 |
Introduction
|
|---|
Apoptosis is an evolutionary conserved process in which the caspase family of cysteine proteases plays an essential role. To date, 14 caspases have been identified in mammals, with some functioning in cytokine processing and inflammation and at least 8 others contributing to programmed cell death. The apoptotic caspases can be further divided into the initiator caspase group, which includes caspase-2, -8, -9, and -10, and the effector caspase group, to which caspase-3, -6, and -7 belong (for reviews see references 1, 2). Depletion experiments in cell-free extracts indicate that caspase-3 is the principal effector caspase (3). On the other hand, knockout studies suggest a partial redundancy in the role of caspase-3 and other caspases such as caspase-7 (4). In addition to cleaving themselves, active caspases proteolyse a set of protein substrates with the loosely conserved recognition sequence X-E-X-D. Cleavage occurs exclusively after the aspartic acid residue (1, 2). Many caspase substrates play key roles in cell function and architecture, and alteration of their normal function by caspase-mediated cleavage is thought to contribute to the characteristic morphological features of apoptotic cells (5).
A large number of pathologies exhibit either too much or too little apoptosis, and it is of considerable interest to develop agents that will modulate programmed cell death in patients (6). A potential target for antiapoptotic agents is the microbial-elicited systemic inflammatory response known as sepsis. This disease is fatal in 30–40% of cases and is the highest cause of mortality in intensive care units (7). Recent studies uncovered a depletion of B and T cells in the lymphoid organs and the presence of apoptotic markers in lymphocytes and intestinal epithelial cells of septic patients (8, 9). Loss of B and T cells was observed in the spleen and thymus of rodents in which sepsis was induced by cecal ligation and perforation (CLP; references 10, 11). Overexpression of breakpoint cluster (Bcl)-2 in B, T, or intestinal epithelial cells reduced CLP- or pneumonia-induced murine sepsis and increased survival (12–15), as did the administration of caspase inhibitors (16). Based on these studies, blockade of apoptosis using caspase inhibitors constitutes a potential treatment. Development of such inhibitors will require an accurate quantitation of caspase-dependent events during sepsis and the percentage of active caspases that must be inhibited for efficacy in vivo. To this end, we examined various manifestations of apoptosis during CLP-induced sepsis in both rats and mice. We found that monitoring of DNA fragmentation and 
II-spectrin cleavage, as opposed to phosphatidylserine (PS) exposure, provides a more accurate measurement of apoptosis-related events during sepsis. Surprisingly, studies with both caspase-3–specific and polycaspase inhibitors reveal different potencies at curbing these apoptotic manifestations, both in vivo and in cell culture, illustrating the need to follow several cell death markers. From these findings, we conclude that a high degree of fractional caspase inhibition is necessary to completely block apoptotic cell death. This establishes, in an animal model of inappropriate apoptosis (CLP-induced sepsis), the required levels of caspase inhibitors needed for improved survival and the potential challenges that face the use of caspase inhibitors in human diseases.
|
Materials and Methods
|
|---|
Animals.
Female Sprague-Dawley rats (250–300 g; Charles River) and C57Bl/6-TgN(BCL-2)25 Wehi mice, heterozygous and WT siblings (20–25 g; stock no. 2320; Jackson Laboratories) were housed in a 12-h light–dark cycle with free access to food and water. All procedures were performed under appropriate Animal Care Committee approval in strict accordance to Merck and Co. animal care policies.
Surgical Procedures.
Animals were anesthetized with 2.5% isoflurane in oxygen, and body temperature was maintained by use of a thermoregulated heated blanket.
