Overexpression of Copper/Zinc Superoxide Dismutase in Transgenic Mice Protects against Neuronal Cell Death after Transient Focal Ischemia by Blocking Activation of the Bad Cell Death Signaling Pathway

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The Journal of Neuroscience, March 1, 2003, 23(5):1710

Overexpression of Copper/Zinc Superoxide Dismutase in Transgenic Mice Protects against Neuronal Cell Death after Transient Focal Ischemia by Blocking Activation of the Bad Cell Death Signaling Pathway
Atsushi Saito, Takeshi Hayashi, Shuzo Okuno, Michel Ferrand-Drake, and Pak H. Chan
Department of Neurosurgery, Department of Neurology and Neurological Sciences, and Program in Neurosciences, Stanford University School of Medicine, Stanford, California 94305-5487

  ABSTRACT

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
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The Bad signaling pathway contributes to the regulation of apoptosis after a variety of cell death stimuli, and Bad playsa key role in determining cell death or survival. We have reportedthat overexpression of copper/zinc superoxide dismutase (SOD1)reduces apoptotic cell death after transient focal cerebral ischemia(tFCI). However, both the role of the Bad pathway after tFCI andthe role of oxygen free radicals in the regulation of apoptosisremain unknown. To clarify these issues, we used an in vivo tFCImodel of SOD1 transgenic mice and wild-type mice. Moreover, toexamine the role of protein kinase A (PKA) in the Bad pathwayafter tFCI, we administered the PKA inhibitor, H89, into the mousebrain after tFCI. Immunohistochemistry and Western blot analysisshowed that dephosphorylation and translocation of Bad were detectedearly after tFCI and that they were promoted by H89 treatmentbut prevented by SOD1. Coimmunoprecipitation revealed that thedimerization of Bad progressed with 14-3-3 (Bad/14-3-3) and withBcl-x_L (Bad/Bcl-x_L) after tFCI. Moreover, Bad/14-3-3 was preventedby H89 treatment but promoted by SOD1. Bad/Bcl-x_L was preventedby SOD1 but promoted by H89 treatment. A cell death assay revealedthat apoptotic-related DNA fragmentation was aggravated by H89treatment but reduced by SOD1. These results suggest that theBad pathway mediated by PKA is involved in apoptotic cell deathafter tFCI and that overexpression of SOD1 may attenuate thisapoptotic celldeath.

Key words: cerebral ischemia; apoptosis; Bad; Bcl-x_L; 14-3-3; superoxide

  Introduction

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ABSTRACT
Introduction
Materials and Methods
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Discussion
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The cell survival pathway has been the focus in clarifying the machinery of apoptotic neuronal cell death after cerebral ischemia.The Bcl-2 family of proteins and many kinase-signaling pathwaysplay pivotal roles in regulation of the balance between cell deathand survival (Adachi et al., 1997; Datta et al., 2000). The Bcl-2family comprises proapoptotic and anti-apoptotic proteins; someproteins within this family, such as Bcl-2, Bcl-x_L, and Bcl-w,inhibit apoptosis, whereas others, including Bad, Bax, Bid, andBcl-x_S, promote apoptosis (Yang and Korsmeyer, 1996; Kroemer,1997). Dimerization of Bcl-2 family members involves interactionsbetween amino acid sequences, known as Bcl-2 homology domains(Yang and Korsmeyer, 1996; Kroemer, 1997; Reed, 1997; Kelekarand Thompson, 1998). Bad, an important proapoptotic member ofthe Bcl-2 family, links signal transduction events to this family(Yang et al., 1995; Zha et al., 1996). Via the phosphorylationof four serine residues (Ser-112, 136, 155, 170) Bad resides inan inactive complex with the molecular chaperone 14-3-3 in invitro studies (Zha et al., 1996; Datta et al., 2000; Lizcano etal., 2000; Dramsi et al., 2002). In the presence of apoptoticstimuli Bad is dephosphorylated, dissociated from 14-3-3, andtranslocated to the outer membrane of mitochondria, where it subsequentlydimerizes with Bcl-x_L (Zha et al., 1996; Hsu et al., 1997; Zhanget al., 1999). Ser-155 residue is critical to the direct interactionof Bad with Bcl-x_L after apoptotic stimuli in many in vitro studies(Tan et al., 1999, 2000; Datta et al., 2000). Ser-155 phosphorylationis regulated by protein kinase A (PKA) or mitogen-activated proteinkinase-activated protein kinase 1 (also called RSK) (Tan et al.,1999; Lizcano et al., 2000). However, Bad prophosphorylation anddephosphorylation after apoptotic stimuli remain unclear in vivo.Intraventricular injection of H89, a specific inhibitor of PKA,effectively suppresses the activity of PKA (Cervo et al., 1997;Kimura et al., 1998). To clarify the Bad signaling pathway andthe role of PKA in vivo, we used a mouse transient focal cerebralischemia (tFCI) model and administered H89 aftertFCI.

Reactive oxygen species (ROS) has been implicated in the machinery of reperfusion injury after cerebral ischemia (Chan, 1994;Fujimura et al., 1999). The electron flow in isolated brain mitochondriaproduces superoxide anions, which are scavenged by superoxidedismutase (SOD) (Boveris and Chance, 1973). We have shown thatcopper/zinc-SOD (SOD1), a cytosolic antioxidant isoenzyme, ishighly protective against ischemia and reperfusion injury aftercerebral ischemia (Kinouchi et al., 1991; Chan, 1996; Kondo etal., 1997). In examining the mechanism of the proapoptotic pathway,our studies have demonstrated that SOD1 affected the early releaseof cytochrome c (Fujimura et al., 2000) and the second mitochondria-derivedactivator of caspases (Sugawara et al., 2002) from mitochondriato the cytosol after cerebral ischemia. However, whether SOD1could affect the balance between cell survival and the apoptoticpathway has not been demonstrated. The present study was designedto clarify the role of SOD1, an endogenous antioxidant, in theBad signaling pathway aftertFCI.

  Materials and Methods

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

SOD1 transgenic mice. Heterozygous SOD1 transgenic (Tg) mice of the SOD1 TGHS/SF-218-3 strain with a CD-1 background, carryinghuman SOD1 genes with a threefold increase in copper/zinc-SOD,were derived from the founder stock described previously (Chan,1994). They were bred further with CD-1 wild-type mice to generateheterozygous mice. The SOD1 Tg mice were identified by quantitativedemonstration of SOD1 with the use of nondenaturing gel electrophoresis,followed by nitroblue tetrazolium staining. There were no differencesin the phenotypes, including the anatomy of the circle of Willis,between the SOD1 Tg mice and their wild-type littermates. Therewas no difference in the regional cerebral blood flow before andafter FCI between the SOD1 Tg and wild-typemice.

