From the Department of Animal Biology and the Mari Lowe Center for Comparative Oncology, School of Veterinary Medicine, University of Pennsylvania, Philadelphia, Pennsylvania 19104
Received for publication, February 20, 2003
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ABSTRACT |
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INTRODUCTION |
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Mitochondria play a crucial role in maintaining the metabolic homeostasis and are important regulators of cell death (11). The mitochondrial electron transport chain accounts for nearly 90% of the molecular O2 consumed by cells and tissues. ROS are generated as undesirable side products of the energy yielding oxidative metabolism, leading to mitochondrial and cellular damages (11). Detoxification of intracellular ROS is catalyzed by antioxidant molecules such as vitamin E and GSH as well as a number of enzyme systems, including superoxide dismutase, catalase, GSH peroxidase, and GST. Recently, it has been shown that transfection with GSTA4-4 cDNA protects cells against oxidative stress and HNE-induced apoptosis (12). Although mitochondria have enzyme systems to regulate ROS produced in the electron transfer chain (13), induced ROS production under various pathophysiological conditions can be overwhelming, leading to mitochondrial DNA and membrane damages. Regulation of ROS by intramitochondrial GSH and GSH-metabolizing enzymes would therefore be critical for maintaining the antioxidant potential and structural/functional integrity of the mitochondrial membrane.
A majority of GSTs in mammalian cells are localized in the cytosol, where they exist as homodimers or heterodimers of subunits with molecular masses from 24 to 29 kDa (14). However, GSTs have also been reported in microsomes (15, 16), nucleus (17), plasma membrane (18), and mitochondria (19, 20, 21, 22). Various subcellular locations of GSTs are consistent with their role in protecting cell components against chemical and oxidative damage. Recently, we showed the presence of three different forms of GSTs belonging to the alpha and mu family, namely, GSTA1-1, A4-4 and M1-1 in mouse liver mitochondria (22). We have also provided evidence that the mitochondrial GSTA4-4 level markedly increases in COS cells under oxidative stress conditions, suggesting its critical role in maintaining the GSH homeostasis under conditions of chemical and oxidative stress (21, 22).
In the present study, we have investigated the mechanism of targeting of recombinant mouse GSTA4-4 to mitochondria. Using in vivo and in vitro systems, we show that the mitochondrial targeting is highly dependent on the intact C-terminal end as well as the phosphorylation status of the protein. Translocation of GSTA4-4 is vastly increased under increased intracellular PKA and PKC activities. Results suggest that phosphorylation increases the affinity of the protein for binding to cytoplasmic chaperone, Hsp70, as a possible basis for its enhanced mitochondrial targeting.
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EXPERIMENTAL PROCEDURES |
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Construction of Wild Type and Mutant cDNA Constructs and Fusions with DHFRFull-length mouse GSTA4-4 cDNA was generated by reverse transcriptase-based PCR, using RNA extracted from mouse liver (25). N- and C-terminal deletions containing a start codon preceded by a Kozak consensus sequence were constructed essentially as described before (26). Mutant GSTA4-4 cDNA constructs with substitutions at the phosphorylation site and C-terminal-positively charged residues were constructed using a QuikChange site-directed mutagenesis kit supplied by Stratagene. These included T113A (Mut 113), T130A (Mut 130), S189A/T193A (Mut 189/193), and mutations at the C-terminal signal domain R217A/K221A (Mut RK/AA). The 172222 sequence of GSTA4-4 was fused to the C terminus of mouse DHFR by in-frame ligation of DNA through an EcoRI linker as described before (27). The cDNAs were engineered to contain 5' XbaI and 3' Hind III restriction sites and cloned in pCMV4 and pGEM7zf (Promega Biotech, Madison, WI) vectors, for cell transfection and in vitro translation studies, respectively.
In Vitro Translation and Phosphorylation of GSTA4-4 In vitro translation of mouse GSTA4-4 cDNA was performed in WGL or RRL systems (Promega Biotech, Madison, WI) in the presence of added [35S]Met (40 µCi/50-µl reaction, PerkinElmer Life Sciences, Boston, MA) as described before (26). In some experiments, GSTA4-4 translation product was phosphorylated either by PKA or PKC. PKA-dependent phosphorylation was performed for 45 min at 30 °C in Mg(CH3COO)2 acetate buffer (pH 6.5) by adding 10 units of PKA and 100 µM ATP to the translation mix as described (28). PKC-dependent phosphorylation of GSTA4-4 was carried out for 45 min at 30 °C in 50 mM MES buffer (pH 6) containing 1 mM EGTA, 10 mM MgCl2, 10 units of PKC, and 100 µM ATP as recommended by the manufacturer (Calbiochem, San Diego, CA). In some cases, translation products were generated in the WGL in the absence of [35S]Met, and phosphorylation was carried out in the presence of [32P]ATP.