CLP was performed as follows. A midline incision was made in the abdominal wall of the animal and the cecum exteriorized. The cecum was ligated with a nylon (4–0) suture proximal to the ileocecal valve. In mice, perforation of the cecum was done using a 23-gauge needle passed through the distal portion of the cecum. Femoral vein cannulation of rats was performed by a small incision in the inguinal region, and the femoral vein was isolated. A Silicone catheter (0.02 inches x 0.037 inches; Lomir) connected to a polyurethane catheter (PU-C30, 3 French, 80 cm; Instech Solomon) was inserted into the vena cava, exteriorized at the nape of the neck, and clamped for the duration of the surgery. Cannulation was immediately followed by CLP using a 20-gauge cannula (Abbott Ireland) passed through and through the distal portion of the exteriorized cecum. Braided silk (size 0) was threaded through the cannula and secured in place to allow leakage of the cecal content into the peritoneum. Sham-operated animals had the cecum exteriorized but no ligation or puncture of the cecum. The abdominal wall was sutured with polydioxane suture (4–0) and the skin sutured with surgical glue (mice) or clips (rats). Immediately after surgery, all animals received 1 c.c. of 0.9% saline administered by subcutaneous injection. A 2 ml/kg bolus of vehicle or compound (M867) was administered via the i.v. catheter, which was then connected to a Medfusion 2010i Syringe pump (Medex Inc.) at a delivery rate of 2 ml/h/kg for 24 h.
Thymic Protein Extract Preparation.
Thymi from rats or mice were recovered 24 h postsurgery and processed within 20 min of their removal. A cell suspension was obtained by grinding tissues in 50 µm Medicon and Medimachine (Dako) with 2 ml of ice cold thymocyte isolation buffer (PBS, 2 mM glucose, 2 mM L-glutamine, 1% FBS) with 2 x 15-s pulses. Cell suspensions were filtered through 50 µm nylon mesh filters (Becton Dickinson). Red blood cells were eliminated by a 10-min incubation in hypotonic buffer (17 mM Tris-Cl, pH 7.5, 140 mM NH4Cl). For some experiments, thymocytes were put in culture for 24 h at a density of 10 x 106 cells/ml in CytoSF4 (Kemp Technologies) supplemented with L-glutamine and antibiotics. Thymi fragments were lysed in cell lysis buffer (50 mM Tris-Cl, pH 7.5, 2 mM EDTA, 1% NP-40) supplemented with complete protease inhibitor (Roche), caspase inhibitor (M029), and calpain inhibitor (M638). Protein in the soluble fraction was quantitated with the BCA protein detection kit (Pierce Chemical Co.).
Enzyme-linked Immunosorbant Assays.
DNA-histone sandwich ELISA was performed using the Cell Death Detection ELISA kit (Roche) according to the manufacturer's specifications. All assays were performed on protein extracts that had not been frozen since freeze-thawing alters results. II-spectrin ELISA was performed on rat thymus extracts only, since the neoepitope anti-p120 II-spectrin antibody is unreactive toward mouse-cleaved II-spectrin. The anti–II-spectrin neoepitope antibody was raised against the NH2-terminal portion of the human caspase-3–specific p120 fragment (immunizing peptide: NH2-SVEALIKC-COOH). The assay plates were washed with Superblock/0.05% Tween-20 buffer (Pierce Chemical Co.) between each of the following steps. Goat anti–rabbit–coated 96-well plates (Pierce Chemical Co.) were incubated with 80 ng/well of anti–II-spectrin neoepitope antibody overnight. The plates were washed, and thymus protein lysate (200 µg in a final volume of 100 µl) was added to each well for 1 h. The plates were washed and consecutively incubated for 1 h with a 1:1,000 dilution of anti–II-spectrin antibody (mab1622; Cedarlane), a 1:6,000 dilution of anti–mouse biotin (Amersham Biosciences), and a 1:6,000 dilution of streptavidin-horseradish peroxidase (Amersham Biosciences). Color was developed with K-blue max substrate (Cedarlane) and absorbance read at 650 nm on a Spectromax photospectrometer (Molecular Devices). Units are expressed as OD values or as standard units from pooled thymus extracts with previously quantitated p120 II-spectrin.
Western Blotting.
Western blotting was performed on 40 µg of heat-denatured thymic protein extract migrated through a 10–20% acrylamide gradient SDS-PAGE Tris-Glycine gel (Invitrogen). The following antibodies and dilutions were used: rabbit anti–caspase-3 antibody R280 (1:2,000 Merck-Frosst); goat antimurine poly(ADP-ribose) polymerase (PARP) (fragment 71–329; 1:2,000; R&D Systems); murine antispectrin (mab1622; 1:1,000; Cedarlane); and anti–rabbit IgG-HRP (1:5,000; Amersham Biosciences). Chemiluminescence was performed with Supersignal West Femto chemiluminescent reagent (Pierce Chemical Co.) and exposed to Hyperfilm ECL (Amersham Biosciences).
