(Received for publication, May 30, 1996, and in revised form, December 27, 1996)
From the Institute of Cell and Molecular Biology, University of
Edinburgh, Edinburgh, EH9 3JR Scotland, United Kingdom, the
¶ Division of Oncology Research and ** Protein Core Facility, Mayo
Clinic, Rochester, Minnesota 55905, and Athena
Neurosciences, Inc., S. San Francisco, California 94080
Recent genetic and biochemical studies have
implicated cysteine-dependent aspartate-directed proteases
(caspases) in the active phase of apoptosis. In the present study,
three complementary techniques were utilized to follow caspase
activation during the course of etoposide-induced apoptosis in HL-60
human leukemia cells. Immunoblotting revealed that levels of
procaspase-2 did not change during etoposide-induced
apoptosis, whereas levels of procaspase-3 diminished markedly
2-3 h after etoposide addition. At the same time, cytosolic peptidase
activities that cleaved DEVD-aminotrifluoromethylcoumarin and
VEID-aminomethylcoumarin increased 100- and 20-fold, respectively; but
there was only a 1.5-fold increase in
YVAD-aminotrifluoromethylcoumarin cleavage activity.
Affinity labeling with
N-(N-benzyloxycarbonylglutamyl-N
-biotinyllysyl)aspartic
acid [(2,6-dimethylbenzoyl)oxy]methyl ketone indicated that multiple
active caspase species sequentially appeared in the cytosol during the
first 6 h after the addition of etoposide. Analysis on one- and
two-dimensional gels revealed that two species comigrated with
caspase-6 and three comigrated with active caspase-3 species,
suggesting that several splice or modification variants of these
enzymes are active during apoptosis. Polypeptides that comigrate with
the cytosolic caspases were also labeled in nuclei of apoptotic HL-60
cells. These results not only indicate that etoposide-induced apoptosis
in HL-60 cells is accompanied by the selective activation of multiple
caspases in cytosol and nuclei, but also suggest that other caspase
precursors such as procaspase-2 are present but not activated during
apoptosis.
Recent studies (reviewed in Refs. 1-5) indicate that the cytotoxicity of virtually all chemotherapeutic agents is accompanied by apoptosis in susceptible cell lines. Likewise, experiments in animals (6-9) and studies of circulating blasts from leukemia patients (10) have provided evidence that chemotherapy is accompanied by apoptosis in vivo. Moreover, it has been suggested that resistance to the cytotoxic effects of chemotherapeutic agents can result from resistance to chemotherapy-induced apoptosis (8, 11, 12). These observations highlight the potential importance of understanding the factors that control apoptosis.
A variety of experimental results suggest that
ICE1 family proteases (now termed
caspases)2 might play a critical role in
initiating and sustaining the biochemical events that result in
apoptotic cell death (reviewed in Refs. 5 and 13-15). Caspases are
unusual in several respects. First, although they are
cysteine-dependent proteases, the members that have been
examined are insensitive to antipain and E64, two broad spectrum
inhibitors of sulfhydryl proteases (16, 17). Second, caspases cleave at
the carboxyl side of aspartate residues (17-20), a specificity that is
unusual for mammalian proteases. Third, activation of caspases appears
to require cleavage at Asp-X sequences in the proenzymes to
yield the large and small subunits that are present in the active
2
2 tetramer (reviewed in Refs. 15, 17, and 21). The last two observations raise the possibility that caspases
might undergo autoactivation and/or activate each other in a cell death
cascade (17, 22, 23).
In Caenorhabditis elegans, deletion of the ced-3 gene, which encodes the single caspase known for this organism, abolishes all developmentally regulated cell death (24, 25). In higher eukaryotes, the situation appears to be more complex. First, proenzyme forms of multiple caspases are expressed in many cell types (17, 22, 26, 27). Second, deletion of the genes for several of these proteases does not appear to alter the features of apoptosis induced by many stimuli, perhaps because of functional redundancy in the substrate recognition properties of these proteases (14, 28).
Previous studies have also identified a number of cellular polypeptides
that are cleaved during apoptosis (reviewed in Refs. 5, 14, 15, and
28). These include the DNA damage recognition protein PARP, which is
cleaved at the sequence DEVDG (29), and the lamins, which are
cleaved by a protease that recognizes the sequence VEID
N (20). After
treatment of HL-60 human acute myelomonocytic leukemia cells with a
variety of chemotherapeutic agents, PARP and lamin B1 are
cleaved just prior to or concomitant with the appearance of other
apoptotic changes (30, 31). Other polypeptides that appear to be
cleaved by caspases during apoptosis in various cell types include the
DNA-activated protein kinase DNA-PK, the retinoblastoma gene product,
the 70-kDa polypeptide subunit of U1 small nuclear ribonucleoprotein
complexes, steroid response element binding proteins, protein kinase
C
, actin, and the intermediate filament-associated polypeptide Gas2
(reviewed in Refs. 5 and 15). The individual proteases responsible for
these cleavages in situ have not been conclusively
identified. Recent studies have indicated that PARP can be cleaved
in vitro by a variety of caspases including caspase-1, -2, -3, -4, -6, -7, and -8 (17, 22, 26, 32-34), although cleavage of
expressed fragments of PARP by caspase-1, -2, and -4 appears to require enzyme concentrations that are stoichiometric rather than catalytic (17, 29, 33). To date, caspase-6 (previously termed Mch2) is the only
caspase known to be capable of cleaving the lamins (20, 35).
In the present study, we have examined HL-60 cells undergoing apoptosis after treatment with the topoisomerase II-directed agent etoposide (reviewed in Ref. 36). These studies have focused on determining 1) the number of caspases that are activated during etoposide-induced apoptosis, 2) the subcellular distribution of these active caspases, and 3) the identity of the active caspases. In order to address these questions, a novel affinity label for active caspases was synthesized and characterized, and a new fluorogenic assay for caspase-6-like protease activity was developed.
