Proteasome Involvement and Accumulation of Ubiquitinated Proteins in Cerebellar Granule Neurons Undergoing Apoptosis

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The Journal of Neuroscience, January 15, 2000, 20(2):589-599

Proteasome Involvement and Accumulation of Ubiquitinated Proteins in Cerebellar Granule Neurons Undergoing Apoptosis
Nadia Canu¹, Christian Barbato¹, Maria Teresa Ciotti², Annalucia Serafino³, Laura Dus², and Pietro Calissano¹^,²
¹ Dipartimento di Neuroscienze, Facoltà di Medicina e Chirurgia, Università di Tor Vergata, 00133 Roma, Italia, ² Istituto di Neurobiologia, Consiglio Nazionale delle Ricerche (CNR), 00137 Roma, Italia, and ³ Area di Ricerca di Roma, Tor Vergata, CNR, 00133 Roma, Italia

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We investigated the potential role of the ubiquitin proteolytic system in the death of cerebellar granule neurons inducedby reduction of extracellular potassium. Inhibitors of proteasomalfunction block apoptosis if administered at onset of this process,but they do not exert such effect when added 2-3 hr later. Thesame inhibitors also prevent caspase-3 activity and calpain-caspase-3-mediatedprocessing of tau protein, suggesting that proteasomes are involvedupstream of the caspase activation. Although the proteasomes seemto play an early primary role in programmed cell death, we foundthat with progression of apoptosis, during the execution phase,a perturbation in normal ubiquitin-proteasome function occurs,and high levels of ubiquitinated proteins accumulate in the cytoplasmof dying cells. Such accumulation correlates with a progressivedecline of proteasome chymotrypsin and trypsin-like activitiesand, to a lower extent, of postacidic-like activity. Both intracytoplasmicaccumulation of ubiquitinated proteins and decline of proteasomefunction are reversed by the pan-caspase inhibitor Z-VAD-fmk.The decline in proteasome function is accompanied by, and likelyattributable to, a marked and progressive decline of deubiquitinatingactivities. The finding that the proteasomes are early involvedin apoptosis and that ubiquitinated proteins accumulate duringthis process prospect granule neurons as a model system aimedat correlating these events with neurodegenerativediseases.

Key words: apoptosis; neurodegeneration; ubiquitin-protein conjugates; proteasome activity; deubiquitinating activity; cerebellar granule neurons

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The presence of intracellular inclusions of insoluble aggregates of ubiquitin protein conjugates is a hallmark of chronicneurodegenerative diseases and, to lesser extent, of physiologicalbrain aging (Lowe et al., 1993). To date, the mechanism or mechanismsleading to such aberrant deposits is unknown. Over time, the accumulationof ubiquitinated proteins results in pathological aggregates thatperturb the normal physiology of affected neurons and lead toproteotoxicity.

Ubiquitination of proteins is required for rapid degradation of short-lived or of damaged proteins by the ubiquitin-proteasomesystem. This is the major proteolytic system in the cytosol ofeukaryotic cells endowed with multiple activities, referred toas chymotrypsin-like, trypsin-like, and postacidic or caspase-likeactivities (Peters, 1994).

In the ubiquitin-proteasome pathway, proteins are first modified by the covalent conjugation to multiple ubiquitin moleculesthat subsequently tag the conjugates for rapid hydrolysis by theproteasome. This complex hydrolyzes exhaustively target proteinsreleasing small peptides, most of which are further degraded bycellular exopeptidases, with concomitant recycling of ubiquitinmolecules by deubiquitinating enzymes (Wilkinson, 1997).

A growing number of studies indicate that ubiquitin-mediated proteolysis plays important roles in a variety of basic cellularprocesses such as regulation of cell cycle and division, responseto cellular stress, morphogenesis of neuronal network, long-termsynaptic plasticity, transcriptional regulation of cell surfacereceptors (Jentsch 1992; Ciechanover 1994; Hochstrasser 1995),and activation of the transcription factor NF-KB (Palombella etal., 1995). Moreover, several observations suggest that a perturbationin ubiquitin-proteasome function plays a critical role in theaccumulation of misfolded or modified proteins such as pairedhelical filaments in Alzheimer's disease (Morishima-Kawashimaet al., 1993), nuclear aggregates of huntingtin in Huntington'sdisease (DiFiglia et al., 1997), and aggregation of $alpha$ -synucleinin Parkinson's disease (Takeda et al., 1998). The inability ofremoving ubiquitin conjugates may result from an altered proteolyticdegradation or from a modification of damaged proteins that makesthem inaccessible to proteolyticmachinery.

It has been recently reported that the proteasome system is critically involved in programmed cell death, by acting upstreamof caspase activation. Generally, proliferating cells respondto inhibitors of proteasome function by activation of apoptosis,whereas in nondividing cells (sympathetic neurons or T-cells)such inhibitors exert antiapoptotic effects (Grimm et al., 1996;Sadoul et al., 1996; Drexler, 1997). On the other hand, it hasbeen postulated that apoptosis plays a role in the pathogenesisof neurodegenerative diseases (Su et al., 1994; Smale et al.,1995; Thompson, 1995).

