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Previous Article | Next Article
The Journal of Neuroscience, June 15, 2000, 20(12):4506-4514
Activation of Mitogen-Activated Protein Kinases after Transient Forebrain Ischemia in Gerbil Hippocampus
Toshiyuki Sugino1, Kazuhiko Nozaki1, Yasushi Takagi1, Itaro Hattori1, Nobuo Hashimoto1, Tetsuo Moriguchi2, and Eisuke Nishida2 1 Department of Neurosurgery, Graduate School of Medicine, Kyoto University, Kyoto 606-8507, Japan, and 2 Department of Biophysics, Graduate School of Science, Kyoto University, Kyoto 606-8502, Japan
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
We investigated the expression, activation, and distribution of c-Jun N-terminal kinases (JNKs), p38 mitogen-activated protein kinases (p38s) and extracellular signal-regulated kinases (ERKs) using Western blotting and immunohistochemistry in gerbil hippocampus after transient forebrain ischemia to clarify the role of these kinases in delayed neuronal death (DND) in the CA1 subfield. Immunoblot analysis demonstrated that activities of JNK, p38, and ERK in whole hippocampus were increased after 5 min of global ischemia. We used an immunohistochemical study to elucidate the temporal and spatial expression of these kinases after transient global ischemia. The immunohistochemical study showed that active JNK and p38 immunoreactivities were enhanced at 15 min of reperfusion and then gradually reduced and disappeared in the hippocampal CA1 region. On the other hand, in CA3 neurons, active JNK and p38 immunoreactivities were enhanced at 15 min of reperfusion and peaked at 6 hr of reperfusion and then gradually reduced but was continuously detected 72 hr after ischemia. Active ERK immunoreactivity was observed transiently in CA3 fibers and dentate gyrus. Pretreatment with SB203580, a p38 inhibitor, but not with PD98059, an ERK kinase 1/2 inhibitor, reduced ischemic cell death in the CA1 region after transient global ischemia by inhibiting the activity of p38. These findings indicate that the p38 pathway may play an important role in DND during brain ischemia in gerbil. Components of the pathway are important target molecules for clarifying the mechanism of neuronal death.
Key words: mitogen-activated protein kinase (MAPK); c-Jun N-terminal kinase (JNK); p38 mitogen-activated protein kinase (p38); extracellular signal-regulated kinase (ERK); transient global ischemia; delayed neuronal death (DND); hippocampus; gerbil
INTRODUCTION
The members of the mitogen-activated protein kinase (MAPK), which are characterized as proline-directed serine-threonine-protein kinases, in particular, c-Jun N-terminal kinases (JNKs), p38 mitogen-activated protein kinases (p38s), and extracellular signal-regulated kinases (ERKs), play important roles in transducing stress-related signals in eukaryotic cells (Kyriakis and Avruch, 1996
). On activation by phosphorylation on both Thr and Tyr residues, these kinases phosphorylate intracellular enzymes and transcription factors. The JNK and p38 are activated by stress signals such as inflammatory cytokines, heat shock, ultraviolet light, and ischemia (Kyriakis and Avruch, 1996
Recent studies demonstrate that the members of MAPK, in particular JNK and p38, are activated in heart, kidney, and brain after ischemia and ischemia-reperfusion (Hu and Wieloch, 1994
A brief period of global ischemia causes delayed neuronal death (DND) in the CA1 region of hippocampus in gerbil (Kirino, 1982
Although there are some in vivo reports about MAPK cascade and brain ischemia (Hu and Wieloch, 1994
In the present study, we investigated the activations of JNK, p38, and ERK during transient forebrain ischemia in gerbil to clarify the roles of these kinases in DND in the hippocampal CA1 region. We demonstrated for the first time the activation and distribution of MAPKs after transient forebrain ischemia in gerbil hippocampus. Moreover, inhibitors of p38 and ERK were used to confirm the involvement of these kinases on DND in the CA1 region.
MATERIALS AND METHODS
Induction of global ischemia. Adult male Mongolian gerbils (Shimizu Laboratory Supplies Co. Ltd., Kyoto, Japan) weighing 60-80 gm were used. They were kept in a temperature-controlled (23 ± 1°C) and light/dark cycle-controlled animal room (lights on at 8 A.M., off at 8 P.M.).