Reagents were obtained from the following
suppliers: etoposide, leupeptin, pepstatin, tetrapropylammonium
hydroxide, PMSF, AMC, and AFC from Sigma; aprotinin
from Mobay Pharmaceuticals (New York, NY); poly(A)+ RNA
from HL-60 cells from Clontech (Palo Alto, CA); AmpliTaq polymerase
from Perkin-Elmer; Superscript RT reverse transcriptase and the
Bac-to-BacTM system from Life Sciences, Inc.; rabbit
anti-caspase-1 (PC84) from Calbiochem; murine monoclonal anti-caspase-2
and anti-caspase-3 from Transduction Laboratories (Lexington, KY);
peroxidase-labeled secondary antibodies from KPL (Gaithersburg, MD);
14C-labeled thymidine (57.8 mCi/mmol), Hybond-N membranes,
and ECL enhanced chemiluminescence reagents from Amersham Corp.;
N-hydroxysuccinimidobiotin from Pierce;
N-(Z)-aspartic acid -t-butyl ester
and YVAD-cmk from Bachem (King of Prussia, PA); DEVD-AFC, YVAD-AFC, and
DEVD-fmk from Enzyme Systems Products (Dublin, CA); and Biolytes from
Bio-Rad.
HL-60 cells (a kind gift from Ron Schnaar, Johns Hopkins University School of Medicine) were cultured in RPMI 1640 medium containing 10% (v/v) heat-inactivated fetal bovine serum, 100 units/ml penicillin G, 100 µg/ml streptomycin, and 2 mM glutamine (medium A). THP.1 cells (American Type Culture Collection, Rockville, MD) were propagated in medium A containing 50 µM 2-mercaptoethanol. All cell lines were maintained at concentrations of <1 × 106 cells/ml to ensure logarithmic growth.
Induction of ApoptosisAt the start of each experiment, nonviable cells were removed by sedimentation at 200 × g for 20 min on Ficoll-Hypaque step gradients (density = 1.119 g/cm3). Cells harvested from the interface were diluted with RPMI 1640, sedimented at 200 × g for 10 min, and resuspended in fresh growth medium. Etoposide (prepared as a 1000-fold concentrated stock in Me2SO) was added to HL-60 cells at a concentration of 68 µM, a high but clinically achievable concentration (37) that has previously been shown to induce apoptosis in >85% of HL-60 cells within 6 h (31).
Preparation of Cytosol and Nuclei (Modified from Ref. 38)After drug treatment, all steps were performed at 4 °C.
Cells were sedimented at 200 × g for 10 min, washed
twice in serum-free RPMI 1640 or phosphate-buffered saline, and
resuspended in buffer C (25 mM HEPES (pH 7.5 at 4 °C), 5 mM MgCl2, 1 mM EGTA supplemented immediately before use with 1 mM PMSF, 10 µg/ml pepstatin
A, and 10 µg/ml leupeptin). After a 20-min incubation on ice, cells
were lysed with 20-30 strokes in a tight fitting Dounce homogenizer. Following removal of nuclei by sedimentation at 800 × g for 10 min (see below) or 16,000 × g for
3 min, the supernatant was supplemented with 0.5 mM EDTA
and sedimented at 280,000 × gmax for 60 min in a Beckman TL-100 ultracentrifuge. After the addition of DTT to a
final concentration of 2 mM, the supernatant (cytosol) was
frozen in 50-µl aliquots at 70 °C. Experiments revealed that
aliquots of cytosol retained DEVD-AFC cleavage activity without
noticeable decrement for at least 3 months. All experiments described
in the present study were performed within 1 month of extract
preparation.
To isolate nuclei, the homogenates prepared above were sedimented at 800 × g. The pellet was washed once with buffer C, resuspended in 1 ml of buffer C, and layered over 4 ml of 50 mM Tris-HCl (pH 7.4) containing 2.1 M sucrose and 5 mM MgSO4. The nuclei were sedimented through the 2.1 M sucrose at 80,000 × gmax for 1 h and resuspended in storage buffer (39) consisting of 10 mM PIPES (pH 7.4), 80 mM KCl, 20 mM NaCl, 250 mM sucrose, 5 mM EGTA, 1 mM DTT, 0.5 mM spermidine, 0.2 mM spermine, 50% (w/v) glycerol, 1 mM PMSF, 10 µg/ml leupeptin, and 10 µg/ml pepstatin. To assess purity of the nuclei, the activity of the cytosolic marker enzyme lactate dehydrogenase was assayed as described (40).
Organic SynthesesTo synthesize VEID-AMC, the tetrapeptide
portion (Z-VEID) was first synthesized from
Fmoc-L-glutamic acid -t-butyl ester, Fmoc-L-isoleucine, Fmoc-L-aspartic acid
-t-butyl ester, and Z-L-valine on
an acid-labile 2-chlorotrityl chloride polystyrene resin (Advanced ChemTech, Louisville, KY). After assembly of the peptide on an ABI 431A
peptide synthesizer using deprotection and coupling protocols provided
by the instrument's manufacturer (Perkin-Elmer), the t-butyl-protected tetrapeptide was released by treatment of
the peptidyl-resin with acetic acid:trifluoroethanol:dichloromethane (1:2:7) for 30 min at 20 °C. Following dilution with 50 volumes of
cold H2O, the protected peptide was lyophilized for 2 days to remove acetic acid and organic solvents, purified by gel filtration on LH-20 (Pharmacia Biotech Inc.) in 1:1
dichloromethane:n-propanol, and coupled to AMC through its
free C-terminal end by a mixed anhydride method with isobutyl
chloroformate. In brief, after gel filtration, 48 mg of protected
tetrapeptide was dissolved in 2 ml of 1-methyl-2-pyrrolidinone and 50 µl of triethylamine, cooled to
5 °C, and treated with 40 µl of
isobutyl chloroformate for 35 min. A solution containing 13.1 mg of AMC
in 1.5 ml of 1-methyl-2-pyrrolidinone was then added dropwise, and the
coupling was allowed to proceed for 18 h at 20 °C. The
protected peptide-AMC conjugate was precipitated by dilution of the
reaction mixture with cold H2O, extracted with ethyl
acetate, and evaporated to dryness. After treatment with
trifluoroacetic acid:H2O (19:1) for 30 min to remove the
t-butyl protecting groups, the resulting product was
purified to homogeneity by reversed phase HPLC on a Vydac Analytical
C18 column (4.6 × 250 mm; 10 µm; Hesperia, CA) with
a gradient of 0.1% trifluoroacetic acid containing 70% acetonitrile.
