Selective and Protracted Apoptosis in Human Primary Neurons Microinjected with Active Caspase-3, -6, -7, and -8

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The Journal of Neuroscience, November 15, 2000, 20(22):8384-8389

Selective and Protracted Apoptosis in Human Primary Neurons Microinjected with Active Caspase-3, -6, -7, and -8
Yan Zhang¹^,³, Cynthia Goodyer², and Andréa LeBlanc¹^,³
Departments of ¹ Neurology and Neurosurgery and ² Pediatrics, McGill University, Montreal, Quebec, Canada H3A 1W9, and ³ The Bloomfield Center for Research in Aging, Lady Davis Institute for Medical Research, Jewish General Hospital, Montreal, Quebec, Canada H3T 1E2

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We have shown previously that caspase-6 is activated in serum deprivation-mediated human neuronal cell death and correlateswith increased production of Alzheimer's disease (AD) amyloid $beta$ peptide (A $beta$ ). Here, we show by direct microinjection of recombinantactive enzymes that caspase-6 (>0.5 pg/cell) induces a protractedcourse of apoptosis in neurons in a caspase-specific, dose- andtime-dependent manner in the presence of serum. Only transientactivation of caspase-6 is required to initiate apoptosis. Caspase-6induces apoptosis directly without the activation of other caspaseeffectors. Doses of caspase-6 of <0.25 pg/cell induce only 20%cell death within 16 d but render neurons vulnerable to oxidativestress, indicating that caspase activation affects neurons despitethe absence of cell death. Caspase-3 induces neuronal apoptosisin 20% of the cells, whereas caspase-7 or -8 do not induce apoptosis.In contrast, astrocytes undergo apoptosis within 24 hr when microinjectedwith caspase-3 but not caspase-6, -7, or -8. These results showcell type-specific vulnerability to caspases in the CNS. The resultssuggest that activation of caspases in human neurons does notlead to an immediate and rapid process of cell death but provokesa protracted form of apoptosis. Activation of caspases in humanneurons may participate in the long-term overproduction of A $beta$ and other potential toxic fragments resulting from caspase-mediatedproteolysis. These results are consistent with the protractedand age-dependent nature ofAD.

Key words: caspase; primary neurons; Alzheimer's disease; oxidative stress; astrocytes; apoptosis

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Neuronal loss correlates with neuronal dysfunction (Gomez-Isla et al., 1996, 1997) in Alzheimer's disease (AD), and caspasesare involved in neuronal death (Masliah et al., 1998; Yang etal., 1998; Gervais et al., 1999; LeBlanc et al., 1999; Selznicket al., 1999; Shimohama et al., 1999; Stadelmann et al., 1999).However, specific features of caspase-mediated neuronal apoptosisare difficult to address in vivo because of the rapid clearanceof apoptotic cells from organs. In addition, species and celltype specificity of apoptotic mechanisms make it hard to extrapolatefrom in vitro to in vivo. We have shown that apoptosis of humanprimary neurons results in an increased production of amyloid $beta$ peptide, suggesting that apoptosis-related activation of proteasesin implicated in the metabolism of amyloid precursor protein (APP)(LeBlanc 1995). Further studies showed that caspase-3, -6, -7,and -8 can cleave APP directly (Barnes et al., 1998; Gervais etal., 1999; LeBlanc et al., 1999; Pellegrini et al., 1999; Weidemannet al., 1999). Furthermore, caspase inhibitors eliminate the apoptosis-mediatedincrease in amyloid $beta$ peptide (Barnes et al., 1998; Gervais etal., 1999; LeBlanc et al., 1999). These studies raise the possibilitythat increased amyloid $beta$ peptide production is, in some cases,the result of caspase activation. To fully understand the potentialimpact of caspase activation in human CNS neurodegenerative diseases,it is important to determine how caspase activation affects humanCNS neuronalapoptosis.

Caspase-3 and -9 activities are likely critical in developmental neuronal cell death because elimination of caspase-3 activityleads to extra numbers of neurons in the frontal lobe of animalsand premature death of mice (Kuida et al., 1996, 1998; Hakem etal., 1998). Increased immunoreactivity to caspase-3 and to caspase-3-cleaved $beta$ -actin or APP has been shown in AD brains (Masliah et al., 1998;Yang et al., 1998; Gervais et al., 1999; Shimohama et al., 1999).Whereas the immunoreactivity to the CM1 antibody to active caspase-3is not increased in neurons associated with senile plaques orneurofibrillary tangles, it is increased in granulovacuolar degenerationin AD (Selznick et al., 1999; Stadelmann et al., 1999). In addition,caspase-6 and caspase-9 active p10 fragments increase in AD braintissue (LeBlanc et al., 1999; Lu et al., 2000). These resultsimplicate caspases in AD pathogenesis. However, the use of postmortemtissue cannot address the initial role of these caspases in humanneurons.