Animals were deprived of food overnight before the induction of ischemia to exclude the influence of hyperglycemia on ischemic brain damage (Pulsinelli et al., 1982
Pretreatment with SB203580 and PD98059. To examine the effect of SB203580 (Calbiochem, La Jolla, CA), a p38 inhibitor (Lee et al., 1994
To examine the effect of PD98059 (Calbiochem), an ERK kinase 1/2 (MEK1/2) inhibitor (Pang et al., 1995
Tissue and sample preparation. For Western blot analysis of the total amounts of JNK, p38, and ERK in hippocampus, the gerbils were killed 0, 15, and 30 min and 2, 6, 24, and 72 hr after ischemia. For immunoblotting of the active forms of JNK, p38, and ERK, the gerbils were killed 0 and 30 min after ischemia and 30 min after sham operation (each n = 3). The whole hippocampus was rapidly excised and frozen in liquid nitrogen.
For immunohistochemical study, 0, 15, and 30 min and 2, 6, 18, 24, 48, and 72 hr (each n = 3) after reperfusion, the animals were killed and perfused transcardially with a buffer (0.1 M PBS, pH 7.4, and 0.2 mM sodium orthovanadate) followed by 4% buffered paraformaldehyde. To examine the effects of SB203580 (0, 1, 10, and 100 µM) on phosphorylation of p38, ATF-2, and JNK and PD98059 (0, 3, 30, and 300 µM) on phosphorylation of ERK after ischemia, gerbils (n = 3 for each dose) were perfused as described earlier at 0 and 15 min after ischemia. The brains were rapidly removed and cryoprotected in 25% sucrose in 0.1 M PBS overnight at 4°C.
Antibodies. Anti-JNK1 (FL) antibody, anti-p38 (c-20) antibody, anti-ERK2 (c-14) antibody, anti-phosphorylated ATF-2 (p-ATF-2) (F-1) antibody (Santa Cruz Biotechnologies, Santa Cruz, CA) and antibodies for the active forms of (anti-ACTIVE) JNK, p38, and MAPK (ERK; Promega, Madison, WI) were used in the present study. Anti-ACTIVE JNK polyclonal antibody recognizes the dually phosphorylated JNK2 enzyme but also reacts with the dually phosphorylated JNK1 enzyme. Anti-ACTIVE ERK polyclonal antibody recognizes the dually phosphorylated ERK2 enzyme.
Absorption test. The specificity of the antibodies against JNK1, p38, and ERK2 (Santa Cruz) were verified using whole-brain homogenate of gerbils and rats as control (male SD rats weighing 280-320 gm; Shimizu Laboratory Supplies). The absorption test was performed using the antibodies against p38 and ERK2 incubated 30 min at 37°C with 0, 1, 10, 100, and 1000 times molar concentration of p38 and ERK2, respectively. The procedure of electrophoresis and immunoblotting was then performed in the same way as described in the next section. With regard to JNK1, an absorption test was not able to be performed because a control peptide of JNK1 was not available (Santa Cruz).
The antibodies recognized JNK1, p38, and ERK2 and each band corresponding to the JNK1, p38, and ERK2 molecular weight in the gerbil brain homogenate, respectively. The antibodies against JNK1 and ERK2 also recognized the bands corresponding to JNK2 and ERK1, respectively. The absorption test showed that no bands corresponding to p38 and ERK2 were demonstrated when the antibodies were preincubated with 1 and 1000 times molar concentrations of the antigens, respectively (data not shown).