Electrospray ionization mass spectrometry verified that the final
product (1.2 mg) had the predicted molecular mass of 764.3.
The synthesis of Z-EK(bio)D-aomk was initiated using the
methodology described by Krantz (41-43).
N-(Z)-aspartic acid -t-butyl ester
was activated as a mixed anhydride (1.4 equivalents of
N-methylmorpholine, 1.3 equivalents of ethyl chloroformate
in tetrahydrofuran at
15 °C) and then treated with 2 equivalents
of CH2N2 in Et2O to yield the
corresponding diazoketone, which was treated with a 1:1 mixture of
excess glacial acetic acid and 45% HBr at 0 °C to generate the
bromomethyl ketone. Treatment of the bromomethyl ketone with 1.2 equivalents of 2,6-dimethylbenzoic acid and 2.5 equivalents of KF in
dimethylformamide yielded Z-Asp-(
-((arylacyl)oxy)methyl ketone). After removal of the Z- protecting group by
catalytic hydrogenation (1 atmosphere, 10% Pd/C, 1 M
solution of compound in ethanol) in the presence of 1.05 equivalents of
HCl, the lysine residue was added using conventional amino acid
coupling conditions (1 equivalent of
Z-Lys(t-Boc)-OH, 1.6 equivalents of
benzotriazol-1-yloxytris(dimethylamino)phosphonium hexafluorophosphate,
6 equivalents of N-methylmorpholine, dimethylformamide). After the Z- protecting group was again removed by catalytic
hydrogenation, the glutamic acid residue was added using identical
conditions to yield
Z-Glu(OtBu)-Lys(t-Boc)-Asp(OtBu)-(
-((arylacyl)oxy)methyl ketone). The t-butanol and t-Boc protecting
groups were removed with trifluoroacetic acid in methylene chloride to
yield Z-Glu-Lys-Asp-(
-((arylacyl)oxy)methyl ketone),
which was then reacted with a 2-fold molar excess of N-hydroxysuccinimidobiotin to derivatize the
-amino group
of lysine. The product Z-EK(bio)D-aomk was separated from
unreacted aomk and excess reagents by reversed phase HPLC. Fractions
containing active Z-EK(bio)D-aomk were identified using
recombinant bacterial ICE, pooled, and concentrated.
Aliquots containing 50 µg of cytosolic or nuclear protein (estimated by the bicinchoninic acid method (44)) in 50 µl of buffer C were diluted with 225 µl of freshly prepared buffer D (25 mM HEPES (pH 7.5), 0.1% (w/v) CHAPS, 10 mM DTT, 100 units/ml aprotinin, 1 mM PMSF) containing 100 µM substrate and incubated for 2 h at 37 °C. Reactions were terminated by the addition of 1.225 ml of ice-cold buffer D. Fluorescence was measured in a Sequoia-Turner fluorometer using an excitation wavelength of 360 nm and emission wavelength of 475 nm. Reagent blanks containing 50 µl of buffer C and 225 µl of buffer D were incubated at 37 °C for 2 h and then diluted with 1.225 ml of ice cold buffer D. Standards containing 0-3000 pmol of AMC or 0-1500 pmol of AFC were utilized to determine the amount of fluorochrome released. Control experiments (not shown) confirmed that the release of substrate was linear with time and with protein concentration under the conditions specified. To determine the effect of various protease inhibitors, aliquots containing 50 µg of protein were incubated with the indicated inhibitor for 5 min at 21 °C and then diluted with substrate in buffer D and assayed as described above.
IRP Expression in Sf9 CellsFull-length cDNAs encoding P45 forms of caspase-1, -2, -3, -4, and -6 were cloned by RT-PCR from Jurkat or THP.1 cell RNA using primers flanking the respective open reading frames. The primers were designed based upon the published sequences (21, 22, 26, 45-51), and all clones were sequenced before expression. High titer recombinant baculovirus expressing caspase-1 was generated by cloning the cDNA into pVL1392 using standard methods (52). Recombinant baculoviruses expressing the other caspases were produced by transposon-mediated recombination (53) in bacteria using the Bac-to-BacTM system according to the supplier's instructions.
Expression cultures of the caspases were produced using high titer
viral stocks (>107 plaque-forming units/ml) infected at
MOIs ranging from 2.5 to 10. At 48 h (high MOI infections) or
72 h (low MOI infections) after infection, a time when caspases
are activated during virus-induced apoptosis, cells were washed twice
with phosphate-buffered saline and lysed in 0.2-0.5 ml of buffer
containing 20 mM HEPES (pH 7.0), 2 mM EDTA, 2 mM DTT, 0.1% Triton X-100, 5 µg/ml leupeptin, 2 µg/ml pepstatin, 2 µg/ml E64, and 0.1 mM PMSF. After a 10-min
incubation at 4 °C, nuclei were removed by centrifugation at
12,000 × g. The supernatants were stored at 80 °C
until treated with Z-EK(bio)D-aomk as described below.
