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Article |
Identification of prothymosin-
1, the necrosis–apoptosis switch molecule in cortical neuronal cultures
Correspondence to Hiroshi Ueda: ueda{at}nagasaki-u.ac.jp
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We initially identified a nuclear protein, prothymosin-
1 (ProT), as a key protein inhibiting necrosis by subjecting conditioned media from serum-free cultures of cortical neurons to a few chromatography steps. ProT inhibited necrosis of cultured neurons by preventing rapid loss of cellular adenosine triphosphate levels by reversing the decreased membrane localization of glucose transporters but caused apoptosis through up-regulation of proapoptotic Bcl2-family proteins. The apoptosis caused by ProT was further inhibited by growth factors, including brain-derived neurotrophic factor. The ProT-induced cell death mode switch from necrosis to apoptosis was also reproduced in experimental ischemia-reperfusion culture experiments, although the apoptosis level was markedly reduced, possibly because of the presence of growth factors in the reperfused serum. Knock down of PKCßII expression prevented this cell death mode switch. Collectively, these results suggest that ProT is an extracellular signal protein that acts as a cell death mode switch and could be a promising candidate for preventing brain strokes with the help of known apoptosis inhibitors.
, prothymosin-1.
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Introduction |
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We recently demonstrated that cultured cortical neurons die by necrosis under low-density (LD) and starvation stress without serum or any supplements (Fujita et al., 2001; Fujita and Ueda, 2003a,b). Of particular interest are the findings that neuronal death in high-density (HD) cultures is markedly inhibited and that addition of conditioned medium (CM) from HD cultures prevents necrosis in LD cultures (Fujita and Ueda, 2003b). Here, we report the identification of a CM molecule, prothymosin-1 (ProT), that mediates necrosis inhibition and note the clinical potential of this protein to prevent brain strokes.
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Results |
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20-kD protein was obtained by molecular weight cutoff ultrafiltration, ion-exchange filtration, and SDS-PAGE from 20 ml of the CM (Fig. 1 d–f; and Table S1, available at http://www.jcb.org/cgi/content/full/jcb.200608022/DC1). After SDS-PAGE, this 20-kD protein was analyzed by matrix-assisted laser desorption/ionization–time of flight (MALDI-TOF) mass spectrometry (MS), and a search in the nonredundant National Center for Biotechnology Information protein database for matching peptide mass fingerprints revealed 17 peptides that were unique to rat ProT. Moreover, tandem MS analysis confirmed that the N terminus of purified ProT was an acetylated serine (129.612 vs. Ser 87.343 m/z; Fig. 1 g), in agreement with a previous report (Pineiro et al., 2000).
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IgG, which had already been characterized (Figs. S1 and S2, available at http://www.jcb.org/cgi/content/full/jcb.200608022/DC1). When CM factors were applied to anti-ProT IgG-conjugated beads, the eluates obtained from acid-treated beads exhibited a single band that corresponded to recombinant ProT on SDS-PAGE and an "acidic blot," with no substantial signal in the flow-through, whereas the ProT signal was observed in the flow-through from preimmune IgG-conjugated beads, but not in the control eluates (Fig. 2 a).
After pretreatment of the CM with anti-ProT IgG-conjugated beads, but not preimmune IgG-conjugated beads, 80% of the original CM-induced survival activity was lost (Fig. 2 b). Thus, it is evident that a large proportion of the survival activity in the CM can be attributed to the action of ProT.