In view of the postulated connection of apoptotic death, altered proteasome function, and neurodegenerative diseases, we investigatedthe role of ubiquitin-proteasome system in an in vitro model ofcerebellar granule cells (CGCs) undergoing massive apoptotic deathafter removal of depolarizing concentration of potassium (D'Melloet al., 1993). We report that the proteasome system appears twiceinvolved during apoptosis: first, its function is crucial in theearly phase, upstream caspase activation, then, in the executionphase, proteasome function declines with consequent accumulationof ubiquitinated proteins. Moreover, an impairment of deubiquitinatingactivities accompanies and likely contributes to the proteasomefailure.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The proteasome inhibitors PSI [Z-Ile-Glu (OtBu)-Ala-Leucinal] and Lactacystin and the caspase inhibitor z-VAD-fmk (Benzyloxycarbonyl-Val-Ala-Asp-fluoromethylchetone)were from Calbiochem (La Jolla, CA). The proteasome inhibitorMG132 (N-CBZ-Leu-Leu-Leu-Al), the calpain inhibitor II ALLM (N-acetyl-Leu-Leu-Methioninal),E64d (trans-epoxy succinyl-L-leucylamydo-3-methyl-butane ethylester), and leupeptin were purchased from Sigma (St. Louis, MO).Substances were dissolved in dimethylsulfoxide at 1000× concentration.No more than 0.1% solvent was present in culture medium. The fluorogenicsubstrates for proteasome assay Suc-LLVY-MCA (succinyl-Leu-Leu-Val-Tyr-7-amido-4-methylcoumarin),Boc-LRR-MCA (N-t-boc-Leu-Arg-Arg-7-amido-4-methylcoumarin), andZ-LLE- $beta$ Nap (N-CBZ-Leu-Leu-Glu- $beta$ -naphtylamide) were from Sigma.Multi-ubiquitin chains [Ub4, Ub3 and Ub2, and the monoclonal antibody(mAb) to $alpha$ -type subunits (PW8195)] were from AFFINITI ResearchProducts Ltd. Ac-DEVD-AMC was from BIOMOL">Biomol (Plymouth Meeting, PA).Rabbit anti-ubiquitin was from Dako (Carpinteria,CA).

Neuronal cultures. Cultures enriched in granule neurons were obtained from dissociated cerebella of 8-d-old Wistar rats (CharlesRiver, Calco, Italy), as described by Levi et al. (1984). Cellswere plated in basal medium Eagle (BME; Life Technologies, Gaithersburg,MD) supplemented with 10% fetal bovine serum, 25 mM KCl, and 2mM glutamine (Life Technologies) on dishes (Nunc, Roskilde, Denmark)coated with poly-L-lysine. Cells were plated at 2.5 × 10⁶ per 35 mm dish or 7 × 10⁶ per 60 mm dish. 1 $beta$ -Arabinofuranosylcytosine (10 mM) was addedto the culture medium 18-22 hr after plating to prevent proliferationof non-neuronalcells.

Induction of apoptosis. Cultures at 6-7 days in vitro (DIV) were washed two times and switched in serum-free BME containing5 mM KCl supplemented with glutamine and gentamicin. Control cellswere washed with BME and maintained in serum-free medium containing25 mM KCl (D'Mello et al., 1993).

Assessment of neuronal viability. Viable granule neurons were quantified by counting the number of intact nuclei after lysingthe cells in detergent-containing solution by the method of Sotoand Sonnenschein (1985) modified by Volontè et al. (1994) andby the MTT tetrazolium salt assay , as described by Manthorpeet al. (1986). Briefly, MTT tetrazolium salt (0.25 mg/ml) wasadded to neurons grown in 24-well plates and incubated for 1-2hr at 37°C. The reaction media were then gently aspirated, andisopropanol containing 0.08 N HCl was added to solubilize theblue formazan product. Formazan-isopranol mixtures were then transferredto 96-well plates and quantified using a Multiskan plate readerat 570 nm (Labsystems Multiskan MCC/340).

Immuofluorescence. Cerebellar granule cells were fixed with 4% paraformaldehyde (w/v in PBS) for 15 min at room temperature,washed in PBS, pH 7.5, and then permeabilized with 0.1%TritonX-100 and Tris-Cl, pH 7.5, for 5 min. The coverslips were treatedwith polyclonal antibody against ubiquitin (Dako; 1:100) in amoist chamber overnight at 4°C, rinsed in PBS, and stained withFITC-conjugated secondary antibodies (Sigma) for 30 min. Nucleiwere stained with propidium iodide (Sigma; 5 µg/ml) and RNase(100 µg/ml) in PBS for 5 min at room temperature. Confocal microscopywas performed with a Leica (Nussloch, Germany) TCS 4D system,equipped with 100× 1.3-0.6 oil-immersion objective (optical section,1 µM). Images of double-labeled samples were recorded with simultaneousexcitation and detection of both dyes to ensure proper image alignment.Optical sections were stereo-pair and three-dimensional reconstituted.To correct for possible crosstalk resulting from overlapping excitationand emission spectra of the dyes used, when necessary, recordedimages were corrected using the MultiColor analysis package softwarebyLeica.

Caspase-3 activity: DEVD-MCA cleavage assay. DEVD-MCA cleavage activity was measured , as described by Armstrong et al. (1997).After 12 hr in S-K5, 500,000 granule cells were washed once withPBS and lysed in 100 µl of buffer A (10 mM HEPES, pH 7.4, 42 mMKCl, 5 mM MgCl₂, 1 mM DTT, and 1 mM PMSF, 0.5% 3-[(3-cholamidopropyl)dimethylammonio]-1-propanesulfonicacid (CHAPS), and 1 µg/ml leupeptin). Twenty-five microlitersof lysate was combined with 75 µl of buffer B (25 mM HEPES, 1mM EDTA, 0.1% CHAPS, 10% sucrose, and 3 mM DTT, pH 7.5) containing30 µM Ac-DEVD-AMC and incubated for 20 min at room temperature.Fluorescence was measured at an excitation of 380 nm and an emissionof 460 nm using a Kontron AG (Zurich, Switzerland) SFMspectrofluorometer.

Fluorogenic peptide substrate assay for proteasome activity. CGCs were lysed in ice-cold homogenization buffer [20 mM Tris/HCl,pH 7.2, 0.1 mM EDTA, 1 mM 2-mercaptoethanol, 5 mM ATP, 20% (v/v)glycerol, and 0.04% (v/v) Nonidet P-40, as described in Beyetteet al. (1998)]. Lysates (10 µg) of CGCs were incubated at 37°Cwith the fluorogenic substrates Suc-LLVY-MCA (50 µM), Boc-LRR-MCA(100 µM), and Z-LLE- $beta$ Nap (400 µM) in 100 µl of 50 mM HEPES, pH8, 5 mM EGTA, for 20, 30, and 60 min, respectively. The reactionwas stopped by adding 900 µl of SDS (1%). Hydrolysis of peptideswas measured at 380 nm excitation and 460 emission for MCA andat 335 nm excitation and 410 nm emission for $beta$ Nap using a KontronSFMspectrofluorometer.

