Article |
Address correspondence to Peter Mundel, Division of Nephrology, Albert Einstein College of Medicine, 1300 Morris Park Ave., Bronx, NY 10461. Tel.: (718) 430-3219. Fax: (718) 430-8963. E-mail: mundel{at}aecom.yu.edu
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Abstract |
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Key Words: actin-binding protein; muscle differentiation; nuclear-cytoplasmic translocation; synaptopodin gene family; Z-disc
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Introduction |
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Although the Z-disc is generally viewed as the site where actin filaments from opposing half-sarcomeres are cross-linked by -actinin, it has become clear over the past years that more proteins are involved in the formation of the common structural unit of all Z-discs, the Z-unit. Most notably, the NH2 terminus of titin participates by providing binding sites for
-actinin (Ohtsuka et al., 1997; Sorimachi et al., 1997; Young et al., 1998) and T-cap/telethonin (for review see Gregorio et al., 1999). Further, nebulin (and nebulette in cardiac muscle; Moncman and Wang, 1995) also enters the Z-disc at its COOH terminus (Labeit and Kolmerer, 1995; Millevoi et al., 1998), it is possible that this polypeptide also provides attachment sites for
-actinin, actin, and perhaps titin. At the periphery of the Z-disc, interaction between actin and titin has been reported in cardiac muscle, thereby rendering this titin region functionally inextensible (Linke et al., 1997; Trombitas and Granzier, 1997). However, the peripheral Z-disc region of titin could well be complexed with F-actin by additional proteins. A potential candidate to form ternary complexes with actin and titin is myopodin, the second member of the synaptopodin gene family.
Synaptopodin is a proline-rich actin-associated protein, strongly expressed in differentiated kidney glomerular podocytes and telencephalic dendrites. Due to its high content of equally distributed proline residues, synaptopodin is a linear molecule without globular domains. In both brain and kidney, the gene expression is differentiation dependent (Mundel et al., 1997a). This is consistent with data obtained from cultured podocytes, in which synaptopodin expression occurs during differentiation and coincides with growth arrest and process formation (Mundel et al., 1997b). Database searches with the synaptopodin cDNA identified an expressed sequence tag (EST)* clone from human skeletal muscle that showed 50% homology in a region of 95 amino acids. Here, we describe the corresponding protein, which we termed myopodin. Evidence is provided that myopodin has actin-binding and -bundling activity and shuttles between the nucleus and the cytoplasm in a differentiation-dependent and stress-induced fashion. We also discuss the possible role of myopodin in the nucleus.
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Results |
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A single 3.6-kb myopodin mRNA encodes an 80-kD protein in skeletal muscle and a 95-kD protein in the heart
Northern blots were performed with 400 ng of polyA+ RNA from mouse skeletal and heart muscle. A strong band of 3.6 kD was detected in skeletal muscle and in the heart a somewhat weaker expression of the same band was seen (Fig. 2 a). Immunoblots of cytosolic extracts from mouse skeletal and heart muscle with antimyopodin antibody SRIB1 showed one band of 80 kD in skeletal muscle and one band of 95 kD in the heart, corresponding to myopodin (Fig. 2 b). The expression was stronger in skeletal muscle than in the heart. Since Northern blot analysis revealed only one message for both skeletal muscle and heart tissues (Fig. 2 a) the different molecular weight on protein level seems to be due to posttranslational modification. Similar findings have been described previously for synaptopodin (Mundel et al., 1997a). Preincubation with the SRIB1 peptide used for immunization blocked the immunoreaction, thereby showing the specificity of the myopodin bands (Fig. 2 b). Identical results were obtained with the myopodin-specific SRIB2 antibody (Fig. 2 b and unpublished data). Using the synaptopodin antibody NT, a major band of 110 kD was found in both tissues, which was clearly different from the myopodin band seen with SRIB1 and SRIB2. Similar to synaptopodin (Mundel et al., 1997a), myopodin is highly susceptible to proteolytic degradation. Several proteolytic myopodin fragments could be detected by Western blot analysis when extracts from muscle tissues where stored at -20°C instead of direct boiling in SDS sample buffer (unpublished data).
