Recruitment of the Mitochondrial-Dependent Apoptotic Pathway in Amyotrophic Lateral Sclerosis

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The Journal of Neuroscience, September 1, 2001, 21(17):6569-6576

Recruitment of the Mitochondrial-Dependent Apoptotic Pathway in Amyotrophic Lateral Sclerosis
Christelle Guégan¹, Miquel Vila¹, Gorazd Rosoklija², Arthur P. Hays², and Serge Przedborski¹^,²
Departments of ¹ Neurology and ² Pathology, Columbia University, New York, New York 10032

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Molecular mechanisms of apoptosis may participate in motor neuron degeneration produced by mutant superoxide dismutase-1 (mSOD1),the only proven cause of amyotrophic lateral sclerosis (ALS).Consistent with this, here we show that the proapoptotic proteinBax translocates from the cytosol to the mitochondria, whereascytochrome c translocates from the mitochondria to the cytosolin spinal cords of transgenic mSOD1 mice during the progressionof the disease. Concomitantly, caspase-9 is activated in the spinalcord of transgenic mSOD1 mice. Only in end-stage transgenic mSOD1mice is the downstream caspase-7 activated and the inhibitor ofapoptosis, XIAP, cleaved. These results indicate a sequentialrecruitment of molecular elements of the mitochondrial-dependentapoptotic pathway in transgenic mSOD1 mice. We also provide immunohistochemicalevidence that cytochrome c translocation occurs in the spinalcord of sporadic ALS patients. Collectively, these data suggestthat the mitochondrial-dependent apoptotic pathway may contributeto the demise of motor neurons in ALS and that targeting key moleculesof this cascade may prove to beneuroprotective.

Key words: amyotrophic lateral sclerosis; apoptosis; Bax; caspase; cytochrome c; mitochondria; superoxide dismutase; neurodegeneration

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Amyotrophic lateral sclerosis (ALS) is a fatal paralytic disease characterized by a progressive loss of spinal cord motorneurons (Rowland, 1995). Important insights into its pathogenesiscome from the discovery that missense mutations in superoxidedismutase-1 (mSOD1) are linked to familial ALS (Deng et al., 1993;Rosen et al., 1993) and that overexpression of different mSOD1sin mice replicate the clinical and pathological hallmarks of ALS(Brown, 1995). mSOD1 cytotoxicity is not triggered by a loss ofenzymatic activity or by a dominant negative mechanism but bya gain of function (Brown, 1995) of unknownnature.

Mounting evidence indicates that mSOD1-induced spinal cord motor neuron death involves, in part, the apoptotic machinery.Indeed, the expression of the anti-apoptotic protein Bcl-2 isdecreased, whereas that of the proapoptotic protein Bax is increasedin the spinal cords of human ALS cases and of transgenic mSOD1mice (Martin, 1999; Vukosavic et al., 1999). Furthermore, theoverexpression of Bcl-2 delays the disease process in transgenicmSOD1 mice (Kostic et al., 1997). In addition, caspase-1 and caspase-3,which belong to the family of apoptotic effector cysteine proteases(Earnshaw et al., 1999), are sequentially activated in spinalcords of affected transgenic mSOD1 mice (Pasinelli et al., 1998,2000; Vukosavic et al., 2000). Activation of these caspases likelyparticipates in the neurodegenerative process of ALS, becauseoverexpression of the dominant negative mutant M17Z of caspase-1(Friedlander et al., 1997) or the chronic infusion of a pan-caspaseinhibitor (Li et al., 2000) provide neuroprotection to transgenicmSOD1mice.