In Vitro Import of GSTA4-4 into MitochondriaMitochondria were isolated from rat liver and used for in vitro import using a system described before (26). The import assays (containing 80,000 cpm of 35S-labeled GSTA4-4) were carried out in a 200-µl final volume and treated with 0300 µg/ml trypsin for 20 min on ice, as described before (26). Trypsin-treated samples were mixed with a 10-times excess of trypsin inhibitor, and mitochondria were recovered by sedimentation through 1 M sucrose. Untreated samples were diluted with mitochondrial isolation buffer and similarly banded through sucrose 1 M sucrose. Resulting mitochondrial pellets were washed twice with mitochondrial isolation buffer, and mitochondrial proteins were solubilized in 2x Laemmli buffer for 10 min at 75 °C and analyzed by SDS-PAGE (29) and fluorography.
Expression of GSTA4-4 cDNA in COS Cells and Isolation of Subcellular FractionsCOS-7 cells were grown in Dulbecco's modified Eagle's medium to 50% confluency and GSTA4-4 cDNA cloned in pCMV4 vector was transfected using FuGENE, a non-liposomal transfection reagent (Roche Applied Science, Molecular Biochemicals, Indianapolis, IN) as described before (30). After 48 h of transfection, cells from six to eight plates (100 mm) were homogenized in sucrose-mannitol buffer containing protease inhibitor mixture with a Teflon-fitted glass homogenizer (about 25 strokes). Mitochondria were isolated by differential centrifugation and sucrose density banding as described before (26). The post-mitochondrial supernatant was centrifuged for 1 h at 100,000 x g, and the cytosolic fraction was recovered in the supernatant.
ImmunoprecipitationMitochondria and cytosol (100 µg each) from GSTA4-4-transfected COS cells were solubilized in 250 µl of phosphate-buffered saline containing 0.1% Triton X-100 and protease inhibitors. The 15,000 x g supernatant fraction was incubated with rabbit polyclonal GSTA4-4 antibody (5 µg of IgG) overnight at 4 °C. 30 µl of protein A-agarose beads was added to the sample and shaken for 3 h at room temperature. Beads were pelleted by centrifugation and washed three times with phosphate-buffered saline containing 0.05% Triton X-100 and protease inhibitors. Immunoprecipitated proteins were eluted from the protein A-agarose beads by heating at 95 °C for 5 min in 30 µl of 2x Laemmli buffer without added -mercaptoethanol and analyzed by immunoblot using phosphoserine, phosphothreonine, and GSTA4-4 antibodies.
SDS-PAGE and Immunoblot AnalysisProteins were resolved by SDS-PAGE (29) and transferred to a nitrocellulose membrane for immunoblot analysis as described previously (31). Immunoblots were developed with a chemiluminescence Super Signal Ultra kit (Pierce Chemical Co., Rockford, IL). Imaging and quantitation were performed using a Fluor-S imaging system (Bio-Rad, Hercules, CA).
GST ActivityGST activity in the COS cell mitochondrial and cytosolic extracts was assayed using CDNB and HNE as substrates following the procedures of Habig et al. (32) and Alin et al. (33), respectively.
Depletion of Hsp70 from WGLGSTA4-4 was translated in the WGL as described above, and 25 µl of the translation mix was incubated for 30 min at room temperature with 25 µl of 8 M urea in 50 mM Tris-HCl, pH 7.5, containing 0.1 mM EDTA. The mixture was dialyzed for 12 h against two changes of 20 mM Tris-HCl (pH 7.5) containing 1 mM MgCl2, 50 mM KCl, and 0.5 mM dithiothreitol. Monoclonal Hsp70 antibody (10 µg of IgG) was added and incubated overnight at 4 °C. The mixture was incubated for 3 h at room temperature with protein A-agarose beads under agitation, and the beads were removed by centrifugation. The supernatant was tested for Hsp70 content and used as a GSTA4-4 translation product devoid of Hsp70.
Co-immunoprecipitation of Hsp70 with GSTA4-4 GSTA4-4 protein was synthesized in the WGL in the absence or the presence of PKC inhibitors (6 µM H7 or 50 nM GF109203X) or PKA inhibitors (50 nM H89 or 50 nM MPI). Interaction of GSTA4-4 with Hsp70 from the WGL under these conditions was analyzed by co-immunoprecipitation. Reaction mixtures were immunoprecipitated with a polyclonal antibody to GSTA4-4 as described above and resolved by SDS-PAGE on a 12% gel. The proteins were transferred to a nitrocellulose membrane, and co-immunoprecipitated proteins were analyzed by fluorography and immunoblot analysis using mouse monoclonal antibody for Hsp70.
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RESULTS |
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The in vivo targeting of GSTA4-4 to mitochondria was investigated using COS cells transfected with GSTA4-4 cDNA (Fig. 1B). Mitochondria and cytosol were isolated from cells transfected with the vector alone (mock) or with GSTA4-4 cDNA. Results show that both mitochondrial and cytoplasmic fractions from mock transfected cells contain endogenous, albeit low levels, of GSTA4-4, which co-migrates with purified GSTA4-4. Mitochondrial and cytoplasmic fractions from transfected cells, however, contain 6- to 10-fold higher levels of antibody-reactive protein. Quantification of blots and calculations based on a 3:1 ratio of cytosolic and mitochondrial protein recovery from cell homogenates showed that the mitochondrial GSTA4-4 pool in transfected cells represents about 20% of that detected in total homogenates. To further confirm the intramitochondrial location of GSTA4-4 protein, freshly isolated mitochondrial particles and cytoplasmic proteins were subjected to limited treatment with trypsin. Results (Fig. 1B) show that mitochondria-associated GSTA4-4 was resistant to trypsin treatment, whereas the cytoplasmic protein was completely degraded under this treatment condition. Control experiments with antibodies to specific marker proteins also showed that the mitochondrial fraction contained mitochondrial inner membrane translocase protein TIM44 but lacked the detectable cytosolic protein -actin. The cytosolic fraction, on the other hand, lacked significant TIM44 protein but contained
-actin, suggesting the purity of subcellular fractions used.