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Myopodin localizes to the Z-disc in mature striated muscle
To determine the intracellular distribution of myopodin, frozen tissue sections from skeletal and heart muscle were immunostained with SRIB1 and SRIB2. A striated pattern was observed in skeletal (Fig. 3 a) and heart muscle (Fig. 3 b). The localization of myopodin in the sarcomere was further analyzed in double labeling experiments with antibodies against titin (Fig. 3 c) and -actinin (Fig. 3 d). The epitope stained by the titin antibody BD6, which localizes to the AI junction (Whiting et al., 1989), flanked the myopodin epitope but did not overlap with it (Fig. 3 c). In contrast,
-actinin, which is a constituent of the Z-disc, completely overlapped with myopodin (Fig. 3 d), indicating that myopodin is localized in the Z-disc region. Preabsorption of both antisera with the corresponding peptides abrogated the immunolabeling, thereby proving the specificity of the Z-line staining (unpublished data). The association of myopodin with the Z-disc was confirmed by immunogold labeling. On ultra-thin frozen sections from stretched rat psoas muscle and heart, the electron-dense gold particles, representing sites of myopodin expression, were found at the center (Fig. 4 a) and periphery of the Z-disc (Fig. 4 b), but were absent from other parts of the sarcomere (Fig. 4 a). In the heart, myopodin was also detected at the Z-disc (Fig. 4 c). This staining pattern was comparable to that found for
-actinin, an established component of the Z-disc (unpublished data).
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Discussion |
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As described previously for synaptopodin (Mundel et al., 1997a), myopodin seems to be differentially modified in different tissues. Northern blot analysis revealed only one message of 3.6 kb in both heart and skeletal muscle (Fig. 2 a). However, by Western blot analysis, a protein of
80 kD was detected in skeletal muscle, whereas the corresponding protein in the heart had a size of
95 kD (Fig. 2 b). The cause of this size difference remains to be established, but for several reasons, it appears to be due to posttranslational modification(s). First, cDNA sequencing of mouse skeletal muscle and heart myopodin revealed identical results. Second, the same message could be detected in both heart and skeletal muscle (Fig. 2 a). Third, alternative splicing can be ruled out because myopodin is an intronless gene (unpublished data). Fourth, in vitro translation from the myopodin cDNA gives only one product of
80 kD (Fig. 6 a). Finally, both polyclonal antisera (SRIB1 and SRIB2) directed against different internal peptides revealed the same results on Western blots (Fig. 2 b).
The high degree of overall homology of 50% with synaptopodin gave the first hint of the function of myopodin. Both proteins are rich in prolines (synaptopodin 20%, myopodin 13%), which are equally distributed along the molecule and may result in a linear protein structure and may explain the high susceptibility to proteolytic degradation of both proteins. Myopodin and synaptopodin are rapidly degraded in protein extracts stored at -20°C before dilution with SDS sample buffer and boiling (unpublished data). On the other hand, this degradation could be avoided when protein extracts were directly mixed with SDS sample buffer and boiled. In fact, synaptopodin, but not myopodin, contains two so-called PEST motifs (Fig. 1) that may target the protein to rapid degradation by the proteasome (Rechsteiner and Rogers, 1996). A linear structure would also allow fast and efficient interactions with multiple other proteins. The idea of myopodin serving as an adaptor protein is supported by the presence of multiple PXXP motifs for potential SH3 domain binding and by the presence of a single PPXY motif in myopodin, which is conserved between mouse and human (Fig. 1). PPXY motifs mediate the interaction with the WW domain of a variety of structural and signal transduction proteins (Kay et al., 2000). In contrast to synaptopodin, myopodin contains two potential NLS (see below).