The release of cytochrome c from the mitochondria to the cytosol is pivotal in the activation of caspases and the ensuingcell death (Kroemer and Reed, 2000). After a death stimulus, cytosolicBax translocates to mitochondria (Wolter et al., 1997; Gross etal., 1998) in which it can promote the release of cytochrome c(Gross et al., 1998; Jürgensmeier et al., 1998). Once released,cytosolic cytochrome c interacts with apoptotic protease-activatingfactor-1 (Apaf-1) in the presence of dATP, which stimulates theprocessing of pro-caspase-9 to its active form, which in turncan then activate the executioner caspase-3 and caspase-7 (Liet al., 1997; Pettmann and Henderson, 1998). Translocation ofcytochrome c occurs in several experimental models of acute neurologicaldisorders, such as strokes and encephalitis (Gillardon et al.,1997; Yakovlev et al., 1997; Krajewski et al., 1999; Guégan andSola, 2000; Vereker et al., 2000). However, whether mitochondrialcytochrome c is released in a chronic neurodegenerative processsuch as in ALS is not yetknown.

Here we show that Bax and cytochrome c translocation occurs in the spinal cord of transgenic mSOD1 mice in parallel with theneurodegenerative process. Concurrently, caspase-9 is activatedfollowed by the activation of caspase-7 and the cleavage of theX chromosome-linked inhibitor of apoptosis protein (XIAP). Wealso present immunohistochemical evidence supporting the occurrenceof cytochrome c translocation in motor neurons of spinal cordsfrom sporadic ALS patients. These findings support the recruitmentof the mitochondrial-dependent apoptotic pathway in mice and humanALScases.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Time course of behavioral abnormalities in transgenic mSOD1 mice. As described previously (Vukosavic et al., 2000), the firstbehavioral abnormality appeared at ~3 months of age in transgenicmSOD1 mice and consisted of a fine tremor and posturing of atleast one limb when the animal was held in the air by the tail.Then, progressively, the animals became paralyzed; they were thenkilled at ~5 months of age, corresponding to the endstage.

Animals. Two lines of hemizygous transgenic mice were used: (1) line G1H (The Jackson Laboratory, Bar Harbor, ME), which carrieda substitution of glycine by alanine at codon 93 of the humanSOD1 protein and expressed ~18 copies of human mutant SOD1 gene(Gurney et al., 1994); and (2) line N1029 (The Jackson Laboratory),which expressed >10 copies of human wild-type (wt) SOD1 gene (Gurneyet al., 1994).

Isolation of cytosolic and mitochondrial fractions. Protein extraction of both mitochondrial and cytosolic fractions was performedfrom fresh spinal cords (n = 4-6 per group) obtained from transgenicwtSOD mice (3 months of age) and from transgenic mSOD1 mice andtheir nontransgenic littermates of different ages (1, 2, 3, and5 months). Tissues were gently homogenized with a glass-glasshomogenizer in 10 vol (w/v) of cold buffer consisting of (in mM):250 sucrose, 10 KCl, 1.5 MgCl₂, 2 EDTA, 20 HEPES, and proteaseinhibitor cocktail (Complete mini; Boehringer Mannheim, Indianapolis,IN). Homogenates were centrifuged (500 × g, 5 min, 25°C), andsupernatants were collected and centrifuged (13,000 × g, 20 min,4°C). Resulting pellets were designated mitochondrial fractions,whereas supernatants were further centrifuged (100,000 × g, 60min, 4°C). Resulting supernatants were designated cytosolic fractions.To verify the relative mitochondrial purification, each fractionwas subjected to Western blotting for $beta$ -actin as a cytosolic markerusing a mouse monoclonal antibody anti- $beta$ -actin (clone AC15; Sigma,St. Louis, MO) and cytochrome c oxidase (COX) as a mitochondrialmarker using a mouse monoclonal antibody anti-COX subunit IV (MolecularProbes, Eugene,OR).