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was extracted from the CM by acid phenol (Fig. S1 and supplemental text), subjected to SDS-PAGE, and directly detected by the highly sensitive blue stain method without a blotting procedure, as transfer of ProT to a blotting membrane is unstable because of its acidity. ProT was detected in the CM as early as 1 h after the onset of serum-free culture, and the level was maintained for up to 12 h, whereas the intracellular ProT level was reduced (Fig. 2 c). The amount of ProT in the CM of HD culture (72 h) was determined to be 66 pmol/cm2. This release into the CM was observed in serum-free, but not in serum-containing (serum-plus), cultures. Because cortical neurons showed no substantial plasma membrane damage at 12 h after the start of serum-free HD culture in terms of PI staining or transmision EM analysis (Fujita and Ueda, 2003a,b), the ProT in the CM is likely to have been released from neurons whose membranes have not yet been disrupted. ProT lacking a signal peptide sequence is probably released in a nonvesicular manner (unpublished data), as seen in the case of FGF-1 (LaVallee et al., 1998; Matsunaga and Ueda, 2006). When anti-ProT IgG was simply added to HD cultures, a concentration-dependent decrease in the survival activity was observed, despite no extra incubation for immunoabsorption (Fig. 2 d). This finding provides strong evidence that ProT released under serum-free stress plays a substantial neuroprotective role.
ProT purified to homogeneity exhibited a concentration dependency equivalent to that of the recombinant protein and had a maximum survival activity in LD cultures that was equal to that in HD cultures (Fig. 2 e). Furthermore, addition of ProT mutants that lacked the N-terminal region (
1–29), including thymosin-1 (Pineiro et al., 2000), or the C-terminal region (102–112), including the nuclear localization signal TKKQKK, retained the original activity of ProT. As the culture plates were precoated with ProT in the aforementioned experiments, the site of ProT action seems to be through unidentified cell surface membrane targets, but not through thymosin-1 receptors or nuclear binding sites. In this experiment, the survival activities of ProT were equivalent when the same amount of protein (25 pmol/cm2) was used to precoat culture plates or added directly to cultures (initial medium concentration: 80 nM; Fig. 2 f).
Recombinant ProT reversed the rapid decrease in survival activity in cortical neurons caused by the serum-free or permanent ischemia model (Fig. 3 a).
The addition of ProT abolished all the typical necrotic features, such as disrupted plasma membranes and swollen mitochondria, but no damage to the nucleus, at 6 h in the transmission EM analysis, and instead caused apoptosis, as observed by nuclear fragmentation, at 12 h (Fig. 3 b). A similar cell death mode switch from necrosis to apoptosis was observed by pretreatment with CM factors (20%) derived from HD cultures, whereas treatment with 1 µg/ml anti-ProT IgG inhibited the cell death mode switch (Fig. 3 b). When the cell death mode was evaluated by double staining with necrosis (PI) and apoptosis (annexin V, caspase-3, and TUNEL) markers, 69, 86, and 92% of neurons, respectively, died by necrosis under serum-free stress, whereas only 15, 22, and 5% of neurons, respectively, died by apoptosis (Fig. 3 c). Addition of ProT or CM totally switched the cell death mode from necrosis to apoptosis, and the CM-induced changes were abolished by further addition of anti-ProT IgG. These findings suggest that the cell death mode switch induced by CM factors is largely attributable to the action of ProT. A pharmacological study using various inhibitors revealed that the survival activity of recombinant ProT was mediated through activation of PLC and PKC (Fig. 3 d), consistent with a previous report regarding CM factors (Fujita and Ueda, 2003b). In the present study, we used 1 µM U73122, a PLC inhibitor, and GF109203X, a pan-type PKC inhibitor. These findings were supported by a biochemical study, in which addition of ProT significantly increased the PKC activity and the effect was reversed by U73122 (Fig. 3 e). This survival activity at 12 h was inhibited by Go6976, a PKC/ß inhibitor, but not by HBDDE, a PKC/
inhibitor, or Rottlerin, a PKC/
/
inhibitor (Fig. 3 d). Therefore, the PKCß isoform is likely to be involved.
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-induced survival activity was observed after 12 h of serum-free culture, but not at 24 h (Fig. 4 a).