Aliquots containing the indicated amounts
of nuclear or cytosolic protein were incubated for 1 h at room
temperature with 1 µM Z-EK(bio)D-aomk (added
from a 25 µM stock in Me2SO). At the completion of the incubation, extracts were diluted with 1/2 volume of 3 × concentrated SDS sample buffer, heated to 95 °C
for 3 min, subjected to SDS-PAGE on 16% (w/v) acrylamide gels,
transferred to nitrocellulose, probed with peroxidase-labeled
streptavidin, and visualized by enhanced chemiluminescence. Control
experiments using purified ICE indicated that this approach could
detect as little as 1 ng of caspase-1. Alternatively, samples treated
with Z-EK(bio)D-aomk were precipitated using
methanol/chloroform and resuspended in 100 µl of urea solubilization
buffer (9 M urea, 4% (v/v) Nonidet P-40, 2% (v/v)
-mercaptoethanol, 20% (v/v) BioLyte 3-10 carrier ampholytes).
Two-dimensional gel electrophoresis was performed using an ISO-DALT
system (Hoeffer, San Francisco, CA) as described previously (54).
Samples were focused on an isoelectric focusing gel for 10,200 V-h,
transferred to the top of a 16% (w/v) SDS-polyacrylamide gel,
subjected to SDS-PAGE at 12 mA for 16 h, transferred to
nitrocellulose, and probed with streptavidin as described above.
A series of mixing experiments was performed to compare affinity-labeled proteases in HL-60 cytosol with recombinant human caspases expressed in Sf9 cells. Z-EK(bio)D-aomk-labeled Sf9 extracts containing caspase-3 were electrophoresed either individually or after mixing with labeled Sf9 extracts containing caspase-2 or caspase-6. A composite image was then created by merging and aligning scans from the various blots using Adobe Photoshop. The location of the known enzyme large subunits in the composite image was then overlaid upon the distribution of active caspase subunits in two-dimensional gel analysis of HL-60 cell cytosol. Caspase-3 species present in all blots were used as reference points for the alignment.
Inhibitor Competition ExperimentsAliquots containing 37 µg of cytosolic protein from etoposide-treated HL-60 cells were incubated for 1 min on ice with the tetrapeptide inhibitor YVAD-cmk dissolved in phosphate-buffered saline containing 10% Me2SO. Z-EK(bio)D-aomk was then added to a final concentration of 1 µM. After a 5-min incubation at 37 °C, the samples were diluted with 1/2 volume of 3 × concentrated SDS sample buffer, heated to 95 °C for 3 min, subjected to SDS-PAGE, and reacted with peroxidase-coupled streptavidin as described above.
Preparation of Whole Cell Lysates for ImmunoblottingAfter
incubation with etoposide for the indicated lengths of time, HL-60
cells were sedimented at 200 × g for 10 min at
4 °C, washed once with ice-cold RPMI containing 10 mM
HEPES (pH 7.4 at 4 °C), and solubilized at a concentration of 3 × 107 cells/ml in SDS sample buffer consisting of 4 M deionized urea, 2% (w/v) SDS, 62.5 mM
Tris-HCl (pH 6.8 at 21 °C), 1 mM EDTA, and 5% (w/v)
freshly added -mercaptoethanol. Samples were immediately sonicated
and frozen at
70 °C. Aliquots were subsequently heated to 65 °C
for 20 min, subjected to SDS-PAGE on gels with 5-15% (w/v) acrylamide
gradients, transferred to nitrocellulose, and probed with antibodies as
described previously (55). Antibodies utilized for these experiments
included murine monoclonal antibodies that recognize PARP (56), chicken
polyclonal antisera raised against rat lamin B1 (57) and
rat nucleolar protein B23 (58), and the commercially available
antibodies described above.
Primers were generally designed to amplify cDNA
sequences encompassing the pro domain into the amino-terminal half of
the respective P20 subunits, regions of the caspase cDNAs that
display relatively low sequence homology. In brief, 1 µg of
poly(A)+ RNA from HL-60 cells was reverse transcribed with
a combination of random hexamer and oligo(dT) primers using Superscript
RT under standard conditions (59). One-twentieth of the cDNA
product was used for each amplification. PCR reactions were performed in 50-µl volumes containing 50 mM KCl, 10 mM
Tris-HCl (pH 8.3), 1.5 mM MgCl2, 0.001% (w/v)
gelatin, 1 µM each primer, 200 µM dNTPs, and 2.5 units of AmpliTaq. Reactions were initiated under hot start
conditions and continued for a total of 30 cycles under step cycle
conditions on a Perkin-Elmer PE-480 DNA thermal cycler using 92 °C
for denaturation, 60 °C for annealing, and 72 °C for extension
(30 s/step). The caspase-5 product was amplified for 35 cycles using a
55 °C annealing step. For each procaspase (accession number
indicated in parentheses), the forward and reverse primers were as
follows: procaspase-1 (X65019),
GGGTACAGCGTAGATGTGAAAAAAAATCTCACTGCTTCG and GCCCATTGTGGGATGTCTCCAAGAA;
procaspase-2 (U13022), GTGCACTTCACTGGAGAGAAA and GGGCAGTCTCATCTTCGGCAA;
procaspase-3 (U13737), AAGGTATCCATGGAGAACACTGAAAAC and
AACCACCAACCAACCATTTCT; procaspase-4 (U28014), CAGAGCACAAGTCCTCTGACA and
AGGGCTGGGCTGCTTGTG; procaspase-5 (U28015), GTATCCTTCAGAGTGGATTGG and
AATTCTTCACGAGGACAAAGTTTGA; procaspase-6 (U20536), CCGGCAGGTGGGGAAGAAAA and TGCAACAGAGTAACACATGAGGAAGTC; procaspase-7 (U37449),
CCGCCGTGGGAACGATGGCAGATG and TGACCCATTGCTTCTCAGCTAGAATGTAC;
procaspase-8 (U60519), ACAAGGAAGCCGAGTCGTATCAAGGAGAGG and
TCGTTGACAGCAGTGAGGATGGATAAGATG; procaspase-10 (U60520),
TAAACACTAGAAAGGAGGAGATGGAAAGGGAACT and CATGGGAGAGGATACAGCAGATGAAGCA.