Focal cerebral ischemia. Adult male mice (3 months old, 35-40 gm) were subjected to tFCI by intraluminal middle cerebral artery(MCA) blockade with a nylon suture as described previously. Themice were anesthetized with 1.5% isoflurane in 30% oxygen and70% nitrous oxide, using a face mask. The rectal temperature wascontrolled at 37°C with a homeothermic blanket. Cannulation ofa femoral artery allowed for the monitoring of blood pressureand arterial blood gases, samples for analysis being taken immediatelyafter cannulation, 10 min after occlusion, and 10 min after reperfusion.Blood gas was analyzed with a pH/blood gas analyzer (Chiron Diagnostics,Essex, UK). After a midline skin incision the left external carotidartery was exposed, and its branches were electrocoagulated. A11.0 mm 5-0 surgical monofilament nylon suture, blunted at theend, was introduced into the left internal carotid artery throughthe external carotid artery stump. After 60 min of MCA occlusionthe blood flow was restored by the withdrawal of the nylon suture.To examine the role of PKA in the Bad signaling pathway, we intraventricularlyinjected a PKA inhibitor, H89, after tFCI. H89 [N-(2- [p-bromocinnamylamino]ethyl)-5-isoquinolinesulfonamide-2HCl]was purchased from Sigma (St. Louis, MO) and dissolved in MilliQH₂O (Millipore, Bedford, MA). The dose of the drug was decidedby referring to a previous intraventricular injection study (Cervoet al., 1997). The scalp was incised on the midline, and the skullwas exposed. H89 (4 µg/µl in MilliQ H₂O) and the vehicle (MilliQH₂O alone) were injected intraventricularly (2 µl, bregma; 1.0mm lateral, 0.2 mm posterior, 3.1 mm deep). H89 and the vehiclewere injected 1 hr before MCAocclusion.

Immunohistochemistry. Anesthetized animals, as well as normal controls (n = 4 each), were perfused with 10 U/ml heparin andsubsequently with 4% paraformaldehyde in 0.1 M PBS, pH 7.4, at1, 2, 4, 8, and 24 hr of reperfusion. The brains were removed,postfixed for 12 hr, sectioned at 50 µm on a vibratome, and processedfor immunohistochemistry. The sections were incubated with blockingsolution and reacted with rabbit polyclonal anti-Bad antibody,which detects total (phosphorylation state-independent) Bad levels(Cell Signaling Technology, Beverly, MA) at a dilution of 1:400,and rabbit polyclonal anti-phosphorylated Bad (Ser-155) antibody,which detects Bad only when phosphorylated at Ser-155 (Cell SignalingTechnology) at a dilution of 1:400, plus rabbit polyclonal anti-Bcl-x_Lantibody (Cell Signaling Technology) at a dilution of 1:1000,rabbit polyclonal anti-14-3-3 antibody (Cell Signaling Technology)at a dilution of 1:400, and heat shock protein (HSP) 60 (Chemicon,Temecula, CA) at a dilution of 1:400. Immunohistochemistry wasperformed via the avidin-biotin technique, and then the nucleiwere counterstained with methyl green solution for 2 min. Forhistological assessment alternate slices from each brain sectionwere stained with cresylviolet.

Terminal deoxynucleotidyl transferase-mediated uridine 5'-triphosphate-biotin nick end labeling staining. To clarify the spatialdistribution of DNA fragmentation, we performed terminal deoxynucleotidyltransferase-mediated uridine 5'-triphosphate-biotin nick end labeling(TUNEL; n = 4 each). The sections fixed by 4% paraformaldehydewere prepared as described above and were incubated with NeuroPore(Trevigen, Gaithersburg, MD) for 30 min. They were placed in 1×terminal deoxynucleotidyl transferase (TdT) buffer (Invitrogen,Carlsbad, CA) for 30 min, followed by reaction with TdT enzyme(Invitrogen) and biotinylated 16-dUTP (Roche Diagnostics, Indianapolis,IN) at 37°C for 90 min. The sections were washed two times insaline-sodium citrate (150 mM sodium chloride, 15 mM sodium citrate,pH 7.4) for 15 min, followed by washing in PBS two times for 15min. The avidin-biotin technique was applied, and then the nucleiwere counterstained with methyl green solution for 2min.

Immunofluorescent double-labeling staining. To evaluate colocalization of Bad and neuron-specific nuclear protein (NeuN) andBad and HSP 60, we performed double immunofluorescent stainingfor these proteins (n = 4 each). The sections fixed by 4% paraformaldehydewere immunostained with anti-Bad antibody as described above,with biotinylated goat anti-rabbit immunoglobulin G (IgG; VectorLaboratories, Burlingame, CA), followed by fluorescein avidinDCS (Vector Laboratories). Then the sections were incubated witha blocking solution and reacted with anti-NeuN or HSP 60 antibody(Cell Signaling Technology) as described above, followed by TexasRed-conjugated donkey anti-mouse IgG antibody (Jackson ImmunoResearch,West Grove, PA) at a dilution of 1:400. The sections were placedon slides, which then were covered with Vectashield mounting mediumwith 4',6-diamidino-2-phenylindole (DAPI; Vector Laboratories).Fluorescence of fluorescein was observed at excitation (Ex) of495 nm and emission (Em) of >515 nm, and fluorescence of TexasRed was observed at Ex of 510 nm and Em of >580 nm. Fluorescenceof DAPI also was observed at Ex of 360 nm and Em of >460nm.

Immunofluorescent double labeling with phosphorylated Bad immunohistochemistry and TUNEL. To clarify the spatial relationshipbetween phosphorylated Bad at Ser-155 (pBad) expression and DNAfragmentation, we performed double staining for pBad and TUNEL,using a fluorescent method (n = 4 each). The sections fixed by4% paraformaldehyde were immunostained with the pBad antibodyas described above with biotinylated goat anti-rabbit IgG (VectorLaboratories), followed by fluorescein avidin DCS (Vector Laboratories).Then the sections were incubated with NeuroPore (Trevigen) for30 min and placed in 1× TdT buffer (Invitrogen) for 30 min, followedby reaction with TdT enzyme (Invitrogen) and biotinylated 16-dUTP(Roche Diagnostics) at 37°C for 90 min. The sections were washedtwo times in saline-sodium citrate (150 mM sodium chloride, 15mM sodium citrate, pH 7.4) for 15 min, followed by washing inPBS two times for 15 min. Texas Red avidin DCS (Vector Laboratories)was applied to the sections for 30 min. Subsequently, the slideswere covered with Vectashield mounting medium with DAPI (VectorLaboratories). Fluorescence was assessed as describedpreviously.

