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Key Words: apoptosis-inducing factor • Apaf-1 • chromatin condensation • caspases • caspase-activated DNase
Immunofluorescence Staining.
Electron Microscopy.
DNA Gel Electrophoresis.
Cell-free Systems of Nuclear Apoptosis.
Introduction
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Abstract
Introduction
Materials and Methods
Results and Discussion
References
One of the hallmarks of apoptosis is the degradation and concomitant compaction of chromatin. It has been generally assumed that caspases as well as downstream effectors such as caspase-activated DNase (CAD) and Acinus are rate limiting for the development of nuclear apoptosis 12345. Accordingly, the inactivation of the caspase-3 gene 67 and that of the caspase activator Apaf-1 8 can delay cell death and largely abolish the type of chromatin condensation observed in normal control cells treated with apoptosis inducers such as staurosporine (STS) or etoposide. Similarly, the inactivation of CAD prevents advanced chromatin condensation in different cell types 9. However, caspases and CAD are not the only effectors causing nuclear apoptosis. Thus, chromatin condensation has been observed in lymphoid cells treated with STS, anti-CD2 10, anti-CD4, or anti-CXCR4 11, as well as in fibroblasts overexpressing PML 12, even when caspase activation is inhibited. Partial chromatin condensation is found in thymocytes undergoing apoptosis in the presence of the pan-caspase inhibitor Z-VAD.fmk 13. Recently, apoptosis-inducing factor (AIF), a mitochondrial intermembrane flavoprotein, has been found to translocate from mitochondria to nuclei in a caspase-independent fashion. When added to purified nuclei, recombinant AIF causes caspase-independent large scale (
50 kb) DNA fragmentation and a type of peripheral chromatin condensation that resembles the first stage of nuclear apoptosis (stage I) observed in intact cells undergoing apoptosis 1415. Here, we examined the question of whether several independent pathways may lead to nuclear apoptosis.
Materials and Methods
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Abstract
Introduction
Materials and Methods
Results and Discussion
References
Cells and Microinjection.
Mouse embryonic fibroblasts (MEFs) obtained from caspase 3–/– 7, Apaf-1–/– 8, or control mice were cultured with STS (2 µM), etoposide (100 µM), cisplatin (150 µM), arsenite (50 µM; Sigma-Aldrich), and/or Z-VAD.fmk (50 µM; Enzyme Systems). Cells were microinjected (pressure 150 hPa; 0.4 s; reference 16) with the following: buffer only; recombinant AIF; an inactive deletion mutant of AIF (
1-351; reference 14); horse cytochrome c (Cyt-c; Sigma-Aldrich); recombinant active caspase-3 17; or inactive inhibitor of CAD (ICAD)/CAD or active CAD (generated by digestion of the 250 nM ICAD–CAD complex with 3 U of caspase-3 in 10 µM of CAD buffer; 30 min at room temperature, followed by addition of 100 µM Ac-DEVD.fmk; Enzyme systems). After microinjection, cells were cultured for 180 min and stained for 10 min with the mitochondrial transmembrane potential (
m)-sensitive dye CMXRos (100 nM) and the DNA-intercalating dye Hoechst 33342 (1.5 µM; reference 16). Microinjected viable cells (100 per session; two to three independent sessions of injection) were identified by inclusion of 0.25% (wt/vol) FITC-dextran (green fluorescence) in the injectate. Only the blue and red fluorescence was recorded.
Fixed and permeabilized MEFs were stained for AIF and Cyt-c as described 1415. A rabbit polyclonal antiserum, CM1 (revealed as anti-AIF), was used to detect the p18 subunit of cleaved caspase-3 18. Unfixed cells were incubated for 15 min with 1.2 µM m-sensitive JC-1 (Molecular Probes). Confocal microscopy was performed on a Leica TC-SP equipped with an ArKr laser mounted on an inverted Leica DM IFBE microscope with an 63 x 1.32 numerical aperture oil objective. Two stages of nuclear apoptosis were distinguished by staining with 25 nM Sytox-green (Molecular Probes) for 15 min at room temperature. Stage I was characterized by rippled nuclear contours and a rather partial chromatin condensation, and stage II by a more pronounced pattern of chromatin condensation 1415.
Cells were fixed in pellets for 1 h at 4°C with 1.6% glutaraldehyde in 0.1 M sodium phosphate buffer, pH 7.4, washed three times, and then post-fixed in 1% osmic acid in phosphate buffer before scrapping, dehydration, and embedding. Ultrathin sections mounted on 200 mesh grids were examined in a JEOL 1200 EX electron microscope.
Oligonucleosomal DNA fragmentation was detected by agarose gel electrophoresis 19. For pulse field gel electrophoresis, DNA was prepared from agarose plugs (106 cells; reference 20) and analyzed in a Bio-Rad CHEF-DR II (1% agarose; TBE; 200 V; 24 h; pulse wave 60 s; 120° angle; Bio-Rad Laboratories).
Cytosols from MEFs stimulated for 24 h with STS (2 µM), etoposide (100 µM), or cisplatin (150 µM) were prepared in cell-free system buffer (50 µl/106 cells) supplemented with 50 µM Z-VAD.fmk, as previously described 21. Immunodepletion of AIF (or sham immunodepletion) was performed using an anti-AIF antiserum (or preimmune serum) and protein A/G coupled to agarose (Santa-Cruz Biotechnology, Inc.; reference 14). Purified HeLa cell nuclei were exposed to cytolic extracts (2 µg/µl protein), AIF 14, CAD, ICAD 4, caspase-3 17, and/or the AIF inhibitor para-chloromercuriphenylsulfonic acid (PCMPS; Sigma-Aldrich; reference 22) in cell-free system buffer 23, and nuclear DNA content was quantitated by cytofluorometry after staining with propidium iodide 14.