Myopodin (Fig. 6, a and b) and synaptopodin (unpublished data) directly bind to actin. In skeletal and heart muscle, myopodin (Fig. 4) and synaptopodin (unpublished data) are found at the Z-disc. In fibroblasts, -actinin and the stress fiber proteins have an arrangement similar to that in striated muscle. Based on these observations, a sarcomeric model of stress fiber structure in nonmuscle cells was proposed (Sanger et al., 1983). The regular and punctuated arrangement of synaptopodin along the actin filaments in podocytes (Mundel et al., 1997a,b), the colocalization of myopodin and synaptopodin with
-actinin in differentiating myoblasts and transfected NIH3T3 cells (unpublished data) indicate that members of the synaptopodin gene family may be involved in the organization or regulation of the Z-disc in striated muscle cells and a Z-disc equivalent in podocytes.
The expression of synaptopodin in neurons and podocytes is restricted to late stages of cellular differentiation (Mundel et al., 1997a). In podocytes, synaptopodin expression coincides with process formation and reorganization of the actin cytoskeleton and is a marker of a differentiated podocyte phenotype (Mundel et al., 1991). During myocyte differentiation, synaptopodin is constitutively expressed in both undifferentiated myoblasts and differentiated myotubes without changes in protein expression levels (unpublished data). In contrast, myopodin is regulated in a temporal and spatial fashion during myocyte differentiation (Fig. 5). In undifferentiated myoblasts, myopodin is expressed preferentially in the nucleus and only weakly in the cytoplasm. In differentiated myotubes it is incorporated into the Z-disc and shows no detectable nuclear expression (Fig. 5, c and d). Notably, this redistribution coincides with an increase in protein expression (Fig. 5 e). Together, these findings indicate that myopodin may be involved in the regulation of myocyte differentiation, a function not shared with synaptopodin.
The most significant difference between myopodin and synaptopodin is the ability of myopodin to translocate into the nucleus and induce nuclear actin bundling. We noted thick bundles of filamentous actin in the nuclei of cells overexpressing GFP-myopodin (Fig. 8), but never in nuclei of cells expressing GFP-synaptopodin (unpublished data). The loops were similar in appearance to those induced by supervillin (Wulfkuhle et al., 1999). Supervillin is a membrane-associated, F-actinbinding protein of the villin/gelsolin superfamily (Pestonjamasp et al., 1997). Similar to myopodin, supervillin contains several NLSs, translocates to the nucleus, and bundles F-actin (Wulfkuhle et al., 1999). However, in contrast to the supervillin-induced loops, the myopodin-induced loops are sensitive to disruption of actin filaments with lat-A (Fig. 8) and do not contain the nuclear cytoskeleton protein lamin (unpublished data). The functional significance of the nuclear actin loops remains elusive. They may simply represent an artifact of strong overexpression. On the other hand, they show the actin-bundling activity of myopodin and its ability to translocate into the nucleus.
It remains to be established whether the myopodin-induced actin bundles arise from a pool of preexisting nuclear actin alone or whether their formation requires additional import of cytoplasmic actin. There is growing evidence for both constitutive presence in and import of actin and actin-associated proteins into the nucleus. The COOH-terminal domain of lamin A binds to nuclear actin, suggesting that an actin-associating molecular motor linked to the nuclear lamina could be involved in the movement or modification of chromatin domains (Sasseville and Langelier, 1998). This hypothesis is further supported by the finding that type I myosin is present in the nucleus (Nowak et al., 1997). A novel isoform of nonmuscle -actinin, termed actinin-4, shifted steadily from the cytoplasm to the nucleus upon inhibition of phosphatidylinositol 3 kinase or actin depolymerization (Honda et al., 1998). Conformational differences between cytoplasmic and nuclear actin were described using a monoclonal antibody (Gonsior et al., 1999). This antibody, 2G2, recognizes a specific conformation of native actin which is present in the nucleus and specified by compaction of the antibody-reactive region into a coherent patch (Gonsior et al., 1999). Actin itself contains two NES sequences in the middle part of the molecule, and LMB treatment of cells prevented nuclear exclusion of endogenous actin, inducing its nuclear accumulation (Wada et al., 1998). Expression of actin mutants with disrupted NESs, but not of wild-type actin, induced a decrease in the proliferative potential of the cell, indicating a role of actin in cell division (Wada et al., 1998). Zyxin, a regulator of actin filaments, shuttles between focal contacts and the nucleus (Nix and Beckerle, 1997), where it targets the mitotic apparatus by interacting with the h-warts/LATS1 tumor suppressor (Hirota et al., 2000). The EAST protein of Drosophila controls an expandable nuclear endoskeleton by promoting nuclear import of CP60 and actin (Wasser and Chia, 2000). Together, these findings indicate that components of the actin cytoskeleton are present in the nucleus under physiological conditions. Modulation of nuclear actin content or polymerization state may be required to maintain normal cell function. Further studies will aim to define the precise role of myopodin in these processes.