The antibodies against active forms of JNK, p38, and ERK (Promega) were raised against a dually phosphorylated peptide sequence representing the catalytic core of the active JNK, p38, and ERK enzymes, respectively. The phosphorylated amino acid residues correspond to Thr-183 and Tyr-185 of these enzymes in mammalians. Because the rodents including gerbils and rats belong to the mammalians, these antibodies should recognize the homogenate of the gerbil brain (Walton et al., 1998
Western immunoblot analysis for JNK1, p38, and ERK2. For gel electrophoresis and Western blotting of JNK1, p38, and ERK2, the hippocampi were homogenized with 0.5 ml of ice-cold buffer containing 20 mM Tris-HCl, pH 7.5, 1 mM EDTA, 5 mM MgCl2, 1 mM DTT, 20 µg/ml aprotinin, and 1 mM phenylmethylsulfonyl fluoride (PMSF). Aliquots of total tissue homogenate were frozen and kept at
80°C. The protein content was determined using the method of Bradford (1976)
Western immunoblot analysis for ACTIVE JNK, p38, and ERK. For gel electrophoresis and Western blotting of active forms of JNK, p38, and ERK, the hippocampi were homogenized with 0.5 ml of ice-cold buffer containing 20 mM Tris-HCl, pH 7.5, 1 mM EDTA, 5 mM MgCl2, 1 mM DTT, 20 µg/ml aprotinin, 1 mM PMSF, and 2 mM sodium orthovanadate. After SDS-PAGE, blotting to PVDF membranes, and blocking overnight at 4°C with 5% skim milk, the membranes were incubated 2 hr at room temperature with the primary anti-rabbit polyclonal active forms of JNK, p38, and ERK (catalog #8031). Polyclonal anti-ACTIVE p38 antibody was used at a dilution of 1:1000; JNK and ERK were used at a dilution of 1:2000. After washing, the membranes were incubated for 1 hr at room temperature with secondary antibody (Donkey anti-rabbit IgG-alkaline phosphatase conjugate; Promega) diluted 1:10,000 for active forms of JNK and p38 and 1:5000 for ERK. The other procedure was performed as described above.
Measurement of the densities of the immunoblot bands. For quantitative analysis of the densities of the immunoblot bands (JNK1, p38, ERK2, p-JNK2, p-p38, and p-ERK2), the densities were measured by NIH Image analyzer 1.61 (Dr. Wayne Rasband, National Institutes of Health, Bethesda, MD). The data of the densities (JNK1, p38, and ERK2) were statistically analyzed by ANOVA followed by post hoc Bonferroni test between groups using Stat View II (Abacus Concepts, Berkeley, CA). Data are presented as mean ± SD, and when p < 0.05, differences were considered significant.
Immunohistochemistry. Frozen coronal sections (40 µm in thickness) of the brains were prepared using a microtome. For immunohistochemistry, antibodies against active forms of JNK, p38, and ERK (catalog #6671; Promega) were used. The sections were processed by the free-floating method. After washing three times in 0.1 M PBS, quenching endogenous peroxidase in 2% H2O2 in 60% methanol, and blocking with 5% goat serum, the sections were incubated overnight at 4°C with polyclonal antibodies against active forms of JNK, p38, and ERK. The sections were washed three times in 0.1 M PBS and incubated in biotinylated anti-rabbit IgG antibody (Vector Laboratories, Burlingame, CA) at a 1:200 dilution for 2 hr and in avidin-biotin complex (ABC kit; Vector) for 60 min. Peroxidase was demonstrated with a DAB substrate kit (Vector). Negative control sections received identical treatment except for the primary antibody. For evaluation of morphological change, adjacent sections were stained with cresyl violet. Each section was mounted on glass slides, air-dried, dehydrated in ascending ethanol series, immersed in xylene, and coverslipped with M·X (Matsunami Glass Industries, Ltd., Osaka, Japan).
Measurement of survival neurons in CA1 and CA3. To examine the effect of intraventricular administration of SB203580 30 min before the ischemia on the development of DND in CA1 and neuronal death in CA3, the animals were anesthetized with diethyl ether and perfused transcardially with a buffer (0.1 M PBS, pH 7.4, and 0.2 mM sodium orthovanadate) followed by 4% buffered paraformaldehyde 7 d after the operation. Twenty-one gerbils were used (n = 6, 5, 5, and 5 for vehicle and doses of 1, 10, and 100 µM, respectively). As for PD98059, 15 gerbils were used (n = 5, 5, and 5 for doses of 3, 30, and 300 µM, respectively). Frozen coronal sections (20 µm in thickness) of the brains were prepared (described earlier) and stained with cresyl violet.