Western blot analysis. Protein extraction of the cytosol fraction was performed as described previously with some modification(Fujimura et al., 1999). Samples were obtained from the MCA territorybrain tissue on the ischemic sides and from nonischemic controls(n = 4 each). Fresh brain tissue was removed after 1, 2, 4, 8,and 24 hr (n = 4 each) of reperfusion and homogenized by gentlydouncing 35 times in a glass tissue grinder (Wheaton, Millville,NJ) in 7 vol of cold suspension buffer [containing (in mM) 20HEPES-KOH, pH 7.5, 250 sucrose, 10 KCl, 1.5 MgCl₂, 1 EDTA, and1 EGTA plus 0.7% protease and phosphatase inhibitor mixtures (Sigma)].The homogenate was centrifuged at 750 × g for 10 min at 4°C andthen at 8000 × g for 20 min at 4°C. The 8000 × g pellets wereused to obtain the mitochondrial fraction. The supernatant wascentrifuged further at 100,000 × g for 60 min at 4°C. This supernatantwas used for the cytosolic analysis. After adding the same volumeof Tris-glycine sodium dodecyl sulfate sample buffer (Invitrogen)to the supernatant, we loaded equal amounts of the samples perlane. The primary antibodies were 1:600 dilution of rabbit polyclonalantibody against Bad (Cell Signaling Technology), 1:1000 dilutionof mouse polyclonal antibody against Bcl-x_L (Cell Signaling Technology),1:1000 dilution of mouse polyclonal antibody against 14-3-3 (CellSignaling Technology), 1:10,000 dilution of anti- $beta$ -actin monoclonalantibody (Sigma), and 1:2000 dilution of anti-cytochrome oxidaseIV monoclonal antibody (Molecular Probes, Eugene, OR). Westernblots were performed with horseradish peroxidase-conjugated anti-rabbitIgG (Cell Signaling Technology) or anti-mouse IgG (Chemicon) byusing enhanced chemiluminescence Western blotting detection reagents(Amersham Biosciences, Buckinghamshire, UK). The film was scannedwith a GS-700 imaging densitometer (Bio-Rad Laboratories, Hercules,CA) and the results were quantified with Multi-Analyst software(Bio-Rad).

Coimmunoprecipitation. The protein extraction of the cytosol and the mitochondrial fraction was performed as described previouslywith some modification (Fujimura et al., 1999). The procedurefor precipitation was performed as described previously with somemodification (Springer et al., 2000). Samples were obtained fromthe MCA territory brain tissue on the ischemic side and from nonischemiccontrols (n = 4 each). Fresh brain tissue was removed after 1,2, 4, 8, and 24 hr (n = 4 each) of reperfusion and was preparedfor collection of the cytosolic fraction and the mitochondrialfraction in the same manner as for Western blotting. Protein concentrationswere determined by the Bradford method (Bio-Rad). Three hundredmicrograms of protein from the cytosol fraction and 15 µg fromthe mitochondrial fraction were used for coimmunoprecipitation.Whole brain extract was included as a positive control. The proteinsample was incubated with 50% slurry of protein G-Sepharose (AmershamBiosciences, Uppsala, Sweden) for 1 hr at 4°C, and this mixedsample was centrifuged at 12,000 × g for 1 min. The supernatantwas incubated with 2 µg of polyclonal rabbit anti-Bcl-x_L antibody(Cell Signaling Technology) or polyclonal mouse anti-14-3-3 antibody(Cell Signaling Technology) and 15 µl of protein G-Sepharose (50%slurry) for 1 hr at 4°C. The negative control was prepared withprotein G-Sepharose without antibody. The 14,000 × g pellets werewashed three times and used as the samples bound to each antibody.After adding the same volume of Tris-glycine sodium dodecyl sulfatesample buffer (Invitrogen) to the sample, we boiled these samplesto remove Sepharose beads. After centrifugation at 14,000 × gfor 1 min, the supernatant was immunoblotted with a 1:600 dilutionof anti-Bad antibody (Cell Signaling Technology) as describedin the Western blottingmethod.

In situ detection of superoxide anion production. The early production of superoxide anions (O₂^-) in cerebral ischemia was investigated by using hydroethidine(HEt) via a previously described method. HEt is diffusible intothe CNS parenchyma after an intravenous injection and is oxidizedto ethidium selectively by O₂^-, but not by other ROS such as hydrogen peroxide, hydroxyl radical,or peroxynitrite. HEt solution (200 µl; 1 mg/ml in PBS) was administeredintravenously 15 min before ischemia induction as described. Inthe brains of the animals intravenously injected with HEt, fluorescencewas assessed microscopically at Ex = 355 nm and Em > 415 nm forHEt detection or at Ex = 510-550 nm and Em > 580 nm for ethidiumdetection. Animals were killed 1 hr after tFCI by transcardialperfusion as described (n = 4 each). After fixation with 4% paraformaldehydefor 12 hr the brains were sectioned at 50 µm on a vibratome. Subsequently,the slides were covered with Vectashield mounting medium withDAPI (Vector Laboratories). These sections were observed witha microscope under fluorescentlight.

Cell death assay. For quantification of apoptotic-related DNA fragmentation we used a commercial enzyme immunoassay to determinecytoplasmic histone-associated DNA fragments (Roche MolecularBiochemicals, Mannheim, Germany), which detect apoptotic but notnecrotic cell death (Leist et al., 1998). Samples were obtainedfrom the entire MCA territory on the ischemic side and from nonischemiccontrols (n = 4 each). Fresh brain tissue was cut into piecesafter 1, 2, 4, 8, and 24 hr of reperfusion and homogenized witha Teflon homogenizer in 5 vol of ice-cold buffer (50 mM KH₂PO₄,0.1 mM EDTA, pH 7.8) and spun for 10 min at 750 × g. The supernatantwas collected and spun for 20 min at 10,000 × g and was centrifugedfurther at 100,000 × g for 60 min at 4°C. The resulting supernatantwas collected, and the protein concentration was determined. Acytosolic volume containing 20 µg of protein was used for theenzyme-linked immunosorbent assay by following the manufacturer'sprotocol.

Quantification and statistical analysis. The data are expressed as mean ± SD. Comparisons among multiple groups were performedwith a one-way ANOVA with appropriate post hoc tests (SigmaStatsoftware, Jandel, San Rafael, CA). Comparisons between two groupswere achieved with Student's t test. Significance was acceptedwith p < 0.05.