To determine which caspase contributes to cell death and altered APP metabolism in human neurons, we have used a unique modelof primary cultures of well differentiated human neurons. Caspase-6,but not caspase-3, is activated in serum deprivation-mediatedhuman neuronal apoptosis (LeBlanc et al., 1999). Caspase-6 knock-outsare developmentally normal (Zheng et al., 1999), but the roleof caspase-6 in adulthood or aging may be important. Althoughcaspase-1 knock-outs appear normal, they delay Huntington-relatedsymptoms in transgenics carrying excess trinucleotide repeats,indicating that some caspases may function in nonphysiologicalcell death (Ona et al., 1999). These results warrant further studieson the role of caspase-6 in human neuronal apoptosis. Here, wedirectly address the role of caspase-3, -6, -7, and -8 in apoptosisof human neurons and astrocytes by microinjection of recombinantactivecaspases.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Neuron cultures. Primary cultures of neurons were established from cortical and subcortical regions of 12- to 14-week-oldfetal brains as described previously, according to ethical regulationsof the Medical Research Council of Canada and approved by theMcGill University Institutional Review Board (LeBlanc, 1995).Briefly, the brain tissue is dissociated in 0.25% trypsin, trypsininactivated with 10% serum, and the dissociated tissue trituratedafter addition of 0.1 mg/ml deoxyribonuclease I. The dissociatedtissue is successively passed through 130 and 70 µm filters andcentrifuged to pellet the cells. The cells are washed once inPBS and once in complete media. The cells are plated at 3 × 10⁶/ml on poly-L-lysine-coated tissue culture dishes or ACLAR (33C;5 mm; Allied Chemical, Minneapolis, MN) coverslips in minimalessential media in Earle's balanced salt solution containing 0.225%sodium bicarbonate, 1 mM sodium pyruvate, 2 mM L-glutamine, 0.1%dextrose, 1× antibiotic Pen-Strep (all products from Life Technologies,Gaithersburg, MD), and 5% decomplemented fetal bovine serum (HyClone,Logan, UT). One millimolar the anti-mitotic agent 5'fluoro-2'-deoxyuridineis added to the culture media after the cells have attached toprevent proliferation of dividing cells. The cells attach rapidlyand establish intricate neuritic networks within 3 d. Typically,the culture is composed of 90-95% neurons and 5-10% astrocytesthat survive in culture for 4-6 weeks (LeBlanc, 1995). Experimentson neurons were conducted at 10 d ofculture.

Microinjection of recombinant caspase-6. Glass micropipettes pulled by a Flaming/Brown micropipette puller (P-87) with a tipdiameter of ~0.5 µm were used for microinjection. The glass micropipetteswere made from 1.0 mm outer diameter and 0.5 mm inner diameterthin-walled glass capillaries with microfilaments (borosilicatewith filament MTW100F-4; World Precision Instruments, Sarasota,FL). Recombinant active caspase-6 (R-Csp-6) (BIOMOL">Biomol, PlymouthMeeting, PA) was prepared in caspase-6 active buffer containing20 mM piperazine-N,N'-bis-(2-ethanesulfonic acid) (PIPES), 100mM NaCl, 10 mM dithiothreitol (DTT), 1 mM EDTA, 0.1% 3-[(3-cholamidopropyl)-dimethylammonio]-2-hydroxy-1-propanesulfonicacid (CHAPS), and 10% sucrose, pH 7.2. Dextran Texas Red (DTR)(at 100 µg/ml) (Cedarlane, Hornby, Ontario, Canada) was coinjectedwith R-Csp-6 as a fluorescent marker to recognize injected neurons.Control microinjections were made with caspase-6 active bufferand DTR only. As an additional control for the specificity ofcaspase-6-mediated apoptosis, caspase-6 was denatured by boilingfor 10 min and injected at 100 pg/cell. Microinjections were performedusing an Eppendorf Microinjector 5246 and Micromanipulator (MIS-5000;Burleigh Instruments Inc., Fishers, NY), at an injection pressureof 100 hectoPascal (hPa), compensation pressure of 50 hPa, andan injection time of 0.1 sec. The injected volume was 1 nl/cell.Neurons were injected into the cytosolic area of the cell soma.Approximately 90% human neurons survive the microinjection ofDTR for at least 16 d indicating, the resistance of the neuronsto the physical stress ofmicroinjection.