Western blot analysis. Concentrations of proteins were determined by BCA protein assay (Pierce, Rockford, IL), and immunoblotswere processed as described previously (Vukosavic et al., 2000).For analyzing the subcellular localization of cytochrome c, 30µg of protein from the cytosolic fraction and 4 µg of proteinfrom the mitochondrial fraction were electrophoresed on a 15%SDS-polyacrylamide gel. For Bax, caspases, and XIAP analysis,30-70 µg were used. Gels were blotted to nitrocellulose membrane.The primary antibodies used were as follows: a mouse monoclonalcytochrome c antibody (1:1500 and 1:10,000 final dilutions forcytosolic and mitochondrial fractions, respectively; clone 7H8.2C12;PharMingen, San Diego, CA), a mouse monoclonal anti-Bax antibody(1:250 final dilution for both fractions; SC-7480; Santa CruzBiotechnology, Santa Cruz, CA), a rabbit polyclonal anti-XIAPantibody (1:150 final dilution; catalog #2042; Cell SignalingTechnology, Beverly, MA), a rabbit polyclonal anti-caspase-7 antibodyrecognizing the pro- and cleaved forms (1:250 final dilution;catalog #9492; Cell Signaling Technology), and a rabbit polyclonalanti-caspase-9 antibody recognizing the pro- and cleaved forms(1:1000 final dilution; catalog #AAP-109; StressGen Biotechnologies,Victoria, Canada). Bands were visualized by using enhanced chemiluminescentsubstrate (SuperSignal Ultra; Pierce). Films (Kodak BioMax MS;Eastman Kodak, Rochester, NY) were scanned, and bands were quantifiedby using the NIH Image 1.62software.

Immunohistochemistry. The immunohistochemical analyses of the experimental mice were performed using our standard protocolon cryostat-cut sections (30 µm) obtained from cervical and lumbarsegments from spinal cord of transgenic mSOD1 mice at the beginningof symptoms (~3 months of age) and the end stage (~5 months ofage) (Kostic et al., 1997). The immunostaining for cytochromec was performed using the Vector M.O.M. immunodetection kit (PK-2200;Vector Laboratories, Burlingame, CA) for eliminating the nonspecificbackground. Sections were incubated overnight at 4°C with thefollowing primary antibodies: anti-cytochrome c mouse monoclonalantibody (1:1000; PharMingen), anti-cleaved caspase-7 rabbit polyclonalantibody (1:100; catalog #9491; Cell Signaling Technology), andanti-cleaved caspase-9 rabbit polyclonal antibody (1:50; catalog#9501; Cell Signaling Technology). Then the sections were incubatedwith the biotinylated anti-rabbit IgG (1:200; Vector Laboratories)for 1 hr at room temperature and processed with the ABC system.The peroxidase reaction was revealed with the diaminobenzidinesubstrate.

The immunohistochemical staining of human spinal cord was applied to 6-µm-thick paraffin sections mounted on coated glassslides. The sections were cleared, rehydrated, and subjected tomicrowave retrieval before staining them for cytochrome c usingthe same method as formice.

Human samples. The tissues used originated from six spinal cord samples from patients with ALS and seven from neurologicalpatients with no spinal cord pathology; samples were obtainedfrom the Brain Bank, Department of Pathology at Columbia University.In the ALS group, the cause of death was pneumonia (n = 3) andrespiratory failure (n = 3); in the control group, it was pneumonia(n = 2), respiratory failure (n = 3), pulmonary embolism (n =1), and septic shock (n = 1). At autopsy, brains and spinal cordswere removed and processed for banking as described previously(Przedborski et al., 1996). Half of the brain and selected blocksof each level of the spinal cord were immediately placed in 10%buffered formalin, embedded in paraffin, and subjected to neuropathologicalexamination. There was no significant difference between the timefrom death to autopsy between the two groups (mean ± SD; ALS,10.7 ± 5.9 hr; control, 14.6 ± 3.6 hr; p = 0.17; Student's t test).The clinical diagnosis of ALS was confirmed pathologically inall six ALS patients. In these spinal cord specimens, dramaticneuronal loss was observed in the anterior horn with mild to moderategliosis, whereas no remarkable pathological changes were notedin spinal cords from controls. For the ALS patients, the meanage at onset was 64.3 ± 13.2 years, with a mean duration of diseaseof 3.3 ± 2.7 years. None of the ALS patients had a family historyfor theillness.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Release of mitochondrial cytochrome c to the cytosol in ALS