Flow Cytometry.
Phosphatidylserine exposure and propidium iodide (PI) permeability were measured with fluorescein-labeled annexin V (TACS; R&D Systems) according to the manufacturer's specification and two-color flow cytometric analysis. The presence of II-spectrin neoepitope was also determined by flow cytometry. Rat thymocytes were fixed in PBS/0.1% sodium azide/0.25% paraformaldehyde on ice for 1 h and permeabilized in PBS/0.1% sodium azide/0.05% Triton X-100 for 15 min at room temperature. After a wash step, the cells were incubated in primary antibody solution (PBS/0.1% sodium azide, 1% normal goat serum [NGS], 1 ng/ml anti–II-spectrin neoepitope antibody) for 1 h. Primary antibody binding was detected using a 1:500 dilution of goat anti–rabbit IgG-Alexa 488 (Molecular Probes) in PBS/0.1% sodium azide/1% NGS. Antibody-binding specificity was assessed by competition with the immunizing peptide. Subdiploid DNA content was determined on thymocytes fixed for 30 min on ice in 70% EtOH. Cells were washed with PBS and suspended in 500 µl of PI staining solution (PBS/0.1% Triton X-100/RNase A [Roche]/25 µg/ml PI [Sigma-Aldrich]). Flow cytometric analysis was performed on FACSCalibur (Becton Dickinson) on 20,000 events/sample, each sample prepared in duplicates. Very small cell debris was electronically gated out based on forward light scatter.
|
Results
|
|---|
Apoptotic Markers and Their Bcl-2 Dependency during Sepsis.
We first determined the contribution of necrosis and the relevance of various apoptotic markers during sepsis by examining several indicators of cell viability in transgenic mice that overexpress Bcl-2 in T cells. Bcl-2 is a potent antiapoptotic protein that works in part by blocking cytochrome-c release from mitochondria and the ensuing caspase activation (17, 18). CLP was used to induce sepsis and resulted in the appearance of the processed form of caspase-3 (p17 fragment) in thymocytes from WT but not of Bcl-2 transgenic animals. The p17 product was not detected in sham animals regardless of their genotype (Fig. 1
A). Hence, caspase-3 processing is induced during sepsis but can be blocked by Bcl-2 overexpression. Next, we examined whether caspase substrates were proteolytically processed and whether thymocytes exhibited characteristic signs of apoptosis. The markers chosen reflect either direct substrate cleavage (II-spectrin and PARP) or the consequence of caspase activation on cell function (membrane permeability, PS exposure, and DNA fragmentation). PARP is a nuclear enzyme that participates in DNA repair and has been one of the first proteins identified as a caspase substrate (19). The 24-kD NH2-terminal PARP cleavage fragment was abundant in all WT mice that had undergone CLP but was absent in most Bcl-2–overexpressing animals. Some of the CLP-operated Bcl-2 transgenic and sham-operated WT animals showed slight PARP 24-kD cleavage product (Fig. 1 A). Another caspase substrate, II-spectrin, is a major component of the cortical cytoskeleton and is proteolytically cleaved during lymphocyte apoptosis (20). Both calpain and caspase-3 cleave II-spectrin at multiple sites, with the p120 fragment specifically generated upon caspase-3 cleavage (21–23). The p120 II-spectrin product was prominent in WT mice but was absent in thymi from septic Bcl-2 animals. No p120 fragment was observed in sham-operated animals (Fig. 1 A). The 150-kD II-spectrin cleavage product, which