Western blot analysis. Equal amounts of proteins were subjected to SDS-PAGE on 8-15% linear gradient gels (Laemmli, 1970).After electroblotting to nitrocellulose (Hybond-C), proteins werevisualized using appropriate primary antibodies. All primary antibodieswere diluted in 0.5% (w/v) nonfat dry milk and incubated withthe nitrocellulose blot overnight at 4°C. Incubation with secondaryperoxidase-coupled anti-mouse or anti-rabbit antibodies was performedat room temperature for 45 min. Blots were developed by usingthe ECL system (Amersham, Arlington Heights, IL). Developmentsof Western blots were terminated before band intensity was saturated;relative optical densities and areas of bands were quantifiedusing a computerized image analysissystem.

Preparation of protein extracts from CGCs and assay for deubiquitinating activity. CGCs were collected and resuspended inice-cold lysis buffer (20 mM Tris-HCl, pH 7.2, 10 mM MgCl₂, 1mM EDTA, 5% glycerol, 1 mM DTT, 1 µg/ml aprotinin, and 1 µg/mlpepstatin) and frozen and thawed three times. The extracts werecentrifuged, and supernatants were stored at $-$ 70°C as 50% glycerolsolutions. Assay of deubiquitinating enzyme (DUB) activity wasconducted at 22°C in a buffer containing 50 mM Tris-HCl, pH 7.3,and 5 mM DTT in a total volume of 30 µl. Reaction mixture contained5 µg of CGC extract and 1 µg of multi-ubiquitin chains. Aliquotsof 5 µl were removed and separated by 12.5% polyacrylamide gels,using a Tricine gel system (Schagger and von Jagow, 1987), transferredto Immobilon P membranes (Millipore, Bedford, MA) and analyzedby anti-ubiquitinantibody.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Inhibition of proteasome function rescues granule neurons from K⁺ deprivation-induced cell death

Rat cerebellar granule neurons can be induced to undergo apoptosis if the potassium concentration is reduced to 5 mM (K5)and serum is removed (S $-$ ) after a period of initial growth in25 mM potassium (K25) and serum (S+) (D'Mello et al., 1993; Galliet al., 1995). Commitment to apoptosis occurs between 2 and 6hr after K⁺ deprivation (Galli et al., 1995; Schulz et al., 1996; Nardi etal., 1997) and at 6-8 hr degenerative changes such as chromatincondensation, vacuole formation, DNA fragmentation, and neuriteretraction become detectable (D'Mello et al., 1993; Schulz etal., 1996; Armstrong et al., 1997). Moreover, during the sameperiod the microtubule-associated protein tau is being degradedby caspase-3 and calpain to a 17 kDa fragment that accumulatesin perikarya of dying neurons (Canu et al., 1998), and an amyloidogenicroute leading to an increased secretion of $beta$ -amyloid is activated(Galli et al., 1998).

Because the proteasome system has been implicated as a positive mediator of apoptosis triggered by damaging stimuli in terminallydifferentiated cell types e.g., by degrading regulatory proteinsthat normally inhibit the apoptotic pathway or activating proteinsthat promote cell death likely working upstream the caspase-activation(Grimm et al., 1996; Sadoul et al., 1996), we investigated theinvolvement of proteasome system in the CGC model of neuronalapoptosis. To this aim the effects of a panel of proteasome inhibitorson the survival of CGCs were examined. The peptide aldehydes MG132and PSI [Z-IE(OtBu)AL-CHO] have been shown to reversibly inhibitthe proteolytic activity of proteasomes (Figueiredo-Pereira etal., 1994; Rock et al., 1994), whereas Lactacystin, a microbialmetabolite, irreversibly blocks the proteasome function (Fenteanyet al., 1995). These substances were added before or simultaneouslywith the induction of apoptosis, and neuronal survival was assessed12 hr later because at longer incubation times these inhibitorsbecome toxic. Cell viability was analyzed by counting the numberof intact nuclei and by the MTT assay, as described in Materialsand Methods. Results shown in Figure 1, A and B, provide evidencethat MG132 and Lactacystin significantly inhibit apoptosis. MG132was a more potent inhibitor of cell death, producing >90% inhibitionof cell death at 2 µM as compared with Lactacystin, which inhibitscell death by 85% at 25 µM. In the presence of these compounds,the cell bodies of neurons and the neurites remained intact for12-18 hr (data not shown). By contrast, PSI protects CGCs fromapoptosis only partially (20%) and at 50-100 µM as assessed bycounting the number of intact nuclei. Very similar results areobtained when viability is assayed with the MTT procedure (Fig.1B) with a slight difference at high concentration of PSI (50µM), indicating that the mitochondrial function is still partiallyoperative in a portion of neurons. Because MG132 also affectscalpain and cathepsin besides proteasomes, we also tested theeffect of ALLM (5-50 µM), E64d ester (20-100 µM), and leupeptin(20-100 µM), which are cell-permeable inhibitors of calpain andcathepsin. As indicated in Figure 1C, these agents failed to rescueCGCs from apoptosis, suggesting that MG132 elicits its effectsby acting primarily on proteasomes.

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Figure 1. Inhibitors of proteasome rescue cerebellar neurons from apoptosis. Cultures at 6 DIV were washed and maintained in high-potassium and serum-free medium (S-K25) or switched to K5 and serum-free medium (S-K5) in the absence or in the presence of different concentrations of proteasome inhibitors. After 12 hr, cell viability was determined by counting the number of intact nuclei (A) or by MTT assay (B), as described in Materials and Methods. C, Effect of calpain and cathepsin inhibitors on cell survival. ALLM, E64d, and leupeptin were added to the medium at the concentrations indicated. Twelve to 15 hr after apoptosis induction, granule neurons were analyzed for survival, as described in Materials and Methods. Results are means ± SD of duplicate determinations of three independent experiments.

We found that MG132 must be added within 1 hr after induction to efficiently block apoptosis (Fig. 2), whereas no rescuingeffect was noticed when this agent was given 3 hr after the apoptoticstimulus. Identical results were obtained with Lactacystin (datanot shown). This finding supports the hypothesis that proteasomeinhibitors act on the early events of apoptosis (Grimm et al.,1996; Sadoul et al., 1996) and become ineffective after the commitmentpoint that occurs between 2-6 hr after apoptotic stimulus (Galliet al., 1995; Schulz et al., 1996; Nardi et al., 1997).