Cytochrome c immunoreactivity was detected by Western blot analysis as a single specific band of 15 kDa (Fig. 1A,C), consistentwith the gel resolution of the commercially purified cytochromec protein (data not shown). In nontransgenic mice, the levelsof cytochrome c in the cytosolic and mitochondrial fractions didnot change over a period corresponding to the lifespan of thetransgenic mSOD1 counterparts (Fig. 1). Conversely, in spinalcord of early symptomatic (~3 months old) and end stage (~5 monthsold) and, to a lesser extent, of asymptomatic transgenic mSOD1mice (1-2 months old), levels of cytochrome c were increased inthe cytosolic fraction and decreased in the mitochondrial fractioncompared with age-matched nontransgenic controls (Fig. 1). TransgenicwtSOD mice age-matched with early symptomatic transgenic mSOD1mice showed no alteration of cytosolic and mitochondrial cytochromec levels (Fig. 1). Likewise, no significant change in cytochromec level was seen in unaffected brain regions of transgenic mSOD1mice, such as the cerebellum (data not shown).

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Figure 1. Western blot analysis of cytochrome c. Protein extracts from cytosol (A, B) and mitochondria (C, D) were obtained from spinal cords of wtSOD1 mice (3 months old), of transgenic mSOD1 mice at asymptomatic stage (AS; 1 and 2 months old), at the beginning of symptoms (BS; 3 months old), at end stage (ES; 5 months old), and of their age-matched nontransgenic mice littermates (Non-Tg). $beta$ -Actin and COX were used as internal controls for the cytosolic and mitochondrial fractions, respectively. The results of densitometric analysis are shown in B and D. The mean values (n = 4-6 per group; mean ± SEM) obtained for transgenic mSOD1 mice (black columns) were compared with the values of their age-matched littermates (white columns). *p < 0.05; **p < 0.01; Student's t test.

Cytochrome c immunostaining

To provide more detailed information regarding the cellular localization of released cytosolic cytochrome c, we immunostainedspinal cord sections from nontransgenic and symptomatic transgenicmSOD1 mice, both at the beginning of symptoms and at end stage.In nontransgenic mice, numerous neurons immunoreactive for cytochromec were observed throughout the gray matter of the spinal cord(Fig. 2A). Notably, all of these cytochrome c-positive neuronsshowed immunostaining confined to the cell body and with a finepunctate appearance (Fig. 2B,C). In symptomatic mice, many remainingspinal cord neurons in the anterior horn showed a more robustimmunoreactivity (Fig. 2D,E) like that described previously inan ischemic model (Fujimura et al., 1999, 2000). In those motorneurons, the fine punctate cytochrome c immunoreactivity appearedmarkedly reduced, giving way to a more diffuse immunostaining(Fig. 2E,F), consistent with the redistribution of cytochromec from mitochondria to cytosol in motor neurons of symptomaticmice.

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Figure 2. Cytochrome c immunostaining in spinal cord from age-matched littermate nontransgenic mice (A-C) and mSOD1 transgenic mice at end stage (D-F). In nontransgenic controls, the staining was faint and punctate (A-C), whereas in end-stage transgenic mSOD1 mice, it was robust and diffuse (D-F).

mSOD1-related neurodegeneration stimulates Bax translocation

Because translocation of Bax to mitochondria promotes cytochrome c release (Wolter et al., 1997; Jürgensmeier et al., 1998),we determined Bax content in both cytosolic and mitochondrialfractions of the spinal cord of different groups of mice at differenttime points. In transgenic mSOD1 mice, cytosolic Bax levels wereunchanged in the spinal cords of asymptomatic animals comparedwith that of nontransgenic controls (Fig. 3A,B). In contrast,cytosolic Bax levels were reduced in the spinal cord of both earlysymptomatic and end-stage mice compared with age-matched nontransgenic(Fig. 3A,B) and transgenic wtSOD animals (data not shown). Inthe same transgenic mSOD1 mice, mitochondrial Bax levels steadilyaugmented in the spinal cords compared with nontransgenic controlsduring the progression of the disease (Fig. 3C,D), reaching atend stage more than a twofold increase.

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Figure 3. Subcellular localization of Bax. Bax expression was analyzed by Western blot in cytosolic (A, B) and mitochondrial (C, D) fractions of spinal cords from transgenic mSOD1 mice (black columns) at the asymptomatic stage (AS), at the beginning of symptoms (BS), and at the end stage (ES) and was compared with their age-matched nontransgenic littermates (Non-Tg; white columns). Represented values (n = 4-6 per group) correspond to mean ± SEM. *p < 0.05; **p < 0.01; Student's t test.

