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© The Rockefeller University Press,
0021-9525/2000//1011 $5.00
The Journal of Cell Biology, Volume 149, Number 5,
, 2000 1011-1018
Brief Report |
Inhibition of Apoptotic Signaling Cascades Causes Loss of Trophic Factor Dependence during Neuronal Maturation
ejohnson{at}pcg.wustl.edu
During development, neurons are acutely dependent on target-derived trophic factors for survival. This dependence on trophic support decreases dramatically with maturation in several neuronal populations, including sympathetic neurons. Analyses of nerve growth factor deprivation in immature and mature sympathetic neurons indicate that maturation aborts the cell death pathway at a point that is mechanistically indistinguishable from Bax deletion. However, neither the mRNA nor protein level of BAX changes with neuronal maturation. Therefore, BAX must be regulated posttranslationally in mature neurons.
Nerve growth factor deprivation in immature sympathetic neurons induces two parallel processes: (a) a protein synthesis–dependent, caspase-independent translocation of BAX from the cytosol to mitochondria, followed by mitochondrial membrane integration and loss of cytochrome c; and (b) the development of competence-to-die, which requires neither macromolecular synthesis nor BAX expression. Activation of both signaling pathways is required for caspase activation and apoptosis in immature sympathetic neurons. In contrast, nerve growth factor withdrawal in mature sympathetic neurons did not induce the translocation of either BAX or cytochrome c. Moreover, mature neurons did not develop competence-to-die with cytoplasmic accumulation of cytochrome c. Therefore, inhibition of both BAX-dependent cytochrome c release and the development of competence-to-die contributed to the loss of trophic factor dependence associated with neuronal maturation.
Key Words: BAX • caspase • cytochrome c • mitochondria • neurotrophin
© 2000 The Rockefeller University Press
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Introduction |
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 TopAbstract Introduction Materials and MethodsResults and DiscussionReferences |
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Genetic and biochemical studies have identified several critical regulators of apoptosis in mammals: caspases, Apaf-1, and the BCL-2 family of proteins. In the mammalian nervous system, most naturally occurring programmed cell death requires the expression of BAX, a proapoptotic member of the BCL-2 family of proteins (Deckwerth et al. 1996; Shindler et al. 1997; White et al. 1998).
Analyses of the biochemical and molecular events induced by trophic factor deprivation in immature and mature sympathetic neurons indicate that the latter are functionally indistinguishable from Bax-deficient cells (Easton et al. 1997). That is, mature sympathetic neurons phenocopy Bax–/– immature neurons: all known biochemical and molecular events induced by trophic factor withdrawal that occur upstream of the BAX/BCL-2 checkpoint do so with similar kinetics in both Bax–/– immature and Bax+/+ mature neurons. However, neither the mRNA nor protein level of BAX increases during NGF deprivation–induced apoptosis in neonatal neurons (Greenlund et al. 1995) or decreases with neuronal maturation (Easton et al. 1997), suggesting that BAX is regulated posttranslationally in both immature and mature sympathetic neurons.
In immature sympathetic neurons, NGF deprivation induces two parallel processes: (a) a protein synthesis–dependent, caspase-independent translocation of BAX (Putcha et al. 1999) from the cytosol to mitochondria, followed by loss of mitochondrial cytochrome c (Deshmukh and Johnson 1998; Neame et al. 1998; Martinou et al. 1999; Putcha et al. 1999); and (b) the development of competence-to-die with cytoplasmic accumulation of cytochrome c, which requires neither macromolecular synthesis nor BAX expression (Deshmukh and Johnson 1998). Activation of both pathways is required for caspase activation and apoptotic cell death in immature sympathetic neurons. In this study, we examined whether decreased trophic factor dependence in mature sympathetic neurons results from inhibition of one or both of these pathways. We found that NGF deprivation in mature sympathetic neurons, which causes Jun NH2-terminal kinase (JNK) activation and some immediate–early gene transcription (Easton et al. 1997), did not induce the translocation of either BAX or cytochrome c. Moreover, mature neurons did not develop competence-to-die with cytoplasmic accumulation of cytochrome c, even after prolonged periods of NGF deprivation. Therefore, failure of both BAX-dependent cytochrome c release and the development of competence-to-die caused the loss of trophic factor dependence in mature sympathetic neurons.
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Materials and Methods |
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TopAbstractIntroductionMaterials and MethodsResults and DiscussionReferences |
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Sympathetic Neuronal Cultures
Primary cultures of sympathetic neurons were established from the superior cervical ganglia of each postnatal day-1 (P1) mouse by using previously described methods (Johnson and Argiro 1983; Deckwerth et al. 1996; Easton et al. 1997). Neurons were grown in AM50 for 
5 d (immature; 5 d in vitro [DIV 5]) or 25 d (mature; DIV 25) and then either maintained in AM50 or treated as follows: for NGF deprivation, cultures were rinsed with AM0, followed by the addition of AM0 containing goat anti–mouse 2.5S NGF neutralizing antiserum (anti-NGF) (Ruit et al. 1990); for NGF deprivation in the presence of various reagents, 1 µg/ml cycloheximide or 50 µM BAF, respectively, was added to AM0 containing anti-NGF.