For the dose and time response curves, 0.01, 0.05, 0.1, 0.25, 0.5, 5, 10, 20, 50, or 100 pg/cell R-Csp-6 were coinjected withDTR in 100 cells on each of two coverslips per neuron preparation.The injected neurons were incubated for various times at 37°Cin serum containing normal neuron media in the presence or absenceof 5 µM BOC-D-fmk, N-benzyloxycarbonyl-Val-Ala-Asp-fluoromethylketone (Z-VAD-fmk), N-benzyloxycarbonyl-Val-Glu-Ile-Asp-fluoromethylketone (Z-VEID-fmk), N-benzyloxycarbonyl-Ile-Glu-Thr-Asp-fluoromethylketone (Z-IETD-fmk), and N-benzyloxycarbonyl-Asp-Glu-Val-Asp-fluoromethylketone (Z-DEVD-fmk) (BIOMOL">Biomol) dissolved at 5 mM in DMSO. As a controlfor the solvent, 0.001% of DMSO was added to DTR-microinjectedneurons. The negative controls were injected with DTR preparedin caspase-6 active buffer. The positive controls were injectedwith DTR only and treated for 24 hr with 10 µM staurosporine toshow that neurons can succumb to an apoptoticsignal.

Astrocytes were injected at an injection pressure of 50 hPa, compensation pressure of 30 hPa, and an injection time of 0.1sec. The injected volume was 0.3 nl/cell. Astrocytes were injectedinto the cytosolic area of the cell soma. Approximately 50% humanastrocytes survive the injection for at least 16 d. Twenty or100 pg/cell R-Csp-6 were coinjected with DTR in 100 cells on eachof two coverslips per astrocytepreparation.

Immunostaining of microinjected caspase-6. Microinjected neurons (0.5 pg/cell R-Csp-6) were fixed at 0, 1, 2, 3, 4, and 8d after injection in fresh 4% paraformaldehyde and 4% sucrosefor 20 min at room temperature and permeabilized in 0.25% TritonX-100 for 10 min at room temperature. Ten percent fetal goat serumin PBS was used for blocking for 20 min at room temperature. Antibodyto active caspase-6 p10 fragment (1:250) (PharMingen, San Diego,CA) was incubated for 2 hr at room temperature. Secondary goatanti-mouse antibody conjugated to FITC (1:200) was used fordetection.

Sublethal oxidative stress treatment. As an oxidative stress, a sublethal dose of 0.1 µM H₂O₂ was added to the media of R-Csp-6(0.1 pg/cell) or control microinjected neurons (Paradis et al.,1996). The neurons were incubated for 0, 2, and 4 d afterinjection.

Measurement of apoptosis. Neurons and astrocytes were fixed in fresh 4% paraformaldehyde and 4% sucrose for 20 min at roomtemperature and permeabilized in 0.1% Triton X-100 and 0.1% sodiumcitrate for 2 min on ice. Terminal deoxynucleotidyl transferase-mediatedbiotinylated UTP nick end labeling (TUNEL) was performed usingthe in situ cell death detection kit I as described by the manufacturer(Roche Products, Hertforshire, UK). The percentage of neuronalapoptosis was determined by the ratio of the number of DTR andTUNEL double-positive neurons over the total number of DTR-positiveneurons. The number of DTR-positive neurons or astrocytes didnot decrease with time, indicating the retention of all apoptoticand nonapoptotic microinjected neurons on thecoverslip.