However, more potent and long-lasting survival activity was observed in the low-oxygen and low-glucose (LOG) ischemia and reperfusion model. It should be noted that no change in the survival activity was observed between 24 and 48 h in the latter condition. The incidence of apoptosis in ProT-treated samples was markedly lower in the latter reperfusion model (38.4 ± 6.16%; n = 4) than in the serum-free model (86.0 ± 8.25%; n = 6), suggesting that this difference could be attributed to the action of antiapoptotic serum factors. This view was clearly confirmed when antiapoptotic growth factors and ProT were added to the serum-free culture (Fig. 4 b). At 48 h after the start of serum-free culture, the survival activity was as low as 5%, even in the presence of ProT alone. However, further addition of NGF, brain-derived neurotrophic factor (BDNF), basic FGF, or interleukin-6 rescued the survival activity to >80% of the control level, whereas these factors alone had no effects on the survival. There was no mitochondrial cytochrome c (cyto c) release, which induces apoptosis through the formation of the apoptosome with Apaf- 1 and caspase-9, whereas addition of ProT caused cyto c release (Fig. 4 c). It should be noted that ProT-induced cyto c release was abolished by further addition of BDNF or BIP-V5, which blocks the translocation of Bax to mitochondria (Yoshida et al., 2004), but not by zVAD-fmk, a pan-type caspase inhibitor.
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and BDNF, zVAD-fmk, or BIP-V5. The addition of ProT alone inhibited necrosis throughout 48 h and increased the number of living cells (or necrosis, apoptosis double negative) more prominently at the early stage (12 h), but not at the later stage (24 or 48 h). On the contrary, the number of cells showing apoptosis time-dependently increased in the presence of ProT. Further addition of BDNF or BIP-V5 showed complete survival by inhibiting apoptosis throughout 48 h. However, zVAD-fmk caused a marked cell death by necrosis at the later stage, though it showed complete survival at the early stage.
It is generally accepted that necrosis is caused by energy failure because of the loss of cellular ATP (Eguchi et al., 1997; Fujita and Ueda, 2003a,b; Zong and Thompson, 2006). The cellular ATP levels of cortical neurons rapidly decreased immediately after the start of serum-free culture (Fig. 5 a).
This decrease was markedly inhibited by the addition of ProT or CM, and further addition of anti-ProT IgG abolished the CM effects. As previously reported (Fujita and Ueda, 2003b), this rapid decrease and its reversal by ProT seem to be parallel to the activity of glucose transport, as [3H]-2-DG uptake was markedly decreased by serum-free treatment and reversed by ProT (Fig. 5 b). Similar changes were also observed in the ischemia-reperfusion model of culture (Fig. 5 c). Addition of ProT reversed the rapid decrease in the cellular ATP levels of cortical neurons after LOG ischemic stress and reperfusion with serum-containing medium (Ueda and Fujita, 2004). We previously revealed that the membrane translocation of the glucose transporters GLUT1 and -4 is largely inhibited in serum-free cultures of cortical neurons, which leads to necrotic cell death (Fujita and Ueda, 2003a). In the present study, inhibition of GLUT1 and -4 membrane translocation was also observed under LOG stress by immunocytochemistry (Fig. 5 d). Biochemical evidence was also found when the cell surface proteins were biotinylated before Western blot analysis (Fig. 5 e).
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activated PKC, -ßI, and -ßII at 10 min (Fig. 5, f and g). A knockdown study using antisense oligodeoxynucleotides (AS-ODNs) for these kinases demonstrated that only PKCßII, not PKC or -ßI, plays roles in the ProT-induced GLUT1/4 translocation (Fig. 5, h and i). Further characterization revealed that ProT induced GLUT1/4 translocation by activation of PLC through pertussis toxin–sensitive Gi/o, but not Gq/11, suggesting that a putative Gi/o-coupled ProT receptor may be involved in this action. Furthermore, the PKCßII AS- ODN treatment reversed the ProT-induced necrotic PI staining (Fig. 5 j).
The molecular machineries for apoptosis are relatively better characterized than those for necrosis. In terms of the activation of various caspases, caspase-3 is believed to be the final execution molecule for apoptotic cell death linked to DNA breakdown and nuclear fragmentation (Ferri and Kroemer, 2001; Danial and Korsmeyer, 2004). ProT activated caspase-3 in the serum-free or permanent ischemia model (Fig. 6 a).