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Figure 2. Rescue time by MG132 on granule neurons undergoing apoptosis. Cells were exposed to 5 µM MG132 either 1 hr before (<1 hr) or at different times after apoptotic stimulus. The number of viable cells was determined 12 hr later, as described in Materials and Methods.

Inhibition of proteasome function prevents caspase-3 activity and cleavage of the microtubule-associated protein tau

The execution phase of apoptosis is initiated by activation of specific proteases of the caspase family (Steller, 1995). Ofthe caspases, caspase-3 is that involved in the cleavage of mostapoptotic substrates (Cohen, 1997). An increase of caspase-3 activityis also present in extracts of granule neurons undergoing apoptosis(Eldadah et al., 1997; Marks et al., 1998; Bobba et al., 1999).We investigated the role of proteasome with respect to this proteaseactivity. Primary CGCs were induced to die in the absence or inthe presence of MG132 (5 µM), Lactacystin (25 µM), and PSI (20and 50 µM). Twelve hours later caspase-3 activity was assayedby the cleavage of the fluorogenic substrate Ac-DEVD-MCA (Enariet al., 1996). As shown in Figure 3A, neurons undergoing apoptosisexhibited a 12- to 13-fold elevation of caspase-3 activity ascompared to controls. Caspase activation induced by apoptosisis partially inhibited by MG132, Lactacystin, and PSI to an extentwhich, at least in part, mirrors their anti-apoptotic effect.To date, only few intracellular substrates of activated caspase-3have been identified in CGCs undergoing apoptosis (Nath et al.,1996; Canu et al., 1998). For instance we have reported that inCGCs undergoing apoptosis the microtubule-associated protein tauis a substrate for both caspase-3 and calpain with a productionof a diagnostic fragment of 17 kDa and concomitant collapse ofthe microtubule network (Canu et al., 1998). Whole-cell extractsprepared from CGCs incubated in the presence of MG-132 and lactacystinwere analyzed by SDS-PAGE, electroblotted, and probed with theanti-tau antibody, mAb Tau-1. As shown in Figure 3B we found thatthe 17 kDa band, corresponding to the major cleavage product oftau previously described, is not detectable in the presence ofproteasome inhibitors. These findings suggest that these agentsblock proteasome function upstream the activation of proteasessuch as caspase-3 and calpain, a conclusion also supported bythe observation that the same inhibitors prevent the release ofcytochrome c (A. Bobba, N. Canu, A. Atlante, E. Marra, and P.Calissano, unpublished observation), an event preceding caspase-3activation in CGCs undergoing apoptosis (Bobba et al., 1999).

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Figure 3. Inhibitors of the proteasomes block caspase activity and prevent cleavage of tau. A, Cultures were switched to S-K5 medium in the absence or in the presence of proteasome inhibitors MG132 (5 µM), Lactacystin (25 µM), or PSI (20 or 50 µM). Control cultures were switched to S-K25. After 12 hr, cultures were lysed and assayed for DEVD-MCA cleavage. Accumulation of MCA was assayed fluorometrically after 20 min at room temperature. Data are reported as the percentage of the rate of cleavage in S-K25 extracts (100%). B, Tau cleavage was analyzed by immunoblotting of cell extracts 12 hr after induction of apoptosis triggered in the absence or in the presence of 1 µM MG132 or 25 µM Lactacystin (LC). The mouse monoclonal antibody Tau-1 was used to detect tau cleavage (Canu et al., 1998).

Proteasome activity decreases during apoptosis

The proteasome can cleave peptides on the carboxyl side of hydrophobic, basic, and acid residues (Orlowski, 1990). These proteolyticfunctions commonly referred to as the chymotryptic, tryptic, andpostacidic or caspase-like, can be measured by evaluating thehydrolysis of the fluorogenic substrates Suc-LLVY-MCA, Boc-LRR-MCA,and Z-LLE- $beta$ Nap, respectively. We therefore determined whetherand which of these specific activities are modulated during neuronalapoptosis. To this aim, control cells and cells undergoing apoptosiswere homogenized in a buffer containing 5 mM ATP and 20% glycerolto preserve the integrity of the 26 S proteasome (Hough et al.,1987), and their supernatant fractions were tested for the abilityto hydrolyze these fluorogenic substrates. Assays were performedin a buffer (pH 8.0) containing 5 mM EGTA to inhibit lysosomalpeptidases and calpains. As shown in Figure 4A, the supernatantfractions of CGCs undergoing apoptosis exhibit a progressivelyreduced hydrolysis of Suc-LLVY-MCA to ~60% of control value at12 hr of apoptosis. The time course analysis of this activitydemonstrates that this decline parallels the number of apoptoticnuclei (Fig. 4D). A similar trend was also observed for trypsin-likeand caspase-like activities of proteasome as detected using thefluorogenic substrates Boc-LRR-MCA and Z-LLE- $beta$ Nap respectively(Fig. 4B,C), although the decline of caspase like-activity isless pronounced and does not mirror the extent of apoptosis. Itis interesting to note, moreover, that the time course analysisof the three distinct peptidase activities of proteasome revealed,in the early phase of apoptosis, a slight, but consistent increasecompared to control cells (Fig. 4A-C).

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Figure 4. Profile of proteasome activities and proteasome concentration during the apoptosis of CGCs. A, Cultures at 6 DIV were washed and maintained in high-potassium and serum-free medium (S-K25) for 12 hr or switched to K5 and serum free-medium (S-K5). At the time indicated after the induction of apoptosis, 10 µg of supernatants were incubated with substrates specific for chymotrypsin-like (Suc-LLVY-MCA) (A), trypsin-like (Boc-LRR-MCA) (B), and caspase-like (Z-LLE- $beta$ Nap) activities (C) at 37°C for 20, 30, and 60 min, respectively, and assayed in triplicate. Specific activities are expressed as the percentage of activities of control cells, which have been given a value of 100. Results are the mean ± SD of experiments from three separate CGC preparations. D, For each time point the corresponding viability was determined, as described in Materials and Methods. E, Western blot analysis of proteasome content in 20 µg of whole extracts, from control cells and cells undergoing apoptosis for different times, performed with a mAb against the $alpha$ -subunits of 20S proteasome.