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Introduction
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Physiological data and cerebral infarction

Physiological data demonstrated no significant differences in body temperature, mean arterial blood pressure, and arterialblood gas analysis between the groups. The preischemic physiologicalvalues were as follows (in mmHg): 36.4 ± 0.3°C body temperature,83 ± 3.1 mean arterial blood pressure, 7.3 ± 0.1 pH, 164.9 ± 19PaO₂, 30 ± 10 PaCO₂ (values are mean ± SD; n = 4). There was nodeviation from these values over the period of assessment. Anischemic lesion of the core of the caudate-putamen was visibleas a pale, slightly stained area in the ischemic hemisphere asearly as 1 hr after reperfusion and extended to the entire MCAterritory at 4 hr by cresyl violet staining (data not shown).The time-dependent increase in infarction in the mouse brainswith the intraluminal suture blockade is consistent with previousreports that used the same FCI model in mice (Yang et al., 1994;Kondo et al., 1997).

14-3-3 protein and Bcl-x_L expression were not different among the time courses and between SOD1 Tg mice and wild-type mice after tFCI

14-3-3 protein immunoreactivity was evident as bands with a molecular mass of 30 and 33 kDa in the cytosolic fraction fromthe MCA territory (Fig. 1A). 14-3-3 expression showed no differenceamong all time courses after tFCI (Fig. 1A). 14-3-3 protein-immunopositivecells were seen in the cortex and the caudate-putamen of boththe nonischemic and ischemic hemispheres, and there was no conspicuousdifference in the reactivity between the hemispheres (data notshown). Double immunofluorescent staining for 14-3-3 and NeuNdemonstrated that 14-3-3 protein expression colocalized with neuronsin the ischemic cortex 24 hr after reperfusion (Fig. 1B). Bcl-x_Lwas expressed as a single band with a molecular mass of 30 kDain the cytosolic fraction (Fig. 1A). Bcl-x_L expression did notchange time dependently (Fig. 1A). Bcl-x_L-immunopositive cellswere seen in the cortex and the caudate-putamen of both the nonischemicand the ischemic sides, and there was no difference in the reactivitybetween the hemispheres (data not shown). Double immunofluorescentstaining for Bcl-x_L and NeuN demonstrated that Bcl-x_L expressioncolocalized with neurons in the ischemic cortex 24 hr after reperfusion(Fig. 1B). Western blot analysis demonstrated that neither 14-3-3protein nor Bcl-x_L immunoreactivity was different between theSOD1 Tg mice and the wild-type mice 24 hr after reperfusion (Fig.1C). These results suggest that the expression of both 14-3-3and Bcl-x_L was neither increased nor reduced after tFCI and thatit also was not affected by intrinsic SOD1.

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Figure 1. A, Western blot analysis of 14-3-3, Bcl-x_L, and $beta$ -actin after tFCI. Shown are 14-3-3, Bcl-x_L, and $beta$ -actin from the cytosolic fraction samples in the nonischemic control brains (cont. lane) and ischemic brains (lanes 1-24 hr; n = 4 each). 14-3-3 immunoreactivity is evident as bands with a molecular mass of 30 and 33 kDa in the cytosolic fraction from the MCA territory in mouse brains (top row). Bcl-x_L immunoreactivity is evident as a band with a molecular mass of 30 kDa (middle row). Both 14-3-3 and Bcl-x_L were expressed constitutively in the control brain (top, middle rows, cont. lane) and showed no prominent increase or decrease after ischemia (top, middle rows, lanes 1-24 hr). The results of the $beta$ -actin analysis are shown as an internal control (bottom row). B, Representative photomicrographs show double immunofluorescent staining for 14-3-3, Bcl-x_L, and NeuN 4 hr after tFCI (n = 4 each). Expression of 14-3-3 was observed in the ischemic cortex (top left panel, green) and showed no prominent change in any of the time courses. NeuN immunoreactivity (red) showed the distribution of neurons in the same view (top middle panel). Overlapped image of 14-3-3 and NeuN immunoreactivity demonstrated that 14-3-3 expression colocalized with neurons in the same view (top right panel, yellow). Expression of Bcl-x_L was observed in the ischemic cortex (bottom left panel, green) and showed no prominent change in any of the time courses. NeuN immunoreactivity (red) showed the distribution of neurons in the same view (bottom middle panel). Overlapped image of Bcl-x_L and NeuN immunoreactivity demonstrated that Bcl-x_L expression colocalized with neurons in the same view (bottom right panel, yellow). Scale bars, 4 µm. C, Western blot analysis of 14-3-3, Bcl-x_L, and $beta$ -actin 24 hr after tFCI in SOD1 Tg mice and wild-type mice (n = 4 each). No difference was observed between the SOD1 Tg mice and the wild-type mice in either 14-3-3 or Bcl-x_L expression (top, middle rows). $beta$ -Actin was used as an internal control, and no difference was observed between the samples (bottom row).

Phosphorylated Bad at Ser-155 was diminished after tFCI and did not colocalize with TUNEL-positive cells

pBad immunoreactivity was evident as a single band with a molecular mass of 23 kDa (Fig. 2A). pBad expression decreased 1hr after reperfusion and was diminished significantly 8 hr afterreperfusion (Fig. 2A) (p < 0.05). TUNEL-positive cells were seenin the caudate-putamen and the cortex of the MCA territory surroundingthe ischemic core, most obviously 24 hr after reperfusion (datanot shown). These results are consistent with previous reportsthat used the same FCI model in mice (Fujimura et al., 1999).The pBad-positive cells were seen in the nonischemic hemisphere,and fewer positive cells were seen in the ischemic cortex (datanot shown). In the area in which TUNEL-positive cells were observed,many fewer pBad-positive cells were seen, and most TUNEL-positivecells did not colocalize with pBad immunoreactivity (Fig. 2B).These results suggest that the dephosphorylation of Bad at Ser-155progressed during the very early period after tFCI and that thedecrease in pBad might be related to the beginning of apoptoticcell death after tFCI.