Similar activation was also observed for caspase-9, but not for caspase-8 or -12. These findings suggest that ProT causes apoptosis through a caspase-9–mediated mitochondrial pathway. This view was clearly confirmed by the findings that ProT increased the expression of proapoptotic Bax and Bim, but slightly decreased the expression of antiapoptotic Bcl-2 and -xL, which regulate mitochondrial apoptotic signaling (Fig. 6 b). On the other hand, the PKCßII AS-ODN also reversed the ProT-induced proapoptotic Bax expression in the LOG stress model (Fig. 6 c). However, it should be noted that the Bax expression was also abolished by treatment with the AS-ODN for PKCß1, but not that for PKC.
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-induced apoptosis, we performed the experiments using siRNA in the LOG ischemic stress and reperfusion model. As shown in Fig. 6 d, the ProT treatment markedly up-regulated the Bax expression in all cells. The pretreatment of Bax siRNA 24 h before ProT treatment caused a complete loss of Bax in 10–18% of total cells, and these Bax-negative cells did not show any apoptotic active caspase-3 or necrotic PI staining. This finding was also confirmed by the quantification of incidence of apoptotic, necrotic, and living cells in experiments without and with Bax siRNA treatment. As mentioned in Fig. 3 (b and c), the ProT treatment alone abolished the necrosis, whereas it increased the survival with some apoptosis (Fig. 6 e, left). A similar cell death ratio was observed in Bax-positive cells, which are unlikely to be transfected with siRNA. However, Bax-negative cells were all alive, or apoptosis and necrosis negative. However, the down-regulation of Bim showed less significant changes in the number of cells showing apoptosis (Fig. S4, available at http://www.jcb.org/cgi/content/full/jcb.200608022/DC1). These results strongly suggest that ProT causes apoptosis through an up-regulation of Bax. |
Discussion |
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is a highly acidic nuclear protein of the -thymosin family and is widely distributed throughout the body (Haritos et al., 1985; Clinton et al., 1991). It is generally thought to be an oncoprotein that is correlated with cell proliferation by sequestering anticoactivator, a repressor of estrogen receptor activity, in various cells (Martini et al., 2000; Bianco and Montano, 2002). On the other hand, ProT has also been reported to act as an extracellular signaling molecule, as observed in the activation of macrophages, natural killer cells, and lymphokine-activated killer cells, and in the production of interleukin-2 and TNF- (Pineiro et al., 2000). Here, we isolated ProT from CM of primary cultures of cortical neurons as a molecule providing protection against neuronal necrosis (Fujita and Ueda, 2003b). By using a specific antibody, ProT was proven to be the major CM factor involved in density-dependent survival under conditions of serum-starvation stress.
The identity of the target of ProT in respect to cell death regulation is a very interesting issue. ProT was reported to inhibit apoptosome formation in NIH3T3 cells (Jiang et al., 2003). This observation is in good contrast with the present finding that addition of ProT to neuronal cultures caused apoptosis, suggesting that ProT has opposite functions inside and outside of the cell. Furthermore, as a ProT deletion mutant lacking the nuclear localization signal retained the full survival activity, it is unlikely to be the aforementioned genomic action. The most probable candidate would be a cell surface receptor. Indeed, the presence of a cell surface ProT receptor has been reported in lymphoid cells (Pineiro et al., 2001; Salgado et al., 2005), and we confirmed this in cortical neurons by using ProT–Alexa 488 (Fig. S5, available at http://www.jcb.org/cgi/content/full/jcb.200608022/DC1). Further strong evidence to support the presence of a cell surface ProT receptor is the fact that ProT-induced membrane transport of GLUT1/4 was mediated through a Gi/o-coupled receptor, which activated PLC and PKCßII. Because ProT-induced translocation of PKCßII was observed within 10 min, it is evident that this signaling can be attributed to a direct action through a membrane receptor.