The severity of neuronal damage in CA1 and CA3 regions was evaluated by the number of surviving neurons. The mean number of surviving neurons of the pyramidal cell layer per 450 µm length was calculated in the CA1 region for each group. In the CA3 region, the number of surviving neurons per 0.2 mm2 indicated by the rectangular fields in Figure 11 was calculated (see Fig. 11C). Cell counting was performed using the light microscope equipped with a 10× objective by independent observers in a blind manner (Tokime et al., 1996
Physiology. In randomly selected animals treated with 100 µM SB203580, 30 µM PD98059, or 1% DMSO (n = 4 in each group), arterial blood pressure was monitored by using an RMP-6004M transducer amplifier (Nihon Kohden, Tokyo, Japan) through a femoral artery catheterized with a PE-8 polyethylene tube. Arterial blood samples (50 µl) were collected through the tube and analyzed by using a blood gas-pH analyzer (Corning 248; Ciba-Corning Diagnostics, Tokyo, Japan). During the operation, and until animals became awake, a rectal temperature was maintained at 37-38°C with a thermoregulator (Animal Blanket Controller ATB-1100; Nihon Kohden) and a heating pad and lamp and did not change significantly during the operative procedure and postoperative period (~2 hr).
RESULTS
Total amounts of MAPKs were not changed after transient global ischemia
To determine whether the total amounts of JNK1, p38, and ERK2 were altered by ischemia, whole hippocampal extracts were subjected to Western analysis using the anti-JNK1, p38, and ERK2 antibodies. No significant changes in the amounts of JNK1 (Fig. 1A,B), p38 (Fig. 1A,C), and ERK2 (Fig. 1A,D) at each time point were observed after global ischemia compared with ischemic control animals (0 min; each n = 3).
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Figure 1. Total amounts of JNK, p38, and ERK were not changed after 5 min of transient forebrain ischemia. A, Western blotting of hippocampal homogenates of postischemic gerbils at 0 min (ischemic control, lane 1), 15 min (lane 2), 30 min (lane 3), 2 hr (lane 4), 6 hr (lane 5), 24 hr (lane 6), and 72 hr (lane 7) after 5 min of transient forebrain ischemia (top panel, JNK1; middle panel, p38; bottom panel, ERK2). B-D, Quantitative representation of immunoblots (mean ± SD) showing no significant change of total amounts of JNK1 (B), p38 (C), and ERK2 (D) in the hippocampal extracts.
These results indicate that the induction of immunoreactivities of active forms of JNK, p38, and ERK might not be attributable to the increase of total protein amounts.
MAPKs are activated after transient global ischemia
To determine whether the phosphorylated forms of JNK, p38, and ERK were altered by ischemia, whole hippocampal extracts were subjected to Western analysis using the antibodies against active forms of JNK, p38, and ERK. No activations of JNK, p38, and ERK were detected in sham-operated animals (Fig. 2, A, lane 1, B). Significant increases in the activities of JNK and p38 were observed 30 min after global ischemia (Fig. 2, A, lane 3, B) compared with the ischemic control animal (0 min; Fig. 2, A, lane 2, B). The activity of ERK was increased immediately after global ischemia (Fig. 2, A, lane 2, B, triangle) and slightly decreased 30 min of reperfusion (Fig. 2, A, lane 3, B, triangle). The data presented are representative of at least three separate experiments.
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Figure 2. Increased phosphorylation of JNK, p38, and ERK after 5 min of transient forebrain ischemia. A, Western immunoblots of hippocampal homogenates of sham-operated gerbils (lane 1) and postischemic gerbils at 0 min (lane 2) and 30 min (lane 3) after 5 min of transient forebrain ischemia (top panel, active JNK; middle panel, active p38; bottom panel, active ERK; p-, phosphorylated). B, Quantitative representation of immunoblots showing activation of JNK1 and p38 30 min after ischemia and ERK2 immediately after ischemia in the hippocampal extracts. The data presented are representative of at least three separate experiments.
These results indicate that transient global ischemia induced the activations of JNK, p38, and ERK.
DND occurs after transient global ischemia
Cresyl violet staining demonstrated that only a few neurons showed ischemic changes, such as pyknosis and cell shrinkage, in the hippocampal CA1 region after 24 hr of reperfusion (Fig. 3C). At 72 hr of reperfusion, almost all neurons showed ischemic changes in the CA1 region (Fig. 3E). After 7 d of reperfusion, almost all neurons died in the CA1 subfield (Fig. 3G).
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Figure 3. Nissl staining after transient global ischemia. Cresyl violet staining in CA1 (A, C, E, G) and CA3 (B, D, F, H) of the hippocampus is shown. Almost all neurons were preserved in the hippocampal CA1 region 24 hr after reperfusion (C). At 72 hr of reperfusion, almost all neurons showed ischemic changes in the CA1 region (E). Almost all neurons died in the CA1 region 7 d after the ischemia (G). A, B, 5 min of ischemia; C, D, 5 min of ischemia followed by reperfusion for 24 hr; E, F, 5 min of ischemia followed by reperfusion for 72 hr; G, H, 5 min of ischemia followed by reperfusion for 7 d. Scale bar, 100 µm.