To ascertain if the decline in proteasome activity was attributable to a decrease in the actual proteasomes content, equalamounts of proteins from control cells and cells undergoing apoptosisfor different times were subjected to SDS-PAGE, electroblotted,and probed with a monoclonal antibody directed against all $alpha$ -proteasomesubunits. As shown in Figure 4E, the intracellular level of proteasomesremained unchanged in apoptotic granule neurons as compared withcontrol cells, indicating that the observed decline in proteasomeactivity during apoptosis is attributable to other causes (seeDiscussion). A similar result was also obtained using a mAb againstthe $alpha$ -subunit C9 (data notshown).

It has been reported that MG132, lactacystin, and PSI have different inhibitory potencies on the proteasomal activities (forreview, see Lee and Goldberg, 1998). Because they protect CGCsfrom apoptosis to a different extent (Fig. 1), we determined theireffectiveness by incubating granule neurons in their presenceand assessing the chymotrypsin, trypsin-like, and postacidic-likeactivities of proteasomes with specific substrates. As shown inFigure 5 all compounds inhibit the chymotrypsin-like activityto the same extent (MG132, $-$ 90 ± 6%; PSI, $-$ 80 ± 10%; lactacystin, $-$ 85 ± 10%). Considerable differences, on the contrary, were observedfor trypsin-like activity ( $-$ 34 ± 10% with MG132, $-$ 50 ± 5% withLactacystin, and $-$ 70 ± 10% with PSI) as well as postacidic-likeactivity ( $-$ 65 ± 5% with MG132, $-$ 50 ± 7% with Lactacystin, and $-$ 38 ± 11% with PSI). The data reported demonstrate that the inhibitorstested are able to enter the cells and to block the proteasomeactivity to an extent comparable to that previously reported fortheir antiapoptotic action. Moreover, on the basis of these resultswe hypothesize that the anti-apoptotic effect is exerted by inhibitorsable to inhibit also the postacidic-like activity.

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Figure 5. Effect of proteasome inhibitors on apoptosis-induced change in proteasome activity. Extracts of granule neurons deprived of K⁺ and serum for 12 hr in the absence or in the presence of proteasome inhibitors were incubated with substrates specific for the chymotrypsin, trypsin, and postacidic-like activities and assayed, as described in Materials and Methods. Data are expressed as the percentage of activities in S-K5. Results are the means ± SD from two separate granule neurons preparations.

Proteasome failure occurs downstream caspase activation

To determine whether the reduced proteasome activity is a regulated event located downstream the caspase activation, we measuredproteasome activities in supernatant fractions from CGCs inducedto undergo apoptosis for 12 hr in the presence or absence of thegeneral caspase inhibitor Z-VAD-fmk (100 µM). The hydrolysis ofSuc-LLVY-MCA, Boc-LLR-MCA, and ZLLE $beta$ -Nap by CGCs was decreasedto 53 ± 8%, 58 ± 11%, and 73 ± 4%, respectively, after the apoptoticstimulus. When CGCs were induced in apoptosis in the presenceof 100 µM of Z-VAD-fmk, the chymotrypsin, trypsin, and caspase-likeactivities were partially restored mirroring the antiapoptic effectof this general caspase inhibitor in this model of neuronal apoptosis(Fig. 6).

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Figure 6. Effect of the general inhibitor, Z-VAD-fmk, on proteasome activities. CGCs were washed and maintained in high-potassium and serum-free medium (S-K25) for 12 hr or switched to K5 and serum free-medium (S-K5) in the absence or in the presence of 100 µM Z-VAD-fmk. Twelve hours later, 10 µg of supernatants were incubated with substrates specific for chymotrypsin-like (Suc-LLVY-MCA), trypsin-like (Boc-LRR-MCA), and caspase-like (Z-LLG- $beta$ Nap) activities at 37°C for 20, 30, and 60 min, respectively, and assayed in triplicate. Specific activities are expressed as the percentage of activities of control cells, where control cells have been given a value of 100. Results are the mean ± SD of experiments from three separate CGC preparations.

Accumulation of ubiquitinated-proteins in cerebellar granule neurons undergoing apoptosis

The progressive failure of proteasomal enzymatic activities prompted a study aimed at ascertaining whether induction of apoptosiswas accompanied by changes in protein ubiquitination, as suggestedby the marked reduction in the chymotrypsin-like activity of proteasomes.In fact, an impairment of this specific activity is closely relatedto the accumulation of ubiquitinated proteins (Heinemeyer et al.,1991; Figueiredo-Pereira et al., 1994).

We therefore examined the ubiquitin immunoreactivity using an antibody that is routinely used for immunohistochemical identificationof ubiquitin-conjugated filamentous inclusions in neurodegeneratingbrains (Perry et al., 1987).

As shown in Figure 7A, neurons undergoing apoptosis and in the execution phase, recognizable as those having a small condensedor fragmented nucleus strongly stained by propidium iodide (Fig.7B), are characterized by a prominent ubiquitin immunoreactivityin the cytoplasm (Fig. 7A) and in the degenerating neurites (Fig.7C), whereas the nuclear staining is markedly reduced. In contrast,cells with a normal nuclear morphology exhibit a heterogeneouspattern of ubiquitin immunofluorescence barely detectable as avery faint staining of dendrites, perikarya, and nucleus.

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Figure 7. Ubiquitin immunostaining in cerebellar granule neurons undergoing apoptosis analyzed by confocal microscopy. Apoptosis in CGC was induced by potassium and serum withdrawal, as described in Materials and Methods. Double immunostaining of ubiquitin (A, C) and DNA (B, D) in CGCs was performed 6 hr after induction, using a polyclonal anti-ubiquitin antibody and propidium iodide, as described in Materials and Methods. Notice that only few, scattered neurons are heavily stained (A) compared to the number of neurons present in the same field (B) and already stained with propidium. Arrows indicate the immunostaining with anti-ubiquitin (A) and their corresponding nuclei (B). Arrowheads indicate ghost cells that have lost the cytoplasm content (C) and their corresponding nuclei (D). Large arrows indicate beaded neurites stained very brightly for ubiquitin (C). Scale bar, 7 µm.