results from both calpain and caspase activity, was present in all animals but was more abundant in thymi from CLP-operated mice. Thus, both PARP and II-spectrin cleavage at the p120 site are protected from caspase cleavage in Bcl-2–overexpressing thymocytes during sepsis. Bcl-2 overexpression did not affect significantly the II-spectrin p150 cleavage site. Loss of membrane phospholipid asymmetry and PS externalization are detected by FITC-labeled annexin V (24). During sepsis, a higher proportion of thymocytes were annexin V positive in CLP relative to sham-operated WT animals (49 versus 18%, respectively, P < 0.001). In contrast, the number of annexin V–positive thymocytes was virtually identical in CLP or sham animals overexpressing Bcl-2 (11.8 versus 9.3%, respectively; Fig. 1 B) but was lower than in sham-treated WT animals. Similar results were obtained with membrane permeability and PI uptake (Fig. 1 C). We conclude that the loss of membrane integrity and phospholipid asymmetry is largely dependent on the mitochondrial apoptotic pathway during sepsis. Cleavage of DNA at internucleosomal spaces is a well-known apoptotic marker and is mediated by DFF40/caspase-activated DNase (CAD) (25–27). CAD activation requires cleavage of DFF45/inhibitor of caspase-activated DNase (ICAD) by caspases (25–27), principally caspase-3 (23, 28–30). We measured DNA fragmentation by the Cell Death ELISA (CDE) method and by flow cytometry using PI staining (as described in Materials and Methods). Thymocytes from mice that have undergone CLP exhibited high levels of DNA fragmentation. Overexpression of Bcl-2 in T cells abrogated DNA cleavage and brought the signal level to or near values found in sham-operated animals (Fig. 1, D and E). We conclude that DNA fragmentation, annexin V binding and II-spectrin cleavage are dependent on the mitochondrial apoptotic pathway during sepsis (Table I).
1 Nicholson, D.W. 1999. Caspase structure, proteolytic substrates, and function during apoptotic cell death. Cell Death Differ. 6:1028–1042.[CrossRef][Medline]
2 Shi, Y. 2002. Mechanisms of caspase activation and inhibition during apoptosis. Mol. Cell. 9:459–470.[CrossRef][Medline]
3 Slee, E.A., C. Adrain, and S.J. Martin. 2001. Executioner caspase-3, -6 and -7 perform distinct, non-redundant roles during the demolition phase of apoptosis. J. Biol. Chem. 276:7320–7326.[Abstract/Free Full Text]
4 Kuida, K., T.S. Zheng, S. Na, C. Kuan, D. Yang, H. Karasumaya, P. Rakik, and R.A. Flavell. 1996. Decreased apoptosis in the brain and premature lethality in CPP32-deficient mice. Nature. 384:368–372.[CrossRef][Medline]
5 Thornberry, N.A., and Y. Lazbenik. 1998. Caspases: enemies within. Science. 281:1312–1316.[Abstract/Free Full Text]
6 Nicholson, D.W. 2000. From bench to clinic with apoptosis-based therapeutic agents. Nature. 407:810–816.[CrossRef][Medline]
7 Angus, D.C., W.T. Linde-Zwirble, J. Lidicker, G. Clermont, J. Carcillo, and M.R. Pinsky. 2001. Epidemiology of severe sepsis in the United States: analysis of incidence, outcome, and associated cost of care. Crit. Care Med. 29:1303–1310.[CrossRef][Medline]
8 Hotchkiss, R.S., P.E. Swanson, B.D. Freeman, K.W. Tinsley, J.P. Cobb, G.M. Matuschak, T.G. Buchman, and I.E. Karl. 1999. Apoptotic cell death in patients with sepsis, shock and multiple organ dysfunction. Crit. Care Med. 27:1230–1251.[CrossRef][Medline]