Caspase fluorogenic activity assays. Recombinant caspases -3, -6, -7, or -8 (PharMingen) were assayed for activity using relevantfluorogenic peptide substrates. Caspase activity in 10 ng of enzymewas measured using 7 µM Ac-DEVD-AFC for caspases-3 and -7, Ac-VEID-AFCfor caspase-6, and Ac-IETD-AMC (BIOMOL">Biomol) in caspase reaction buffer(20 mM PIPES, 30 mM NaCl, 10 mM DTT, 1 mM EDTA, 0.1% CHAPS, and10% sucrose, pH 7.2). Release of the fluorogenic moiety Ac, N-acetylcoumarin (AFC) or 7-amino-4-trifluoromethyl coumarin (AMC) wasmonitored over time in a Bio-Rad (Hercules, CA) Fluoromark apparatus.Excitation was at 390 nm for AFC or AMC, and emission was at 538nm for AFC or at 460 nm for AMC. Readings were recorded at 2 minintervals over 1 hr. A standard curve of fluorescence of AFC orAMC allowed calculation of nanomoles of released AFC/AMC in thereactions. Specific activities were expressed as nanomoles ofAFC/AMC released per microgram of protein per minute, based onthe linear range of thecurve.

Statistical evaluation of the results. For the dose response, H₂O₂ stress, and recombinant caspase-3, -7, and -8 activities,statistical evaluations were assessed using two-tailed, unpairedStudent's t test. For the time and dose response of R-Csp-6, two-wayANOVA was performed with independent variables as time factor(df = 7) and dosage factor (df = 7). Post hoc analysis with two-tailedunpaired t test was applied as a follow-up for the significantdifference shown by ANOVA for both time and dosage factors. p< 0.05 was used as indicative of statisticalsignificance.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Microinjected recombinant active caspase-6 confers a dose-dependent increase in apoptosis of primary human neurons in culture

In our previous study, we showed the loss of procaspase-6 and the presence of caspase-6 activity in serum-deprived neurons(LeBlanc et al., 1999). These results indicated that caspase-6is responsible for neuronal apoptosis. However, because otherproapoptotic proteins may be activated by serum deprivation, wedetermined whether caspase-6 activation is directly responsiblefor neuronal apoptosis by microinjecting serum-treated neuronswith various amounts of R-Csp-6 and DTR as a fluorescent markerdye. Apoptosis was identified by TUNEL staining 48 hr after themicroinjection. Figure 1A shows a representative example of thedetection of DTR-positive (red) and TUNEL-positive (green) inDTR-microinjected neurons. The TUNEL-positive neuron has the shrunkenappearance of apoptotic cells compared with TUNEL-negative cells.To determine the life span of the microinjected caspase-6 in theneurons, we incubated caspase-6-microinjected neurons for 24,48, 72, and 96 hr and immunostained the cells with a caspase-6antibody. The results show the detection of R-Csp-6 in 95% ofmicroinjected neurons until 24 hr of injection (Fig. 1B). At 48hr, the immunoreactivity is considerably decreased. At 72 or 96hr, caspase-6 is detected only in 2-5% of injected neurons (resultsnot shown).

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Figure 1. Dose-response curve of R-Csp-6 on neuronal apoptosis. A, Detection of apoptotic microinjected neurons. Cells were injected with the marker dye DTR (top), and apoptosis was detected by TUNEL (bottom). The white arrow shows a green TUNEL-positive neuron. B, Immunodetection of caspase-6 after microinjection in neurons. Neurons were microinjected with 5 pg/cell recombinant active caspase-6 and DTR and submitted to immunocytochemistry with monoclonal caspase-6 p10 antibody at various times after the microinjection. C, Survival of neurons microinjected with caspase-6. Neurons in culture were microinjected with DTR and various amounts of R-Csp-6 and stained for TUNEL after 48 hr to determine the percentage of neuronal apoptosis after injection. STS represents apoptosis in non-caspase-6-microinjected neurons incubated with 10 µM staurosporine for 24 hr. Denatured represents neuronal apoptosis 48 hr after neurons were microinjected with 100 pg/cell denatured caspase-6. Data represent the mean and SD of four independent experiments. *p < 0.002. D, Caspase-6 peptide inhibitor effect on cell death. Neurons in culture were microinjected with DTR and 5 pg/cell R-Csp-6 and treated in the absence or presence of 5 µM caspase inhibitors for 48 hr. Data represent the mean and SD. p < 0.004 for BOC-D-fmk, Z-VAD-fmk, and Z-VEID-fmk.

Microinjected neurons show a dose-dependent increase in apoptosis from 0.25 to 20 pg/cell R-Csp-6 (Fig. 1C). Higher dosesof 50 and 100 pg/cell do not result in more TUNEL-positive cells.The maximum amount of apoptosis observed at 48 hr is 50%, indicatingthat some cells are either resistant or undergoing a delayed celldeath after microinjection of R-Csp-6. A high dose of kinase inhibitor,staurosporine (10 µM), provokes over 90% cell death within 24hr, indicating that these neurons are able to undergo a rapidapoptotic cell death. Denatured R-Csp-6 (100 pg/cell) was alsomicroinjected to ensure that apoptosis was directly attributableto active caspase-6 (Fig. 1C). The denatured R-Csp-6 did not causesignificant cell death up to 16 d after injection, suggestingthat the dose-dependent apoptosis is specifically induced by R-Csp-6.