We found that at any given time of apoptosis only a small fraction of the whole population of neurons identified by propidiumstaining demonstrate an high reactivity with the antibody recognizingubiquitinated proteins. The simplest explanation is that suchhigh positivity is transitory because of the subsequent loss ofthe cytoplasmatic content. In fact, cell ghosts that have lostmembrane integrity are not stained with anti-ubiquitin antibody(Fig. 7A,B) suggesting that ubiquitinated proteins, which accumulatein the cytoplasm of dying cells, are subsequently sequesteredin the apoptoticblebs.

We next assessed whether such increased and modified intracellular distribution was also accompanied by an altered cellularamount of polyubiquitinated proteins. Western blot analysis ofcytoplasmatic and nuclear extracts derived from control cellsand cells undergoing apoptosis were immunodeveloped with the sameanti-ubiquitin antibody used for the immunofluorescence analysis.Figure 8A shows that within 6 hr after the apoptotic stimulus,a progressive increase of a heterogeneous population of high molecularweight proteins is detectable in the cytoplasmic extracts. Noticethat at 12 hr after the onset of apoptosis, whereas the extentof dying neurons continues to increase and approximates 50% oftotal neurons, the amount of ubiquitinated polypeptides is lowerthan that detectable at 6 hr, probably because of the sequestrationof proteasome and ubiquitinated proteins in the apoptotic blebsas previously described (Pitzer et al., 1996). A different trendis observed for nuclear proteins, because during the same perioda progressive reduction in the ubiquitin immunostaining occurs.It is interesting to note that the actual increase of ubiquitinatedpolypeptides is a measure of the whole population of dying neurons.Because, as shown in Figure 7, only a small fraction of the totalpopulation of apoptotic neurons exhibit a clear cut increase inubiquitin immunostaining at any given time after the apoptoticstimulus, we are brought to conclude that in these neurons theincrease of ubiquitinated proteins is several fold higher thanthat detected by Western blot. Furthermore, ubiquitinated proteinsaccumulate within 1 hr, despite the slight increase of chymotrypsin-likeactivity (Figs. 4A, 8A). This apparent discrepancy could be attributableto (1) the generation of proteins unable to enter the proteosomecavity because not properly ubiquitinated or edited, (2) the increasedamount of ubiquitinated proteins not completely degraded by theslight increment of chymotrypsin activity shown in Figure 4; and(3) the existence of two populations of CGCs, one undergoing fastand another undergoing slow apoptotic death. (Miller and Johnson,1996).

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Figure 8. Accumulation of ubiquitin conjugates in cerebellar granule cells undergoing apoptosis. A, At 6 DIV cells were induced to apoptosis and after 1, 6, and 12 hr, nuclear (10 µg) and cytoplasmatic proteins (20 µg) were collected, resolved by SDS gel electrophoresis (8-15%), and immunoblotted with the polyclonal anti-ubiquitin antibody, as described in Materials and Methods. Molecular weight markers are indicated on the left. B, Densitometric analysis of Western blot reported above. The absolute scanning values are given as arbitrary units. C, Time course of neuronal death after onset of apoptosis in sister cultures.

Proteasome and caspase inhibitors prevent the intracytoplasmatic accumulation of ubiquitinated proteins in apoptotic neurons

Because proteasome inhibitors counteract apoptosis of CGCs, we examined their influence on the intracytoplasmatic accumulationof ubiquitinated proteins by indirect immunofluorescence analysisperformed 6 hr after onset of the apoptotic stimulus. As can beenseen in Figure 9 the proteasome inhibitor MG132 prevents the diffuseintracytoplasmatic accumulation of ubiquitinated proteins, characteristicof apoptotic cells and shown also in Figure 7. Furthermore, thegeneral caspase inhibitor Z-VAD-fmk, was also able to preventthis event, although to a slightly lower extent, indicating thatthe massive build up of ubiquitinated proteins in degeneratinggranule neurons is an event located downstream the caspase activation,as also suggested by the finding that the decline in chymotrypsin-likeactivity of proteasomes is restored in apoptotic granules treatedwith Z-VAD-fmk (Fig. 6). On the contrary, treatment with calpaininhibitors (such as E64d or ALLM) did not block the accumulationof ubiquitinated proteins or inhibit apoptosis (Fig. 1C).

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Figure 9. Proteasome and caspase inhibitors affect the intracytoplasmatic accumulation of ubiquitinated proteins in apoptotic granules. Apoptosis in CGCs was induced in the absence or in the presence of MG132 (5 µM), Z-VAD-fmk (100 µM), ALLM (40 µM), and E64d (20 µM). Ubiquitin immunostainings were examined 6 hr after induction using anti-ubiquitin antibodies, as described in Materials and Methods. Fluorescent images were taken in a laser confocal microscope (Leica TCS 4D system, equipped with 100× 1.3-0.6 oil-immersion objective, optical section 1 µM). Optical sections were stereo-pair and three-dimensional reconstituted. A representative experiment (of 3) is shown.

Deubiquitinating activities decline during apoptosis

As a first attempt to investigate the possible cause or causes of proteasome failure during neuronal apoptosis we measuredthe activity of DUB. These enzymes, also referred to as ubiquitinC-terminal peptidases, catalyze the removal of ubiquitin fromvarious cellular adducts, thus playing an important role in theediting of ubiquitination state of proteins and in the recyclingof ubiquitin (Wilkinson, 1997). The recycling of free ubiquitinfrom poly-ubiquitin remnants is required for the continued actionof the complete proteolytic system. In fact, polyUb chains, notproperly disassembled, bind avidly to and inhibit the 26 S proteasomecomplex, presumably via competition with polyubiquitinated substrates(Hadari et al., 1992; Amerik et al., 1997). DUB enzymes are encodedby two gene families: the UCH family (ubiquitin C-terminal hydrolases,with molecular weight of ~30 kDa, hydrolyzing small C-terminalderivatives) and UBP family (ubiquitin-specific processing proteases,with molecular weight of ~110 kDa, hydrolyzing large derivativesofubiquitin).