Further proof for mitochondrial targeting of GSTA4-4 in transfected COS cells was sought by assaying the rates of CDNB and HNE conjugation to GSH (Fig. 1C). Cytosolic fractions from mock transfected cells yielded relatively higher activity (400 nmol/mg of protein/min) with CDNB, which is a broad range substrate for GSTs belonging to different subfamilies, and a low activity of about 30 nmol/min/mg of protein with HNE. The corresponding activities representing endogenous GST levels from the mitochondrial fraction were about one-half to one-third of those obtained with the cytosolic fraction. A nearly 2-fold higher activity with CDNB was observed in the mitochondrial and cytosolic fractions of cells transfected with GSTA4-4 cDNA as compared with corresponding fractions of mock transfected cells. The activity with HNE in the mitochondrial and cytosolic fractions of transfected cells was 6- to 8-fold of corresponding fractions from mock transfected cells. Consistent with the results of immunoblot analysis, the GST activity with HNE was generally higher with the cytosolic fraction than with the mitochondrial fraction.
Mitochondrial GSTA4-4 Is HyperphosphorylatedRecent studies in our laboratory showed that CYP enzymes belonging to family 2, which are predominantly microsomal, are also targeted to mitochondria and that the bimodal targeting of these proteins is modulated by PKA-dependent phosphorylation (30, 34). GSTA4-4 contains a number of consensus sites for both PKA- and PKC-mediated phosphorylation (see the schematic at the top of Fig. 2). As shown in Fig. 2A, nascent GSTA4-4 translated in WGL was efficiently phosphorylated by adding PKA and PKC. Phosphorylation was apparent both in the presence of added PKC along with PKA inhibitor H89, or PKA along with PKC inhibitor GF109203X. PKA and PKC inhibitors together markedly reduced the level of phosphorylation. We also investigated the steady-state levels of Ser and Thr phosphorylation of cytosolic and mitochondrial GSTA4-4. As shown in Fig. 2B, GSTA4-4 was immunoprecipitated from both cell fractions, and the immunoprecipitates were subjected to immunoblot analysis with monoclonal antibodies to Ser-phosphate and Thr-phosphate. Fig. 2B shows that nearly the same amounts of immunoprecipitated GSTA4-4 from mitochondria and cytosolic fractions (left-most panel) show vastly varying levels of phosphorylation. As seen from the middle and right-most panels, mitochondrial GSTA4-4 was more heavily phosphorylated both at the Ser and Thr residues as revealed by intense antibody-reactive bands. The cytosolic counterpart carries very low to negligible phosphorylation of Ser and Thr. These results clearly show that the mitochondrial GST is hyperphosphorylated.
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Role of Phosphorylation on Mitochondrial Targeting of GSTA4-4 The role of phosphorylation on mitochondrial targeting of GSTA4-4 was studied using in vitro and in vivo approaches. In the first approach, GSTA4-4 translated in WGL in the presence or absence of added PKA and PKC and, with or without added kinase inhibitors, was used for import in isolated rat liver mitochondria. Although not shown, none of the protein kinase inhibitors affected the translational efficiency of GSTA4-4 at the concentrations used. Results of in vitro import in Fig. 3A (lanes 1 and 2) show that translation products formed in the absence of added kinases or inhibitors bind to mitochondria efficiently (about 70% of input protein), although they were imported at a very low level (6% of input cpm). Addition of PKA (10 units) during translation caused a marked increase of in vitro import to about 40% of input protein as indicated by resistance to trypsin treatment (Fig. 3A, lanes 3 and 4). Addition of PKC also caused a marked increase in import to about 60% of input (Fig. 3A, lanes 5 and 6). Inhibitors of PKA, H89 (50 nM), and MPI (a myristoylated peptide inhibitor of PKA, 50 nM), both selectively abolished PKA-mediated increase of in vitro transport, without affecting PKC-mediated increase (Fig. 3, B and C, lanes 36). PKC-specific inhibitor, GF109203X (50 nM), on the other hand, selectively abolished the PKC-mediated increase of import without affecting the PKA-mediated increase (Fig. 3D, lanes 36). General protein kinase inhibitor H7 and a combination of GF109203X and MPI inhibited both PKC- and PKA-mediated mitochondrial import (Fig. 3, E and F, lanes 36). The PKA and PKC inhibitors as well as the general kinase inhibitor H7 inhibited both mitochondrial binding and import of GSTA4-4 synthesized in the control WGL system, suggesting that the low level of import seen in Fig. 3A (lane 2) may be due to a low level of endogenous kinases (Fig. 3, BF, lanes 1 and 2).