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Figure 2. A, Western blot analysis of phosphorylated Bad at serine-155 residue (pBAD) after tFCI. The expression of pBad was detected as a band with a molecular mass of 23 kDa (n = 4 each). The immunoreactivity of pBad decreased gradually in a time-dependent manner (top row). The quantitative analysis showed that pBad expression was decreased significantly 8 hr after tFCI (bottom panel; *p < 0.05). $beta$ -Actin was used as an internal control, and no difference was observed between the samples (middle row). B, Representative photomicrographs show double immunofluorescent staining for pBad and TUNEL 24 hr after tFCI (n = 4 each). The pBad was expressed strongly in the nonischemic control area and expressed weakly in the ischemic cortex of the MCA territory and the partial caudate-putamen surrounding the ischemic core (left panel, red). TUNEL-positive cells were observed in the ischemic cortex of the MCA territory in the same view (middle panel, green). Overlapped image of pBad and TUNEL demonstrated that most pBad-immunopositive cells were not colocalized with TUNEL-positive cells (right panel). Scale bar, 10 µm. C, D, Western blot analyses of Bad in the cytosolic fraction (C) and in the mitochondrial fraction (D) after tFCI (n = 4 each). The expression of Bad was detected as a band with a molecular mass of 23 kDa (C, D, top row). The cytosolic Bad immunoreactivity decreased in a time-dependent manner (C). In particular, Bad expression 8 and 24 hr after tFCI decreased significantly compared with the nonischemic control sample (cont.) (C, top row, 8 hr, p > 0.05; 24 hr, p > 0.05). Mitochondrial Bad immunoreactivity gradually increased after 1 hr of tFCI (D, top row). At 8 hr after tFCI the Bad expression decreased significantly (D, top row; *p < 0.05). $beta$ -Actin was used as an internal control for the cytosolic fraction, and cytochrome oxidase (COX) was used as an internal control for the mitochondrial fraction (C, D, middle rows). No difference was observed between the fraction samples (C, D, middle rows). E, Representative photomicrographs show double immunofluorescent staining for Bad and NeuN 4 hr after tFCI (n = 4 each). Expression of Bad was observed in the ischemic cortex (left panel, green) and showed no prominent change in any of the time courses. NeuN immunoreactivity (red) showed the distribution of neurons in the same view (middle panel, red). Overlapped image of Bad and NeuN immunoreactivity demonstrated that Bad expression colocalized with neurons in the same view (right panel, yellow). Scale bar, 15 µm. F, Representative photomicrographs show double immunofluorescent staining for Bad and heat shock protein 60 (HSP60) at 8 hr after tFCI (n = 4 each). HSP 60 expression was used as a marker for the distribution of mitochondria. Expression of Bad was observed in the ischemic cortex and showed particle-like punctate stains in the cell body (left panel, green). This particle-like immunoreactivity was observed in the HSP 60 immunoreactivity (middle panel, red). Overlapped image of Bad and HSP 60 immunoreactivity demonstrated that punctate Bad expression colocalized with the distribution in mitochondria in the same view (right panel, yellow). Scale bar, 10 µm. OD, Optical density.

Western blot analysis and immunofluorescent double staining demonstrated translocated Bad after tFCI

Bad expression was detected as a band with a molecular mass of 23 kDa (Fig. 2C,D). Bad expression decreased as early as 2hr after reperfusion, and at 8 hr after reperfusion a significantdecrease was seen (Fig. 2C). In contrast, mitochondrial Bad expressiongradually increased after tFCI (Fig. 2D). One hour after reperfusionthe band was barely visible, but after 4 hr of reperfusion itwas obvious (Fig. 2D). A significant increase was observed 8 hrafter reperfusion (Fig. 2D). Double immunofluorescent stainingfor Bad and NeuN demonstrated that Bad immunoreactivity colocalizedwith neurons in the cortex of the ischemic hemisphere 24 hr afterreperfusion (Fig. 2E). The immunohistochemical expression of HSP60 is reported to be an effective marker for the localizationof mitochondria and is used to examine the colocalization or thetranslocation related to mitochondria (Springer et al., 2000).Double immunofluorescence for Bad and HSP 60 demonstrated thatthe punctate Bad immunoreactivity was obvious in the cortex surroundingthe ischemic core after 8 hr of reperfusion and that the particle-likeimmunoreactivity colocalized with mitochondrial expression (Fig.2F). These results suggest that Bad translocated from the cytosolto mitochondria during the early period after tFCI and that thetiming of Bad translocation was consistent with that of the dephosphorylationof Bad. We could not find the relationship between Bad expressionand glial fibrillary acidic protein in the mouse brains aftertransient focal ischemia (data not shown). However, we cannotexclude completely the possibility that such a relationship existsbetween the Bad signaling reaction and astrocytes after ischemicdamage.

Coimmunoprecipitation demonstrated the direct binding of Bad to 14-3-3 and Bcl-x_L

To investigate the direct interaction of Bad with 14-3-3 and Bcl-x_L, we performed coimmunoprecipitation. In the cytosolicfraction a robust band of Bad precipitated by 14-3-3 protein (Bad/14-3-3)was detected in the sham control, and the bands gradually decreasedby 24 hr after reperfusion (Fig. 3A,B). In contrast, Bad expressionprecipitated by Bcl-x_L (Bad/Bcl-x_L) in the mitochondrial fractionincreased time dependently, and a significant increase was observed8 hr after reperfusion (Fig. 3A,B). These results suggest thatwith a nonischemic stimulus Bad sequestered with 14-3-3 in thecytosol, but it dissociated from 14-3-3 after tFCI and that thetranslocated Bad dimerized with Bcl-x_L concomitant with the dissociationfrom 14-3-3.

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Figure 3. A, B, Coimmunoprecipitation analysis for Bad immunoreactivity precipitated by 14-3-3 in the cytosolic fraction (BAD/14-3-3) (A, top row; B, left panel) and Bad immunoreactivity precipitated by Bcl-x_L in the mitochondrial fraction (BAD/Bcl-x_L) (A, bottom row; B, right panel) after tFCI (n = 4 each). Bad/14-3-3 expression gradually decreased in a time-dependent manner (A, top row; B, left panel). At 24 hr after tFCI the Bad/14-3-3 expression significantly decreased (B, left panel; *p < 0 0.05). Bad/Bcl-x_L expression gradually increased (A, bottom row; B, right panel). At 8 hr after tFCI the Bad/Bcl-x_L expression significantly increased (B, right panel; *p < 0.05). p.c., Positive control; n.c., negative control; cont., nonischemic control sample.

