronal death.Together, these results indicate that Ras is, in part, both necessaryand sufficient for survival of sympathetic neurons and that thiseffect is mediated by activation of both the PI3-K- and MEK-signalingcascades, which in turn suppress a proapoptotic p53pathway.

Key words: Ras; Ras effectors; sympathetic neurons; nerve growth factor; Trk; survival; apoptosis; adenovirus; Raf; PI3-kinase; p53; Bax

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Nerve growth factor (NGF) is essential for maintaining the survival of different subsets of neurons, including sympatheticneurons from the rat superior cervical ganglia (Levi-Montalcini,1987). NGF mediates survival by binding to TrkA (Kaplan et al.,1991a,b; Klein et al., 1991), an event that stimulates the activityof multiple signaling proteins, including the small GTP-bindingprotein p21Ras (Segal and Greenberg, 1996; Kaplan and Miller,1997). Ras activates several downstream effectors, including Rafand phosphatidylinositol 3-kinase (PI3-K) (Rodriguez-Viciana etal., 1994; Vojtek and Der, 1998). Raf binds to and activates MAPkinase kinase 1 (MEK1) and MEK2, activators of the MAP kinases[MAPK or extracellular signal-regulated kinase (ERK)], which playimportant roles in the regulation of neuritogenesis in pheochromocytoma12 (PC12) cells (Cowley et al., 1994; Fukuda et al., 1995; Panget al., 1995). PI3-K is a key regulator of cell survival, morphology,and growth cone extension in neural cells (Yao and Cooper, 1995;Dudek et al., 1997; Crowder and Freeman, 1998; Klesse and Parada,1998). A target of PI3-K activity, the serine/threonine kinaseAkt (or protein kinase B), has been shown to be necessary andsufficient for stimulating the survival of sympathetic, cerebellar,and immortalized hippocampal neurons (Dudek et al., 1997, Philpottet al., 1997; Crowder and Freeman, 1998; Eves et al., 1998). Therole of the Ras effectors has been best defined in non-neuronalcells via the use of Ras effector mutants. Distinct mutationsin the protein recognition, or effector, domain result in theloss of the ability of constitutively activated Ras (RasV12) tostimulate Raf-, PI3-K-, or Ral-GDP dissociation stimulator (GDS)-signalingpathways and of selective biological responses (Rodriguez-Vicianaet al., 1997). For example, the Ras effector mutant Ras^V12Y40C induces membrane ruffling in fibroblasts via its abilityto activate selectively PI3-K and not Raf or RalGDS (Joneson etal., 1996; Rodriguez-Viciana et al., 1997). In several cases,such as the induction of DNA synthesis (Joneson et al., 1996),the concerted action of multiple Ras effectors is needed to mimicthe biological actions of wild-typeRasV12.

In primary neurons, the role of Ras in neurotrophin-regulated cell survival and differentiation varies depending on the celltype assayed. Ras activity is necessary and sufficient for survivaland neuritogenesis of rat and chick sensory but not chick sympatheticneurons (Borasio et al., 1993; Vogel et al., 1995; Klesse andParada, 1998). Paradoxically, Ras activity is required for thesurvival, although not neuritogenesis, of rat sympathetic neurons(Nobes and Tolkovsky, 1995; Nobes et al., 1996; Markus et al.,1997). In these cases, the mechanisms by which Ras stimulatessurvival and suppresses apoptosis remain to bedetermined.

In this report, we examine the signaling pathways used by Ras to stimulate sympathetic neuron survival and to suppress apoptosis.We show that Ras activity is required for a portion of neuronalsurvival and that Ras mediates its actions via both PI3-K andMEK. Ras exerts its effects by suppressing the levels or activitiesof c-jun, the p53 tumor suppressor, and Bax, which are key elementsin the major apoptotic pathway in sympathetic neurons, and apoptosisresulting from suppression of NGF-induced Ras activity requiresp53activity.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Preparation of recombinant adenoviruses. C-myc-tagged RasV12 and dominant-inhibitory Ras (N17Ras) constructs (kind gift ofDr. C. Bazenet) as well as the double mutants Ras^V12T³⁵S, Ras^V12D38E, and Ras^V12E37G (kind gift of Dr. P. Warne) were cloned into the pAd-CMV-F1-IRES-EGFPbicistronic expression vector (Exogen Neurosciences, Montreal,Quebec, Canada). Ras^V12Y40C was cloned into the expression vector pAd-CMV5-F1 (ExogenNeurosciences). Expression of Ras and, for the bicistronic vectors,green fluorescent proteins (GFPs) was confirmed in transientlytransfected 293 cells by Western blot analysis using anti-Ras[Pan Ras (Ab-4); 1:1000; Oncogene Sciences, Uniondale, NY] andanti-GFP (1:2000; Clontech, Palo Alto, CA) antibodies, respectively.Replication-defective recombinant adenoviruses were prepared andpurified as described previously (Slack et al., 1996). Briefly,expression vectors containing the Ras mutants were cotransfectedwith replication-defective adenoviral DNA (Quantum Biotechnologies,Laval, Quebec, Canada) in 293 cells. Plaques were selected andtested for Ras expression by Western blot analysis. Positive plaqueswere repurified twice by limiting dilution. Finally, recombinantadenoviruses were amplified, purified on CsCl gradients, and titeredby plaque assay in 293 cells. As controls, GFP- or Escherichiacoli $beta$ -galactosidase-expressing recombinant adenoviruses (ExogenNeurosciences and Dr. F. Graham, McMaster University, Hamilton,Ontario, Canada, respectively) generated using the same viralbackbone as above were used. The recombinant adenovirus expressingE1B55K was a generous gift of Phil Branton (McGill University,Montreal, Quebec,Canada).

Primary neuronal cultures. Mass cultures of pure sympathetic neurons derived from the superior cervical ganglia (SCG) wereprepared from postnatal day 1 rats essentially as described previously(Ma et al., 1992). Cells were plated in rat tail collagen-coated96 (for survival assays)- or 6 (for Western blot analysis)-wellplates (Falcon Labware; Becton Dickinson, Lincoln Park, NJ) atdensities of 3000-5000 or 0.5-1 × 10⁵ cells, respectively. For nuclear staining, 5000-10,000 neuronswere plated on poly-D-lysine (Sigma, St. Louis, MO) and laminin(Becton Dickinson)-treated glass coverslips. Neurons 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) and initiallycultured for 5 d in the presence of 50 ng/ml NGF (Cedarlane, Hornby,Ontario, Canada) after which they were maintained in the samemedium without serum. This concentration of 50 ng/ml NGF was usedto maximally induce p75NTR, tyrosine hydroxylase, Talpha1 $alpha$ -tubulin,and other differentiation-related genes (Ma et al., 1992). Thereafter,the NGF concentration was reduced to 10 ng/ml. We have shown previouslythat 10 ng/ml is the amount of NGF required for 100% survivalof our neuronal cultures (Belliveau et al., 1997).