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The use of translation mix containing PKA or PKC in the in vitro import experiments in Fig. 3A above leaves open the possibility that phosphorylation of mitochondrial membrane proteins also contribute to the increased import. We carried out two types of experiments to test this possibility. In the first approach, the residual PKC and PKA activities at the end of post-translational phosphorylation were quenched by adding specific inhibitors, and the translation mix in the presence of inhibitors was used for in vitro import. As seen from Fig. 3G, control translation products without added kinase and kinase inhibitor (lanes 1 and 2) yielded a low level of transport. Translation products phosphorylated with PKA and its specific inhibitor H89 (lanes 3 and 4), PKC and its inhibitor GF109203X (lanes 5 and 6), or with both kinases and both inhibitors yielded nearly 5060% import. This same level of import was obtained when kinase reactions were not terminated (see Fig. 3A). In the second approach, control untreated mitochondria and those preincubated with H89 or GF109203X were used for protein import. As seen from Fig. 3H, the levels of import of control translation product or those phosphorylated with PKA or PKC had imported levels correspondingly similar in untreated mitochondria (Fig. 3, A and G). Additionally, PKA and PKC inhibitors did not affect the import of mitochondrial cytochrome oxidase subunit Vb, which contains a cleavable N-terminal targeting signal (results not shown). These results suggest that the increased import in post-translationally phosphorylated translation products is not due to indirect effects of kinases on mitochondrial translocase proteins.
The role of PKA- and PKC-dependent phosphorylation on in vivo targeting of GSTA4-4 to mitochondria was investigated using COS cells transfected with GSTA4-4 cDNA (Fig. 4). Cells were treated with PKA inducers or inhibitors (Fig. 4A) and harvested 48 h post-transfection, and the levels of GSTA4-4 in the subcellular fractions were determined by immunoblot analysis (Fig. 4A). As described before, the cell fractionation procedure yielded mitochondrial preparations with less than 1% extramitochondrial contamination as tested by marker enzyme assays (22, 30, 35). Addition of the cAMP analog, Bt2cAMP (10 µM), or cAMP inducer, forskolin (10 µM), increased the mitochondrial targeting of GSTA4-4 by 40 and 70%, respectively (Fig. 4A, left panel). The cytosolic GSTA4-4 pool under these conditions was reduced by 5060% (Fig. 4A, right panel). Addition of H89 (50 nM) or MPI (50 nM) decreased the mitochondrial GSTA4-4 level to that of control cells, whereas the level of cytosolic GSTA4-4 was increased markedly.
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We used the PKC inducer PMA to assess the effects of PKC on in vivo mitochondrial targeting of GSTA4-4. In all cases, cells were harvested 48 h post-transfection, and PMA (100 nM) was added 1, 3, or 24 h before harvesting. As shown in Fig. 4B, addition of PMA for 1 h caused a rapid increase of intramitochondrial GSTA4-4 with a corresponding decrease in the cytosolic fraction. At longer durations of 3 and 24 h, the mitochondrial GSTA4-4 content steadily declined with corresponding increases in the cytosolic GSTA4-4. These results suggest that PMA-mediated phosphorylation causes a rapid redistribution of cytosolic GSTA4-4 by channeling it to mitochondrial compartment. Consistent with this possibility, PKC-specific inhibitor GF109203X as well as general kinase inhibitor H7 mark-edly retarded the PMA-mediated increase in mitochondrial GSTA4-4 (Fig. 4B).
Localization of Mitochondrial Targeting Signal of GSTA4-4 at the C TerminusWith the goal of localizing the mitochondrial targeting signal of GSTA4-4, we generated deletion cDNA constructs, which express proteins lacking the first 19 amino acids at the N terminus (GSTNT) and 19 amino acids at the C terminus (GST
CT) of GSTA4-4. Both of these segments contain positively charged residues that are characteristics of mitochondrial-targeting signals (Fig. 5A). Wild type GSTA4-4 and the two deletion constructs were transfected in COS cells (Fig. 5B), and translation products were used for in vitro import assay (Fig. 5, B and C). Our results show that the N-terminal deletion had no effect on the mitochondrial targeting of the protein, whereas the C-terminal deletions inhibited it in vivo (Fig. 5B) as well as in vitro (Fig. 5C) transport, indicating that the targeting signal might reside at the C terminus of GSTA4-4. Interestingly, the N-terminal deletion was not recovered in the cytosolic compartment, suggesting that it may be unstable and/or degraded in the cytosol. Because positively charged residues at 217 and 221 are within the putative mitochondrial targeting signal region, we tested the double mutant of R217A/K221A (GSTRK/AA) protein in the in vitro transport assay. Fig. 5D shows that the GSTRK/AA mutant protein synthesized in the absence of kinases was imported very poorly. The proteins synthesized in the presence of PKA and PKC were imported at a slightly higher level of about 8%. This rate, however, is markedly lower than the 4050% import with WT protein (Fig. 3). The residual activity with the GSTRK/AA mutant may be a result of two additional positive residues at positions 204 and 205. The results of protein transport with deletion and point mutations show that the C-terminal 20-amino acid stretch functions as a cryptic mitochondrial targeting signal.