Immunocytochemistry
Neuronal cultures were immunostained as described previously (Easton et al. 1997). Cytochrome c was detected with mouse monoclonal primary antibodies (1:1,000) (PharMingen) and FITC-conjugated donkey anti–mouse secondary antibody (1:300) (Jackson ImmunoResearch). BAX was detected with a rat monoclonal primary antibody (1:250) (catalog number 13401A, lot M024742; PharMingen) and a Cy3-conjugated anti–rat secondary antibody (1:400) (Jackson ImmunoResearch).
Cell Counts: BAX and Cytochrome c Immunocytochemistry
Sympathetic neurons that had been maintained in NGF for 5 or 25 DIV in AM50 were deprived of NGF in the presence of the caspase inhibitor BAF (as described above). At various times after deprivation, cultures were fixed and immunostained with anti-BAX or anti–cytochrome c antibodies. For each timepoint, the number of cells that had acquired a punctate staining pattern for BAX or had lost the punctate staining pattern for cytochrome c was determined by a blinded observer from a random sampling of 200–250 cells. All experiments were conducted in the presence of BAF to prevent any cell loss that would otherwise affect the counts.
Subcellular Fractionation
Sympathetic neurons (106) were harvested in 10 ml of isotonic fractionation buffer (250 mM sucrose, 0.5 mM EDTA, 20 mM Hepes, 500 µM Na3VO4, pH 7.2) supplemented with protease inhibitor cocktail Complete (Roche Molecular Biochemicals) and centrifuged at 900 g for 5 min. All steps were conducted at 4°C. The pellet was then resuspended in 200 µl fractionation buffer, homogenized by using a ball-bearing homogenizer, and centrifuged at 900 g for 5 min to remove nuclei and intact cells. The postnuclear supernatant was transferred to a microfuge tube (Beckman) and centrifuged at 25,000 g for 10 min to collect the heavy membrane (HM) fraction enriched in mitochondria, followed by centrifugation of the post-HM supernatant at 100,000 g for 10–20 min to obtain the microsomal and cytosolic fractions. All pellets were resuspended in a volume of fractionation buffer equivalent to the cytosolic volume. All fractions were then resuspended to equivalent volumes with lysis buffer and evaluated by Western blotting.
We were unable to detect cytochrome c in the cytosolic fractions of both nonneuronal and neuronal primary cells and cell lines undergoing apoptosis induced by a variety of stimuli, even at multiple timepoints. The lack of detectable cytochrome c in the cytosol may indicate its rapid degradation once it has been released into the cytosol (Deshmukh and Johnson 1998; Neame et al. 1998; Martinou et al. 1999; Putcha et al. 1999).
Alkali Extraction
The postnuclear supernatant from sympathetic neurons (2–4 x 106) was isolated as described above and aliquoted equally into three microfuge tubes. Samples were centrifuged at 25,000 g for 10 min to collect the HM fractions. The post-HM supernatants were pooled, centrifuged at 100,000 g for 10–20 min to obtain the microsomal and cytosolic fractions, and prepared for immunoblot analysis as described above. The HM pellets were then resuspended in 800 µl fractionation buffer, 0.2 M Na2CO3, pH 11.5, or 1% (wt/vol) SDS, incubated at 4°C for 30 min while rotating, and centrifuged at 25,000 g for 10–20 min to retrieve the HM pellets. These pellets were resuspended in a volume of fractionation buffer equivalent to one-third the cytosolic volume and prepared for Western blot analysis as described above. Mitochondrial integral membrane proteins are resistant to extraction by 0.2 M Na2CO3, yet sensitive to extraction by 1% SDS, whereas peripheral membrane proteins are extracted by both treatments.
Microinjections and Quantitation of Cell Death
These experiments were performed as described previously (Deshmukh and Johnson 1998). In brief, sympathetic neurons were maintained in NGF for either 5 or 25 DIV and treated for 36–48 h with NGF, anti-NGF, or anti-NGF plus 1 µg/ml cycloheximide. Cells were then microinjected with 25 mg/ml bovine cytochrome c and rhodamine dextran dye. At each timepoint after the injections, the number of microinjected cells that remained viable was determined by using morphological criteria and expressed as a percentage of the total number of microinjected cells.