In the CA3 region, no remarkable ischemic change was observed after transient global ischemia (Fig. 3B,D,F,H).
Immunolocalization for active JNK and p38 after transient global ischemia
Few neurons in the hippocampus showed immunoreactivity for active JNK and p38 in sham-operated animals (results not shown) and immediately after the ischemia (Figs. 4, 5A,B). After 15 min of reperfusion, active JNK, and p38 immunoreactivities were enhanced in neurons in CA1 (Figs. 4, 5C) and CA3 (Figs. 4, 5D). After 6 hr of reperfusion, active JNK and p38 immunoreactivities reduced in CA1 (Figs. 4, 5E), and the immunoreactivities almost disappeared after 18 hr of reperfusion (Figs. 4, 5G). In the CA3 region, the immunoreactivities were intensely enhanced after 6 hr of reperfusion (Figs. 4, 5F), and then the immunoreactivities reduced (Figs. 4, 5H) but were continuously observed up to 72 hr of reperfusion (results not shown).
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Figure 4. Phosphorylated JNK in CA1 and CA3 after ischemia. Immunohistochemical staining for the active form of JNK in CA1 (A, C, E, G) and CA3 (B, D, F, H) of the hippocampus is shown. The photographs represent 0 min (A, B), 15 min (C, D), 6 hr (E, F), and 18 hr (G, H) after 5 min of transient forebrain ischemia. Scale bar, 100 µm.
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Figure 5. Phosphorylated p38 in CA1 and CA3 after ischemia. Immunohistochemical staining for the active form of p38 in CA1 (A, C, E, G) and CA3 (B, D, F, H) of the hippocampus is shown. The photographs represent 0 min (A, B), 15 min (C, D), 6 hr (E, F), and 18 hr (G, H) after 5 min of transient forebrain ischemia. Scale bar, 100 µm.
Immunolocalization for active ERK after transient global ischemia
Few neurons in the hippocampus showed immunoreactivity for active ERK in sham-operated animals (Fig. 6A). Immediately after transient global ischemia, active ERK immunoreactivity was detected in CA3 fibers (Fig. 6B). After 15 min, active ERK immunoreactivity was enhanced in dentate gyrus (Fig. 6C,D) but not in the CA3 region (Fig. 6C). After 30 min, the immunoreactivity reduced in dentate gyrus (Fig. 6E). After 48 hr, no immunoreactivity for active ERK was detected in all hippocampal regions including dentate gyrus (results not shown). In subiculum, there were a few neurons that showed only faint ERK-positive stainings at 30 min after the ischemia (Fig. 6G). In the CA1 region, immunoreactivity for active ERK was never detected after global ischemia (Fig. 6F).
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Figure 6. Phosphorylated ERK in hippocampus after ischemia. Immunohistochemical staining for the active form of ERK in whole hippocampus (A-C), dentate gyrus (D, E), CA1 (F), and subiculum (G) of the hippocampus is shown. The photographs represent sham-operated gerbil (A) and 0 min (B), 15 min (C, D), and 30 min (E-G) after 5 min of transient forebrain ischemia. Scale bars: A-C, 1 mm; D, E, 100 µm; F, G, 400 µm.
Although the activity of ERK was moderately detected 30 min after the transient forebrain ischemia in immunoblot analysis (Fig. 2C), immunoreactivity for active ERK reduced in dentate gyrus at the same time point (Fig. 6E). The discrepancy might be attributable to the differences of sensitivities of the antibodies (catalog #6671 and #8031) or to the inclusion of whole hippocampal tissues in samples for Western blot analysis.