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Phosphorylation Sites of GSTA4-4 That Are Critical for Mitochondrial TargetingAs shown in Fig. 6A, the mouse GSTA4-4 contains five PKA and PKC target sites. Deletion studies shown in Fig. 5 (B and C) showed that the N-terminal 19-amino acid stretch of GSTA4-4 does not play a significant role in mitochondrial import suggesting that the PKA/PKC site at Ser-18 may not be important for mitochondrial transport. We therefore generated T113A and T130A (Mut113 and Mut130) and a double mutant of S189A and T193A (Mut189/193) constructs as shown in Fig. 6A. It is seen that the in vitro transport of both Mut113 and Mut130 proteins (Fig. 6B) exhibit PKA- and PKC-mediated increase in transport similar to the WT protein. Furthermore, PKA inhibitor, H89, and PKC inhibitor, GF190203X, inhibited the specific kinase-mediated increase of in vitro import. The double mutant Mut189/193, on the other hand, showed a vastly reduced mitochondrial binding and mitochondrial import. Post-translational incubation with PKA and PKC had no significant effect on the import of this protein. In support of our studies with CYP2B1 and CYP2E1 (30, 34), these results suggest that the PKA and PKC sites closest to the C-terminal targeting signal are important for mitochondrial targeting and that phosphorylation at these positions may have a role in the activation of cryptic signal.
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Phosphorylation Enables the Cryptic Mitochondrial Signal to Target Heterologous Proteins to MitochondriaTo further as-certain the mitochondrial targeting property of the C-terminal end of GSTA4-4 and the role of phosphorylation at the Ser-189 and Thr-193 sites, we generated fusion constructs with DHFR. The construct contained sequence 172222 of GSTA4-4, which includes the PKA and PKC phosphorylation sites, fused to DHFR (Fig. 7A). The second construct consisted of sequence 172222 of GSTA4-4 with mutated Ser-189 and Thr-193 residues fused to DHFR (Fig. 7A). Results of in vitro import in Fig. 7B show that the fusion construct DHFR-C50GST was imported at a high level of 5060% when phosphorylated with PKA or PKC. The fusion construct (DHFR-C50GST/Mut189, 193), carrying mutations at the phosphorylation sites, was imported poorly even when the protein was subjected to post-translational phosphorylation with PKA or PKC.
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The mitochondrial targeting of the fusion proteins under in vivo conditions was tested by expressing the proteins in COS cells by cDNA transfection and by probing the cell fractions with antibody to DHFR. Fig. 8A shows the immunoblot analysis of cytosolic and mitochondrial fractions with DHFR antibody from cells transfected with the DHFR-C50GST construct and treated with either inducers or inhibitors of cAMP. It is seen (upper panels) that the mitochondrial fusion protein content was increased 2- to 3-fold by Bt2cAMP and forskolin as compared with control cells and was reduced to near control cell level by H89 and MPI, known inhibitors of PKA. The cytoplasmic fraction (Fig. 8A, upper panel), on the other hand, showed a relatively high DHFR fusion protein level but markedly reduced levels in cells treated with Bt2cAMP and forskolin. Additionally, treatment with H89 and MPI reversed the PKA-mediated reduction of fusion protein in the cytoplasm. These results suggest that, similar to that observed with WT GSTA4-4, PKA and PKC treatment cause a reduction in the cytosolic fusion protein by increased targeting to mitochondria. However, there was no significant change in the level of mitochondrial TIM44 and cytoplasmic -actin used as loading controls. The fusion construct DHFR-C50GSTMut189/193, on the other hand, was not targeted to mitochondria in control cells as well as in cells treated with cAMP inducers and inhibitors. The level of this protein in the cytoplasm remained at relatively high and constant level under all the treatment conditions, suggesting that the protein does not respond to cellular PKA levels.
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Fig. 8B shows the effects of PKC inducers and inhibitors on the mitochondrial and cytoplasmic levels of the fusion proteins as well as DHFR-C50GST and its 189/193 mutant. The relative distribution under different treatment conditions is nearly similar to that with PKA inducers and inhibitors shown above. In confirmation with the results of in vitro transport in Fig. 7, these results show that the C-terminal 50-amino acid sequence of GSTA4-4, when fused in the same orientation as the parent GSTA4-4, not only directs the mitochondrial targeting of a heterologous protein DHFR but also imparts responsiveness to PKA and PKC.