9 Hotchkiss, R.S., K.W. Tinsley, P.E. Swanson, R.E. Schmieg, Jr., J.J. Hui, K.C. Chang, D.F. Osborne, B.D. Freeman, J.P. Cobb, T.G. Buchman, and I.E. Karl. 2001. Sepsis induces progressive profound depletion of B and CD4+ T lymphocytes. J. Immunol. 166:6952–6953.[Abstract/Free Full Text]
10 Hotchkiss, R.S., P.E. Swanson, J.P. Cobb, A. Jacobson, T.G. Buchman, and I.E. Karl. 1997. Apoptosis in lymphoid and parenchymal cells during sepsis: findings in normal and T- and B-cell-deficient mice. Crit. Care Med. 25:1298–1307.[CrossRef][Medline]
11 Ayala, A., C.D. Herdon, D.L. Lehman, C.A. Ayala, and I.H. Chaudry. 1996. Differential induction of apoptosis in lymphoid tissues during sepsis: variation in onset, frequency and the nature of the mediators. Blood. 87:4261–4275.[Abstract/Free Full Text]
12 Hotchkiss, R.S., P.E. Swanson, C.M. Knudson, K.C. Chang, J.P. Cobb, D.F. Osborne, K.M. Zollner, T.G. Buchman, S.J. Korsmeyer, and I.E. Karl. 1999. Overexpression of Bcl-2 in transgenic mice decreases apoptosis and improves survival in sepsis. J. Immunol. 162:4148–4156.[Abstract/Free Full Text]
13 Hotchkiss, R.S., K.W. Tinsley, P.E. Swanson, K.C. Chang, J.P. Cobb, T.G. Buchman, and I.E. Karl. 1999. Prevention of lymphocyte cell death in sepsis improves survival in mice. Proc. Natl. Acad. Sci. USA. 96:14541–14546.[Abstract/Free Full Text]
14 Coopersmith, C.M., K.C. Chang, P.E. Swanson, K.W. Tinsley, P.E. Stromberg, T.G. Buchman, I.E. Karl, and R.S. Hotchkiss. 2002. Overexpression of Bcl-2 in the intestinal epithelium improves survival in septic mice. Crit. Care Med. 30:195–201.[CrossRef][Medline]
15 Coopersmith, C.M., P.E. Stromberg, W.M. Dunne, C.G. Davis, D.M. Amiot, II, T.G. Buchman, I.E. Karl, and R.S. Hotchkiss. 2002. Inhibition of intestinal epithelial apoptosis and survival in a murine model of pneumonia-induced sepsis. JAMA. 287:1716–1721.[Abstract/Free Full Text]
16 Hotchkiss, R.S., K.C. Chang, P.E. Swanson, K.W. Tinsley, J.J. Hui, P. Klender, S. Xanthoudakis, S. Roy, C. Black, E. Grimm, et al. 2000. Caspase inhibitors improve survival in sepsis: a critical role for the lymphocyte. Nat. Immunol. 1:496–501.[CrossRef][Medline]
17 Kluck, R.M., E. Bossy-Wetzel, D.R. Green, and D.D. Newmeyer. 1997. The release of cytochrome c from mitochondria: a primary site for Bcl-2 regulation of apoptosis. Science. 275:1129–1132.[Abstract/Free Full Text]
18 Yang, J., X. Liu, K. Bhalla, C. Naekyung Kim, A.M. Ibrado, J. Cai, T.-I. Peng, D.P. Jones, and X. Wang. 1997. Prevention of apoptosis by bcl-2: release of cytochrome c from mitochondria blocked. Science. 275:1129–1132.[Abstract/Free Full Text]
19 Lazebnik, Y.A., S.H. Kaufmann, S. Desnoyers, G.G. Poirier, and W.C. Earnshaw. 1994. Cleavage of poly(ADP-ribose) polymerase by a proteinase with properties like ICE. Nature. 371:346–347.[CrossRef][Medline]
20 Martin, S.J., G.A. O'Brien, W.K. Nishioka, A.J. McGahon, A. Mahboubi, T.C. Saido, and D.R. Green. 1995. Proteolysis of fodrin (non-erythroid spectrin) during apoptosis. J. Biol. Chem. 270:6425–6428.[Abstract/Free Full Text]
21 Harris, A.S., D. Croall, and J.S. Morrow. 1988. The calmodulin-binding site in alpha-fodrin is near the calcium-dependent protease-I cleavage site. J. Biol. Chem. 263:15754–15761.[Abstract/Free Full Text]
22 Wang, K.K.W., R. Posmantur, R. Nath, K. McGinnis, M. Whitton, R.V. Talanian, S.B. Glantz, and S.J. Morrow. 1998. Simultaneous degradation of II- and ßII-spectrin by caspase 3 (CPP32) in apoptotic cells. J. Biol. Chem. 273:22490–22497.[Abstract/Free Full Text]