Activation of caspase-9 and caspase-7 in transgenic mSOD1 mice

During apoptotic cell death, pro-caspase-9 (52 kDa) is processed into a large active subunit (35 kDa) and a small unit (17kDa), whereas pro-caspase-7 (37 kDa) is processed into proteolyticfragments of 28 and 20 kDa. In agreement with this, pro-caspase-9and pro-caspase-7 were detected, respectively, as 52 and 37 kDafull-length inactive proteins in cytosolic fractions of spinalcords obtained from nontransgenic age-matched with end-stage,asymptomatic, and symptomatic transgenic mSOD1 mice (Figs. 4A,5A). However, levels of pro-caspase-9 and pro-caspase-7 were decreasedin symptomatic transgenic mSOD1 mice compared with nontransgeniccontrols (Figs. 4A, 5A). Although neither active caspase-9 orcaspase-7 could be detected in nontransgenic mice, they were bothfound in symptomatic transgenic mSOD1 (Figs. 4A, 5A); note thatactive caspase-9 was detected sooner than active caspase-7 (Figs.4A, 5A).

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Figure 4. Activation of caspase-9 in spinal cords of transgenic mSOD1 mice. A, Using an antibody recognizing both forms of caspase-9, the expression of pro-caspase-9 (52 kDa) and its active fragment (35 kDa) was analyzed by Western blot in cytosolic fractions of spinal cords from transgenic mSOD1 mice at the asymptomatic stage (AS), at the beginning of symptoms (BS), and at the end stage (ES) and was compared with their age-matched nontransgenic littermates (Non-Tg). Each lane corresponds to a different animal. B, The immunolocalization of active caspase-9 was performed on spinal cord sections from transgenic (Tg) mSOD1 mice at end stage (ES) and their age-matched nontransgenic (Non-Tg) littermates.

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Figure 5. Activation of caspase-7 in spinal cords of transgenic mSOD1 mice. A, Using an antibody recognizing both forms of caspase-7, the expression of pro-caspase-7 (37 kDa) and its cleaved fragment (28 kDa) was analyzed by Western blot in cytosolic fractions of spinal cords from transgenic mSOD1 mice at the asymptomatic stage (AS), at the beginning of symptoms (BS), and at the end stage (ES) and was compared with their age-matched nontransgenic littermates (Non-Tg). The top panel corresponds to $beta$ -actin. Each lane corresponds to a different animal and is representative of four to six animals per group. B, The immunolocalization of active caspase-7 was performed on spinal cord sections from transgenic (Tg) mSOD1 mice at end stage (ES) and their age-matched nontransgenic (Non-Tg) littermates.

To determine the cellular localization of activated caspases, we immunostained spinal cord sections from age-matched nontransgenicand transgenic mSOD1 mice at end stage with antibodies directedagainst cleaved caspase-9 and caspase-7. In nontransgenic controls,neither of the two antibodies generated any significant cellularimmunostaining for caspase-9 or caspase-7 fragments (Figs. 4B,5B). On the contrary, in transgenic mSOD1 mice, numerous largemotor neurons of anterior horn showed a strong immunostainingfor active caspase-9 and caspase-7 (Figs. 4B, 5B).

Cleavage of XIAP reflects caspase activation

The member of the inhibitor of apoptosis family, XIAP, antagonizes the caspase cascade through a direct inhibition of caspase-3,caspase-7, and caspase-9 (Deveraux and Reed, 1999). Cleavage ofXIAP reflects an excess of activated caspases and produces a 30kDa fragment with reduced ability of inhibiting caspases (Deverauxet al., 1999). We used an anti-XIAP antibody recognizing the aminoacid residues (~240) corresponding to the cleavage site of XIAP(Deveraux et al., 1999). The full-length protein was detectedas a band of 53 kDa in nontransgenic and transgenic mice (Fig.6). However, at the end stage of the disease, the level of XIAPwas dramatically depleted and a ~30 kDa fragment was concomitantlygenerated (Fig. 6). A nonspecific band migrating slightly largerthan XIAP was also detected as described previously (Deverauxet al., 1999).