Control PCR reactions included 1) HL-60 cDNA template and
human -actin primers (forward, GTGGGGCGCCCCAGGCACCA; reverse,
CTCCTTAATGTCACGCACGATTTC) to validate the cDNA and 2) 0.05 µg of
HL-60 poly(A)+ RNA template to confirm that the products
observed were derived from cDNA rather than contaminating genomic
DNA. Following amplification, one-tenth of the PCR reactions were
electrophoresed for 160 V-h on a 3.5% composite agarose gel (2.5%
NuSieve, 1% Seakem-GTG; FMC Bioproducts, Rockland, ME) containing 0.5 µg/ml ethidium bromide in 1 × TAE buffer. Products were
visualized on a UV transilluminator (256 nm), excised, and
sequenced.
The present studies focused
on HL-60 cells, a human leukemia cell line that readily undergoes
apoptosis in response to a variety of chemotherapeutic agents (30, 31,
60-63). Recent studies suggesting that caspase activation plays a
critical role in initiating the active phase of apoptosis (5, 13, 14,
17, 27, 28, 32) prompted us to compare the expression and
activation of caspase precursors in this cell line. RT-PCR revealed
that transcripts for the nine caspases examined are expressed
constitutively in these cells (Fig. 1). Northern blot
analysis (not shown) indicated that full-length messages for these
transcripts are present. Sequencing of the PCR products confirmed that
the observed gel bands corresponded to the indicated caspase
precursors. In addition, this sequence analysis revealed that the
multiple PCR products observed using procaspase-8 and procaspase-10
primers are derived from alternate splicing of the target mRNAs as
described by Boldin et al. (64). These results indicated
that HL-60 cells constitutively express at least nine procaspases.
Detection of Multiple Caspase Activities in Cytosol from Etoposide-treated HL-60 Cells
In order to follow caspase
activation during apoptosis, cytosol from cells treated with 68 µM etoposide for increasing lengths of time was incubated
with the fluorogenic substrate DEVD-AFC, VEID-AMC, or YVAD-AFC. The
first two of these substrates correspond to the apoptotic cleavage
sites of PARP (29) and lamin A (20), respectively, whereas the third
substrate is derived from the cleavage site preferred by caspase-1
(21). Results of these assays are shown in Fig. 2.
Etoposide treatment of HL-60 cells was accompanied by a marked increase in activity that cleaved DEVD-AFC (Fig. 2A). The specific activity in cytosolic extracts from control HL-60 cells was 2 pmol of product released/min/mg of protein. There was a 20-fold increase in activity within 2 h of the addition of etoposide and a 100-fold increase within 3 h (Fig. 2A). Control experiments (Fig. 2B) revealed that the DEVD-AFC cleavage activity in cytosolic extracts from etoposide-treated HL-60 cells was extremely sensitive to DEVD-fmk (IC50 ~10 nM) compared with YVAD-cmk (IC50 ~10 µM) and completely insensitive to E64 at concentrations of 100 µM.
VEID-AMC cleavage activity also increased during the course of etoposide-induced apoptosis, albeit somewhat more modestly (Fig. 2C). The specific activity in extracts from control HL-60 cells was 15 pmol of product released/min/mg of protein. There was a 4-fold increase in activity 2 h after the addition of etoposide and a 20-fold increase over the 6-h time course. Examination of the effect of inhibitors (Fig. 2D) revealed that the VEID-AMC cleavage activity was at least 10-fold more sensitive to DEVD-fmk (IC50 < 1 nM) and 3-fold more sensitive to YVAD-cmk (IC50 ~3 µM) than the DEVD-AFC cleavage activity in the same extract, suggesting that the DEVD-AFC and VEID-AMC cleavages are mediated, at least in part, by different caspases (20). The VEID-AMC-cleaving enzyme was also somewhat more sensitive to 1-chloro-3-tosylamido-7-amino-2-heptanone (Fig. 2, compare TLCK in panels B and D).
The YVAD-AFC cleavage activity in cytosol from control HL-60 cells was <10 pmol of product released/min/mg of protein. In contrast to the marked increase in DEVD-AFC and VEID-AMC cleavage activities, there was little change in YVAD-AFC cleavage activity after the addition of etoposide (Fig. 2E). Additional experiments with cytosol from THP.1 cells, which are known to contain caspase-1 activity (38), not only confirmed that the assay could detect YVAD-AFC cleavage activity in cytosolic extracts, but also indicated that the inhibitor profile of the apoptotic proteases (Figs. 2, B and D) differed substantially from that of caspase-1 (Fig. 2F).
The Protease Activities Represent Activation of Preexisting PolypeptidesTo determine whether the appearance of active
apoptotic proteases depends on de novo synthesis of the
proenzymes, HL-60 cells were treated with 68 µM etoposide
in the absence or presence of cycloheximide or puromycin at
concentrations that inhibited [35S]methionine
incorporation into protein by >90%. Results of this experiment (Fig.
3) revealed that neither cycloheximide nor puromycin inhibited the etoposide-induced increase in DEVD-AFC cleavage activity.