Phosphorylated GSTA4-4 Exhibits a Higher Affinity for Binding to Cytosolic Hsp70 Binding of newly synthesized proteins to the cytoplasmic Hsp70 family chaperones is an important first step of mitochondrial targeting, which ensures efficient presentation of properly unfolded polypeptide to the mitochondrial translocase proteins (36). With the goal of understanding the role of phosphorylation on mitochondrial targeting, we investigated its role on GSTA4-4 binding to cytoplasmic Hsp70 proteins. We examined the role of Hsp70 at two different levels: 1) during the translation of GSTA4-4 protein and 2) post-translationally, during the import process. When GSTA4-4 was translated in WGL in the presence of a monoclonal antibody to Hsp70, the translation efficiency was reduced by 2- to 3-fold (Fig. 9A, lanes 1 and 2). In lanes 310 (Fig. 9A), we compared the rate of in vitro import of GSTA4-4 synthesized in the presence and absence of added antibody (80,000 cpm each). It is seen that addition of Hsp70 antibody to the translation mix strongly inhibited both binding and import of the protein, even when the protein was phosphorylated (Fig. 9A, lanes 9 and 10). Addition of mouse IgG affected neither the binding nor the import into mitochondria (not shown). The GSTA4-4 synthesized in the absence of added Hsp70 antibody was imported in a significant amount, and the import was further enhanced by PKA (Fig. 9A, lanes 36). Although not shown, complete depletion of Hsp70 from the WGL by immunoadsorption resulted in a vastly reduced GSTA4-4 translation, suggesting that Hsp70 is required for the synthesis and/or stabilization of GSTA4-4 protein.
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To understand the role of Hsp70 in the mitochondrial import of GSTA4-4, we carried out two types of experiments. In the first series, Hsp70 antibody was added to the WGL following complete synthesis of GSTA4-4 and just prior to the start of in vitro import reaction. Addition of antibody to translation products programmed in the absence (lanes 14) as well as presence of PKA (lanes 510) inhibited the in vitro import in a concentration-dependent manner (Fig. 9B), whereas mouse IgG had no effect (not shown). Although not shown, the import competence of GSTA4-4 was not restored by the addition of pure Hsp70 protein, probably due to excess of antibody present in the translation mixture. In the second series of experiments, therefore, the translation mixture was depleted of Hsp70 as well as the residual antibody by adsorption to protein A-Sepharose beads. To reduce the loss of GSTA4-4 bound to Hsp70 during immunodepletion, the translation mixture was subjected to urea treatment followed by dialysis before immunodepletion. Fig. 9C shows the immunoblot analysis of translation products in the presence of PKA at different steps of immunodepletion (left panel) and autoradiography of the same gel (right panel) to determine the levels of 35S-labeled GSTA4-4. As seen from Fig. 9C, immunodepleted lysate lacks detectable Hsp70 (left panel, lane 2) as compared with control lysate (left panel, lane 1). As expected, the protein adsorbed to the protein A-Sepharose beads contains Hsp70 (left panel, lane 3) and a number of unidentified proteins. The autoradiogram (Fig. 9C, right panel) shows that nearly 50% of GSTA4-4 was lost even when the lysate was subjected to urea treatment (lane 2), which was nearly quantitatively recovered in the protein A-Sepharose-bound fraction (lane 3). Fig. 9D shows the mitochondrial import of PKA-phosphorylated GSTA4-4 from control and Hsp70-depleted lysates. It is seen that control WGL supported both mitochondrial binding and import of GSTA4-4 efficiently (lanes 1 and 2). However, both mitochondrial binding and import of GSTA4-4 were drastically reduced with Hsp70-depleted lysate (lanes 3 and 4). Furthermore, addition of purified Hsp70 restored both binding and import, suggesting its direct role in the mitochondrial import of GSTA4-4 (lanes 5 and 6).
In the second series of experiments, we investigated the effect of phosphorylation on the affinity of GSTA4-4 for binding to Hsp70 protein. GSTA4-4 was translated and phosphorylated (PKA and PKC) in WGL in the absence or presence of specific inhibitors, and the in vitro translation products were immunoprecipitated with GSTA4-4 antibody. In some cases, the immunoprecipitation was carried out with pre-immune serum or antibody to -actin as negative controls. The immunoprecipitated proteins were resolved on SDS-polyacrylamide gels and transferred to nitrocellulose membrane. The blot was successively probed with a monoclonal antibody to Hsp70 protein (Fig. 10A, top panel) and subjected to autoradiography (Fig. 10A, bottom panel). The autoradiogram shows that almost the same amount of GSTA4-4 was immunoprecipitated in lysates with or without added inhibitors when GSTA4-4 antibody was used. Both pre-immune serum and antibody to
-actin failed to co-immunoprecipitate significant amount of Hsp70, suggesting the specificity of HSP 70 binding. The top panel shows the level of Hsp70 pulled down along with immunoprecipitated GSTA4-4 protein. The control reaction, without added inhibitor, shows a prominent Hsp70 protein band indicating physical interaction between the two proteins. The amount of Hsp70 in the immunoprecipitate was reduced by 4060% by added PKC (GF109203X) or PKA (MPI or H89) inhibitors. A drastic reduction in the level of Hsp70 was seen when either PKA and PKC inhibitors (MPI plus GF109203X) or when nonspecific H7 kinase inhibitor were added together during translation.
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The role of phosphorylation on binding to HSP was further verified using antibody pull-down with phosphorylation site mutant GSTA4-4 WT. As shown in Fig. 10B, WT GSTA4-4, Mut130, and Mut189/193 proteins were translated in the WGL system and phosphorylated post-translationally when both PKA and PKC were added. The translation mix was immunoprecipitated with Hsp70 antibody, and the immunoprecipitates were probed with Hsp70 antibody and GSTA4-4 antibody by immunoblot analysis. It is seen from Fig. 10B that in all three cases nearly similar amounts of Hsp70 protein were immunoprecipitated. However, the levels of GSTA4-4 protein varied markedly. Wild type and Mut130 proteins were co-immunoprecipitated at comparably high levels, whereas the Mut189/193 protein was co-immunoprecipitated at very low levels. These results provide confirmatory evidence that phosphorylation at Ser-189/Thr-193 is important for binding to Hsp70.