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Figure 6. Cleavage of XIAP in spinal cords of transgenic mSOD1 mice. XIAP expression was analyzed by Western blot in cytosolic fractions of spinal cords from transgenic mSOD1 mice at the asymptomatic stage (AS), at the beginning of symptoms (BS), and at the end stage (ES) and was compared with their age-matched nontransgenic littermates (Non-Tg). The top panel corresponds to $beta$ -actin. Each lane corresponds to a different animal and is representative of four to six animals per group.

Immunostaining of cytochrome c of human spinal cord from ALS patient

As indicated above, translocation of cytochrome c is pivotal in the mitochondrial-dependent caspase activation. Therefore,to determine whether this pathway, as in transgenic mSOD1 mice,is in play in human patients with ALS, we assessed cytochromec immunostaining in spinal cord specimens from sporadic ALS patientsand controls. Very similar to the situation seen in mice, neuronswith punctate cytochrome c immunostaining were seen in both controlsand ALS (Fig. 7). As in mice, in ALS specimens but not in controls,several anterior horn neurons exhibited a strikingly more robustand more diffuse cytosolic cytochrome c immunostaining (Fig. 7).

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Figure 7. Immunostaining for cytochrome c of spinal cord from ALS patients and controls. The immunostaining for cytochrome c was processed on spinal cord sections obtained from control (A-D; n = 7) and from ALS (E-H; n = 6) patients. In controls, cytochrome c-positive neurons were faintly stained and punctuate (A-D). In ALS cases, some neurons exhibited a control-like appearance (H), whereas most others were much more intensely and evenly immunostained (F, G).

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We studied selected key molecular factors of the mitochondrial-dependent apoptotic pathway in the spinal cord of transgenicmSOD1 mice and human ALS because of its major potential clinicaland therapeutic significance. Herein, we found that cytochromec contents rose in the cytosolic fraction of transgenic mSOD1mice, whereas, concomitantly, it dropped in the mitochondrialfraction over the course of the disease. This finding indicatesthat, during the neurodegenerative process, the spinal cord oftransgenic mSOD1 mice is the site of a translocation of cytochromec from the mitochondria to the cytosol, which is a critical eventin the mitochondrial-dependent apoptotic pathway (Kroemer andReed, 2000). However, mitochondria in the spinal cord of transgenicmSOD1 mice develop, over the course of the disease, major structuralalterations, including cristae distortions, vacuolization, andvariable degrees of swelling (Kong and Xu, 1998). Therefore, theappearance of cytochrome c immunostaining in some areas of motorneurons in affected transgenic mSOD1 mice could correspond todistended mitochondria (Fig. 2E,F), which could possibly accountfor some of the cytosolic-like cytochrome c immunostaining. Furthermore,cytochrome c may have leaked out from these damaged organelles.Against these hypotheses is the fact that cytochrome c releasewas detected in transgenic mSOD1 mice before the appearance ofthose mitochondria alterations (Kong and Xu, 1998). Supportingthe pathological significance of cytochrome c translocation inthe transgenic mouse model of ALS are the following observations.First, the redistribution of cytochrome c appeared specific foraffected brain regions, because cerebellum, which is devoid ofneuropathological changes in this model (Dal Canto and Gurney,1995), did not show evidence of cytochrome c translocation. Second,the cytochrome c release was related to the cytotoxic effectsof the mutant protein and not to increased SOD1 activity, becauseage-matched transgenic wtSOD1 mice, with also approximately fourfoldincreased SOD1 activity (Mena et al., 1997), did not show spinalcord cytochrome c translocation. Third, cytochrome c translocationculminates in 3-month-old transgenic mSOD1 mice, the age at whichthe most active wave of motor neuron death occurs in these animals(Kong and Xu, 1998).