The distinctive advantage of ProT-induced neuroprotection can be attributed to the inhibition of necrosis. Necrosis is characterized by bioenergetics failure and rapid loss of plasma membrane integrity, which may result from decreased glucose transport (Fujita and Ueda, 2003a), as well as enzymatic destruction of cofactors required for ATP production, increased mitochondrial reactive oxygen species production, and channel-mediated calcium uptake (Nordberg and Arner, 2001; Xiong et al., 2004; Zong and Thompson, 2006). In our serum-free or LOG stress model, most cortical neurons died by necrosis. We found that rapid cell death or necrosis was accompanied by decreased glucose uptake and cellular ATP levels. The glucose transport mechanism is one of the most important sets of molecules for maintaining cell survival. Various species of GLUT have been identified in different cell types (McEwen and Reagan, 2004). Because GLUT3, which is most abundant in neurons, is constitutively localized in membranes, its function is unlikely to be regulated by environmental factors. In contrast, it was reported that some survival factors induce translocation of GLUT1 and -4 into plasma membranes through activation of protein kinases, including AKT and PKCs (Perrini et al., 2004; Ishiki and Klip, 2005; Welsh et al., 2005). This is consistent with our previous study showing that serum-free stress reduces GLUT1/4 translocation (Fujita and Ueda, 2003a). Here, we successfully demonstrated that ProT prevented the stress-induced reduction of GLUT1/4 transport through PKCßII activation.
The second important issue is that ProT switches the cell death mode by causing apoptosis. Because serum-free stress alone did not cause mitochondrial cyto c release, this stress by itself is unlikely to induce the machinery for apoptosis as well as that for necrosis. This view is supported by our previous report that addition of pyruvate to serum-free cultures to maintain the cellular ATP levels prevented necrosis but did not induce apoptosis (Fujita and Ueda, 2003a). Although the possibility still remains that pyruvate has an unidentified mechanism to remove the trigger for apoptosis, it is very likely that apoptosis does not always occur after the prevention of necrosis. This finding strongly supports the view that ProT induces apoptosis. In the present study, we have demonstrated that ProT up-regulates proapoptotic Bax and Bim, and down-regulates antiapoptotic Bcl-2 and -xL. Because the treatment with Bax siRNA blocked the ProT-induced apoptosis, and the treatment with BIP-V5 blocked the ProT-induced cyto c release and apoptosis, it is evident that the up-regulation of Bax plays an important role in ProT-induced apoptosis. On the other hand, the caspase inhibitor zVAD-fmk blocked the ProT-induced apoptosis and caused necrosis. This may be explained by the view that the up-regulation of Bax by ProT causes a cyto c depletion from mitochondria, followed by the necrosis induction through a damage of mitochondrial ATP production (Chipuk et al., 2006; Malhi and Gores, 2006), as apoptosis is inhibited by zVAD-fmk.
ProT-induced up-regulation of Bax was found to be mediated by PKCßI and -ßII activation, consistent with previous reports that PKCß activates the I-
B kinase complex, IKK (Mattson and Camandola, 2001; Herrmann et al., 2005), leading to NF-B activation followed by Bax up-regulation. Thus, PKCßII is likely to be an important switch molecule to determine the cell death mode. The lack of contribution of PKCß1 to the ProT-induced necrosis inhibition may be related to the deficiency of the membrane-anchoring C-terminal peptide of PKCßII (Ono et al., 1986).
By use of acid-phenol extraction and blue staining, the amount of ProT in the CM was determined to be 66 pmol/cm2. The data of Fig. 2 c revealed that CM amounts are 50% of the total (CM + cells) at 6–12 h after the start of serum-free HD culture. As this value in CM (30 pmol/cm2 of ProT) corresponds to the concentration of ProT (25 pmol/cm2) required to make the conversion of necrosis to apoptosis, this mechanism seems to be physiologically relevant.