To confirm that caspase-6 is directly responsible for the neuronal apoptosis and is not activating downstream caspases, wetested the effect of general caspase inhibitors BOC-D-fmk andZ-VAD-fmk, caspase-6-specific inhibitor Z-VEID-fmk, caspase-3-specificinhibitor Z-DEVD-fmk, and caspase-8-specific inhibitor Z-IETD-fmkon R-Csp-6-microinjected neurons (Fig. 1D). Z-VEID-fmk was themost potent inhibitor of caspase-6-mediated neuronal apoptosis.The general caspase inhibitors also inhibited caspase-6-mediatedapoptosis, and Z-DEVD-fmk and Z-IETD-fmk were the least efficientand did not show significant inhibition of caspase-6-mediatedapoptosis. Because DEVD also inhibits caspase-2, -7, and -10 (Thornberryet al., 1997), these results indicate that active caspase-6 islethal to human neurons in the absence of other effector caspaseactivity.

To determine whether caspase-6-microinjected neurons that do not exhibit neuronal apoptosis 48 hr after microinjection willeventually succumb or are naturally protected against apoptosis,neuronal cell death was examined over time with varying dosesof microinjected caspase-6 (Fig. 2A). The results show that eventhe lowest lethal dose of caspase-6 (0.5 pg/cell) induces celldeath in ~90% of neurons within 6 d after injection. Thereafter,the remaining 10% of neurons resist the lethal injection of R-Csp-6.The 10% of remaining neurons are either completely resistant tocaspase-6-mediated cell death, or an even longer time is requiredfor apoptosis to occur. A striking feature of these results isthe length of time required for neurons to undergo apoptosis aftera lethal injection of R-Csp-6. We have also observed this extendeddeath in serum deprivation-mediated neuronal loss in which only35% of the human neurons show TUNEL-positive apoptosis after 4d of serum deprivation (Fig. 3B). In contrast, staurosporine-mediatedcell death occurs within 24 hr (Fig. 1C). These results indicatethat caspase-6 induces a protracted course of apoptosis in humanneurons.

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Figure 2. Time-dependent cell death by microinjected R-Csp-6. A, Microinjected neurons were assayed for apoptosis from 1 to 16 d. Data represent the mean and SD from three independent neuron preparations. Two-way ANOVA on doses $>=$ 0.25 pg/cell and time factors (df = 7 for both) results in a statistical significance of p < 0.001. Doses of 0.1 and 0.05 pg/cell showed a statistically significant increase of apoptosis at 6 and 16 d, respectively. In time, doses of 0.5 pg/cell and above were significantly different at 1 d after microinjection, whereas 0.25 pg/cell required 2 d. No increase in apoptosis was observed in time with 0.01 and 0.05 pg/cell up to 16 d after microinjection. B, Percentage of apoptotic neurons in serum-deprived neurons. Data represent the mean and SEM from 18 independent neuron preparations.

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Figure 3. Sublethal dose of caspase-6 renders neurons vulnerable to normally nonlethal doses of oxidative stress. Neurons were microinjected with DTR in the absence or presence of 0.1 pg/cell R-Csp-6 and submitted to serum deprivation or 0.1 µM H₂O₂. Cells were fixed at 0, 48, and 96 hr and analyzed for apoptosis by TUNEL. Data represent the mean and SD of three independent neuron preparations.