The transgenic mSOD1 mouse is a faithful model of the mSOD1-linked familial form of ALS (Bruijn and Cleveland, 1996), buthow good this experimental model is for sporadic ALS is uncertain.Relevant to this issue is the observation that cytochrome c is,as in the transgenic mice, translocated in human postmortem spinalcord samples from sporadic ALS cases. This finding not only providesfurther credibility to the transgenic mSOD1 mouse model of ALSbut also demonstrates that cytochrome c translocation is probablya consistent neuropathological feature of ALS, regardless of whetheror not the disease is linked to mSOD1. Of note, as in ALS cases,several controls died from respiratory failure and yet they showedno evidence of spinal cord cytochrome c translocation. It canthus be suggested that the redistribution of cytochrome c in ALSresults from the disease process and not from the cause ofdeath.

Proteins of the Bcl-2 family regulate cell death in part by affecting mitochondrial cytochrome c redistribution (Vander Heidenand Thompson, 1999). In symptomatic transgenic mSOD1 mice, expressionof Bcl-2 and Bcl-xL, which inhibit apoptosis, is reduced, whereasexpression of Bad and Bax, which promote apoptosis, is increased(Vukosavic et al., 1999). In neuronal death induced by trophicfactor deprivation or in Fas-inducing cell death, the redistributionof Bax from the cytosol to the mitochondria is a critical eventfor exerting its proapoptotic activity (Putcha et al., 1999).Given this, it is important to indicate that Bax does translocatefrom the cytosol to the mitochondria in spinal cords of affectedtransgenic mSOD1 mice. This finding agrees with the compartmentalredistribution of selected Bcl-2 members in vulnerable regionsin ALS patients (Martin, 1999). Here we found that the redistributionof Bax to the mitochondria occurs either just before or at thesame time as the release of cytochrome c to the cytosol, suggestingthat Bax in this model of ALS, as in other cell death settings(Finucane et al., 1999; Putcha et al., 1999), participates intriggering cytochrome crelease.

Once released from the mitochondria, cytochrome c interacts in the cytosol with Apaf-1, forming an ATP-dependent complex thatactivates caspase-9 (Liu et al., 1996; Li et al., 1997; Zou etal., 1997; Hu et al., 1999; Saleh et al., 1999), which is instrumentalin the mitochondrial-dependent activation of downstream effectorcaspases such as caspase-3 and caspase-7 (Slee et al., 1999).In the spinal cord of transgenic mSOD1 mice, a weak activationof caspase-9 is detected in early symptomatic animals, which coincideswith the peak of cytosolic cytochrome c, and becomes conspicuousin end-stage animals. In contrast, activation of caspase-7, likethat of caspase-3 (Pasinelli et al., 2000; Vukosavic et al., 2000),appears later over the course of the disease in these mice. Thissequence of events is consistent with our current knowledge ofthe hierarchical organization of these different molecules withinthis apoptotic cell death-related machinery (Pettmann and Henderson,1998). Accordingly, it is likely that activated caspase-9 probablyinitiates the processing of caspase-7 (Fig. 5) and of caspase-3(Pasinelli et al., 2000; Vukosavic et al., 2000). Activated caspase-3and caspase-7 can cleave other caspases, including caspase-9 (Sleeet al., 1999). Consequently, the late and enhanced surge in caspase-9activation could result in part from a feedback effect of activatedcaspase-3 and caspase-7.

Aside from the dramatic loss of motor neurons, spinal cord specimens from both human ALS cases and transgenic mSOD1 mice exhibita strong glial reaction (Adams et al., 1984; Almer et al., 1999;Levine et al., 1999). Because glial cells can produce potent proapoptoticmolecules, including tumor necrosis factor- $alpha$ and interleukin-1- $beta$ ,it is plausible that gliosis triggers and/or enhances the apoptoticdemise of motor neurons in ALS. Alternatively, the described spinalcord apoptotic markers could have originated, at least in part,from glial cells as in Alzheimer's disease (Shimohama, 2000).In the spinal cord of transgenic mSOD1 mice, however, it appearsthat glial apoptosis is either absent or minimal and that most,if not all, apoptotic cells are reminiscent of neurons (Pasinelliet al., 2000; Vukosavic et al., 2000). Consistent with these previousfindings, the present study shows that activated caspase-9 andcaspase-7 were found in cells exhibiting a morphology of neuronsand not of glial cells. Moreover, the neurons immunopositive forcaspase-9, caspase-7, and for diffuse cytochrome c are likelyengaged in the dying process, because they appear, in almost allcases, condensed and shrunken. Our observation is consistent withthat made by Martin (1999), indicating in human ALS postmortemsamples that most of the remaining motor neurons are at an "attritionalstage" and thus are suffering-diseasedneurons.