The possible in vivo roles of ProT in brain stroke represent the most important issue to be discussed. ProT inhibits the rapid cell death of neurons after serum-free ischemic stress by inhibiting necrosis. This property seems to be beneficial, as the representative growth factors used in the present study had no effects on the necrosis, although they have potent antiapoptosis activities. Furthermore, ProT is a unique cell death regulatory molecule in that it converts the intractable cell death necrosis into the controllable apoptosis. Because this apoptosis would be inhibited by growth factors secreted upon ischemic stress, it is expected that ProT may have neuroprotective roles in brain stroke. As mentioned in Fig. 4 (b–d), the combined use of ProT with growth factors, but not caspase inhibitors, may have a potential clinical availability. In conclusion, we have identified the survival factor secreted from cortical cultures as the nuclear protein ProT. We have also demonstrated that this protein plays an in vivo neuroprotective role in brain ischemic events. Moreover, it has the potential for clinical use against brain strokes.
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Materials and methods |
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, -ßI, -ßII, -, -
, and - (all from Santa Cruz Biotechnology, Inc.); activated caspase-3 and phosphorylated PKC
(Cell Signaling); and cyto c (BD Biosciences). The reagents for staining were PI (Sigma-Aldrich), TUNEL, Hoechst 33342 (Invitrogen), and Gelcode blue stain reagent (Pierce Chemical Co.).
Purification of ProT
After several trials, we optimized our procedures for purifying ProT. Purification was started with 20 ml CM, which had been collected at 72 h after the start of HD culture, as previously reported (Fujita and Ueda, 2003b). The CM was first subjected to ultrafiltration (Vivaspin 2; Sartorius KK), and the active materials observed in the >5-kD fraction were applied to an ion-exchange membrane spin column (Vivapure Q Mini; Sartorius KK), which had been equilibrated with 20 mM sodium acetate, pH 5.2. The sample was eluted with different concentrations of NaCl (0.2–1 M), and the active fraction was finally separated by SDS-PAGE and stained with Gelcode blue stain. The appropriate band was excised from the gel, washed with 50 mM NH4HCO3 and 50% acetonitrile, and incubated with 100% acetonitrile for 10 min. The gel segment was rehydrated in 50 mM NH4HCO3 and then dehydrated in 100% acetonitrile. The resulting gel plug was incubated overnight with 5 ng/µl trypsin in 25 mM NH4HCO3. The digested peptide mixture was diluted with the matrix 4-hydroxy--cyanocinnamic acid (HCCA) in 1:1 acetonitrile/0.1% TFA (vol/vol), deposited on a target, and dried to allow MALDI-TOF MS analysis (Bruker Daltonik).
Preparation and detection of recombinant proteins
Purification of recombinant rat ProT was performed as described previously (Evstafieva et al., 1995). This procedure using acid phenol was also available for simple purification of endogenous ProT for SDS-PAGE analysis. In the recombinant protein preparation, the genes for ProT and its deletion mutants (1–29 and 102–112) were first amplified from cDNAs derived from rat embryonic brain using specific primers (rat and mouse 5'-primer, 5'-AACATATGTCAGACGCGGCAGTGGA-3'; rat 3'-primer, 5'-AAGGATCCAGTGGAGGGTGAATAGGTCAC-3'; rat 1–29 5'-primer, 5'-AAGAATTCGGAAGAGACGCACCTGCC-3'; rat 3'-primer, 5'-GAGTCGACCTAGTCATCCTCATCAGTCTTC-3'; rat 102–112 5'-primer, 5'-AAGAATTCATGTCAGACGCGGCAGTG-3'; rat 3'-primer, 5'-GAGTCGACCTACTCAACATCATCATCCTCATC-3'). The PCR products were cloned into pGEM-T Easy and subcloned into pET16b. BL21 (DE3) cells were transformed with pET16b-ProT. Recombinant rat ProT and its derivatives were induced by 0.1 mM IPTG, purified (Biophoresis; ATTO), and dialyzed against PBS for later use. Recombinant and endogenous ProT isolated by the acid-phenol extraction procedure were detected as described previously (Evstafieva et al., 1995).