In addition to a role under physiological conditions, there is growing evidence for a role of the actin cytoskeleton in the nucleus in situations of cellular stress. Sanger et al. (1980) showed a reversible translocation of cytoplasmic actin into the nucleus and formation of intranuclear actin filament bundles after treatment with DMSO. Subsequently, Ono et al. (1993) showed the association of cofilin with nuclear actin and proposed that nuclear import of actin in DMSO-treated cells is mediated by cofilin. Similar results were obtained in heat-shocked cells (Courgeon et al., 1993). Interestingly, T cell costimulation causes nuclear translocation of cofilin (Samstag et al., 1994) and inhibition of the translocation by dephosphorylation induces T cell apoptosis (Samstag et al., 1996). We now show that heat shock of myoblasts (Fig. 10, af) and myotubes (Fig. 10, gi) induces cytoplasmic depletion and nuclear accumulation of myopodin, even after incorporation into a mature Z-disc. This nuclear accumulation was even stronger after inhibition of CRM1-mediated nuclear export with LMB. As described above, actin has two NESs and accumulates in the nucleus after inactivation of the NESs (Wada et al., 1998). In contrast, myopodin does not have a known NES (Fig. 1), but still accumulates in the nucleus after LBM treatment (Fig. 10). Therefore, future studies will have to clarify whether the nuclear accumulation of myopodin is mediated by a novel NES or via binding to actin or another NES-carrying protein. In any case, our studies indicate a role of myopodin in situations of cellular stress. The stress might trigger certain cellular responses during which myopodin may serve as a signaling or regulator molecule.
Another intriguing question is how myopodin is translocated into the nucleus. The two potential NLSs present in the molecule appear to be not necessary for nuclear import, since deletion or inactivation by mutagenesis of both NLSs did not prevent nuclear import and actin bundling in myoblasts (Fig. 9, a and b). In addition to NLS-mediated nuclear import, proteins can be imported into the nucleus through so-called nuclear-shuttling (NS) sequences (Michael, 2000). NS sequences are stretches of 30 and 60 aa and bind to transportin proteins that mediate both nuclear import and export (Michael, 2000). All proteins currently known to contain this type of signal also associate with mRNA. In contrast to basic amino acid type NLSs and leucine-rich NESs, the NS motifs are less well preserved and therefore need to be experimentally established for each protein (Michael, 2000). Future studies will focus on testing whether myopodin contains a (novel) NS or whether it shuttles between the cytoplasm by binding to another protein, including actin.
What could be the functional role of myopodin? Myopodin directly binds to actin. It bundles actin filaments, both in the cytoplasm and in the nucleus, and is found along cytoplasmic actin filaments in a punctuated pattern and at the Z-disc, where it colocalizes with -actinin. In contrast, in the nucleus myopodin is not coexpressed with
-actinin, indicating that myopodin may interact with different proteins in the cytoplasm and the nucleus. In the nucleus, myopodin shows a speckled pattern reminiscent of actin snRNP aggregates (Sahlas et al., 1993). Thus, one can imagine that myopodin is involved in an actin-based mRNA transport pathway. Alternatively, it may bundle nuclear actin and thereby modulate the actin-based nuclear endoskeleton similar to the Drosophila EAST protein (Wasser and Chia, 2000). Striated muscle cells are highly differentiated and specialized cells that must be able to adequately respond to various physiological and pathological challenges. We propose that, similar to zyxin at focal contacts (Nix and Beckerle, 1997), myopodin may play a dual role as a structural protein at the Z-disc and a regulator protein participating in a signaling pathway between the nucleus and the Z-disc during development and in situations of cellular stress.