The IAPs family members are very well conserved evolutionary proteins that are characterized by the presence of baculoviral-inhibitorof apoptosis repeat (BIR) domains. The overexpression of eachmember or just the BIR domains is sufficient to block apoptosisin different paradigms of cell death (Liston et al., 1996; Deverauxet al., 1997; Roy et al., 1997). For instance, overexpressionof XIAP attenuates cellular and behavioral deficits produced byan ischemic injury to the rat hippocampus, and adenovirus-mediatedtransgene expression of XIAP blocks the death of dopaminergicneurons in the substantia nigra after the administration of theparkinsonian toxin 1-methyl-4-phenyl-1,2,3,6-tetrahydropyridine(Xu et al., 1999; Eberhardt et al., 2000). Moreover, some IAPfamily members can delay motor neuronal death after axotomy (Perreletet al., 2000). Here we found that XIAP, the most potent inhibitorof apoptosis in the IAP family (Deveraux and Reed, 1999), wascleaved, and thus inactivated, in end-stage transgenic mSOD1 mice.This data, in association with our previous demonstration of adownregulation of Bcl-2 in transgenic mSOD1 (Vukosavic et al.,1999), suggests that not only does the activity of effectors ofapoptosis rise over the course of the disease but also that theactivity of inhibitors of apoptosis drops. Our demonstration ofXIAP cleavage in affected transgenic mSOD1 mice provides meaningfulfunctional information, which allows one to conclude that caspaseactivation may have real pathological consequences in this modelofALS.

The present study shows that some common apoptotic steps, namely mitochondrial translocation of Bax, cytosolic translocationof cytochrome c, and activation of caspase-9 and caspase-7 arerecruited during the degeneration of motor neurons in the spinalcord of transgenic mSOD1 mice. All of these events arise in asequential manner and are associated with the cleavage of theinhibitor of apoptosis XIAP. Previously, we have demonstratedthat caspase inhibition (Li et al., 2000) and Bcl-2 overexpression(Kostic et al., 1997) succeed in prolonging survival but not instopping the disease in transgenic mSOD1 mice. This suggests that,although the mitochondrial apoptotic machinery may be pivotalin the demise of motor neurons in ALS, its multifactorial naturemay require combining several anti-apoptotic strategies to achieveoptimal neuroprotection. In keeping with this possibility, thepresent study, by unraveling key apoptotic factors and the sequencein which they intervene, should help in the development of moreeffective therapeutic approaches forALS.

  FOOTNOTES

Received April 11, 2001; revised June 1, 2001; accepted June 6, 2001.

This study is supported by the Muscular Dystrophy Association, the Amyotrophic Lateral Sclerosis Association, Project AmyotrophicLateral Sclerosis, National Institute of Neurological Disordersand Stroke Grants R01 NS38586, R29 NS37345, and P50 NS38370, UnitedStates Department of Defense Grant DAMD 17-99-1-9471, the LowensteinFoundation, the Smart Foundation, and the Parkinson's DiseaseFoundation. M.V. is a recipient of a fellowship from the HumanFrontier Science Program Organization. We are grateful to NormaRomero for technical help, Dr. Caiping Chen for genotyping, Dr.Brigitte Sola and Dr. Brigitte Onténiente for their continualsupport, and Dr. Vernice Jackson-Lewis for critical reading ofthismanuscript.
Correspondence should be address to Dr. Serge Przedborski, Departments of Neurology and Pathology, BB-307, Columbia University,650 West 168th Street, New York, NY 10032. E-mail: SP30{at}columbia.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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