Primary culture
Primary culture of the cerebral cortex from 17 d of embryonic rats was performed according to the previously reported protocol (Fujita et al., 2001; Fujita and Ueda, 2003b). They were seeded onto 96-well culture dishes, 8-well Lab-Tek chambers (Nunc), and 3.5- and 9.0-cm culture dishes that had been all coated with poly-DL-ornithine (Sigma-Aldrich) and cultured in DME/F-12 medium at 37°C in 5%-CO2 atmosphere. For ProT coating, recombinant ProT was added to culture dishes and incubated for 2 h at 25°C. The dishes were washed twice with PBS for immediate use.
In vitro ischemia-reperfusion stress model
Primary cultures of 17-d-old embryonic rat cerebral cortex were prepared as described previously (Fujita and Ueda, 2003b). After being cultured for 3 d, cortical neurons were washed twice with glucose-free balanced salt solution (BSS; 116 mM NaCl, 5.4 mM KCl, 1.8 mM CaCl2, 0.8 mM MgSO4, and 1 mM NaH2PO4, pH 7.3), which had been deaerated using a vacuum. After replacement of the BSS with fresh BSS containing 1 mM glucose, neurons were exposed to hypoxia (<0.4% O2, 5% CO2, and 95% N2) for 2 h at 37°C in a commercially available culture incubator (Nuair). After the ischemic stress, the culture medium was exchanged for fresh DME/F-15 medium (1:1) containing 5% horse serum and 5% FBS, and the neurons were further incubated for the indicated periods in a 5% CO2 atmosphere (reperfusion).
Characterization of the modes of cell death
Survival activity was determined by the WST-8 reduction assay throughout the experiments. The modes of cell death were determined by various means, including PI staining, activated caspase-3, GLUT1, GLUT4, TUNEL, ATP measurement, and scanning and transmission EM analyses, as previously reported (Fujita et al., 2001; Fujita and Ueda, 2003a,b). In the GLUT translocation analyses, the cortical neurons were biotinylated (Pierce Chemical Co.), lysed, immunoprecipitated with streptavidin-conjugated beads, and subjected to Western blot analysis. Characterization of the modes of cell death and the immunocytochemistry analysis are described in the supplemental text.
Immunocytochemistry and immunoblot analysis for PKCs
Cortical cells on 8-well Lab-Tek chamber slides were fixed with 4% PFA in PBS for 30 min at 25°C, followed by permeabilization with 50 and 100% methanol for 5 min each at 25°C. The cells were then rinsed twice with PBS and preincubated in blocking buffer (2% BSA with 0.1% Tween 20 in PBS) for 1 h at 25°C. Next, the cells were incubated with each primary antibodies in blocking buffer overnight at 4°C, rinsed with PBS, and incubated with FITC-conjugated anti-rabbit IgG (1:200; Santa Cruz Biotechnology, Inc.) or FITC-conjugated anti-goat IgG (1:200; Rockland) for 2 h at 25°C. The immunolabeled cells were mounted with Permafluor (Thermo Scientific). For imaging cells, a laser-scanning confocal microscope imaging system consisting of a microscope (Axiovert 200 M; Carl Zeiss MicroImaging, Inc.) and a scan module (LSM 510 META and LSM 5 PASCAL; Carl Zeiss MicroImaging, Inc.) with image browser software (Carl Zeiss MicroImaging, Inc.) were used at ambient temperature, equipped with 40x/1.3 and 63x/1.4 oil-immersion lens and nonimaging photodetection device (photomultiplier tube; Carl Zeiss MicroImaging, Inc.). The imaging medium used was immersion oil (Immersol 518; Carl Zeiss MicroImaging, Inc.). A dynamic range adjustment was used to optimize the signal for the fluorophores, and images were collected in multitrack mode (Carl Zeiss MicroImaging, Inc.). Any brightness and contrast adjustments were performed in Photoshop (Adobe).