23 Janicke, R.U., P. Ng, M.L. Sprengart, and A.G. Porter. 1998. Caspase-3 is required for -fodrin cleavage but dispensable for cleavage of other death substrates in apoptosis. J. Biol. Chem. 273:15540–15545.[Abstract/Free Full Text]
24 Vermes, I., C. Haanen, H. Steffens-Nakken, and C. Reutelingsperger. 1995. A novel assay for apoptosis: flow cytometric detection of phosphatidylserine expression on early apoptotic cells using fluorescein labelled annexin V. J. Immunol. Methods. 184:39–51.[CrossRef][Medline]
25 Liu, X., P. Li, P. Widlak, H. Zu, X. Luo, W.T. Garrard, and X. Wang. 1998. The 40-kDa subunit of DNA fragmentation factor induces DNA fragmentation and chromatin condensation during apoptosis. Proc. Natl. Acad. Sci. USA. 95:8461–8466.[Abstract/Free Full Text]
26 Enari, M., H. Sakahira, H. Yokoyama, K. Okawa, A. Iwamatsu, and S. Nagata. 1998. A caspase-activated DNase that degrades DNA during apoptosis and its inhibitor ICAD. Nature. 391:43–50.[CrossRef][Medline]
27 Sakahira, H., M. Enari, and S. Nagata. 1998. Cleavage of CAD inhibitor in CAD activation and DNA degradation during apoptosis. Nature. 391:96–99.[CrossRef][Medline]
28 Wolf, B.B., M. Schuler, F. Echeverri, and D.R. Green. 1999. Caspase-3 is the primary activator of apoptotic DNA fragmentation via DNA fragmentation factor-45/inhibitor of caspase-activated DNase inactivation. J. Biol. Chem. 274:30651–30656.[Abstract/Free Full Text]
29 Tang, D., and V.J. Kidd. 1998. Cleavage of DFF-45/ICAD by multiple caspases is essential for its function during apoptosis. J. Biol. Chem. 273:28549–28552.[Abstract/Free Full Text]
30 Sharif-Askari, E., A. Alam, E. Rhéaume, P.J. Beresford, C. Scotto, K. Sharma, D. Lee, W.E. DeWolf, M.E. Nuttall, J. Lieberman, and R.-P. Sékaly. 2001. Direct cleavage of the human DNA fragmentation factor-45 by granzyme B induces caspase-activated DNase release and DNA fragmentation. EMBO J. 20:3101–3113.[CrossRef][Medline]
31 McIlroy, D., M. Tanaka, H. Sakahira, H. Fukuyama, M. Suzuki, K. Yamamura, Y. Ohsawa, Y. Uchiyama, and S. Nagata. 2000. An auxiliary mode of apoptotic DNA fragmentation provided by phagocytes. Genes Dev. 14:549–558.[Abstract/Free Full Text]
32 Lechardeur, D.L. 2000. Drzymala, M. Sharma, D. Zylka, R. Kinach, J. Pacia, C. Hicks, N. Usmani, J.M. Rommens, and G.L. Lukacs. 2000. Determinants of the nuclear localization of the heterodimeric DNA fragmentation factor (ICAD/CAD). J. Cell Biol. 150:321–334.[Abstract/Free Full Text]
33 Chen, D., R.A. Stetler, G. Cao, W. Pei, C. O'Horo, X.-M. Yin, and J. Chen. 2000. Characterization of the Rat DNA fragmentation factor 35/inhibitor of caspase-activated DNase (short form). J. Biol. Chem. 275:38508–38517.[Abstract/Free Full Text]
34 Han, B.H., D. Xu, J. Choi, Y. Han, S. Xanthoudakis, S. Roy, J. Tam, J. Vaillancourt, J. Colucci, R. Siman, A. Giroux, G. Robertson, R. Zamboni, D.W. Nicholson, D.M., and D.M. Holtzman. 2002. Selective, reversible caspase-3 inhibitor is neuroprotective and reveals distinct pathways of cell death after neonatal hypoxic-ischemic brain injury. J. Biol. Chem. 277:30128-30136.[Abstract/Free Full Text]
Top
Abstract
Introduction
0.5 mg/kg/h and an almost complete inhibition at 2 mg/kg/h (Fig. 4
A). Inhibition of DNA fragmentation was dose dependent but required larger amounts of drug (50% inhibition at 
CiteULike 
Complore 
Connotea 
Del.icio.us 
Digg 
Reddit 
Technorati What's this?