Effect of SB203580 on activation of p38, ATF-2, and JNK
Few neurons showed immunoreactivity for active p-ATF-2 in sham-operated animals (Fig. 7A). Consistent with the activation of the p38 signaling cascade, an increase in phosphorylated ATF-2 levels was observed 15 min after global ischemia in the CA1 region (Fig. 7B). Intraventricular administration of SB203580 (0, 1, 10, and 100 µM) 30 min before the ischemic insult could not reduce the immunoreactivity for active p38 15 min after ischemia (results not shown) but reduced the immunoreactivity for p-ATF-2, a substrate of p38 (Fig. 7C), because SB203580 is not able to inhibit the phosphorylation of p38 but inhibits the activity of the phosphorylated form of p38 (Larsen et al., 1997
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Figure 7. Representative photomicrographs of immunohistochemical study for phospho-ATF-2 in CA1 of the hippocampus of sham-operated animals (A) and at 15 min after ischemic insult in animals that received intraventricular injection of vehicle (B) and 100 µM SB203580 (C) 30 min before ischemic insult. Intraventricular injection of SB203580 reduced the immunoreactivity 15 min after global ischemia (B). Scale bar, 100 µm.
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Figure 8. Representative photomicrographs of immunohistochemical study for active JNK in CA1 of the hippocampus 15 min after ischemic insult in animals that received intraventricular injection of vehicle (A) and 100 µM SB203580 (B) 30 min before ischemic insult. Intraventricular injection of SB203580 moderately reduced the immunoreactivity 15 min after global ischemia (B). Scale bar, 100 µm.
Effect of PD98059 on activation of ERK
Intraventricular administration of PD98059 (0, 3, 30, and 300 µM) 30 min before the ischemic insult reduced the immunoreactivity for active ERK immediately after ischemia in a dose-dependent manner; the maximum reduction of the immunoreactivity for active ERK was obtained with a dose of 30 µM (Fig. 9B). Concerning p38- or JNK-dependent cascades, PD98059 could not reduce the activation of p38, ATF-2, and JNK in the immunohistochemical study (results not shown).
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Figure 9. Representative photomicrographs of immunohistochemical study for active ERK in whole hippocampus immediately after ischemic insult in animals that received intraventricular injection of vehicle (A) and 30 µM PD98059 (B) 30 min before ischemic insult. In animals that received vehicle, immunoreactivity of the active form of ERK was the same as in animals that received only ischemic insult (A). Intraventricular injection of PD98059 markedly reduced the immunoreactivity (B). Scale bar, 1 mm.
SB203580, a p38 inhibitor, is neuroprotective, resulting in a decrease in DND
In the sham-operated group, no significant neuronal damage was detected. The mean number of surviving neurons in the CA1 region was 126.3 ± 5.5 (n = 6). Intraventricular administration of SB203580 (0, 1, 10, and 100 µM) 30 min before the ischemic insult significantly reduced DND in the hippocampal CA1 region 7 d after the ischemia in a dose-dependent manner, and the maximum effect was obtained at a dose of 100 µM (Figs. 10G, 11A). We tested
300 µM doses of SB203580, but the protective effect was not increased significantly in our preliminary data. In the CA3 region, no significant effects in survival were observed (Fig. 11B). Rectal temperature was not significantly different between groups during the operative procedure and the postoperative period (data not shown).
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Figure 10. Photomicrographs of Nissl staining of the hippocampus after SB203580 treatment. Cresyl violet staining in CA1 (A, C, E, G) and CA3 (B, D, F, H) of the hippocampus after transient forebrain ischemia is shown. Almost all neurons died in the hippocampal CA1 region pretreated with 1% DMSO (A) and 1 µM SB203580 (C). When pretreated with 10 µM (E) and 100 µM (G) SB203580, more than half of the neurons survived in the CA1 region after forebrain ischemia. A, B, Pretreated with 1% DMSO; C, D, pretreated with 1 µM SB203580; E, F, pretreated with 10 µM SB203580; G, H, pretreated with 100 µM SB203580. Scale bar, 100 µm.
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Figure 11. Effects of SB203580 and PD98059 on neuronal death in CA1 and CA3 regions. Numbers of survival neurons in CA1 (A) and CA3 (B) regions of the hippocampus after SB203580 and PD98059 treatments at various doses are shown. SB203580 showed neuroprotective effects in a dose-dependent manner in the CA1 subfield (A). Neuroprotective effects with 10 and 100 µM SB203580 were significant compared with vehicle (1% DMSO) (*p < 0.0001). PD98059 showed no neuroprotective effects in the CA1 region (A). In the CA3 region, both drugs showed no significant effects on neuronal survival (B). Cell count in the CA3 subfield was done in the squares indicated in the diagram (C).