A dose of 0.05-0.25 pg/cell R-Csp-6 leads to only 18-24% apoptosis within 16 d, whereas no cell death is detected with 0.01pg/cell R-Csp-6 (Fig. 2A). This finding raises the possibilitythat, although these low doses of R-Csp-6 cannot induce significantcell death, they may act on neuronal protein substrates and altercellular homeostasis. To determine whether the neurons microinjectedwith sublethal doses of caspase-6 are more vulnerable to a secondaryinsult, we treated neurons with serum deprivation or a sublethaldose of oxidative stress (0.1 µM H₂O₂) after microinjection with0.1 pg/cell R-Csp-6 (Fig. 3). The results show that microinjectionof 0.1 pg/cell R-Csp-6 does not cause cell death after 48 or 96hr. The induction of apoptosis by serum deprivation in non-R-Csp-6-microinjectedcells is slightly, but not significantly, exacerbated by R-Csp-6at 48 or 96 hr (p < 0.2). In contrast, a 0.1 µM dose of H₂O₂,which in the absence of R-Csp-6 does not induce apoptosis, significantlyenhances neuronal apoptosis by 96 hr of treatment (p $<=$ 0.004).These results indicate that lower doses of active R-Csp-6 aredetrimental to neurons and render neurons vulnerable to oxidativestress but not to growth factor deprivation. Therefore, low levelsof caspase-6 activation could account for increased neuronal vulnerabilityin aging and neurodegenerative diseases in which oxidative stressis stronglysuspected.

Human neurons are more susceptible to caspase-6 than to caspases-3, -7, or - 8

Many investigators have reported that activation of caspase-3 is important in neuronal apoptosis (Du et al., 1997; Keane etal., 1997; Yakovlev et al., 1997; Barnes et al., 1998; Srinivasanet al., 1998). Particularly, the study of caspase-3 and -9 knock-outmice, showing abrogation of the developmentally regulated neuronalcell death in the forebrain, provides convincing evidence foran important role of caspase-3 and -9 in neuronal apoptosis (Kuidaet al., 1996, 1998; Hakem et al., 1998; Zheng et al., 1999). Becausecaspase-6 can activate caspase-3 (Orth et al., 1996) and to determinewhether caspase-3 or other caspases can also cause apoptosis ofhuman neurons in a manner similar to R-Csp-6, we microinjected20 and 100 pg/cell recombinant caspases-3, -7, and -8 in neurons(Fig. 4A). These recombinant caspases show strong specific activity,as determined by in vitro fluorogenic assay (Fig. 4B). However,we find that only caspase-6 induces significant cell death inthe human neurons, even 16 d after microinjection of 100 pg/cell.Caspase-3 induces a slight increase in apoptosis at the dosagesof 20 and 100 pg/cell (p < 0.05). These results indicate thatdifferentiated human primary neurons are more resistant to caspases-3,-7, and -8 than to caspase-6.

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Figure 4. Human neurons are resistant to caspase-3, -7, and -8. A, Neurons were injected with 20 or 100 pg/cell recombinant caspases. Cells were fixed at the indicated times and stained for TUNEL. Data represent the mean and SD of three neuronal preparations. There is no statistical difference between the DTR-injected and caspases-3-, -7-, or -8-injected neurons, except in caspase-3 at 4 (p = 0.01) and 8 (p = 0.04) d. B, The activity of each recombinant caspases was verified by fluorogenic substrate assay. Data represent the mean and SD of three independent experiments

Human astrocytes are more susceptible to caspase-3 than to caspase-6, 7, or 8

To determine whether other CNS cell types are vulnerable to caspase-6 or other caspases, human astrocytes were microinjectedwith 20 and 100 pg/cell recombinant caspase-3, -6, -7, and -8(Fig. 5). In contrast to neurons, astrocytes undergo apoptosiswith caspase-3 but not caspase-6, -7, or -8. These results showCNS cell type vulnerability to different caspases. In addition,the astrocytes undergo maximal apoptosis within 24 hr after microinjection.These results confirm that the caspase-mediated apoptosis in neuronsis protracted compared with other cell types.

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Figure 5. Astrocytes are resistant to caspase-6, -7, and -8 but undergo apoptosis with caspase-3. Astrocytes were injected with 20 or 100 pg/cell. Apoptosis was determined by TUNEL. Data represents the mean and SD of two experiments from three astrocyte preparations. Statistical difference is achieved only with caspase-3 (p < 0.0001).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Resolving the role of caspase activation in neuronal apoptosis is fundamental to the understanding of neurodegenerative diseases.Generally, caspases are considered effectors of programmed celldeath. The role of caspases in AD is supported by evidence ofincreased caspase-3, caspase-6, and caspase-9 immunoreactivityor activation in AD brain tissue (Masliah et al., 1998; Yang etal., 1998; Gervais et al., 1999; LeBlanc et al., 1999; Selznicket al., 1999; Shimohama et al., 1999; Stadelmann et al., 1999;Lu et al., 2000), the observation that Alzheimer's-associatedproteins, presenilins, and APP are substrates of caspases (Kimet al., 1997; Loetscher et al., 1997; Barnes et al., 1998; Gervaiset al., 1999; LeBlanc et al., 1999; Pellegrini et al., 1999; Weidemannet al., 1999), and the fact that amyloid $beta$ peptide, AD-linkedmutations, or overexpression of APP and presenilins induce neuronalapoptosis (Yankner et al., 1989; Loo et al., 1993; Wolozin etal., 1996; Kim et al., 1997; Nishimura et al., 1998). However,the protracted course of AD and the difficulty in detecting considerablenumbers of apoptotic neurons in postmortem tissue argues againstapoptosis being responsible for neuronal dysfunction and cellloss in AD (Stadelmann et al., 1998).