Cell death assay demonstrated that DNA fragmentation after tFCI significantly decreased in SOD1 Tg mice compared with wild-type mice and that it increased with intraventricular administration of H89

Apoptotic-related DNA fragmentation after tFCI was analyzed with a commercial cell death assay kit. As shown in Figure 4A,DNA fragmentation was increased significantly in the ischemicMCA territory 24 hr after reperfusion. It was reduced significantlyin the SOD1 Tg mice compared with the wild-type mice 24 hr aftertFCI (Fig. 4B) (p < 0.05). However, it was increased significantlyin the H89-treated mice compared with the vehicle-treated miceat the same time point (Fig. 4C) (p < 0.05). We performed theintraventricular injection of H89 in the mouse brains as reportedpreviously and confirmed that the administration of H89 effectivelyreduced PKA activity (Cervo et al., 1997; Kimura et al., 1998).TUNEL-positive cells were seen in the caudate-putamen and in thecortex of the MCA territory surrounding the ischemic core andwere observed most obviously 24 hr after reperfusion (data notshown). TUNEL-positive cells were reduced in the SOD1 Tg micecompared with the wild-type mice 24 hr after tFCI (Fig. 4D, toppanels). However, TUNEL-positive cells were increased in the H89-treatedmice compared with the vehicle-treated mice at the same time point(Fig. 4D, bottom panels). To confirm whether free radical inductionafter reperfusion was promoted by H89, we examined O₂^- production by using the H89-treated mice and the vehicle-treatedmice 1 hr after reperfusion. Production of O₂^- was determined by using HEt as described previously (Murakamiet al., 1997). Oxidized HEt signals were observed most stronglyin the ischemic cortex 1 hr after reperfusion and were reducedin the SOD1 Tg mice compared with the wild-type mice (Fig. 4E,top panels). These results are consistent with previous reportsthat used the same tFCI model in mice (Murakami et al., 1997;Fujimura et al., 2000; Noshita et al., 2002). There was no conspicuousdifference in the oxidized HEt signals between the H89-treatedmice and the vehicle-treated mice (Fig. 4E, bottom panels). Theseresults suggest that overexpression of SOD1 attenuates apoptoticcell death after tFCI and that inhibition of PKA activity aggravatedapoptotic cell death after tFCI. Moreover, data on the detectionof O₂^- show that SOD1 prevented the early production of O₂^- after tFCI and that inhibition of PKA did not affect O₂^- production after tFCI, suggesting that ROS might be upstreamof activation of the Bad signaling pathway, which may be mediatedby PKA.

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Figure 4. A, Apoptotic-related DNA fragmentation after tFCI was analyzed with a commercial cell death detection kit (n = 4 each). DNA fragmentation increased significantly in the entire MCA territory lesion 24 hr after tFCI (**p < 0.01). B, In the SOD1 Tg mice DNA fragmentation significantly decreased compared with the wild-type mice 24 hr after tFCI (*p < 0.05; n = 4 each). C, In the H89-treated mice, as a protein kinase A inhibitor sample, DNA fragmentation significantly increased compared with the vehicle-treated mice 24 hr after tFCI (*p < 0.05; n = 4 each). D, Representative photomicrographs show TUNEL staining in SOD1 Tg mice (top left panel) and in the H89-treated mice (bottom left panel) and, as a control, in the wild-type mice (top right panel) and the vehicle-treated mice (bottom right panel) 24 hr after tFCI (n = 4 each). TUNEL-positive cells were observed in the ischemic cortex of the MCA territory and the partial caudate-putamen surrounding the ischemic core 24 hr after tFCI. TUNEL reactivity was strongly observed in the wild-type mice (top right panel), whereas in the SOD1 Tg mice TUNEL reactivity decreased (top left panel). TUNEL reactivity in the H89-treated mice was much stronger compared with the vehicle-treated mice (bottom panels). Scale bar, 50 µm. E, Representative photomicrographs show superoxide production in the H89-treated mice (bottom left panel) and the vehicle-treated mice (bottom right panel) 1 hr after tFCI (n = 4 each). Superoxide production was observed by oxidized HEt signals (red), and nuclei were stained by DAPI (blue) 1 hr after reperfusion injury. The oxidized HEt signal was reduced in the SOD1 Tg mice compared with the wild-type mice (top panels). No conspicuous difference was observed between the H89-treated mice and the vehicle-treated mice (bottom panels). Scale bar, 25 µm.

H89 administration affected phospho-Bad and translocated Bad expression and dimerization with 14-3-3 and Bcl-x_L after tFCI

We examined the role of PKA in the Bad signaling pathway after tFCI by using the tFCI model with H89-treated mice. Westernblot analysis demonstrated that pBad immunoreactivity was reducedsignificantly in the H89-treated mice compared with the vehicle-treatedmice 24 hr after reperfusion (Fig. 5A) (p < 0.05). In the wild-typemice pBad expression was barely visible in the ischemic core,and its weak expression was observed in the caudate-putamen andthe cortex of the MCA territory surrounding the ischemic coreafter 8 hr of reperfusion (data not shown). Western blot analysisdemonstrated that translocated Bad expression in the mitochondrialfraction was significantly greater in the H89-treated mice comparedwith the vehicle-treated mice 24 hr after reperfusion (Fig. 5B)(p < 0.05). Immunohistochemistry also showed that the expressionof pBad in the penumbra regions was diminished in the H89-treatedmice compared with the vehicle-treated mice (Fig. 5C). Coimmunoprecipitationdemonstrated that Bad/14-3-3 immunoreactivity in the cytosolicfraction was reduced significantly in the H89-treated mice comparedwith the vehicle-treated mice 24 hr after reperfusion (Fig. 5D)(p < 0.05), whereas Bad/Bcl-x_L immunoreactivity in the mitochondrialfraction significantly increased in the H89-treated mice comparedwith the vehicle-treated mice 24 hr after reperfusion (Fig. 5E)(p < 0.05). These results suggest that the inhibition of PKA causedprogression of dephosphorylation and translocation of Bad andthat it also caused progression of the dissociation from 14-3-3and the dimerization with Bcl-x_L after tFCI.

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Figure 5. A, Western blot analysis for pBad in the cytosolic fraction in the H89-treated mice and the vehicle-treated mice 24 hr after tFCI. pBad expression was significantly stronger in the vehicle-treated mice compared with the H89-treated mice at the same time course (top row, bottom panel; *p < 0.05). $beta$ -Actin was used as an internal control for the cytosolic fraction, and no difference was seen between the samples (middle row). B, Western blot analysis for translocated Bad (trans. BAD) in the mitochondrial fraction in the H89-treated mice and the vehicle-treated mice 24 hr after tFCI. Translocated Bad expression was significantly stronger in the H89-treated mice compared with the vehicle-treated mice at the same time course (top row, bottom panel; *p < 0.05). Cytochrome oxidase (COX) expression was used as an internal control for the mitochondrial fraction, and no difference was seen between the samples (middle row). C, Representative photomicrographs show the immunohistochemistry for pBad in the H89-treated mice (left) and the vehicle-treated mice (right) in the cortex of the MCA territory 24 hr after tFCI. The immunoreactivity of pBad was stronger in the vehicle-treated mice compared with the H89-treated mice at the same time course. Scale bar, 20 µm. D, Coimmunoprecipitation analysis of Bad/14-3-3 in the cytosolic fraction in the H89-treated mice and the vehicle-treated mice 24 hr after tFCI. The expression of Bad/14-3-3 was significantly stronger in the vehicle-treated mice compared with the H89-treated mice (*p < 0.05). E, Coimmunoprecipitation analysis of Bad/Bcl-x_L in the mitochondrial fraction in the H89-treated mice and the vehicle-treated mice 24 hr after tFCI. Expression of Bad/Bcl-x_L was significantly stronger in the H89-treated mice compared with the vehicle-treated mice (*p < 0.05). OD, Optical density.