Viral infections. After 5 d in culture, a sample well was trypsinized, and cells were counted. Subsequently, medium was removed,and recombinant adenovirus diluted in Ultraculture and DMEM (50:50;DMEM from Life Technologies, Gaithersburg, MD) containing 2 mMglutamine, 100 U/ml penicillin, 100 µg/ml streptomycin, 10% fetalbovine serum, and 30 ng/ml NGF was added to the sympathetic neurons.The multiplicity of infection (MOI) indicates the number of plaque-formingunits added per cell. After 20-24 hr, the virus-containing mediumwas removed and replaced with Ultraculture medium containing 2mM glutamine, 100 U/ml penicillin, 100 µg/ml streptomycin, and20 ng/ml NGF (serum-free). After an additional 24 hr, the mediumwas removed, and the cells were washed 4 times with NGF-free mediumand then incubated in serum-free medium with or without the additionof 10 ng/mlNGF.

Survival assays and pharmacological treatments. Survival assays were performed 72-96 hr after viral infection (2-5 d afterNGF withdrawal) as described previously (Slack et al., 1996),using the nonradioactive cell proliferation assay (MTT; Sigma).Briefly, MTT reagent (final concentration, 0.5 mg/ml) was addedto each well for 2.5 hr. After removing the media and lysing thecells with 100 µl of solubilization solution [HCl acid and isopropanol(0.002:1)], the colorimetric reaction was measured in aspectrophotometer.

For survival assays after pharmacological treatments, neurons were infected where appropriate, and after 2 d, cultures wereexposed to different concentrations of PD 98059 and LY 294002in serum-free media (Calbiochem, San Diego, CA). We establishedthat maximal effects on survival were attained at concentrationsof 75 µM PD 98059 and 100 µM LY 294002 in NGF-treated cultures.Cells treated with the appropriate volume of diluted DMSO, usedto solubilize the drug stocks, served as controls. The volumeof DMSO never surpassed 2 µl/ml ofmedia.

Immunocytochemistry, nuclear staining, and terminal deoxynucleotidyl transferase-mediated biotin-dUTP nick end labeling. ForRas and c-myc immunocytochemistry, cells maintained in the presenceof 10 ng/ml NGF were fixed 48 hr after infection with 2% formalinin PBS for 10 min. Cells were then washed and blocked for 20 minwith 5% goat serum in PBS and 0.02% Triton X-100, followed bya 90 min incubation with either rat anti-Ras (20 µl/ml; Ab-2;Oncogene Sciences) or mouse anti-c-myc (1:150; PharMingen, Mississauga,Ontario, Canada) antibodies. After washing, cells were incubated,where appropriate, with a cy3-conjugated anti-rat or anti-mousesecondary antibody (1:1000; Jackson ImmunoResearch, West Grove,PA) for 45 min, washed, mounted in mounting media (Sigma), andexamined by fluorescencemicroscopy.

For terminal deoxynucleotidyl transferase-mediated dUTP nick-end labeling (TUNEL), cells fixed in ice-cold methanol and acetone(1:1) for 10 min were incubated with 1.5% terminal deoxynucleotidyltransferase (TdT; Promega, Madison, WI) and 1% biotin-16-dUTP(Boehringer Mannheim, Montreal, Quebec, Canada) in TdT bufferfor 1 hr at 37°C. After washing, cells were incubated with cy3-streptavidin(1:3000; Jackson ImmunoResearch) for 45 min at room temperature.Cultures were counterstained with Hoechst 33258 stain (2 µg/ml;ICN Biomedicals, Costa Mesa, CA) for 1 min. Quantitation was doneon randomly selected fields by counting the total number of Hoechst-and TUNEL-positiveneurons.

Western blot analysis. Seventy-two to ninety-six hours after viral infections (2-3 d after NGF withdrawal, where appropriate),cells were washed twice in PBS and lysed in Tris-buffered saline(TBS) lysis buffer (Knusel et al., 1994) (137 mM NaCl and 20 mMTris, pH 8.0) containing 1% NP-40, 10% (v/v) glycerol, 1 mM phenylmethylsulfonylfluoride, 10 µg/ml aprotinin, 0.2 µg/ml leupeptin, 1.5 mM sodiumvanadate, and 0.1% SDS for 10 min at 4°C. After a 5 min centrifugation,the protein concentration in the supernatant was determined usingthe BCA Protein Assay Reagent kit (Pierce, Rockford, IL). Equalamounts of proteins (50-100 µg) were separated on 7.5% (for MAPK,Akt, and p53 proteins) or 15% (for Ras proteins) polyacrylamidegels under denaturing conditions. After gel electrophoresis, proteinswere transferred to nitrocellulose membranes. Membranes were thenblocked in 5% nonfat milk in TBS containing 0.08% Tween 20 (TBST)for 90 min followed by an overnight incubation with the primaryantibodies diluted in 5% nonfat milk in TBST as follows: rabbitanti-phosphorylated-MAPK (1:10,000; Promega), rabbit anti-phosphorylated-Akt(1:1000; New England Biolabs, Beverly, MA), rabbit anti-MAPK1(which recognizes denatured MAPK2 as well; 1:10,000; Santa CruzBiotechnologies, Santa Cruz, CA), mouse anti-Ras [Pan Ras (Ab-4);1:1000; Oncogene Sciences], mouse monoclonal anti-c-jun (1:1000;Santa Cruz Biotechnologies), rabbit anti-Bax (1:500; Santa CruzBiotechnologies), and rabbit anti-p53 (1:1000; Novocastra, Newcastleupon Tyne, United Kingdom). Membranes were then extensively washedand incubated for 90 min with HRP-conjugated goat anti-mouse (forRas and anti c-jun) or goat anti-rabbit (for all other antibodies)IgG (Boehringer Mannheim) diluted 1:10,000 in TBST and 5% nonfatmilk. Immunopositive bands were visualized using enhanced chemiluminescence(Amersham, Arlington Heights, IL) and XAR x-ray film (EastmanKodak, Rochester,NY).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Constitutively activated Ras supports sympathetic neuron survival in the absence of NGF and stimulates phosphorylation of both MAPK and Akt