Instead, treatment with cycloheximide alone or puromycin alone was
associated with increased DEVD-AFC cleavage activity, a result that is
consistent with previous observations that cycloheximide and puromycin
induce apoptosis in HL-60 cells (30, 31, 61). These results suggest
that de novo protein synthesis is not required for the
appearance of caspase activity when HL-60 cells undergo apoptosis.
Sequential Labeling of Multiple Caspases in HL-60 Cells
To
more completely delineate the spectrum of caspases activated in HL-60
cells, aliquots of cytosol were labeled with
Z-EK(bio)D-aomk, an affinity labeling reagent (43, 65)
designed to mimic the EVD motif preferred by the apoptotic proteases
detected in Fig. 2. Control experiments revealed that
Z-EK(bio)D-aomk covalently modified the larger subunits of
all active caspases tested, including caspase-1, -2, -3, -4, and -6 (e.g. Fig. 7A). Titration experiments revealed
that as little as 1 ng of purified caspase-1 could be detected with
this reagent.
When this reagent was utilized to label cytosol from control and
etoposide-treated HL-60 cells, evidence for activation of multiple
caspases was obtained. No active enzymes were detectable when cytosol
from untreated HL-60 cells was incubated with
Z-EK(bio)D-aomk (Fig. 4A,
lane 1). In contrast, 6 h after the addition of
etoposide to HL-60 cells, four discrete bands were detected by this
affinity label (Fig. 4A, lane 6). These bands
were termed IRP1 (relative mobility of 21.5 kDa),
IRP2 (relative mobility of 19.1 kDa), IRP3 (relative mobility of 18.4 kDa), and IRP4 (relative
mobility of 16.6 kDa). When cytosol from apoptotic HL-60 cells was
pretreated with YVAD-cmk (a nonspecific caspase inhibitor at the
concentration used), Z-EK(bio)D-aomk labeling of the
proteases was abolished (Fig. 4B), providing further support
for the view that these four bands are active caspases.
Interestingly, each band appeared at a characteristic time after
etoposide addition (Fig. 4A, lanes 3-6). The
bands denoted IRP2 and IRP3 were faintly
visible 2 h after the addition of etoposide, increased
dramatically by 3 h, and remained relatively constant thereafter.
In contrast, IRP1 and IRP4 were first evident
at 3 h and increased progressively during the remainder of the
incubation. Similar results were obtained when cytosol was labeled with
N-(acetyltyrosinylvalinyl-N-biotinyllysyl)aspartic
acid [(2,6-dimethylbenzoyl)oxy]methyl ketone (YV(bio)KD-aomk) (65)
(data not shown), although Z-EK(bio)D-aomk could be used to
label the IRPs at 10-fold lower concentrations.
Because
several nuclear polypeptides are cleaved during the course of apoptosis
(5, 13, 15, 30), we next examined the possibility that active caspases
might be detected in nuclei as well as cytosol. For these experiments,
HL-60 cells were treated with etoposide and then fractionated into
cytosol and nuclei. The nuclei were purified by sedimentation through
sucrose cushions as described previously (40). Electron microscopy of
these nuclei failed to reveal any identifiable cytoplasmic organelles
(data not shown). Furthermore, assays indicated that the activity of the marker enzyme lactate dehydrogenase was 4.6 ± 1.4 pmol of substrate consumed/min/mg of protein in nuclei compared with 85 ± 14 pmol/min/mg of protein in cytosol after 3 h of etoposide treatment, suggesting that contamination by cytosolic polypeptides was
minimal. Nonetheless, nuclei prepared from etoposide-treated cells
contained DEVD-AFC cleavage activity. Results of time course experiments (Fig. 5A) revealed that this
activity was low or undetectable in nuclei from control cells (0 h) and
increased to ~100 pmol of product released/min/mg of protein after
2 h. In additional experiments, VEID-AMC cleavage activity was
also detected in nuclei from apoptotic cells but not control
cells.
Labeling with Z-EK(bio)D-aomk (Fig. 5B) confirmed the presence of active caspases in nuclei prepared from apoptotic HL-60 cells. Nuclei that were not treated with Z-EK(bio)D-aomk contained a number of polypeptides that reacted with streptavidin (Fig. 5B, lane 7), including a polypeptide of Mr~ 17,000 that migrated just below the expected position of IRP3. These streptavidin-binding polypeptides did not change during the course of etoposide treatment (Fig. 5B, lanes 4-6, and data not shown). Etoposide treatment was, however, accompanied by the appearance of new bands that labeled with Z-EK(bio)D-aomk. These bands, which appeared beginning 3 h after the addition of etoposide to the cells, comigrated with IRP1 and IRP2 (Fig. 5B, lanes 4-6). Interestingly, IRP3 and IRP4 were detectable in cytosol from these cells but not in nuclei (cf. lanes 2 and 5).
Identification of Caspases That Are Activated during Etoposide-induced ApoptosisTaken together, the results in Figs.
2, 3, 4, 5 suggest that etoposide treatment is associated with activation of
multiple caspases from preexisting proenzymes. In order to begin to
identify the proenzymes that are activated, whole cell lysates from
etoposide-treated HL-60 cells were examined by immunoblotting using
antibodies that recognize cloned human caspases. To provide a frame of
reference, the same blots were also probed with antibodies that
recognize the caspase substrates PARP and lamin B1 as well
as the nucleolar protein B23, a polypeptide that is not cleaved during
apoptosis in HL-60 cells (31). Results of these experiments are shown in Fig. 6.