Overexpression of SOD1 increased phospho-Bad, diminished the translocated Bad, and affected the dimerization with 14-3-3 and Bcl-x_L after tFCI

We examined the relationship between the Bad signaling pathway after tFCI and oxidative stress by using the tFCI model withSOD1 Tg mice. Western blot analysis demonstrated that pBad immunoreactivitywas detected as a significantly stronger band in the SOD1 Tg micecompared with the wild-type mice 24 hr after reperfusion (Fig.6A) (p < 0.05). Western blot analysis that used the mitochondrialfraction demonstrated that translocated Bad immunoreactivity wasdiminished significantly in the SOD1 Tg mice compared with thewild-type mice 24 hr after reperfusion (Fig. 6B) (p < 0.05). Inthe penumbra areas of the MCA territory surrounding the ischemiccore, immunoreactivity of pBad was also greater in the SOD1 Tgmice compared with the wild-type mice 24 hr after reperfusion(Fig. 6C). Coimmunoprecipitation demonstrated that the expressionof Bad/14-3-3 in the cytosolic fraction significantly increasedin the SOD1 Tg mice compared with the wild-type mice 24 hr afterreperfusion (Fig. 6D) (p < 0.05) and that Bad/Bcl-x_L immunoreactivitywas diminished significantly in the SOD1 Tg mice compared withthe wild-type mice (Fig. 6E) (p < 0.05). These results suggestthat overexpression of SOD1 prevented dephosphorylation and translocationof Bad and that it also prevented the dissociation from 14-3-3and the dimerization with Bcl-x_L after tFCI.

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Figure 6. A, Western blot analysis for pBad in the cytosolic fraction in the SOD1 Tg mice and the wild-type mice 24 hr after tFCI. pBad expression was significantly stronger in the SOD1 Tg mice compared with the wild-type mice at the same time course (top row, bottom panel; *p < 0.05). $beta$ -Actin was used as an internal control for the cytosolic fraction, and no difference was seen between the samples (middle row). B, Western blot analysis for translocated Bad in the mitochondrial fraction in SOD1 Tg mice and wild-type mice 24 hr after tFCI. Translocated Bad (trans. BAD) expression was significantly stronger in the wild-type mice compared with the SOD1 Tg mice at the same time course (top row, bottom panel; *p < 0.05). Cytochrome oxidase (COX) expression was used as an internal control for the mitochondrial fraction, and no difference was seen between the samples (middle row). C, Representative photomicrographs show immunohistochemistry for pBad in the SOD1 Tg mice (left) and the wild-type mice (right) in the cortex of the MCA territory 24 hr after tFCI. Immunoreactivity of pBad was observed more strongly in the SOD1 Tg mice compared with the wild-type mice at the same time course. Scale bar, 20 µm. D, Coimmunoprecipitation analysis for Bad/14-3-3 in the cytosolic fraction in the SOD1 Tg mice and the wild-type mice 24 hr after tFCI. Expression of Bad/14-3-3 was significantly stronger in the SOD1 Tg mice compared with the wild-type mice (*p < 0.05). E, Coimmunoprecipitation analysis for Bad/Bcl-x_L in the mitochondrial fraction in the SOD1 Tg mice and the wild-type mice 24 hr after tFCI. Expression of Bad/Bcl-x_L was significantly stronger in the wild-type mice compared with the SOD1 Tg mice (*p < 0.05). OD, Optical density.

  Discussion

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

There is clear evidence that neuronal apoptotic cell death after cerebral ischemia involves factors that determine the balanceof cell death and survival (Noshita et al., 2002; Zhu et al.,2002). In recent studies cell survival factors have been the focusas critical regulators of the progress of apoptosis; these includeserine-threonine kinase, the Akt cell signaling pathway, mitogen-activatedprotein kinase (MAPK) and extracellular signal-regulated kinase(ERK) kinase (MEK) and the ERK pathway (Hetman et al., 1999; Rommelet al., 1999; Zimmermann and Moelling, 1999). Phosphorylationof serine or threonine residues interacts with these signalingfactors and plays a pivotal role in the regulation of the balancebetween cell death and cell survival (Burgering and Coffer, 1995;Flanke et al., 1999). As an executor downstream of these signalingfactors, Bad is reported to have an important role and act dynamicallyvia the phosphorylation of its four serine residues in responseto different stimuli (Burgering and Coffer, 1995; Datta et al.,2000; Lizcano et al., 2000; Dramsi et al., 2002). As for Ser-112,one of the serine residues of Bad, it has been demonstrated thattransforming growth factor- $beta$ 1 suppresses Bad expression and increasesphosphorylation via the activation of the MAPK/ERK pathway inboth in vivo and in vitro cerebral ischemia models (Zhu et al.,2002). An in vitro study showed that phosphorylation of Bad atSer-155 was affected by some kinases, such as RSK and PKA, andthat the ERK pathway is upstream of RSK (Bonni et al., 1999; Pastorinoet al., 1999; Tan et al., 1999; Shimamura et al., 2000). In particular,Ser-155 residue is known as the most critical site for the translocationof Bad and dimerization with Bcl-x_L, which is the turning pointfor the regulation of apoptosis (Lizcano et al., 2000; Tan etal., 2000). However, little is known about the relationship betweenBad phosphorylation at Ser-155 and the Bad signaling pathway invivo. In particular, nothing is known about the link between theBad signaling pathway and ischemic stimuli in vivo. In the presentstudy we demonstrated for the first time the following points.(1) The translocation of Bad from the cytosol to the mitochondriawas detected during the early period after tFCI. The expressionof phosphorylated Bad at Ser-155 residue decreased in the cytosol,which was related concomitantly to the translocation of Bad. Thissuggests that, in the absence of ischemic stimuli, Bad localizedin the cytosol and that after reperfusion injury phosphorylatedBad at Ser-155 residue was diminished to translocate from thecytosol to the mitochondria. (2) The direct binding of Bad to14-3-3 in the cytosol and to Bcl-x_L in the mitochondria was detectedafter tFCI. Whereas Bad/14-3-3 binding gradually increased, incontrast Bad/Bcl-x_L binding decreased in a time-dependent mannerafter tFCI. These results demonstrate that after reperfusion injuryBad dissociated from 14-3-3 and the translocated Bad dimerizedwith Bcl-x_L in the mitochondria. (3) A PKA-specific inhibitor,H89, decreased the phosphorylated Bad at Ser-155 and increasedthe translocated Bad. Moreover, it also decreased Bad/14-3-3 bindingand increased Bad/Bcl-x_L binding after tFCI. Quantitative analysisshowed that the PKA inhibitor apparently aggravated apoptoticneuronal cell death after tFCI. These results reveal that theinhibition of PKA accelerated the apoptotic cell death signalingpathway after tFCI by blocking phosphorylation of Bad at Ser-155.PKA seems to phosphorylate Bad, at least at Ser-155, and to affectcell survival in reperfusion injury after tFCI. There is a possibilitythat the PKA inhibitor is related to the dephosphorylation ofBad not only at Ser-155 but also at Ser-112, as reported in anin vitro study. However, in our study we did not elucidate theexact role of Ser-112 residue on Bad after tFCI. Further studyis required to clarify the difference in function among otherserine residues on Bad. PKA inhibitor is thought to affect phosphorylation-relatedmechanisms globally. We cannot exclude completely the possibilitythat PKA inhibition might affect the cell death pathway in a mannerunrelated to the Bad reaction after ischemic insult. (4) Overexpressionof intrinsic SOD1 diminished dephosphorylation of Bad at Ser-155and the translocation of Bad. Moreover, it increased Bad/14-3-3binding and decreased Bad/Bcl-x_L to protect the neurons againstapoptotic cell death after tFCI. In an in situ superoxide detectionanalysis H89 did not affect the production of superoxide afterreperfusion injury, suggesting that the increase in productionof superoxide after reperfusion injury is upstream of the Badphosphorylation pathway mediated byPKA.