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Materials and methods |
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RNA isolation and Northern blot analysis
Total RNA was isolated from mouse skeletal and heart muscle with the RNeasy Kit (QIAGEN) according to the manufacturer's instructions. PolyA+ mRNA was purified with the Oligotex mRNA Purification Kit (QIAGEN), separated on a 1.2% denaturing formaldehyde gel, and transferred onto GeneScreen Plus membranes (NEN Life Science Products). Northern blot analyses were done with a 32P-labeled antisense riboprobe using a 1750-bp fragment of the mouse heart cDNA as template.
Site-directed mutagenesis
The two potential NLSs were inactivated using the Quikchange site-directed mutagenesis kit (Stratagene) by replacing the first two arginines in each NLS with two alanines (Fig. 9 a). Diagnostics digests at newly arising cutting sites and subsequent DNA sequencing confirmed the effective mutagenesis. We generated two GFP full-length constructs, one in which only the COOH-terminal NLS was mutated (mut2) and one in which both NLS were mutated (mut 1+2).
Antibodies
Two polyclonal antisera specific for myopodin were generated by immunization of rabbits with a keyhole limpet hemocyanin-conjugated peptides. The antisera were affinity purified as described previously for synaptopodin (Mundel et al., 1997a). Antisera SRIB1 was directed against aa 634652 (single letter code SGRGAQLFAKRQSRMEKYV, bold and boxed in Fig. 1), and SRIB2 directed against aa 593612 (single letter code FKGPQAAVASQNYTPKPTVS, boxed in Fig. 1) of human myopodin. Antisynaptopodin polyclonal antiserum NT has been described previously (Mundel et al., 1997a).
Immunochemistry
Adult female rats were perfused via the abdominal aorta with 4% PFA in PBS for 3 min at 220 mm Hg followed by cryoprotectant sucrose PBS solution (800 mOsmol) for 5 min at 220 mm Hg. Organs were harvested and tissue slices were frozen in liquid isopentane (Mundel et al., 1997a). 5-µm thick frozen sections from rat heart and skeletal muscle were incubated with SRIB1 (1:25) and SRIB2 (1:10) and NT (1:50). Double labelings were done with monoclonal antibody BD6 against titin (Whiting et al., 1989) and sarcomeric -actinin (Sigma-Aldrich). Immunofluorescence labeling and documentation were done as described previously (Mundel et al., 1997a). The specificity of the myopodin reaction was verified by preabsorption with the corresponding peptides that had been used for immunization. For human heart, 3-µm thick serial sections of formalin-fixed paraffin-embedded tissue were rehydrated in a graded series of alcohol and stained using an avidin-biotin immunoperoxidase technique (Barisoni et al., 1999).
Immunoelectron microscopy
Psoas muscle stretched to different degrees in situ was excised from freshly killed rats, which had been previously perfused with PBS containing 4% paraformaldehyde. Cryosectioning and immunogold labeling with SRIB1 and SRIB2 as well as anti-actinin (Sigma-Aldrich) followed by 10-nm gold particleconjugated secondary antibodies was essentially as described (Mundel et al., 1991; Linke et al., 1998).
Protein extraction and immunoblotting
Skeletal muscles and hearts were harvested from adult C67 black mice. Protein extraction was performed at 4°C in a tight-fitting Potter homogenizer with 15 strokes at 1,400 rpm in 10 vol of homogenization buffer (20 mM Tris, 500 mM NaCl, pH 7.5) supplemented with 1% Triton X-100 (Sigma-Aldrich), 5 mM EDTA, and the following protease inhibitors (all from Roche Diagnostics): 2 µM pepstatin, 2 µM leupeptin, and 200 µM pefabloc. Insoluble material was pelleted at 50,000 g for 35 min at 4°C. The resulting supernatants were immediately diluted with SDS sample buffer, boiled for 5 min, and separated on 8% SDS polyacrylamide gels to avoid proteolysis of myopodin. Proteins were transferred to Immobilon P membranes (Millipore) by semidry blotting. SRIB1 and SRIB2 were used at 1:250, NT was used at 1:1:200, HRP-conjugated secondary antibodies (Promega) at 1:20,000. The immunoreaction was visualized by ECL (Amersham Pharmacia Biotech) and film exposure. The specificity of the myopodin reaction was verified by preabsorption with the corresponding peptide used for immunization. To explore the expression of myopodin in organs other than skeletal and heart muscle, cytosolic extracts from colon, stomach, uterus, lung, brain and liver were analyzed by immunoblotting. In addition, proteins were extracted from C2C12 myoblasts and myotubes.