Cleavage of PARP to its signature 89-kDa fragment (29-31) was evident within 3 h of the addition of etoposide to these cells (Fig. 6A, lane 7). A marked decrease in lamin B1 content, indicative of lamin B1 degradation (39, 66, 67), was also evident 3 h after etoposide addition (Fig. 6B, lane 7). At this time point, a decrease in procaspase-3 was evident (Fig. 6C, lane 7), suggesting that caspase-3 might be activated in these cells. In contrast, there was no significant change in procaspase-2 content in etoposide-treated HL-60 cells (Fig. 6D).
Despite the marked decrease in procaspase-3 signal (Fig. 6C), the appearance of a signal corresponding to active caspase-3 was not observed even after overexposure of the blots. To confirm that the disappearance of procaspase-3 from the immunoblots was associated with appearance of active caspase-3 and to attempt to identify the other IRPs activated in apoptotic HL-60 cells, the mobility of the large subunits of active caspases detected in HL-60 cytosol following Z-EK(bio)D-aomk labeling was compared with the mobility of the corresponding subunits of cloned human enzymes expressed in Sf9 cells (Fig. 7). Unidimensional SDS-PAGE (Fig. 7A) revealed that IRP1 and IRP3 comigrated with two bands observed in Sf9 cells expressing caspase-6 (Fig. 7A, lane 4); IRP2 and IRP4 comigrated with two bands observed in Sf9 cells expressing caspase-3 (Fig. 7A, lane 5); and IRP4 also comigrated with the band observed in Sf9 cells expressing caspase-2 (Fig. 7A, lane 3). In contrast, the large subunits of caspase-1 and -4 did not comigrate with any of the IRPs. These results suggested the tentative interpretation of the HL-60 labeling pattern shown in Fig. 7A.
To further examine the spectrum of IRPs activated after etoposide treatment, labeled HL-60 cytosol was subjected to two-dimensional isoelectric focusing/SDS-PAGE. This analysis revealed as many as eight distinct spots in the Mr ~16,000-18,000 range (Fig. 7, B and C). For convenience, these spots have been termed A1 (pI 6.5), A2 (pI 6.3), A3 (pI 6.2), B (pI 6.6), C1 (pI 6.4), C2 (pI 6.2), C3 (pI 6.0), and C4 (pI 5.9), respectively. In mixing experiments, the mobilities of the large subunits of caspase-2, -3, and -6 expressed in Sf9 cells were also determined (Fig. 7C, bottom). When apoptotic HL-60 cytosol and the recombinant caspases were compared, a number of the labeled spots comigrated (Fig. 7C, middle). This analysis leads to several conclusions. First, spots A1, C1, and C3 comigrate with three different active species of recombinant caspase-3 expressed in Sf9 cells. Second, spot B comigrates with an active species of caspase-6. Finally, none of the spots detected in HL-60 cytosol comigrated with the major form of caspase-6 detected in insect cells or with recombinant caspase-2.
Previous studies have suggested that caspase activation plays a crucial role in the initiation or propagation of apoptotic events. Recent reports also indicate that genes encoding as many as nine caspases are simultaneously expressed in certain human leukemia cell lines. However, it has been unclear whether all of these proteases participate in apoptotic events. Two factors contribute to this uncertainty. First, activation of caspases, which involves proteolytic cleavage of zymogen precursors at Asp-X bonds to yield the large and small subunits of the active heterotetrameric proteases, is poorly understood (reviewed in Refs. 15 and 28). Second, high titer antibodies that are specific for the subunits of mature proteases are not available for all of the caspases. As a result, it has remained unclear whether all of the proenzymes are activated simultaneously, whether the appearance of active enzymes involves de novo synthesis of caspases or activation of preexisting proenzymes, and whether active caspases are localized exclusively to the cytoplasm or are found in other cellular compartments. The present study sheds light on all of these issues.
Analysis of affinity labeling experiments by unidimensional SDS-PAGE revealed that HL-60 cells undergoing etoposide-induced apoptosis contain four distinct bands that covalently label with Z-EK(bio)D-aomk (Fig. 4). Although these polypeptides appear sequentially rather than simultaneously, the apparent stability of the larger bands (IRP1-3) at later time points suggests that the lower bands are not derived from the upper band(s) by proteolytic cleavage. Instead, these polypeptides appear to correspond to the larger subunits of the active forms of multiple discrete caspases. A similar repertoire of five endogenous caspases with distinct cleavage preferences was recently demonstrated by us in apoptosis-inducing S/M extracts prepared from chicken hepatoma cells (20). Thus, apoptosis in higher eukaryotic cells differs in detail from developmental cell death in C. elegans, where a single caspase appears to be required (24, 25).
The results obtained with Z-EK(bio)D-aomk provide the first direct evidence that a number of caspases are activated during apoptosis in HL-60 cells. This caspase activation is accompanied by the appearance of at least two distinct enzyme activities. These activities cleave DEVD-AFC (Fig. 2A) and VEID-AMC (Fig. 2C) but display different inhibitor sensitivities (Fig. 2, B and D). In contrast, activation of a caspase-1-like activity was not observed during etoposide-induced apoptosis in HL-60 cells (Fig. 2E), a result that differs from the recent observation that caspase-1-like protease activity is elevated early in the course of Fas-mediated apoptosis in T cells (68). Whether these disparate findings reflect differences between various cell types or variations in the pathways activated by different apoptotic stimuli requires further investigation.
The observation that several recombinant caspase polypeptides expressed in Sf9 cells comigrate with the IRPs present in HL-60 extracts following labeling with Z-EK(bio)D-aomk enables us to propose a tentative identification of the proteases acting in the course of etoposide-induced HL-60 apoptosis. IRP2 and IRP4 appear to correspond to caspase-3 (Fig. 7B). The appearance of these active species occurs with a time course (Fig. 4) that parallels the appearance of DEVD-AFC cleavage activity (Fig. 2A) and disappearance of procaspase-3 from immunoblots (Fig. 6C). Our demonstration that caspase-3 is enzymatically active in HL-60 apoptosis (i.e. covalently labels with Z-EK(bio)D-aomk) confirms and extends recent claims of caspase-3 activation based solely on appearance of immunoreactive P17 subunit (27, 69).