In our mouse tFCI model such dynamic activities as dephosphorylation, dissociation, translocation, and dimerization of Badafter reperfusion injury were observed, as they have been in manyin vitro studies. However, other important links between Bad andother kinase signaling pathways, for example MEK/ERK and phosphatidylinositol3-kinase/Akt upstream of the Bad signaling pathway or Bax andother Bcl-2 family member pathways downstream of that, remainunknown, especially in in vivo ischemia models (Noshita et al.,2002; Zhu et al., 2002). As for Bax, it translocates from thecytosol to the mitochondria after reperfusion injury in mousetFCI and induces mitochondrial membrane permeabilization by interactingwith proteins of the mitochondrial permeability transition porecomplex, such as voltage-dependent anion channel and adenine nucleotidetranslocator (Cao et al., 2001). The translocation of Bax is suggestedto result in the release of apoptosis-promoting factors, includingcytochrome c (Jürgensmeier et al., 1998; Narita et al., 1998).However, the interaction between Bax translocation and Bad remainsunclear. It was reported that Bcl-x_L resides constitutively boundto Bax in the cytosol and that Bad displaces and releases Baxfrom Bcl-x_L (Yang et al., 1995). Thereafter, Bax translocatesfrom the cytosol to mitochondria (Li et al., 1997; Jürgensmeieret al., 1998). Our data show that Bad/Bcl-x_L binding was detectedin the mitochondrial fraction, and expression of the binding increasedin a time-dependent manner after reperfusion injury, suggestingthat mitochondria are the main site at which Bad interacts withBcl-x_L. Similarly, Bad/Bcl-x_L binding was detected in mitochondriaafter traumatic spinal cord injury in rats, and the binding contrastedwith Bad/14-3-3 binding in the cytosol fraction (Springer et al.,2000). Because Bcl-x_L, which could bind to Bax in mitochondria,decreases as Bad/Bcl-x_L binding increases after reperfusion injury,we suggest that Bcl-x_L unbound to Bad is also important for activationdownstream of the Bad signalingpathway.

Our previous studies demonstrated that overexpression of intrinsic SOD1 has protective effects on ischemic damage (Kinouchiet al., 1991; Chan, 1996; Kondo et al., 1997; Fujimura et al.,1999, 2000). In this study we focused on the role of the Bad signalingpathway on the neuroprotective effect of SOD1. Our results demonstratethat overexpression of SOD1 prevented the Bad cell death pathwayafter reperfusion injury, and it shifted the balance between survivaland death to cell survival. The ERK pathway is reported to beone of the kinase pathways for Bad phosphorylation in in vitrostudies (Pastorino et al., 1999; Lizcano et al., 2000). It isreported that ROS can induce MEK/ERK cell death pathway activationin vitro (Baas and Berk, 1995; Guyton et al., 1996; Seo et al.,2001). We also have demonstrated that oxidative stress plays acrucial role in ERK cell death pathway activation after tFCI (Noshitaet al., 2002). It is not clear whether the ERK pathway regulatesphosphorylation of Bad in vivo, including reperfusion injury aftertFCI. Moreover, transforming growth factor (TGF) also has beensuggested to contribute to activation of the MAPK/ERK pathwayand PKA (Wang et al., 1998; Zhu et al., 2002). There is also apossibility that ROS affect TGF activation or production via reductionin oxidation-sensitive transcription factors, such as NF- $kappa$ B andhypoxia-inducible factor-1 $alpha$ after apoptotic stimuli (Haddad, 2002;Ishida et al., 2002). It remains unclear how oxidative stressis involved with the Bad signaling pathway after tFCI, but itis obvious that oxidative stress plays an important role in theactivation of the Bad cell death pathway. Further study is requiredto clarify the link between the Bad signaling pathway and oxidativestress aftertFCI.

Conclusion

Our results imply that the Bad cell death signaling pathway is activated in neurons after tFCI and that SOD1 contributes tothe inhibition of apoptosis induced by FCI by reducing the earlyformation of superoxide radicals and preventing the dephosphorylationof Bad. We suggest that SOD1 may play a critical role in the Badsignalingpathway.

  FOOTNOTES

Received Oct. 17, 2002; revised Dec. 12, 2002; accepted Dec. 19, 2002.

This work was supported by National Institutes of Health Grants P50NS14543, R0125372, R0136147, and R0138653 and an AmericanHeart Association Bugher Foundation award. P.H.C. is a recipientof the Jacob Javits Neuroscience Investigator Award. We are gratefulto Dr. Charles J. Epstein (Department of Pediatrics, Universityof California, San Francisco, School of Medicine) for the breedingpairs of SOD1 transgenic mice. We thank Cheryl Christensen foreditorial assistance, Liza Reola and Bernard Calagui for technicalassistance, and Elizabeth Hoyte for figurepreparation.

Correspondence should be addressed to Dr. Pak H. Chan, Neurosurgical Laboratories, Stanford University School of Medicine,1201 Welch Road, MSLS #p314, Stanford, CA 94305-5487. E-mail:phchan{at}leland.stanford.edu.

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