Results and Discussion
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Abstract
Introduction
Materials and Methods
Results and Discussion
References
Mitochondrial Membrane Permeabilization, Initial Nuclear Apoptosis, and Large Scale DNA Fragmentation Occur in Apaf-1–/– and caspase-3–/– Cells.
Apaf-1–/– or caspase-3–/– cells, as well as control MEF, responded to four different apoptosis inducers (STS, etoposide, cisplatin or arsenite) by manifesting a decrease in the m, translocation of AIF from mitochondria to nuclei, and translocation of Cyt-c from mitochondria to the cytoplasm (Fig. 1A and Fig. B). As expected, at no time point did Apaf-1–/– or caspase-3–/– MEFs stain with an antibody specific for activated caspase-3 (Fig. 1 A). The nuclear phenotype manifested by Apaf-1–/– or caspase-3–/– cells appeared clearly distinct from that of control cells. Apaf-1–/– or caspase-3–/– cells (Fig. 1AFig. c) only manifested a minor peripheral chromatin condensation (stage I), as was also found in control cells after short-term incubation with STS. However, Apaf-1–/– or caspase-3–/– cells failed to develop the more advanced chromatin condensation (stage II) of control cells (Fig. 1AFig. c). None of the mitochondrial parameters nor the pattern or kinetics of chromatin condensation of Apaf-1–/– or caspase-3–/– cells (Fig. 1A and Fig. B) were influenced by addition of the pan-caspase inhibitor Z-VAD.fmk. However, Z-VAD.fmk arrested the nuclear apoptosis of control wild-type cells at stage I (Fig. 1A and Fig. B). At the ultrastructural level, nuclei from apoptotic Apaf-1–/– or caspase-3–/– cells demonstrated a rather partial chromatin condensation, with patches of chromatin abutting to the apparently intact envelope and without nucleolar degradation (Fig. 1 C). As a biochemical correlation of the morphological features of caspase-independent apoptosis, Apaf-1–/– or caspase-3–/– cells developed large scale DNA fragmentation to 50 kb (Fig. 1 D), yet failed to show the (presumably CAD-mediated; references 1, 2, 9) oligonucleosomal DNA fragmentation (Fig. 1 E).
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m loss, chromatin condensation) in wild-type cells, but not in Apaf-1–/– nor in caspase-3–/– cells (Fig. 2A and Fig. B). In contrast, microinjection of active caspase-3 provoked full-blown apoptosis (stage II) in all three cell types (Fig. 2 B). Similarly, AIF and CAD induced apoptosis in all cell types (Fig. 2A and Fig. B). AIF induced a peripheral type of chromatin condensation (similar to the caspase-independent stage I, Fig. 1 A), whereas CAD (and its activator caspase-3) provoked a more advanced pattern of nuclear compaction (similar to the caspase-dependent stage II, Fig. 1 A). The differential effect of AIF and CAD was confirmed in a cell-free system. When added to purified HeLa nuclei, AIF caused peripheral chromatin condensation (Fig. 3A and Fig. B), whereas CAD induced a much stronger type of chromatin compaction accompanied by a reduction in nuclear size (Fig. 3A and Fig. B). Moreover, AIF alone caused large scale DNA fragmentation (Fig. 3 D), yet was unable to provoke the "ladder type" oligonucleosomal chromatin digestion (Fig. 3 E). In contrast, CAD provoked the digestion of DNA in two steps, first into 50 kb (at low doses; Fig. 3 F) and then into mono- and oligomers of 200 bp (at high doses; Fig. 3 E). Moreover, CAD could act on AIF-pretreated nuclei (which lack oligonucleosomal DNA fragmentation, Fig. 3 E) to induce oligonucleosomal fragmentation (Fig. 3 G). In conclusion, AIF and CAD cause two morphologically and biochemically distinct types of nuclear apoptosis.
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Irrespective of these theoretical considerations, our data indicate the existence of at least two pathways leading to chromatin condensation and degradation during apoptosis. Why the process of apoptotic chromatin condensation is so complex and whether these pathways are connected at the molecular level by a common action on sessile nuclear proteins with proapoptotic potential remains an open question for future investigation.
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Acknowledgments |
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L. Ravagnan and K.F. Ferri received Ph.D. fellowships from the French Ministry of Science & Technology; M. Loeffler received a postdoctoral fellowship from the Austrian Science Foundation; and P. Costantini received a fellowship from the Fondation pour la Recherche Medicale (FRM). This work has been supported by a special grant of the Ligue Nationale contre le Cancer, as well as by grants from Agence National de Recherche sur la SIDA, FRM (to G. Kroemer), Assistance Publique-Hôpitaux de Paris and Caisse Nationale Assurance Maladie (CANAM; contract 98006 to E. Daugas), and the Wellcome Trust (to W.C. Earnshaw).
Submitted: 13 January 2000
Revised: 5 May 2000
Accepted: 13 June 2000
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References |
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| TABLE OF CONTENTS |
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), etoposide (
), cisplatin (
), arsenite (
) and/or Z-VAD.fmk (right panels) are shown in B. This experiment has been repeated three times, yielding comparable results. Electron microscopy (C), large scale DNA fragmentation (D), and oligonucleosomal DNA fragmentation (E) of cells treated as in A are also shown.
10% of nuclear apoptosis. Results are means of triplicates (X ± SD) and are representative of three independent determinations.