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Results and Discussion |
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TopAbstractIntroductionMaterials and MethodsResults and DiscussionReferences |
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5 (immature) or 25 d (mature). Cells were then deprived of NGF for various periods, and the subcellular localization of BAX and cytochrome c was determined by using both immunocytochemistry (Fig. 1) and subcellular fractionation (Fig. 2). The pan-caspase inhibitor BAF was added to the cultures at the time of deprivation to prevent any cell death that might otherwise have complicated cell counts.
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Recently, two groups reported that BAX did not translocate from the cytosol to mitochondria during cell death in nonneuronal cell lines. Instead, they suggested that BAX already at the mitochondria undergoes a conformational change that exposes the NH2 terminus (Goping et al. 1998; Desagher et al. 1999). To distinguish between these two possibilities, we also examined the localization of BAX and cytochrome c by using subcellular fractionation. In NGF-maintained immature sympathetic neurons, BAX primarily localized to the cytosol, whereas cytochrome c was found exclusively in mitochondria (Fig. 2 a). NGF deprivation induced the translocation of BAX from the cytosol to mitochondria, leading to the loss of mitochondrial cytochrome c (Fig. 2 a). Taken together with our previous findings (Putcha et al. 1999), the results shown in Fig. 1 and Fig. 2 demonstrate that trophic factor withdrawal in immature sympathetic neurons induced the translocation of BAX from the cytosol to mitochondria, followed by the loss of mitochondrial cytochrome c.
BAX is found in both the cytosolic and mitochondrial fractions of various tissues and cells, including sympathetic neurons, both in vivo and in vitro (Fig. 2 a and Fig. 3 a; data not shown) (Hsu et al. 1997; Eskes et al. 2000). To determine whether BAX associated with mitochondria is integrated into mitochondrial membranes, we performed alkali extraction of the mitochondrial fractions from NGF-maintained and -deprived immature sympathetic neurons (Fig. 3 a). Mitochondrial integral membrane proteins are resistant to extraction by 0.2 M Na2CO3, yet sensitive to extraction by 1% SDS, whereas peripheral membrane proteins are extracted by both treatments. In NGF-maintained cells, mitochondrial BAX was extracted by alkali treatment, indicating that under normal conditions, a small amount of cellular BAX is loosely associated with mitochondrial membranes. Conversely, mitochondrial BAX from NGF-deprived sympathetic neurons was resistant to alkali extraction, consistent with its insertion into mitochondrial membranes. Thus, trophic factor withdrawal in immature sympathetic neurons induced the translocation of BAX from the cytosol to mitochondria and integration of BAX into mitochondrial membranes.
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Although BAX-dependent cytochrome c release is necessary for NGF deprivation–induced cell death in immature sympathetic neurons, it is not sufficient, since cytoplasmic accumulation of cytochrome c does not induce apoptosis in NGF-maintained cells. Sympathetic neurons must also develop competence-to-die, a process that requires neither macromolecular synthesis nor BAX expression (Deshmukh and Johnson 1998). Only activation of both signaling pathways, BAX-dependent cytochrome c release, and the development of competence-to-die, is sufficient to ensure rapid and efficient neuronal apoptosis after trophic factor withdrawal. To determine whether mature neurons develop competence-to-die after NGF withdrawal, we examined whether cytoplasmic accumulation of cytochrome c was sufficient to induce cell death in NGF-deprived, mature sympathetic neurons. Immature and mature sympathetic neurons were deprived of NGF for 36–48 h in the presence or absence of cycloheximide and then microinjected with holocytochrome c. In immature neurons, cycloheximide prevents cell death yet allows the development of competence induced by NGF deprivation (Deshmukh and Johnson 1998). At various times after microinjection, cell viability was assessed. As shown in Fig. 4, cytoplasmic microinjection of cytochrome c did not induce cell death in NGF-deprived, mature sympathetic neurons, even with 1 wk of deprivation (data not shown) or with a fivefold higher concentration of cytochrome c than that required for immature cells (i.e., 25 vs. 5 mg/ml). Therefore, these neurons did not develop competence-to-die. Thus, the results shown in Fig. 1Fig. 2Fig. 3Fig. 4 demonstrate that inhibition of both BAX-dependent cytochrome c release and the development of competence-to-die was responsible for the loss of trophic factor dependence associated with neuronal maturation.
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Acknowledgments |
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This work was supported by National Institutes of Health grants R37AG-12947 and RO1NS38651 (E.M. Johnson, Jr.) and a Paralyzed Veterans of America Spinal Cord Research grant (M. Deshmukh).
Submitted: 20 March 2000
Revised: 24 April 2000
Accepted: 26 April 2000
Abbreviations used in this paper: BAF, boc-aspartyl(OMe)-fluoromethylketone; DIV, days in vitro; HM, heavy membrane.
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3. Bar, 5 µm. Please note that a, b, e, and f have been reported previously in 