In the present manuscript, we evaluated the role of caspase activation in neuronal apoptosis of human primary neurons. Wehave shown previously the activation of caspase-6, but not caspase-3,in serum deprivation-mediated apoptosis of these highly differentiatedprimary cultures of human neurons (LeBlanc et al., 1999). However,a number of other proapoptotic proteins may be activated by serumdeprivation, raising the possibility that neuronal apoptosis isnot mediated directly by caspase-6. Our study shows six strikingfeatures of caspase-mediated neuronalapoptosis.

First, caspase-6 is directly responsible for neuronal apoptosis. We find that neurons microinjected with caspase-6 undergoapoptosis in the presence of complete media. The possibility thatcaspase-6 is activating other effector caspases was eliminatedby showing that neither caspase-3 nor caspase-8 caspase peptideinhibitors prevent caspase-6-mediated cell death. As expected,the caspase-6-specific inhibitor Z-VEID-fmk and general caspaseinhibitors significantly prevent apoptosis of caspase-6-microinjectedneurons. These results eliminate the possibility that proteinsother than caspase-6 are responsible for neuronal apoptosis andreasonably demonstrate that caspase-6 acts as an effector caspasein these neurons. The known substrates of caspase-6 are laminA and amyloid precursor protein (Gervais et al., 1999; LeBlancet al., 1999; Nicholson, 1999; Pellegrini et al., 1999). Whetherthe downstream events of caspase-6-mediated cell death requiresproteolysis of these proteins remains to be determined. Caspasecleavage of the APP C-terminal 31 amino acids can increase thevulnerability of cells to a cytotoxic insult (Lu et al., 2000).It is reasonable to assume that caspase-6 initiates downstreamevents that eventually result in the demise of thecell.

Second, a threshold level of caspase-6 is required to induce apoptosis. Lower levels of active caspase-6 do not induce neuronalapoptosis but render neurons vulnerable to a secondary insult.The 0.5 pg of R-Csp-6 required to induce maximal apoptosis is~70 times the amount observed in serum-deprived apoptotic neuronsat 12 hr of serum deprivation (LeBlanc et al., 1999). This levelis comparable with the expression levels obtained in transfectedcell lines. The lack of apoptosis in neurons microinjected withcaspase-6 at 0.25 pg/cell or less is intriguing. These neuronsare not normal, as shown by the addition of a sublethal dose ofoxidative stress. H₂O₂ at 0.1 µM increases apoptosis in neuronsmicroinjected with 0.1 pg/cell R-Csp-6. Therefore, it appearsthat caspase activation does not necessarily induce apoptosisbut renders neurons vulnerable to oxidative stress, a well knownage-dependent stress of the brain. Together, these results demonstratethat the level of active caspase in neurons can result in eitherimmediate or delayedapoptosis.

Third, we show that the microinjected caspase-6 disappears from most injected cells within 48 hr. Yet, 80-90% of these microinjectedneurons become apoptotic within 6 d of microinjection. These resultsindicate that caspase-6-mediated apoptosis requires only transientactivation. Therefore, the detection of caspases may be impossibleto detect at the end point of neurodegeneration in postmortemtissue, and the absence of detectable active caspase fragmentsmay not necessarily indicate normal neurons. These results mayexplain the discrepancy between the detection of caspase-cleavedproteins such as $beta$ -actin and amyloid precursor protein and activecaspases in AD postmortem tissues (Yang et al., 1998; Gervaiset al., 1999; Selznick et al., 1999; Stadelmann et al., 1999).