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DISCUSSION |
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Using in vitro and in vivo transport methods (Figs. 1 and 3), we have presented compelling evidence that GSTA4-4 localizes inside the mitochondrial membrane system particularly when cellular PKA or PKC activities are induced. We have used a series of approaches to dispel the possibility that GSTA4-4 associated with the mitochondrial fraction represents a cross-contaminant from the cytosolic fraction: 1) mitochondrial preparations were devoid of -actin, a cytosolic-specific marker but contained mitochondrial-specific membrane protein TIM44 and soluble matrix protein mtTFA, 2) cytosolic GSTA4-4 from transfected COS cells was readily degraded by limited digestion with trypsin, whereas mitochondrial associated GSTA4-4 was resistant to this treatment, and 3) immunohistochemical studies with transfected COS cells showed that a significant amount of immunostained GSTA4-4 was co-localized with punctate membrane structures that were also stained with antibody to mitochondrial genome encoded CytOX I protein (22). Furthermore, treatment with PMA, an inducer of PKC, or forskolin, an inducer of PKA, intensified the staining of punctate structures with GSTA4-4 antibody suggesting increased mitochondrial localization (not shown). Results of this study also suggest that full-length GSTA4-4 translocated to mitochondria is catalytically active as indicated by its ability to conjugate CDNB and HNE.
Mitochondrial compartment is an important subcellular site for ROS production as part of the electron transport chain coupled oxidative metabolism (38). We, as well as others, have shown the occurrence of GST isoforms in the hepatic and brain mitochondria. Our recent study showed that three of the mitochondrial GSTs exhibit size and sequence similar to those of the cytosolic GST counterparts, suggesting that the same primary translation product is translocated to mitochondria (22). In this study we investigated mechanisms of mitochondrial targeting of GSTs using GSTA4-4 as a model system. The choice of this form was based on its known physiological function in the metabolic detoxification of HNE and related end product of lipid peroxidation in human (39), rat (21), and mouse (22, 40). A recent study showed that cytosolic and mitochondrial isoenzymes of fumarase in yeast exhibit identical size and N-terminal sequence and are encoded by the same gene (41). Interestingly, the primary translation product of fumarase with N-terminal extension is first targeted to mitochondria, and following N-terminal processing by the matrix metalloprotease, part of the protein pool is shuttled back to the cytosol (41). However, currently there is no evidence for the expression of GSTs with N-terminal extensions (22). We therefore investigated the possibility of protein phosphorylation playing a role in mitochondrial targeting of GSTA4-4, by a mechanism similar to that shown for CYP2B1 and 2E1 (30, 34).
There is no well documented evidence either for the phosphorylation of any of the soluble GST isoforms, regulation of their expression, or modulation of activity by phosphorylation. However, GSTA4-4 (and other cytosolic GSTs) contains a number of consensus sites for both PKA and PKC (see Fig. 2). Results presented in this study show for the first time that GSTA4-4 is the target for both PKA- and PKC-mediated phosphorylation. Additionally, in both transfected COS cells and in mouse liver, the mitochondrial GSTA4-4 contains a high level of both Ser and Thr phosphorylation, whereas the cytosolic counterparts contained no detectable phosphorylation. These results suggest that phosphorylation plays a direct role in the distribution of soluble GST pool between the cytosolic and mitochondrial compartments. These results are consistent with our previous study showing an increase of mitochondrial GSTA4-4 and parallel decrease in the cytosolic compartment of COS cells subjected to oxidative stress by treatment with HNE or H2O2 (22). Both of these treatments are known to induce cellular PKC activity (42, 43, 44). Preliminary results on enzyme activity with different substrates show no detectable difference in the specific activities of enzymes from the mitochondrial and cytosolic GSTs, suggesting that phosphorylation may not be a major factor in their catalytic function. However, results of both in vitro import and in vivo transport in transfected COS cells clearly show that PKA- and PKC-mediated phosphorylation plays a direct role in mitochondrial translocation of the protein. Because mitochondria are the direct targets of chemical and oxidative stress conditions, which also induce cellular kinase activities (42, 43, 44), we postulate that phosphorylation induced mitochondrial translocation of GSTA4-4, and possibly other GSTs represent an important cellular defense system.