Previous studies have shown that Ras can mediate sympathetic neuron survival (Nobes and Tolkovsky, 1995; Nobes et al., 1996;Markus et al., 1997). However, the downstream effectors activatedby Ras in these neurons remain unknown. To determine this, wegenerated a bicistronic recombinant adenovirus expressing RasV12(Seeburg et al., 1984) and GFP from the same promoter and confirmedthat it was appropriately expressed in sympathetic neurons byWestern blot analysis (Fig. 1A) and fluorescence microscopy (Fig.2A). We then determined whether, as predicted, RasV12 could supportsympathetic neuron survival in the absence of NGF. Specifically,sympathetic neurons were grown for 5 d in 50 ng/ml NGF, infectedfor 24 hr with the RasV12-expressing adenovirus, and 2 d laterwashed free of NGF. MTT assays revealed that control sympatheticneurons infected with GFP died within 2 d of NGF withdrawal (Fig.1B), as observed previously (Chun and Patterson, 1977; Martinet al., 1988; Edwards and Tolkovsky, 1994; Bamji et al., 1998).In contrast, infection with RasV12 adenovirus rescued sympatheticneurons from death after NGF withdrawal in a concentration-dependentmanner (Fig. 1C). This survival response was maximal at 100-200MOI, where it was similar to survival induced by 5 ng/ml NGF (Fig.1C). At 5 d after infection, survival induced by RasV12 was alsosimilar to survival induced by 5 ng/ml NGF (data not shown), indicatingthat RasV12 appears to prevent and not just delay cell death ina portion of our neurons. RasV12 was never able to rescue survivalto the levels seen for those neurons maintained in 10 ng/ml NGF,even though the level of RasV12 expression was high (Fig. 1A)and most of the neurons were expressing the mutated protein asdetermined by anti-c-myc immunocytochemistry (Fig. 2A,C). Typically,77-85% of neurons expressed visible GFP after infection with Ras-expressingviruses.

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Figure 1. Ras is sufficient to sustain sympathetic neuronal survival and stimulates the phosphorylation of Akt and MAPK. A, Expression of RasV12 in sympathetic neurons is shown. NGF-selected sympathetic neurons were infected with 100 MOI of recombinant adenovirus-expressing GFP or RasV12; 3 d later, neurons were lysed, and equal amounts of protein were analyzed by Western blotting with an antibody specific for Ras. Note the high level of expression of RasV12. B, C, Ras is sufficient to prevent apoptotic neuronal death after NGF withdrawal. Sympathetic neurons were cultured for 5 d in the presence of 50 ng/ml NGF and infected with different MOIs of recombinant adenoviruses expressing either GFP (B) or RasV12 (C). Forty-eight hours after the onset of the infection, NGF was withdrawn for 2 d, and survival was assessed using MTT assays. As controls, uninfected sister cultures were maintained in 5 or 10 ng/ml NGF for the final 2 d (black bars in C). Each point represents the mean ± SEM of quadruplicate wells from three representative experiments. Results are normalized to the amount of survival obtained with 5 ng/ml NGF. Values for RasV12 are significantly different from that of control (NGF-deprived) cells at p < 0.05 (*) (one-way ANOVA and post hoc Dunnett's multiple comparison test). D, RasV12 sustains high levels of phosphorylation of Akt and MAPK in the absence of NGF. After 5 d in 50 ng/ml NGF, cultures were infected with 100 MOI of RasV12 or GFP control virus. Twenty-four and forty-eight hours after the onset of the infection, cells were deprived of NGF. As a positive control, cultures were maintained in the continuous presence of 10 ng/ml NGF. After 2 d, cells were lysed, and Western blot analyses were performed using phosphorylation and activation state-specific antibodies against Akt or MAPK. Note that the levels of phosphorylation of these two Ras downstream effectors are similar in cultures infected with RasV12 and in those treated with NGF. To confirm that the amounts of protein were similar in each lane, we reprobed the blots with anti-ERK1 antibody (bottom bands). P-AKT, Phospho-Akt; P-ERKs, phospho-MAPKs.

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Figure 2. Immunohistochemistry of Ras mutants expressed in sympathetic neurons via recombinant adenovirus. Sympathetic neurons were infected with 100 MOI of c-myc-tagged RasV12 (A, C) or 200 MOI of c-myc-tagged N17Ras (B, D) in the presence of NGF, and 48 hr later cells were processed for immunocytochemistry using anti-myc (A, B). Note that the majority of neurons (phase contrast in C, D) express the Ras mutant proteins.

To confirm that the survival effect observed with RasV12 was caused by a rescue from NGF withdrawal-induced apoptosis, wealso examined neurons by TUNEL staining (Fig. 3A). QuantitativeTUNEL analysis confirmed that these neurons were rescued fromapoptosis; 82 ± 6% of neurons withdrawn from NGF for 2 d had TUNEL-positivenuclei, whereas only 28 ± 2% of neurons were TUNEL positive whenthey were infected with RasV12 and then withdrawn from NGF (Fig.3A). Thus, RasV12 expression was able to rescue the majority ofsympathetic neurons from NGF withdrawal-induced apoptosis, indicatingthat Ras signaling is sufficient for neurotrophin-mediated sympatheticneuron survival.

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Figure 3. Ras regulates sympathetic neuron apoptosis. A, Quantitation of TUNEL-positive cells is shown. Cultures (n = 3) were infected with RasV12 (100 MOI) or N17Ras (200 MOI) in the presence of 10 ng/ml NGF. Twenty-four hours after infection, cultures infected with RasV12 were deprived of NGF, while those infected with N17Ras were maintained in 10 ng/ml NGF. Three days after infection, cells were processed for TUNEL and Hoechst staining. As controls, sympathetic neurons were infected with 200 MOI (control for N17 Ras) or 100 MOI (control for RasV12) of a recombinant adenovirus expressing GFP. Results are expressed as a percentage of TUNEL-positive neurons relative to the total number of Hoechst-labeled cells. B, C, Sympathetic neurons infected with N17Ras (200 MOI) and maintained in 10 ng/ml NGF for 3 d after infection were processed for TUNEL (B) and Hoechst staining (C). As determined by fluorescence microscopy, neurons that were TUNEL positive (B) had nuclei containing highly condensed or fragmented chromatin (C), confirming that they were undergoing apoptosis, whereas those that were TUNEL negative always had spherical and uniformly distributed chromatin.

We then determined whether expression of RasV12 led to the activation of multiple signaling pathways, focusing on the Raf/MEK/MAPKas well as on PI3-K/Akt pathways. Sympathetic neurons were infectedwith adenoviruses expressing either GFP or RasV12, maintainedfor an additional day in NGF, withdrawn from NGF for 2 d, andsubsequently analyzed by Western blots for activation of MAPKand Akt using phosphorylation and activation state-specific antibodies(Fig. 1D). As expected, the levels of phosphorylation of bothAkt and the MAPKs were significantly higher in neurons maintainedin NGF than in those infected with GFP adenovirus and withdrawnfrom NGF for 48 hr (Fig. 1D). In neurons maintained in the absenceof NGF, expression of RasV12 led to strong phosphorylation ofboth Akt and the MAPKs to levels comparable with those seen inneurons maintained in 10 ng/ml NGF (Fig. 1D). Thus, these resultsshow that RasV12 expression is sufficient to sustain sympatheticneuron survival and can activate both MAPK- and Akt-signalingpathways in theseneurons.