Western blot analysis
SDS-PAGE using 10–15% polyacrylamide gels and immunoblot analyses were performed as described previously (Fujita and Ueda, 2003a). The primary antibodies were an anti-phosphorylated PKC antibody, anti-PKC antibody, rabbit anti-PKCßI antibody, and rabbit anti-PKCßII antibody (1:1,000; Santa Cruz Biotechnology, Inc.). Visualization of immunoreactive bands was performed using an enhanced chemiluminescent substrate (Super Signaling Substrate; Pierce Chemical Co.) for HRP detection.
AS-ODN treatments
To determine the activation of various PKC isoforms and G protein in the mechanism of GLUT translocation, cultures were grown in the presence of AS-ODNs for PKC, PKCßI, PKCßII, or Gq/11. The AS-ODNs were diluted in water to a concentration of 20 µM and added to the cultures at a final volume of 1/50 of the culture medium every 12 h after seeding for 3 d. In parallel, some cultures were treated with the corresponding missense ODNs containing the same bases as the AS-ODNs but in a random order. None of the ODNs resembled any other sequences in the GenBank database. Using Western blot and immunocytochemical analyses, we demonstrated that treatment of cortical neurons in culture with these AS-ODNs, but not the missense ODNs, reduced the levels of the target proteins. The probes had the following sequences: PKC AS-ODN, 5'-CGGGTAAACGTCAGC-3' (Fleming et al., 1998); PKCßI AS-ODN, 5'-GTTTTAAGCATTTCG-3'; PKCßII AS-ODN, 5'-GTTGGAGGTGTCTCT-3'; PKCßII missense ODN, 5'-ACGAGCCCGAACCACCGT-3' (Simpson et al., 1998); and Gq/11 AS-ODN, 5'-ATGGACTCCAGAGT-3' (Mizota et al., 2005). All the ODNs were purchased from QIAGEN.
Bax and Bim gene silencing by siRNA
Bax and Bim siRNA constructs were purchased from Ambion (siRNA ID 49750 and 47149). Gene silencing was attained by transfection of siRNA into cells using Lipofectamine 2000 transfection reagent (Invitrogen) according to the manufacturer's instructions. The gene silencing was verified by detecting protein with immunocytochemical analysis 48 h after the transfection of primary cortical neurons with siRNA. In brief, cells (1 x 105 cells/cm2) grown in an 8-well Lab-Tek chamber slide were transiently transfected with 50 nM siRNA using 20 µl/ml Lipofectamine 2000 in a total transfection volume of 0.2 ml DME (Invitrogen). After incubation at 37°C in 5% CO2 for 6 h, the medium was replaced by fresh serum–containing medium. 2 d after the incubation, treated neurons were used for the characterization of cell death modes, as described.
Statistical analysis
Multiple comparisons of analysis of variance followed by t test were used for statistical analysis of the data. The criterion of significance was set at P < 0.05. All the results are expressed as the mean ± SEM.
Online supplemental material
The supplemental text contains additional methodological details on characterization of anti-ProT IgG used, as well as protocols used for cell survival activity, intracellular ATP levels, [3H]-2-DG uptake, PKC kinase assay, and immunostaining protocol. Table S1 shows a summary of the procedures for purifying ProT from CM. Fig. S1 shows a characterization of anti-ProT IgG. Fig. S2 shows an evaluation of membrane localization of GLUT1/4 by fluorescence imaging. Fig. S3 shows specific down-regulation of Gq/11 and PKC isoforms by treatment with AS-ODNs. Fig. S4 shows immunostaining of ProT-induced apoptosis under the Bim siRNA–treated LOG stress condition. Fig. S5 shows ProT–Alexa 488 binding to cell membranes. Online supplemental material is available at http://www.jcb.org/cgi/content/full/jcb.200608022/DC1.
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Acknowledgments |
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antibody preparation; and N. Takayama, W. Hamabe, and N. Kiguchi for technical assistance. Parts of this study were supported by grants-in-aid and special coordination funds from the Ministry of Education, Culture, Sports, Science and Technology.
Submitted: 4 August 2006
Accepted: 6 February 2007
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References |
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