Cell culture
C2C12 myoblasts (Yaffe and Saxel, 1977; Blau et al., 1985) were propagated in DME with 4 mM L-glutamine, 1 mM sodium pyruvate and 1.5 g/l sodium bicarbonate, supplemented with 10% FBS. Differentiation was induced by replacing FBS with 2% horse serum when the cells reached 80% confluence. For immunostaining, myoblasts were plated on collagen-coated coverslips. 6 d after switching to horse serum, cells were fixed and processed for immunocytochemistry. M2 cells (ABP280/filamin-deficient) and A7 cells (ABP280/filamin-repleted M2 cells) (Cunningham et al., 1992) were cultured in MEM containing 8% newborn calf serum and 2% fetal calf serum. In case of the rescued A7 cells, G418 (500 µg/ml) was added to retain expression of ABP280/filamin.
Actin cosedimentation
In vitro translation of full-length myopodin was done with the TnT coupled reticulocyte lysate kit (Promega) in the presence of 1 µg plasmid DNA and either 35S-labeled methionine (Amersham Pharmacia Biotech) or unlabeled amino acid mix. Actin cosedimentation assays were essentially performed as described previously (Kaplan et al., 2000). For competitive binding assays, 5 or 15 µl of unlabeled in vitrotranslated myopodin was added to the cosedimentation mix. Myopodin bands were quantified with ImageQuant Software and expressed as a percentage of total labeled protein found in supernatant and pellet (Kaplan et al., 2000).
Mapping of the actin binding site
Myopodin cDNA constructs of decreasing length covering the complete ORF (see Fig. 7) were cloned into the pEGFP-C1 expression vector (CLONTECH). The constructs were transfected into subconfluent myoblasts using GenePORTER transfection reagent (Gene Therapy Systems) and analyzed by direct fluorescence microscopy in living cells. Pictures were captured with a Spot cooled CCD camera (Diagnostic Instruments) and processed with Adobe Photoshop® 5.0 software.
Reversible disruption of the actin cytoskeleton with lat-A
2 d after transfection with GFP-myopodin, cells were treated with 5 µM lat-A (Calbiochem) for 2 h to depolymerize actin filaments (Coue et al., 1987). The effects of lat-A were observed in living cells as described in the previous section. The cells were washed twice with PBS and further cultivated for 4 h in the absence of lat-A to show reversibility.
Heat shock and LMB treatment
C2C12 myoblast and myotubes were incubated for 90150 min at 43°C in a waterbath. In some experiments 10 nM LMB (Sigma-Aldrich) was added to the medium 5 min before heat shock induction to block nuclear export (Nishi et al., 1994). After heat shock, cells were fixed and processed for immunocytochemistry.
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Footnotes |
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* Abbreviations used in this paper: aa, amino acid; EST, expressed sequence tag; GFP, green fluorescent protein; lat-A, latrunculin A; LMB, leptomycin B; NES, nuclear export sequence; NLS, nuclear localization signal; NS, nuclear shuttling.
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Acknowledgments |
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Wolfgang A. Linke is a Heisenberg fellow of the German Research Foundation. This work was supported by a grant from the Howard Hughes Medical Research Institute Research Resources for Medical Schools and the National Institutes of Health (DK57683-01) to Peter Mundel.
Submitted: 11 December 2000
Revised: 31 August 2001
Accepted: 26 September 2001
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References |
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