Dominant-inhibitory Ras blocks NGF-induced survival of sympathetic neurons and Akt and MAPK phosphorylation

Neonatal sympathetic neurons require neurotrophin-mediated TrkA receptor activation for their survival, both in vivo (Levi-Montalciniand Brooker, 1960) and in culture (Levi-Montalcini and Angeletti,1963; Coughlin and Collins, 1985; Belliveau et al., 1997). Todetermine whether this TrkA-dependent survival is mediated viaRas, we generated a bicistronic recombinant adenovirus expressingN17Ras (Sigal et al., 1986) and GFP from the same promoter. Wethen confirmed that this adenovirus generated the appropriateprotein products. Sympathetic neurons were infected with N17Rasadenovirus in the presence of 10 ng/ml NGF, and 3 d later Westernblots for Ras and immunocytochemistry for c-myc were performed.The biochemical analysis (Fig. 4A) demonstrated overexpressionof a Ras-immunoreactive protein of ~21 kDa in neurons infectedwith the N17Ras adenovirus. In control neurons, a similar-sizedband was observed, corresponding to endogenous Ras, which waspresent at much lower levels (Fig. 4A). Fluorescence microscopyalso indicated that the majority of sympathetic neurons expressedN17Ras (Fig. 2B,D).

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Figure 4. Dominant-inhibitory Ras suppresses neurotrophin-mediated sympathetic neuron survival. A, Expression of dominant-inhibitory Ras in sympathetic neurons is shown. NGF-selected sympathetic neurons were infected with adenovirus expressing GFP or N17Ras; 3 d later, neurons were lysed, and equal amounts of protein were separated by gel electrophoresis. After transfer, the blot was probed with anti-Ras. Note that endogenous Ras can be seen in the GFP-infected neurons (arrow), but that N17Ras is expressed at much higher levels. As reported previously, Ras migrates at a slightly higher apparent molecular weight than 21 kDa (Cox et al., 1995). B, MTT assays for sympathetic neurons infected with various MOIs of recombinant adenovirus expressing either N17Ras or GFP in the presence of NGF are shown. Neurons were selected in 50 ng/ml NGF for 5 d, infected with adenovirus, and, 48 hr after the onset of the infection, switched into media containing 10 ng/ml NGF for an additional 2 d, before the MTT assay was performed. Values are normalized to that of 10 ng/ml NGF, which supports 100% neuronal survival (Belliveau et al., 1997), and error bars represent the SEM. A value that is statistically different from that of 10 ng/ml NGF is denoted by an * at p < 0.01(one-way ANOVA and post hoc Dunnett's multiple comparison test). Results are the means from three independent experiments. The GFP adenovirus has no effect on neuronal survival, whereas N17Ras significantly reduces NGF-mediated survival. C, Top, N17Ras decreases the levels of phosphorylation of Akt and MAPK in cultures maintained in NGF. After 5 d in 50 ng/ml NGF, cultures were infected with N17Ras or GFP control virus (200 MOI) for 24 hr in the presence of 10 ng/ml NGF. Three days later, cells were lysed, and equal amounts of proteins were analyzed by Western blotting using phosphorylation and activation state-specific antibodies against Akt or MAPK. Blots were reprobed with an antibody directed against total ERK1 (bottom bands). Shown is a representative blot of the experiment performed at least three times. Bottom, The intensity of each band (top), normalized against those of total ERK1, is shown in the bar graph. Note the decrease in the levels of NGF-mediated phosphorylation of both phospho-Akt (P-Akt) and, to a lesser extent, phospho-MAPK (P-ERK) in cultures infected with N17Ras.

Having confirmed that N17Ras was expressed in neurons, we then asked whether Ras activation was necessary for NGF-mediatedsympathetic neuron survival. Specifically, postnatal day 1 sympatheticneurons were cultured in 50 ng/ml NGF for 5 d, at which time theywere infected for 24 hr with the N17Ras adenovirus at variousMOIs. After infection, neurons were maintained in 10 ng/ml NGFfor 3 additional days, and survival was then quantified usingMTT assays (Manthorpe et al., 1986) (Fig. 4B). N17Ras expressiondecreased NGF-mediated sympathetic neuron survival by up to 43%,whereas infection with a control GFP-expressing adenovirus atthe same MOIs had no effect (Fig. 4B), indicating that Ras activationis required for at least a portion of the NGF-mediatedsurvival.

To confirm that this decrease in neuronal survival was caused by apoptosis, we examined neurons by Hoechst staining and TUNELanalysis 3 d after infection with N17Ras (Fig. 3). Quantitativeanalysis revealed that 4 ± 1% of neurons infected with an adenovirusexpressing only GFP and maintained in 10 ng/ml NGF were TUNELpositive (Fig. 3A). In contrast, infection with the N17Ras adenovirusincreased the percentage of TUNEL-positive nuclei to 32 ± 2% (Fig.3A). In addition, the TUNEL-negative neurons exhibited intact,rounded nuclei as revealed by Hoechst staining, whereas thosethat were TUNEL positive showed condensed and in some cases fragmentednuclei (Fig. 3B,C), the latter an indication of apoptotic deathinduced by growth factor deprivation (Darzynkiewicz et al., 1992;Deckwerth and Johnson, 1993; Edwards and Tolkovsky, 1994).

We then investigated whether infection with the N17Ras adenovirus led to inhibition of two of the signal transduction pathwaysactivated by RasV12 in these neurons, Raf/MEK/MAPK and PI3-K/Akt(Fig. 1D). In one set of experiments, sympathetic neurons werecultured in NGF for 5 d, infected with adenoviruses expressingeither GFP alone or N17Ras for 24 hr, and then maintained in 10ng/ml NGF for 3 additional days. Cells were subsequently lysedand analyzed for phosphorylation of MAPK and Akt using phosphorylationand activation state-specific antibodies. Western blot analysisrevealed that in cultures maintained in 10 ng/ml NGF, N17Ras induceda 42% decrease in phosphorylation of Akt and a 30% decrease inphosphorylation of MAPKs relative to that in neurons maintainedin NGF but infected with the GFP adenovirus (Fig. 4C). These resultsshow that Ras is necessary for a portion of NGF-induced sympatheticneuron survival and that cell death induced by N17Ras is accompaniedby a concomitant reduction in Akt and MAPKphosphorylation.

Ras sustains sympathetic neuron survival via multiple downstream effectors

Together, these results indicate (1) that Ras is a key regulator of sympathetic neuron survival, (2) that it signals via multiplepathways in sympathetic neurons, and (3) that at least one ofthese downstream pathways may mediate sympathetic neuron survival.To determine which of these pathways are involved in this response,we generated recombinant adenoviruses expressing Ras effectormutants that selectively activate downstream targets. Initially,we generated one Ras mutant, Ras^V12Y40C, that binds and activates PI3-K but not Raf, a second, Ras^V12T³⁵S, that binds and activates Raf and RalGDS but not PI3-K, a third,Ras^V12E37E, that activates RalGDS but neither Raf nor PI3-K, and a fourth,Ras^V12D38E, that activates Raf (Rodriguez-Viciana et al., 1997). Wethen confirmed that these effector mutants were expressed in sympatheticneurons at similar levels. Specifically, sympathetic neurons wereinfected with one of these four viruses, and 3 d later, Westernblot analysis was performed with anti-Ras. Ras^V12T³⁵S, Ras^V12Y40C, and Ras^V12E37G adenoviruses expressed immunoreactive proteins of the appropriatesize in sympathetic neurons (Fig. 5A). However, we could not obtainconsistent high Ras levels with the Ras^V12D38E adenovirus. In view of this, we used Ras^V12T³⁵S as a selective Raf/MEK/MAPK inducer.