We measured both activities in cell extracts of CGCs undergoing apoptosis using as substrate multi-ubiquitin chains composedof a mixture of (Ub)₄, (Ub)₃, and (Ub)₂ oligomers. Such oligomersare converted by the action of DUB enzymes into monomeric ubiquitinUB₁ (Wilkinson et al., 1995). These multi-ubiquitin chains aresuitable substrates for measuring the activity of UBP family ofDUB enzymes (Wilkinson et al., 1995). Moreover, the oligomer (UB)₂is also a good substrate for the UCH-L1 (Larsen et al., 1998),which is one of the most abundant enzyme in the brain, comprisingup to 2% of total brain proteins (Leroy et al., 1998).

The cleavage of these substrates was monitored by Western immunoblot using anti-ubiquitin antibody , as described in Materialsand Methods. As shown in Figure 10A, a striking difference in cleavagerate was observed, this being markedly reduced after 12 hr ofapoptosis, as suggested by the finding that the immunoreactivityfor (Ub)₄, (Ub)₃, and (Ub)₂ oligomers is greater in CGCs undergoingapoptosis than in control cells, whereas the immunoreactivityfor (UB)_1, the end product of DUB activity, is lower in apoptoticcells.

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Figure 10. Deubiquitinating activity in granule neurons undergoing apoptosis. A, Cultures at 6 DIV were washed and switched to K5 and serum free-medium (S-K5) and in K25 and serum free-medium (S-K25) for 1, 3, 6, and 12 hr. At the time indicated after the induction of apoptosis, 5 µg of supernatants were incubated with 1 µg of multi-ubiquitin chains, substrates for DUB enzymes, incubated at 22°C for 10 min, and immunoblotted with anti-ubiquitin antibody. B, Effect of the general caspase inhibitor Z-VAD-fmk on deubiquitinating activities. CGCs were washed and maintained in high-potassium and serum free-medium (S-K25) for 12 hr or switched to K5 and serum free-medium (S-K5) in the absence or in the presence of 100 µM Z-VAD-fmk. Twelve hours later deubiquitinating assay was performed as described above.

Notice also that the DUB activity is restored in granule neurons undergoing apoptosis in the presence of a general caspaseinhibitor Z-VAD-fmk (Fig. 10B) This latter finding suggest thatthe impairment of deubiquitinating activity is an event that occursdownstream of caspase activation. Similar results were also obtainedusing as substrate fluorogenic substrate Z-RLRGG-MCA (Stein etal., 1995; Dang et al., 1998), which is based on the C terminusof ubiquitin (data not shown). Further experiments are requiredto clarify, by the use of specific substrate, which family ofDUB enzymes, UCH or UBP, is responsible for the decreased deubiquitinatingactivity detected in apoptoticneurons.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Two major findings reported in this paper deserve some comments and deal with the demonstration that specific inhibitors ofproteasome activities administered at the time of triggering apoptosislargely prevent this otherwise irreversible program of cell death,such inhibition being most probably upstream the caspase activation.The second peculiar finding is that within 12 hr of inducing apoptosis,a progressive accumulation of ubiquitinated proteins occurs, likelyas a result of a progressive deficit in proteasome chymotrypsin-likeactivity, such accumulation being downstream of the caspase activation.A corollary of these studies, in line with some previous hypothesis,postulates that such proteasome involvement may have some relevancewith neurodegenerative diseases. For the sake of clarity, eachof these specific issues will be separatelydiscussed.

Previous studies have attributed to the proteasome a critical role in apoptosis triggered by different stimuli in terminallydifferentiated cells (Grimm et al., 1996; Sadoul et al., 1996).Our findings, using a panel of proteasomal inhibitors with differentinhibitory capabilities against the proteasome, demonstrate thatthis proteolytic machinery plays also a role in death by apoptosisof CGCs. We have found that not all inhibitors exert the sameprotective effect. In fact, the most powerful blockers were MG132and Lactacystin, producing a neuronal survival of 98 and 85%,respectively, after 12 hr of apoptosis. By contrast, another proteasomeblocker PSI (Z-IE (OtBu) AL-CHO) is a poor inhibitor even at thehighest concentration tested (50-100 µM). Such weak inhibitoryactivity is in contrast with the report dealing with the protectiveeffect of PSI (at concentration ranging from 10 to 100 nM) onsympathetic neurons deprived of NGF (Sadoul et al., 1996). Thesimplest explanation is that the composition of the proteasomecomplex in CGCs and sympathetic neurons is not identical, or thatthe pathway or pathways linking their function with other intracellularactivities are distinct and they therefore exhibit markedly differentsensitivity to this inhibitor. For example, proteasomes involvedin antigen presentation differ both in composition and functionfrom proteasomes involved in other processes (Driscoll et al.,1993). On the other side, it is possible that the block of celldeath in CGCs requires the simultaneous repression of more thanone peptidase activity of proteasome, one of which is of caspase-likenature. In fact, as shown in Figure 5, the most powerful inhibitorsare those that also affect more deeply the postacidic activity(MG132 and Lactacystin). This activity could be devoted to cleavea particular substrate that promotes cell death, for example apro-caspase family member into an active form, or could degraderegulatory proteins that normally control the apoptotic pathway.This hypothesis is strengthened by the observation that proteasomescan cleave after Asp in synthetic peptide substrates (Rivett etal., 1994; Kisselev et al., 1999) and that proteasomes are themajor ICE-like proteinase in P19 cells treated with retinoic acid(Kobayashi et al., 1996). On the basis of such considerationsand of previous findings, it is tempting to place the proteasomeactivity in CGCs undergoing apoptosis upstream of the caspaseactivation, as already shown in sympathetic neurons deprived ofNGF (Sadoul et al., 1996) and in thymocytes treated with dexamethasone, $gamma$ -irradiation, or etoposide (Grimm et al., 1996; Hirsch et al.,1998; Stefanelli et al., 1998). The suggestion that the proteasomecomplex is acting upstream of the caspases is also based on thefinding that the proteasomal inhibitors block caspase-3 activityand prevent the cleavage of tau in granule neurons undergoingapoptosis (Fig. 3). Furthermore, these inhibitors block the earlyrelease of cytochrome c from mitochondria (Bobba, Canu, Atlante,Marra, and Calissano, unpublished observations), an event precedingcaspase-3 activation (Bobba et al., 1999).