The two-dimensional analysis presented in Fig. 7 provides the first evidence for the presence of multiple active forms of caspase-3 during apoptosis. Spots A1, C1, and C2 all comigrate with species observed in Sf9 cells expressing human caspase-3. The various forms of the enzyme could arise from alternative splicing of the transcripts (70), alternative processing of the proenzymes, and/or posttranslational modification of the processed subunits. Whether these species correspond to functionally distinct subpopulations of caspase-3 that differ in their substrate recognition properties, time of activation during apoptosis, or intracellular location requires further study. Nonetheless, the observation that cells contain multiple active species of this caspase suggests that the spectrum of active caspases in apoptosis could be even more complicated than previously thought.
Measurements of enzyme activity also indicate that a discrete VEID-AMC cleavage activity appears in etoposide-treated HL-60 cells beginning ~2 h after the addition of etoposide (Fig. 2, C and D). Analysis by one- and two-dimensional isoelectric focusing/SDS-PAGE supports this observation by indicating that IRP3/spot B has the same mobility as one species of active caspase-6 (Fig. 7). Caspase-6 was recently shown to be unique among caspases characterized to date in being able to cleave the VEID-X sequence (20). Although analysis by unidimensional SDS-PAGE strongly suggested that IRP1 might correspond to a second active species of caspase-6 (Fig. 7A), this assignment could not be confirmed by two-dimensional isoelectric focusing/SDS-PAGE because IRP1 did not focus in the two-dimensional gels (Fig. 7, B and C).
Two-dimensional analysis of HL-60 cytosol also revealed the presence of multiple additional Z-EK(bio)D-aomk-reactive species (Fig. 7C) that did not comigrate with any of the recombinant caspases tested to date. Among these, spots C3 and C4 have mobilities on SDS-PAGE similar to species tentatively identified as caspase-3 but have different isoelectric points, suggesting that they might be posttranslationally modified versions of the caspase-3 large subunit. Alternatively, these minor species could correspond to other human caspases, either known or yet to be characterized.
In addition to the caspases detected in cytosol, Z-EK(bio)D-aomk also selectively labeled two polypeptides in nuclei of etoposide-treated HL-60 cells (Fig. 5B). Despite the fact that several of the known caspase substrates are nuclear proteins (reviewed in Refs. 15 and 28), this is the first demonstration of multiple active caspases in nuclei. It is unlikely that the nuclear enzymes represent contaminating cytosolic proteins, since the isolated nuclei were shown to lack significant cytoplasmic contamination as detected either by electron microscopy or assays for the cytosolic marker enzyme lactate dehydrogenase. The comigration of the active caspase subunits in cytosol and nuclei (Fig. 5B) suggests the possibility that some (but not all) of the species activated in the cytosol might be transported into nuclei. Alternatively, we cannot rule out the possibility that certain caspase precursors present in nuclei are activated during the course of apoptosis. Further experiments are required to distinguish between these possibilities.
The present observations also shed light on the origin of the active caspases. We were unable to detect either DEVD-X cleavage activity (Fig. 2A) or Z-EK(bio)D-aomk-labeled polypeptides corresponding to the large subunit of active caspases in cytosol from control HL-60 cells (Fig. 4A). These observations argue against the possibility that caspase-3 (or any related protease) is preactivated in the cytosol of HL-60 cells and effectively rule out a model in which the activity of preactivated proteases is controlled in these cells by regulation of the levels of endogenous inhibitors.
An alternative possibility is that caspases are synthesized de novo in response to apoptotic stimuli (71). We did not observe a reproducible etoposide-induced increase in content of any of the four caspases for which antibodies are currently available (Fig. 6 and data not shown). Moreover, the observation that high concentrations of the protein synthesis inhibitors cycloheximide and puromycin failed to prevent the appearance of DEVD-AFC cleavage activities in etoposide-treated HL-60 cells (Fig. 3) argues against the possibility that this activity results from de novo synthesis of the proenzyme. Instead, it appears that multiple caspase proenzymes are present in HL-60 cells (and several other human cell lines) prior to the application of apoptotic stimuli (Fig. 6; see also Refs. 17, 22, 26, 27, and 45).
In support of this conclusion, RT-PCR (Fig. 1) indicated that untreated HL-60 cells contain transcripts for at least nine caspases. Although procaspase polypeptide levels might not always reflect the levels of the corresponding transcripts, it is reasonable to assume that as many as nine procaspase polypeptides are expressed in HL-60 cells. This does not mean, however, that all nine procaspases are activated during the course of apoptosis. We failed to detect an increase in caspase-1 enzymatic activity (YVAD-AFC cleavage) after etoposide treatment (Fig. 2E). Likewise, immunoblotting indicated that the bulk of procaspase-2 present in HL-60 cells remained intact during apoptosis (Fig. 6D), and two-dimensional analysis failed to detect a Z-EK(bio)D-aomk-labeled spot corresponding to active caspase-2 (Fig. 7C). This is in contrast to the extensive cleavage (Fig. 6C) and activation (Fig. 7C) of procaspase-3. The mechanism for selective apoptotic activation of some caspase precursors (e.g. procaspase-3) and not others (e.g. procaspase-2) is currently unclear and requires further investigation.
We thank Dr. Ivan Lieberburg for making this collaboration possible; Michael Power for DNA sequence confirmation of clones and constructs used in this work; Alastair Mackay and Joe Lewis for help with the two-dimensional gel analysis; and Deb Strauss for secretarial assistance.