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Figure 5. Ras sustains sympathetic neuronal survival via multiple signaling pathways. A, Expression of Ras effector mutants in sympathetic neurons is shown. Cells were infected with 100 MOI of adenoviruses expressing GFP, Ras^V12T³⁵S (RasT35S), or Ras^V12E37G (RasE37G) or with 200 MOI of Ras^V12Y40C (RasY40C) adenovirus for 3 d. Equivalent amounts of protein were separated by gel electrophoresis, as shown by the bottom bands, and Western blots were probed with anti-Ras. Note that the levels of expression of the different Ras effector mutants are comparable. B, Ras effector mutants differentially activate Ras downstream targets. Sympathetic neurons were infected with 200 MOI of Ras^V12Y40C, 100 MOI of Ras^V12T³⁵S, or 100 MOI of Ras^V12E37G in the presence of 30 ng/ml NGF, and 48 hr after the onset of the infection, NGF was withdrawn. As controls, neurons were infected with 100 MOI of GFP adenovirus and maintained in 10 ng/ml NGF (GFP + NGF). Two days after NGF withdrawal, cell lysates were prepared and normalized for equal amounts of proteins. Phosphorylation of MAPK and Akt was examined on Western blots using anti-phospho-MAPK (P-ERK) or anti-phospho-Akt (P-AKT). Note that Ras^V12Y40C only induces phosphorylation of Akt, whereas Ras^V12T³⁵S is able to induce phosphorylation of MAPK (ERK) but not Akt. As expected, Ras^V12E37G did not stimulate the phosphorylation of these two Ras downstream effectors. C-E, Ras sustains sympathetic neuron survival via PI3-K and Raf but not RalGDS. Sympathetic neurons were prepared and after 5 d in vitro infected with increasing MOIs of adenovirus expressing Ras^V12Y40C (C), Ras^V12T³⁵S (D), or Ras^V12E37G (E), which selectively activates PI3-K, Raf/MEK/MAPK, or RalGDS pathways, respectively. Results from the MTT assay performed 2 d after NGF withdrawal are expressed as the percentage of survival with 5 ng/ml NGF and are means ± SEM of quadruplicate wells from three independent experiments. Values are significantly different from that of NGF-deprived cultures (0 MOI) at p < 0.05 (*) or p < 0.01 (**) (one-way ANOVA and post hoc Dunnett's multiple comparison test).

We next confirmed that these effector mutants functioned as predicted in sympathetic neurons. Specifically, NGF-dependentsympathetic neurons were infected with adenoviruses expressingactivated Ras or one of the three effector mutants and were maintainedfor an additional 24 hr in NGF. Two days after NGF withdrawal,Western blot analysis was performed for phosphorylated Akt, adownstream target of PI3-K, or for phosphorylated MAPKs, downstreamtargets of Raf-1 and MEK (Fig. 5B). Ras^V12Y40C, which selectively activates PI3-K, induced phosphorylationof Akt but not phosphorylation of the MAPKs (Fig. 5B). Conversely,expression of Ras^V12T³⁵S led to phosphorylation of the MAPKs but not Akt (Fig. 5B). Finally,as predicted, Ras^V12E37GE failed to induce phosphorylation of these downstream substrates.In the case of each mutant, the phosphorylation of MAPK and Aktwas less than that observed with NGFtreatment.

Because the Ras effector mutants selectively activated the predicted pathways in sympathetic neurons, we next determined whetherthese proteins were capable of mediating sympathetic neuron survival.Neurons were grown for 5 d in 50 ng/ml NGF and infected with oneof the three Ras effector mutant-expressing adenoviruses, and48 hr later they were withdrawn from NGF for 2 d. MTT assays revealedthat Ras^V12Y40C maintained survival of sympathetic neurons in the absenceof NGF in a concentration-dependent manner (Fig. 5C), with a statisticallysignificant increase in survival first detected at 25 MOI. Atthe highest MOI used in this study (200 MOI), Ras^V12Y40C was able to mediate ~60% of the survival mediated by RasV12when these proteins were expressed at similar levels (data notshown). Similarly, Ras^V12T³⁵S was able to promote sympathetic neuron survival (Fig. 5D), althoughto a much lesser degree than was Ras^V12Y40C (Fig. 5C). Ras^V12E37G was unable to mediate sympathetic neuron survival at anyof the MOIs used either alone (Fig. 5E) or in combination withother effector mutants (data not shown), in spite of the factthat it was expressed at levels similar to that of the other twoeffector mutants (Fig. 5A). These results suggest that the RalGDSpathway is not important in mediating sympathetic neuron survivaland that Ras promotes sympathetic neuron survival via pathwaysoriginating primarily from PI3-K but also from Raf-1.

To confirm that Ras mediates neuronal survival via these two downstream pathways, we used two pharmacological agents: (1)PD 98059 that selectively inhibits MEK (which is immediately downstreamof Raf) and (2) LY 294002 that selectively inhibits PI3-K. Initially,we confirmed biochemically the selectivity of these pharmacologicalagents in sympathetic neurons. Specifically, sympathetic neuronswere selected in NGF, infected with adenoviruses expressing GFPor RasV12, and then switched to media without NGF containing 100µM LY 294002 or 75 µM PD 98059 for 2 d. As a control, uninfectedsister cultures were maintained in media containing 10 ng/ml NGFwith or without one of these two drugs. We then analyzed theseneurons for phosphorylation of Akt (downstream of PI3-K) and MAPKs(downstream of MEK) by Western blots. As shown previously in othercell types (Vlahos et al., 1994; Dudley et al., 1995), LY 294002inhibited the NGF-induced phosphorylation of Akt but had no effecton the phosphorylation of MAPK, whereas PD 98059 inhibited NGF-inducedphosphorylation of MAPKs but not of Akt (Fig. 6A). These two drugshad similar effects on substrate phosphorylation in response toactivated Ras. LY 294002 inhibited Ras-induced phosphorylationof Akt, with no effect on the phosphorylation of MAPK, whereasPD 98059 inhibited Ras-induced phosphorylation of MAPK, with noeffect on Akt (Fig. 6A).