PD98059, a MEK1/2 inhibitor, is not neuroprotective on neuronal death in CA1 and CA3
Intraventricular administration of PD98059 (0, 3, 30, and 300 µM) 30 min before the ischemic insult could not significantly reduce DND in the hippocampal CA1 region 7 d after the ischemia (Fig. 11A). In the CA3 region, no significant effects in survival were observed (Fig. 11B). Rectal temperature was also not significantly different between groups during the operative procedure and the postoperative period (data not shown).
SB203580 and PD98059 do not alter respiratory and cardiovascular parameters and body temperatures
SB203580 and PD98059 did not affect respiratory and cardiovascular parameters or produce hypothermia. Mean arterial blood pressure, arterial gas analysis (PCO2, PO2, and pH), blood glucose, and body temperature were not significantly affected by the presence or absence of 100 µM SB203580 or 30 µM PD98059 5 min before the ischemia (Table 1).
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Table 1. Physiological parameters before transient global ischemia under halothane anesthesia
DISCUSSION
Transient forebrain ischemia causes DND in the CA1 region of hippocampus in gerbil (Kirino, 1982
In response to extracellular stimulation such as growth factors (Boulton et al., 1991
Unlike ERK, JNK and p38 are not associated with mitogenesis or differentiation (Cano and Mahadevan, 1995
The role of JNK and p38 in neuronal death is also still controversial. Xia et al. (1995)
Several in vivo studies have been recently reported regarding the participation of the MAPK cascade in brain ischemia (Hu and Wieloch, 1994
In the present study, we demonstrated that the activation of JNK and p38 was induced 15 min after global ischemia in CA1 and CA3 and gradually reduced in CA1 but was continuously observed in CA3 at 72 hr of reperfusion. The decrease in immunoreactivities of JNK and p38 preceded histological changes in CA1. The activation of ERK was mainly transient in CA3 fibers and dentate gyrus. We speculate that transient activation of JNK and p38 in CA1 may be harmful effects on survival of CA1 neurons from ischemic cell death. The activation of ERK might not be significantly related to the determination of the fate of neurons to live or die, because the immunoreactivity was detected mainly temporarily in CA3 and dentate gyrus and was never detected in the CA1 region.
To evaluate the significance of the activation of p38 in transient forebrain ischemia, we tested the effect of SB203580, a p38 inhibitor, on DND in the CA1 region of hippocampus. Intraventricular administration of SB203580 (10 or 100 µM) 30 min before ischemic insult significantly reduced DND in the CA1 region. Kawasaki et al. (1997)
To evaluate the significance of the activation of ERK in transient forebrain ischemia, we tested the effect of PD98059, a MEK1/2 inhibitor, on DND in the CA1 region. Intraventricular administration of PD98059 30 min before ischemic insult could not ameliorate DND in the CA1 region. We suggested that this enzyme may not participate in gerbil hippocampal neuronal survival after brain ischemia, because the inhibition of ERK by PD98059 in the CA3 region did not affect the neuronal survival. Alessandrini et al. (1999)
In the CA3 region, no significant neuronal death was observed in the presence or absence of SB203580 or PD98059 after ischemia. We suggest that there might be a selective vulnerability of the CA1 region to active p38 that might not be present in the CA3 region. We also speculate that different upstream or downstream cascades of MAP kinases might be activated in CA1 and CA3 after ischemia in gerbil brain.
Up to now, a specific inhibitor of JNK has not been available (Maroney et al., 1998
The present study demonstrated for the first time that JNK, p38, and ERK were activated in gerbil hippocampus after transient forebrain ischemia in vivo, that the activation of JNK and p38 in CA1 neurons after ischemia was seen earlier than previously reported (Walton et al., 1998
In conclusion, JNK, p38, and ERK were activated after transient forebrain ischemia in gerbil hippocampus in vivo. We suggest that p38 may play an important role in hippocampal neuronal survival and death during brain ischemia. Components of the pathway are important target molecules in elucidating the mechanism of ischemic neuronal death.
FOOTNOTES Received Oct. 1, 1999; revised March 20, 2000; accepted April 7, 2000.
Correspondence should be addressed to Dr. Kazuhiko Nozaki, Department of Neurosurgery, Graduate School of Medicine, Kyoto University, 54 Kawahara-cho, Shogoin, Sakyo-ku, Kyoto 606-8507, Japan. E-mail: noz{at}kuhp.kyoto-u.ac.jp.
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