After such early involvement, proteasomes become part of a generalized cellular failure that affects the major activitiesof the apoptotic neuron, as shown by the finding that CGCs undergoingapoptosis accumulate ubiquitinated-proteins (Figs. 7, 8A). Althoughseveral mechanisms could account for the building up of ubiquitinatedproteins, a decrease of proteasome activity in CGCs undergoingapoptosis could be one of the major causes. We found that after6 hr of apoptosis there is a significant decline in proteasomeactivity that further decreases by 12 hr and that it tightly reflectsthe extent of apoptosis. This decline involves the chymotrypsin-like,trypsin-like and to, a lower extent, the caspase-like activity(Fig. 4A-C). Among them, the chymotrypsin-like activity has beendirectly linked to the degradation of ubiquitin conjugates. Defectsin the yeast proteasome subunits bearing this catalytic activityresult in decreased ability of cells to cope with stress conditions,cause accumulation of ubiquitin conjugates, and reduce proteindegradation rates (Heinemeyer et al., 1991). Moreover, the inhibitionof chymotrypsin-like activity (by the inhibitor PSI) of proteasomein neuronal cells is sufficient to induce accumulation of ubiquitinatedproteins (Figueiredo- Pereira et al., 1994), and a decrease ofthe proteasome chymotrypsin-like activity is observed in transientischemia (Kamikubo and Hayashi, 1996). Although a decline in proteasomefunction seems to play a major role, the possibility that duringapoptosis the proteolytic machinery may be overwhelmed or incapableof dealing with an increased amount of ubiquitinated proteinscannot be ruled out. It is also possible that the proteasome efficacyis additionally hampered by the generation, during apoptosis,of poor substrates for proteolysis such as cross-linked or aggregatedproteins because, for example, of the disruption of the intracellularsulfhydryl homeostasis (Figueiredo-Pereira et al., 1998).

The significant decrease in proteasome function is likely attributable to a specific downregulation and not of proteasomecontent, as suggested by the finding that the amount of proteasomesubunits does not change within the first 24 hr of apoptosis.Because we have used a broad range antiserum directed againstall $alpha$ -subunits, we cannot exclude that a specific subunit couldbe a target of caspases, resulting in reduced activity. Whateverthe correct explanation, the impairment in proteasome functionis likely correlated and linked to the decline in deubiquitinatingactivities that also occurs downstream of the caspase activation.It is worth noting that deubiquitinating enzymes facilitate theprotein degradation by the proteasome, possibly by supervisingthe ubiquitinated state of proteins and by preventing accumulationof ubiquitin chains generated as intermediates in substrate degradation(Hadari et al., 1992). These chains may need to be disassembledto avoid accumulation to a level that inhibit proteolysis. Disruptionof DUB enzymes in yeast leads to a decrease in protein degradation,accumulation of polyubiquitin proteins, and to depletion of cellularubiquitin pools (Papa and Hochstrasser, 1993; Amerik et al., 1997).Our finding that DUB activity declines downstream of caspase activationsuggests that it could be directly or indirectly a target of caspaseor caspases. In this regard, it must pointed out that a missensemutation in Parkinson's disease (Leroy et al., 1998) or intragenicdeletion in gad mice (Saigoh et al., 1999) of the deubiquitinatingenzyme UCH-L1 cause partial loss of the catalytic activity ofthis enzyme, which could lead to aberration in the proteolyticpathway and aggregation ofproteins.

Our data provide evidence that apoptosis in neuronal cells is accompanied by an early involvement of proteasome activitiesfollowed by a decrease in its function. To date, two other studiesreported the modifications of proteasome activity during dexamethasone-inducedapoptosis in thymocytes (Beyette et al., 1998; Hirsch et al.,1998). Beyette et al., (1998) found that dexamethasone-inducedapoptosis in rat thymocytes is accompanied by a reduction of proteasomeactivity similar to the extent of apoptosis. Hirsch et al. (1998),on the other hand, reported that, in the same experimental paradigm,the proteasome is activated concurrently with the onset of apoptoticdeath. Our data mirror partly those of Beyette et al. (1998),showing a decrease, during apoptosis, after a brief and slightincrease, of all the activities of proteasome. In addition, ourstudies, using as a parameter of proteasome failure the accumulationof ubiquitinated proteins, place the decline of proteasome activitydownstream of the caspase activation as also confirmed by thefinding that the chymotrypsin-like activity is restored in supernatantfraction from CGCs induced to undergo apoptosis in the presenceof Z-VAD-fmk.

It is reported that the high levels of ubiquitin immunoreactivity associated with the inclusion bodies characteristic of arange of neurodegenerative disorders is attributable to the inabilityof the intracellular proteolytic system in lysing these structures.Moreover, inappropriate apoptosis is believed to be the underlyingmechanism in the pathogenesis of neurodegenerative diseases. Thestudies reported in this article define an important role of apoptosisfor proteasome activity failure, likely caused by a deficit indeubiquitinating activities, in the accumulation of ubiquitinatedproteins, giving new insights into the mechanism that generatesubiquitinylated inclusions in many neuropathologies .

The question then arises as to the nature of the mechanism that first involves proteasomes as primary actors of apoptosis,to the extent that their inhibition blocks this event, and subsequently,when their apoptosis-promoting activity has been launched to otherintracellular site or sites, these same structures become objectof their own message so that their most typical and preferredsubstrate, ubiquitinated proteins, accumulate in the cytoplasmof dyingcells.

  FOOTNOTES

Received June 25, 1999; revised Oct. 29, 1999; accepted Nov. 3, 1999.

This work was supported by Telethon-Italy (Grant E855), Progetto Finalizzato Biotecnologie, and Cofinanziamento Ministerodell'Universitá e della Ricerca Scientifica e Tecnologica (40%to P.C.). We thank Dr. Andrea Levi for comments on this manuscriptand Marianna De Bernardinis for helpful suggestions on MTTassay.
Correspondence should be addressed to Dr. Nadia Canu, Istituto di Neurobiologia Consiglio Nazionale delle Ricerche, V.le Marx15, 00137 Roma, Italia. E-mail: nadia{at}biocell.irmkant.rm.cnr.it.

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