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Figure 6. Inhibition of NGF- and Ras-mediated survival by the PI3-K inhibitor LY 294002 and the MEK inhibitor PD 98059. A, NGF-selected sympathetic neurons were infected with 100 MOI of adenoviruses expressing GFP or RasV12. Two days after the initiation of the infection, cultures were switched into media with no NGF but containing 100 µM LY 294002 or 75 µM PD 98059. As controls, mock-infected sister cultures were switched into media containing 10 ng/ml NGF plus one of the same two drugs. Two days later, neurons were lysed and analyzed by Western blotting with anti-phospho-Akt (P-AKT) and anti-phospho-MAPK (P-ERK). To ensure that similar amounts of proteins were present in all lanes, we reprobed the blot with an antibody against ERK1 (bottom bands). Note that, as expected, LY 294002 inhibits phosphorylation of Akt, whereas PD 98059 only affects phosphorylation of MAPK. B, C, PI3-K and MEK are required to mediate Ras survival effects on sympathetic neurons. B, Sympathetic neurons were infected with 100 MOI of GFP adenovirus and were switched to media containing 10 ng/ml NGF plus 100 µM LY 294002 (LY) or 75 µM PD 98059 (PD) 48 hr after the onset of the infection. MTT assays were performed 2 d later. Mock-infected sister cultures were also analyzed after the same treatment. C, Neurons were infected with 100 MOI of adenoviruses expressing GFP, RasV12, Ras^V12T³⁵S, or Ras^V12Y40C adenovirus (200 MOI) and 48 hr later switched to media containing no NGF and 100 µM LY 294002, 75 µM PD 98059, or both for 2 d before MTT assays. In B and C, results represent the means ± SEM of four to five replicates from three independent experiments and are expressed as the percentage of survival attained with 10 ng/ml NGF (B) or RasV12 (C). Results are different from their appropriate control (no drug treatment) at p < 0.05 (*) or p < 0.01 (**) (one-way ANOVA and post hoc Dunnett's multiple comparison test).

Having confirmed the selectivity of action of these two drugs, we next determined whether they inhibited the ability of RasV12to mediate sympathetic neuron survival, as predicted by the Raseffector data. As a baseline, we determined the effects of thesetwo drugs on NGF-induced survival of sympathetic neurons thatwere either mock infected or infected with an adenovirus expressingGFP (Fig. 6B). For this study, neurons were selected in 50 ng/mlNGF for 5 d, infected with GFP-expressing adenovirus (100 MOI),and after 48 hr switched for an additional 2 d to 10 ng/ml NGFwith or without PD 98029 or LY 294002, after which neuronal survivalwas measured by MTT assays. The PI3-K inhibitor LY 294002 decreasedby 70-80% the survival of uninfected or GFP-infected sympatheticneurons (Crowder and Freeman, 1998), whereas PD 98029 decreasedsympathetic neuron survival by <20% (Fig. 6B). Our results showingsuppression of survival by LY 294002 are similar to those of Crowderand Freeman (1998) but differ from those of Philpott et al. (1997).

We next determined the effects of these two drugs on the inhibition of sympathetic neuron survival as mediated by RasV12 orthe two Ras effector mutants Ras^V12T³⁵S and Ras^V12Y40C. NGF-dependent sympathetic neurons were infected with 100MOI of each of these three viruses and were then switched intomedia without NGF, containing either PD 98059 or LY 294002. Twodays later, we performed MTT assays to measure neuronal survival(Fig. 6C). Inhibition of MEK with PD 98059 completely abolishedthe ability of Ras^V12T³⁵S, which selectively activates Raf-1 and MEK, to promote sympatheticneuron survival (Fig. 6C), whereas LY 294002 had no effect. Thisresult further confirms that the effects of Ras^V12T³⁵S are mediated via Raf/MEK/MAPK rather than, or in addition to,RalGDS. Similarly, inhibition of PI3-K activity with LY 290042completely abolished the ability of Ras^V12Y40C, which selectively activates PI3-K, to mediate sympatheticneuron survival (Fig. 6C), whereas PD 98059 had no effect. Finally,as predicted by the Ras effector mutant data, LY 290042 and PD98059 were both independently able to inhibit survival mediatedby RasV12; inhibition of PI3-K by LY 290042 inhibited Ras-mediatedsurvival by ~60%, whereas both LY 290042 and PD 98059 togetherdecreased survival to near background levels. Thus, as indicatedby the effector mutant data, Ras mediates sympathetic neuron survivalvia activation of PI3-K/Akt and Raf/MEK/MAPK signal transductionpathways.

Activated Ras suppresses and dominant-inhibitory Ras induces the c-jun/p53/Bax pathway in sympathetic neurons

We have demonstrated recently that sympathetic neuron apoptosis after NGF withdrawal or p75 receptor activation is dependenton an apoptotic pathway that involves JNK, p53, and Bax (Aloyzet al., 1998). To determine whether activated Ras can suppressthis pathway, we infected sympathetic neurons with RasV12 adenovirusand biochemically examined proteins in this pathway. Sympatheticneurons were infected with RasV12 and withdrawn from NGF, and24-48 hr later, the levels of c-jun, p53, and Bax were examined.Withdrawal from NGF increased, as expected, the level and degreeof phosphorylation of c-jun (Ham et al., 1995; Bamji et al., 1998;Eilers et al., 1998) and increased the levels of p53 and Bax protein(Aloyz et al., 1998) in GFP-expressing adenovirus-infected culturesrelative to that in sister cultures treated with 10 ng/ml NGF(Fig. 7A). RasV12 expression inhibited the increases in c-jun,p53, and Bax protein levels that are observed after NGF withdrawal(Fig. 7A), coincident with its ability to rescue sympathetic neuronapoptosis.

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Figure 7. Dominant-inhibitory Ras induces and activated Ras suppresses the p53 apoptotic pathway. Sympathetic neurons were infected with 100 MOI of RasV12 (A) or GFP (A, labeled GFP $-$ NGF) or 200 MOI of N17Ras (B). Forty-eight hours after infection, the media were changed, and cultures were maintained in the absence (GFP $-$ NGF, RasV12 $-$ NGF) or presence (NGF, N17Ras + NGF) of 10 ng/ml NGF. Two days later, cells were lysed, and equal amounts of proteins were separated electrophoretically and transferred onto nitrocellulose membranes. Western blots were probed with anti c-jun, anti-p53, anti-Bax, anti- P-Akt, anti-P-ERK, and anti-ERK 1. Note that in NGF-treated cultures, N17Ras induces an increase in the levels of expression of c-jun and a shift to a larger apparent molecular weight, indicative of increased phosphorylation (B). RasV12 suppressed (A) whereas N17Ras increased the levels of p53 and Bax protein (B). Shown are representative blots of experiments performed at least four times. The lanes labeled ERK 1 indicate total protein amounts assayed. P-Akt, Phospho-Akt; P-ERK, phospho-MAPK.

To determine whether TrkA-induced activation of Ras mediates survival by suppressing the c-jun/p53/Bax apoptotic pathway,we inhibited Ras activity by infecting sympathetic neurons withN17Ras and examined the levels of c-jun, p53, and Bax. Specifically,neurons were maintained in NGF for 5 d, infected with either GFPor N17Ras-expressing adenovirus, and then maintained with or without10 ng/ml NGF for an additional 2 d. Expression of N17Ras elevatedthe levels of these apoptotic proteins in NGF-treated neurons(Fig. 7B), coincident with its ability to induce apoptosis. Thus,our results suggest that in sympathetic neurons, TrkA-mediatedactivation of Ras normally suppresses the c-jun/p53/Bax apoptoticpathway.