The cryptic mitochondrial targeting signals of CYP1A1, 2B1, and 2E1 have one common feature in that they precede the hydrophobic ER targeting/transmembrane anchor domains (26, 30, 34). The cryptic signals, however, vary markedly in terms of overall secondary structure and number as well as relative positions of positively charged residues that are critical for mitochondrial targeting. Both the N- and C-terminal 20- to 25-amino acid regions of GSTA4-4 show sequence properties reminiscent of the cryptic mitochondrial targeting sequences of CYPs with variable distribution of positive residues. Deletion studies, however, showed that the N-terminal 19 residues had no effect on the mitochondrial targeting under both in vitro and in vivo conditions, although deletion of the C-terminal 19 residues vastly reduced its mitochondrial entry, suggesting its role in mitochondrial targeting. Consistent with other cleaved and uncleaved mitochondrial targeting signals, the positively charged residues Arg-217 and Lys-221 of the cryptic C-terminal signal of GSTA4-4 are important for mitochondrial targeting of protein. Direct support for the mitochondrial targeting property of the C-terminal end of GSTA4-4 comes from experiments showing that the 50-amino acid sequence from the C terminus can drive the mitochondrial targeting of a cytosolic protein, DHFR.
Mutational analysis of putative phosphorylation sites (Fig. 5) showed that two closely located PKA and PKC target sites at Ser-189 and Thr-193 are critical for signal-mediated shuttling of cytosolic GSTA4-4 to the mitochondrial compartment. The concept of activation of cryptic signals for protein targeting is relatively new and emerged mainly from our studies on CYP2B1 and 2E1 targeting to mitochondria. The present results support and extend this concept, because both PKA- and PKC-dependent phosphorylation appears to activate the putative signal. Additionally, similar to that shown for CYPs, the overlapping PKA/PKC sites closest to the cryptic signal at the C-terminal most 20-amino acid region are important for activation and subsequent mitochondrial targeting of the protein. The precise mechanism by which phosphorylation activates the cryptic targeting signal remains unclear, although it may be associated with conformational changes in the protein as shown for CYP2B1 and 2E1 (30, 34).
The cytoplasmic Hsp70 and related chaperones are thought to play important roles in mitochondrial protein targeting, particularly in unfolding the newly synthesized protein in the cytosol, maintaining it in an import-competent state and presenting the protein to mitochondrial contact points (45, 46, 47). An important observation of the present study is that cytoplasmic Hsp70 is critical for both efficient translation of GSTA4-4 under in vitro conditions and for the mitochondrial import. Selective immunodepletion of WGL resulted in vastly reduced translation rates and in vitro mitochondrial import of both phosphorylated and non-phosphorylated GSTA4-4. Addition of purified Hsp70 fully restored the in vitro import competence of the protein further establishing its role in mitochondrial targeting of GSTA4-4. Our results are in general agreement with previous studies showing the requirement for Hsp70 for efficient translation of precursor protein and/or mitochondrial import under in vitro conditions (36, 37, 45, 48). We hypothesize that phosphorylation-induced conformational changes in GSTA4-4 increase its affinity for binding to Hsp70, which in turn helps present the protein to mitochondrial translocase complexes in an import-competent conformation. We also observed a major difference in the import competence of GSTA4-4 translated in the RRL and WGL, the former being an unsupportive system for in vitro transport of GSTA4-4. Interestingly, addition of 4 M urea to RRL-translated protein vastly increased the import competence (not shown). It is known that urea treatment and associated protein unfolding improve the import competence of some proteins (48, 49). Based on this we postulate that reticulocyte Hsp70 either binds to GSTA4-4 inefficiently or is unable to properly unfold the nascent chains, thus contributing to inefficient import of this protein.
In summary, we provide direct experimental evidence for the mitochondrial transport of GSTA4-4 and its organization in the mitochondrial matrix compartment in a catalytically active form. Our results demonstrate that phosphorylation of GSTA4-4 in the cytoplasmic compartment increases its affinity for binding to cytosolic Hsp70, which might be the basis for increased mitochondrial localization under increased cellular PKA and PKC activities. Based on these in vivo and in vitro results we present a model for GSTA4-4 targeting to mitochondria under different physiological conditions (Fig. 11). This study also sheds light on mechanisms by which mitochondrial GSTA4-4 is modulated under chemical or oxidative stress conditions.
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FOOTNOTES |
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These authors contributed equally to the work.
On leave from the Faculty of Medicine and Health Sciences, United Arab Emirates University, Al Ain, United Arab Emirates.
¶ To whom correspondence should be addressed. Tel.: 215-898-8819; Fax: 215-573-6810; E-mail: narayan{at}vet.upenn.edu.
1 The abbreviations used are: GST, glutathione S-transferase; CCCP, carbonyl cyanide-m-chlorophenylhydrazone; CDNB, 1-chloro-2,4-dinitrobenzene; CYP, cytochrome P450; Bt2cAMP, dibutyryl cAMP; GSH, glutathione; HNE, 4-hydroxynonenal; MPI, myristoylated peptide inhibitor; PMA, phorbol-12-myristate-13-acetate; PKA, protein kinase A; PKC, protein kinase C; ROS, reactive oxygen species; RRL, rabbit reticulocyte lysate; TIM, translocase of the inner mitochondrial membrane; WGL, wheat germ lysate; DHFR, dihydrofolate reductase; Hsp70, heat-shock protein 70; CMV, cytomegalovirus; MES, 4-morpholineethanesulfonic acid; MPI, myristoylated peptide inhibitor; WT, wild-type; ER, endoplasmic reticulum.
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ACKNOWLEDGMENTS |
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