Fourth, our study demonstrates that 10% of neurons microinjected with a lethal dose of R-Csp-6 resist apoptosis up to 16 dafter the microinjection. These results show that neurons canresist certain levels of active caspase-6 without an absolutecommitment to cell death. These neurons may represent a subspeciesof neurons that are either insensitive to active caspase-6 orcontain high levels of natural inhibitors of caspase-6. The resistanceof some of the human primary neurons to caspase-6 could explainthe selective neuronal cell death that occurs in neurodegenerativediseases.

Fifth, the microinjected neurons undergo an extended form of apoptosis, even with the highest lethal dose of caspase-6. Thiselongated mode of cell death is also observed in serum-deprivedneurons in which only 35% of apoptosis occurs after 4 d. Althoughit could be argued that terminally differentiated neurons havebecome resistant to growth factor deprivation, the direct microinjectionof active caspase-6 in neurons indicates an unusual extended formof cell death. In contrast, staurosporine treatment of neuronsor microinjection of recombinant caspase-3 in astrocytes inducesrapid apoptosis within 24 hr. These results suggest that humanneurons submitted to caspase-6 activation do not undergo the rapidtype of apoptosis observed in many cell lines. In humans, neuronshave to survive for 8-10 decades, and these cells probably haveevolved the best survival mechanisms to prevent rapid loss ofthis essential cell type. We propose that the extended death ofthe human neuron is the result of the presence of endogenous caspaseinhibitors or activation of a number of survival programs responsiblefor counteracting various insults. This feature is likely oneof all long-lived celltypes.

Last, the resistance of the human neurons to microinjected recombinant active caspase-3, -7, and -8 is also very surprising.In contrast to caspase-6, caspase-3 induces only a slight, albeitstatistically significant, increase in neuronal apoptosis, whereascaspases-7 and -8 do not increase apoptosis. We had presumed thatactive caspase-3 would result in significant neuronal cell death.Others have shown the importance of caspase-3 in developmentalneuronal cell death of mice (Kuida et al., 1996; Srinivasan etal., 1998), and there is evidence for the role of caspase-3 activationin AD (Kim et al., 1997; Masliah et al., 1998; Yang et al., 1998;Gervais et al., 1999; Selznick et al., 1999; Stadelmann et al.,1999). The resistance of neurons to caspase-3 may indicate thepresence of strong natural inhibitors of caspase-3 such as theinhibitors of apoptosis (IAPs) (Roy et al., 1997) or the lackof downstream pathways leading to apoptosis. Whether IAPs decreasewith age or with various insults remains to be determined butour results suggest the presence of strong inhibitors of caspase-3in healthy neurons but not in astrocytes. Conversely, endogenouscaspase-6 inhibitors may be present in astrocytes but not in neurons.The IAPs do not inhibit caspase-6; therefore, other inhibitorsmust be present in thesecells.

Together, these findings are consistent with the protracted course and the age-dependent characteristics of AD. Therefore,activation of caspases in vivo may not be directly linked to immediateneuronal apoptosis in the CNS. However, the neurons are not necessarilynormal. Apoptosis of human neurons increase the production ofamyloid $beta$ peptide, and caspases are involved in APP and presenilinproteolytic processing (LeBlanc, 1995; Kim et al., 1997; Loetscheret al., 1997; Barnes et al., 1998; Gervais et al., 1999; LeBlancet al., 1999; Pellegrini et al., 1999; Weidemann et al., 1999).Therefore, this extended type of apoptosis in human neurons couldresult over time in a significant increased production of amyloid $beta$ peptide, as well as in the degradation of other functional neuronalproteins such as presenilins, leading to a dysfunctional neuronlong before neuronal cell death. In addition, similar to neuronsin culture, AD neurons with increased levels of active caspasescould be induced to undergo apoptosis by a secondary insult suchas oxidative stress, which is a well known age-dependent stressof the brain and is believed to play an important role in neurodegenerativediseases (Mattson et al., 1999).

  FOOTNOTES

Received June 27, 2000; revised Aug. 16, 2000; accepted Aug. 24, 2000.

This work was supported by the Medical Research Council of Canada and the Fond de Recherche en Santé du Québec to A.L.B.The technical assistance of Beverly Akerman and Jennifer Hammondis gratefullyacknowledged.
Correspondence should be addressed to Dr. Andréa LeBlanc, The Bloomfield Center for Research in Aging, Lady Davis Institutefor Medical Research, The Sir Mortimer B. Davis Jewish GeneralHospital, 3755 chemin Côte Sainte-Catherine, Montréal, Québec,Canada H3T 1E2. E-mail: mdal{at}musica.mcgill.ca.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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