To provide genetic evidence that p53 is required for apoptosis induced by suppression of the NGF-activated Ras-signaling pathway,we asked whether suppression of p53 could prevent N17Ras-inducedsympathetic neuronal death in the presence of NGF. To suppressp53, we used an adenovirus vector that functionally ablates p53via the actions of E1B55K and targets p53 for degradation viathe adenovirus E4orf6 product (Yew and Berk, 1992; Querido etal., 1997; Teodoro and Branton, 1997; Aloyz et al., 1998). Wehave shown previously that this vector will suppress p53 levelsand rescue sympathetic neurons from NGF withdrawal and p75NTR-inducedcell death (Aloyz et al., 1998). As reported previously (Aloyzet al., 1998), after NGF withdrawal, E1B55K rescued up to ~55%of the neurons relative to those maintained in 10 ng/ml NGF (Fig.8). Maximal antiapoptotic effects of E1B55K were attained at 300MOI of E1B55K, which was thus used for subsequent experiments.Expression of E1B55K significantly blocked the apoptotic effectsof N17Ras in neurons maintained in the presence of NGF (Fig. 8).In data from three separate experiments, N17Ras expression inhibitedneuronal survival by 42%, whereas coexpression of E1B55K withN17Ras reduced neuronal loss to 17%. Infection with control GFPadenovirus (300 MOI) did not affect the decrease in neuronal survivalinduced by N17Ras (Fig. 8). These results further suggest thatthe antiapoptotic effects of Ras are caused by its inhibitionof the p53 proapoptotic protein in sympathetic neurons.

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Figure 8. p53 is required for neuronal death induced by suppression of NGF-induced Ras activity. Sympathetic neurons maintained in the presence of 10 ng/ml NGF were infected with increasing MOI of E1B55K (which functionally ablates p53) and withdrawn from neurotrophin support 48 hr after infection. Neurons were also infected with 200 MOI of N17Ras either alone or with the simultaneous addition of either 300 MOI of E1B55K (E1B) or, as a control, 300 MOI of GFP and kept in the continuous presence of 10 ng/ml NGF. In all cases, neurons were processed for MTT assays 96 hr after infection. Values are normalized as the percentage of survival attained with 10 ng/ml NGF and represent means ± SEM of quadruplicate wells from three experiments. Values for N17Ras + GFP are significantly different from those for N17Ras + E1B55K at p < 0.05 (*) (one-way ANOVA and post hoc Dunnett's multiple comparison test). E1B55K significantly blocked the apoptotic effects induced by N17Ras in NGF-treated cultures.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In this study, we have examined the role of Ras and its multiple signal transduction pathways in neurotrophin-induced survivalresponses of postnatal rat sympathetic neurons, during the periodcorresponding to the time point when these neurons undergo naturallyoccurring cell death in vivo. Our results support several conclusions.First, activation of Ras is necessary and sufficient for a portionof NGF sympathetic neuron survival. Second, neurotrophins inducethe phosphorylation of both Akt and MAPK in these neurons in aRas-dependent manner. Third, the antiapoptotic effects of Rasare mediated primarily by PI3-K, and partially by MEK, but notby RalGDS. Fourth, Ras appears to regulate sympathetic neuronsurvival by suppressing the activity or levels of c-jun, p53,and Bax, which are components of the key pathway mediating naturallyoccurring cell death in these neurons (Deckwerth et al., 1996;Xiang et al., 1996, 1998; Aloyz et al., 1998; Bamji et al., 1998;Eilers et al., 1998). Fifth, p53 activity is required for apoptosisinduced by suppression of the NGF-activated Raspathway.

Ras as a major mediator of sympathetic neuron survival

In agreement with previous reports on the role of Ras in rat sympathetic SCG neurons (Nobes and Tolkovsky, 1995; Nobes etal., 1996), we show that Ras is a major mediator of NGF-inducedsympathetic neuron survival. The authors of these previous reportsused scrape loading of anti-Ras antibodies into newly isolatedpostnatal sympathetic neurons to show that Ras was responsiblefor approximately one-half of NGF-dependent neuronal survival.Similarly, we find that activated Ras supports, and N17Ras suppresses,approximately one-half of the survival responses of postnatalday 5 sympathetic neurons expressing these proteins via recombinantadenovirus. The observation that only one-half of the sympatheticneurons are affected by these manipulations of Ras activity couldbe attributable to low levels of expression of exogenously expressedRas proteins or to the presence of both Ras- and non-Ras-dependentsurvival pathways in sympathetic neurons. It is unlikely thatthe expression of activated Ras via adenovirus was insufficientto promote complete survival responses, because (1) most cellsin each experiment were infected by adenovirus, (2) increasingthe virus particles per cell did not increase the ability of activatedRas to increase neuronal survival beyond 50% of the cells, and(3) activated Ras strongly stimulated MAPK and Akt phosphorylation,the latter a major mediator of sympathetic neuron survival (Crowderand Freeman, 1998). The same N17Ras adenovirus did fully blockneurite outgrowth responses and induced apoptosis of NGF-dependentPC12 cells (I. E. Mazzoni, F. D. Miller, and D. Kaplan, unpublishedobservations), indicating that the N17Ras adenovirus that we usehas the potential to inhibit NGF responses of cells completely.Therefore, the inability of activated Ras to fully stimulate andN17Ras to fully inhibit survival suggests that TrkA mediates atleast one-half of neuronal survival in a Ras-independent manner.These results suggest to us that multiple signaling pathways regulatesurvival, with some pathways (PI3-K) being crucial for the survivalof most cells and others (Ras) being necessary if completely andefficiently suppressed. It is also possible that the strengthof PI3-K survival signaling depends on the relative importanceof Ras-dependent and -independent signaling in a given neuron.The later may include Ras-independent mechanisms regulating PI3-K-derivedsurvival, such as through Gab-1 (Holgado-Madruga et al., 1997)or TrkA-activated proteins such as phospholipase C- $gamma$ 1, SRC, rAPS1,SH2-B, fibroblast receptor substrate-2, and SVC-associated neurotrophicfactor target (Kaplan and Miller, 1997; Kouhara et al., 1997;Qian et al., 1998).

Studies in non-neuronal cells have shown that Ras has the potential to activate a large number of downstream effectors andmay do so in a cell-specific manner (for review, see Quilliamet al., 1995; Marshall, 1996; Vojtek and Der, 1998). Furthermore,activation of different Ras-dependent pathways can lead to distinctbiological responses (Joneson et al., 1996; Khosravi-Far et al.,1996; Rodriguez-Viciana et al., 1997). Our data provide evidencethat, in sympathetic neurons, Ras can stimulate both MEK/MAPKand PI3-K/Akt pathways and, moreover, that Ras sustains neuronalsurvival via multiple signal transduction pathways as well. Boththe MEK/MAPK- and PI3-K/Akt-signaling pathways, activated by Ras^V12T³⁵S and Ras^V12Y40C, respectively, contributed ~40 and 60% of the maximal survivaleffects induced by activated Ras. Similarly, treatment of neuronswith the MEK inhibitor PD 98059, together with the PI3-K inhibitorLY 294002, completely abolished the survival-inducing effectsof activated Ras. These results suggest that MEK and PI3-K activityaccount for most, if not all, of the survival effects inducedby activated Ras in sympathetic neurons. PI3-K, however, appearedto be the dominant Ras effector protein for survival responses.In this regard, N17Ras blocked Akt phosphorylation more efficientlythan MAPK phosphorylation. Furthermore, expression of Ras^V12T³⁵S, which specifically induces MEK and MAPK activity, was lessefficient at stimulating survival than was Ras^V12Y40C, which specifically stimulates PI3-K and Akt activity. Otherinvestigators have also shown that MEK plays only a minor rolein NGF-mediated survival of sympathetic neurons (Virdee and Tolkovsky,1995a,b; Creedon et al., 1996). In our experiments, PI3-K wasrequired for 60% of Ras-induced and 80% of NGF-induced neuronalsurvival. Although the activities of PI3-K and Akt have been shownto be sufficient to sustain sympathetic neuronal survival, thereare contradictory reports on whether their activities are necessaryto mediate NGF's antiapoptotic effects (Philpott et al., 1997;Crowder and Freeman, 1998). Our results agree with those of Crowderand Freeman (1998), who also used LY 294002, as well as dominant-inhibitoryPI3-K and Akt, to inhibit sympathetic neuron survival. Our resultsalso suggest that much, but not all, of PI3-K-induced neuronalsurvival is caused by Ras activity and agree with recent studiesperformed in sensory neurons showing that Ras-dependent activationof PI3-K is necessary to induce neuron survival (Klesse and Parada,1998).

Another downstream effector stimulated by Ras, RalGDS, did not affect neuronal survival because expression of Ras^V12E37G, which activates this pathway (Rodriguez-Viciana et al.,1997), could not sustain, either in combination with Ras^V12Y40C or Ras^V12T³⁵S (Mazzoni., Miller, and Kaplan, unpublished observations) oralone (Fig. 5E), sympathetic neuron survival after NGF withdrawal.Ras^V12E37G expression did not augment or inhibit the survival effectsobserved with the other Ras effector mutant Ras^V12T³⁵S (Mazzoni, Miller, and Kaplan, unpublished observations). Nevertheless,we cannot rule out a survival role for other Ras effector proteins,such as Rin1, p120GAP, and AF6 (for review, see Quilliam et al.,1995; Marshall, 1996; Vojtek and Der, 1998), whose expressionand function in sympathetic neurons remain to bedetermined.

Mechanism of Ras-mediated suppression of apoptosis

What is the mechanism by which Ras mediates NGF-dependent survival? In postnatal sympathetic neurons, both in vivo duringthe period of naturally occurring cell death and in vitro, thebalance between survival and apoptosis depends on the relativestrengths of TrkA prosurvival signals and p75NTR-mediated apoptoticsignals (Aloyz et al., 1998; Bamji et al., 1998). A similar findinghas been reported in oligodendrocytes (Yoon et al., 1998). Apoptosisof sympathetic neurons induced by both p75NTR and NGF deprivationis regulated via a common cell death sensor, p53. We have shownrecently that p53 is necessary and sufficient for inducing apoptosisin postnatal sympathetic neurons both in vivo and in culture (Slacket al., 1996; Aloyz et al., 1998). In this regard, we demonstratedthat p53 is upregulated in response to NGF withdrawal as wellas after p75NTR activation, both of which involve signaling viathe MEK kinase(MEKK)/JNK pathway (Estus et al., 1994; Ham et al.,1995; Casaccia-Bonnefil et al., 1996; Bamji et al., 1998). Furthermore,we found p53 to lie downstream of JNK and upstream of Bax (Aloyzet al., 1998). Here we show that expression of activated Ras suppresses,whereas N17Ras increases, c-jun, p53, Bax levels, anti-P-Akt,anti-P-ERK, and anti-ERK 1. In addition, functional ablation ofp53 by E1B55K prevents apoptotic neuronal death induced by N17Rasin NGF-treated cultures. The observation that E1B55K could notcompletely rescue N17Ras-treated cultures to control (NGF-treated)values could mean that additional apoptotic pathways are operationalin these cells. These might include Akt-induced phosphorylationof the Bad and forkhead apoptotic proteins (Datta et al., 1997;Brunet et al., 1999), although we have not found Bad to be phosphorylatedin NGF-treated sympathetic neuron cultures. On the basis of ourdata, we propose that Ras and its effectors PI3-K/Akt, and toa lesser extent MEK/MAPK, are major signaling proteins used byTrkA to suppress apoptosis. Thus, sympathetic neuron survivalmay not depend on the relative strengths of independent pro- andantiapoptotic signaling pathways. Rather, neuronal survival maybe dependent on the ability of TrkA-activated Ras, and on theRas-activated effectors PI3-K/Akt and MEK, to suppress the MEKK/JNK/p53/Baxcell death pathway. Because p53 is a primary cell death sensorfor PNS and CNS neurons undergoing cell death because of excitotoxicity,survival factor deprivation, and p75NTR activity (Morrison etal., 1996; Aloyz et al., 1998; Bamji et al., 1998; Xiang et al.,1998), Ras could function in many neuronal contexts as a generalsuppressor of p53 apoptoticactions.

  FOOTNOTES

Received May 12, 1999; revised Aug. 20, 1999; accepted Sept. 1, 1999.

This work was supported by grants from the Medical Research Council of Canada and from the Neuroscience Network to D.K. andF.D.M. D.K. is a recipient of the Harold Johns and Canadian CancerSociety Research Scientist Award, and F.D.M. is a Killam Scholar.I.E.M. is funded by a fellowship from the Natural Sciences andEngineering Research Council of Canada. We thank Dr. P. Warne(Imperial Cancer Research Fund, United Kingdom) and Dr. C. Bazenet(EISAI London Research Laboratories, United Kingdom) for providingus with the mutated Ras constructs, Dr. L. Paquet (Exogen Neurosciences,Montreal, Quebec, Canada) for his helpful advice, and B. Bourqueand M. Ahkavan for technicalassistance.
Correspondence should be addressed to Dr. D. Kaplan or Dr. F. Miller, Center for Neuronal Survival, Montreal NeurologicalInstitute, 3801 rue University, Montreal, Quebec, Canada H3A 2B4.E-mail: mcdv{at}musica.mcgill.ca.

Dr. Mazzoni's present address: Caprion Pharmaceuticals, 6100 Royalmont Avenue, Montreal, Quebec, Canada H4P2R2.

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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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