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(American Journal of Pathology. 1999;155:285-292.)
© 1999 American Society for Investigative Pathology

Regular Articles

Human Cytomegalovirus Infection Decreases Expression of Thrombospondin-1 Independent of the Tumor Suppressor Protein p53

Jindrich Cinatl Jr.^*, Ruslan Kotchetkov^*, Martin Scholz^*, Jaroslav Cinatl, Jens-Uwe Vogel^*, Pablo Hernáiz Driever and Hans Wilhelm Doerr^*

From the Zentrum der Hygiene,^*
Institut für Medizinische Virologie, Zentrum für Kinderheilkunde und Jugendmedizin,
Abteilung Pädiatrische Hämatologie und Onkologie, Klinikum der Johann Wolfgang Goethe-Universität, Frankfurt am Main, Germany, and Department of Neurosurgery,
Georgetown University Medical Center, Washington, D.C.

	Abstract

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Thrombospondin-1 (TSP-1) is a potent inhibitor of angiogenesis. It has been shown that promoter sequences of the TSP-1 gene can be transactivated by the wild-type tumor suppressor protein p53. As human cytomegalovirus (HCMV) infection inactivates wild-type p53 of various cell types, we investigated whether HCMV infection is associated with reduced TSP-1 production. We found, in conjunction with accumulated p53, that TSP-1 mRNA and protein expression was significantly reduced in HCMV-infected cultured human fibroblasts. To determine whether the observed TSP-1 suppression depends on p53 inactivation, the p53-defective astrocytoma cell line U373MG was infected with HCMV. In these cells TSP-1 expression was also significantly reduced by HCMV infection whereas expression of the p53 mutant variant remained unaltered. In both cell lines the decreased expression of TSP-1 mRNA occurred early after infection (4 hours), indicating that HCMV inhibits TSP-1 transcription during the immediate-early phase of infection before HCMV DNA replication. Inhibition of HCMV DNA synthesis by ganciclovir did not influence TSP-1 reduction whereas the antisense oligonucleotide ISIS 2922, complementary to HCMV immediate-early mRNA, completely prevented the HCMV-mediated TSP-1 suppression. These findings strongly suggest a novel role for HCMV in the modulation of angiogenesis due to p53-independent down-regulation of TSP-1 expression.

	Introduction

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The development of new blood vessels (angiogenesis) is necessary to sustain the growth, invasion, and metastasis of tumors.¹² The signals controlling angiogenesis, although directed at the endothelial cells, come from tumor or stromal cells, such as fibroblasts or monocytes/macrophages. A variety of positive regulators of angiogenesis have been isolated from different tissues and have been purified and sequenced.¹³ From the many peptide growth factors known to act on the vasculature, basic fibroblast growth factor (bFGF)¹⁴ and vascular endothelial growth factor (VEGF)¹⁵ represent the most potent ones, but other factors, such as transforming growth factor-ß1 (TGF-ß1) and platelet-derived growth factor (PDGF), may also be involved in tumor angiogenesis.¹³

In contrast, several other proteins negatively control angiogenesis. One of the most potent negative regulators is the extracellular matrix protein thrombospondin-1 (TSP-1).^16,17 Although some positive effects on angiogenesis have been reported,¹⁸ TSP-1 under defined conditions generally inhibits endothelial cell adhesion,¹⁹ motility,²⁰ and growth^20,21 and induces apoptosis in endothelial cells.²²

TSP-1 expression and function are influenced by several growth factors, oncogenes, and tumor suppressor genes.¹⁶ For example, wild-type p53 induced TSP-1 in normal human fibroblasts.²³ Further evidence for the importance of p53 as a transactivator of the TSP-1 gene has been clearly demonstrated with cultured fibroblasts from cancer-prone Li-Fraumeni patients. When these cells, lacking one p53 allele, either lose or mutate the second p53 allele (which occurs during progression to malignancy), TSP-1 is down-regulated by ~96%.²³

HCMV infection of fibroblasts has been associated with increased expression of bFGF and some other cytokines and interleukins that may exert both direct and indirect angiogenic activities.²⁴ However, it has not been shown whether HCMV may also affect the expression of negative regulators of angiogenesis, for example, via HCMV-IE protein interaction with p53. In the present study, the effects of HCMV infection on TSP-1 in wild-type p53-expressing cultured human fibroblasts and in the p53-defective human astrocytoma cell line U373MG²⁵ were studied. The results show that both the laboratory-adapted strain HCMV AD169 and a patient-derived strain, Hi91, inhibited the expression of TSP-1 in infected cell lines, indicating that p53 was not involved. As HCMV-mediated suppression of TSP-1 could be prevented by treatment with antisense oligonucleotides against HCMV-IE mRNA, this suggested that HCMV-IE proteins regulate TSP-1 expression. In contrast, ganciclovir (GCV), a specific inhibitor of DNA replication and consequently late gene expression, had no effect. In conclusion, novel therapeutic strategies targeting the HCMV-IE gene expression could be important for the prevention of HCMV-associated angiogenesis.

	Materials and Methods

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Cell Cultures

Human foreskin fibroblast (HFF) cultures were established in our laboratory as described previously.²⁶ HFF cells between three and six subcultures were used in the experiments. The human astrocytoma cell line U373MG was obtained from American Type Culture Collection (Rockville, MD). Cells were grown in a culture medium composed of Eagle's minimal essential medium supplemented with 20% fetal bovine serum. After reaching confluency, cells were subcultured at 6-day intervals.

Virus Preparation

The HCMV laboratory strain AD169 was obtained from American Type Culture Collection, whereas the clinical strain Hi91 was isolated from a urine sample of a patient with HIV infection. Virus stocks of both strains were prepared in HFF cells incubated in minimal essential medium supplemented with 4% fetal bovine serum. The respective titers were determined by plaque titration in HFF cells as described previously.⁴ Mock-infected inocula were prepared in an identical fashion, except that cell monolayers were not infected with HCMV.

HCMV inactivation was achieved by exposure of virus-containing cell culture medium to ultraviolet (UV) light (220 V, 12 W) for 15 minutes.²⁷ Irradiated virus samples were used as inocula in HFF or U373MG cultures. UV-irradiated samples were free of infectious virus as demonstrated by plaque titration (not shown).

Filtered virus inocula were prepared by filtering virus stocks through a Microsep microconcentrator with a cutoff at 300,000 molecular weight (Filtron Technology Corp., Northborough, MA) at 3000 x g for 12 hours at 4°C. The filtrate collected from the bottom of the filter apparatus was added to HFF or U373MG cultures. The filtrate samples were free of infectious virus as demonstrated by plaque titration.

Antiviral Drugs

GCV (Hoffman-La Roche AG, Grenzach-Wyhlen, Germany) was prepared fresh (on the day of each experiment) in distilled water. ISIS 2922, a phosphorothioate oligonucleotide that is complementary to HCMV IE RNA and the noncomplementary control oligonucleotide ISIS 26062, were kindly provided by ISIS Pharmaceuticals (Carlsbad, CA).²⁸ Both ISIS 2922 and ISIS 26062 were dissolved in phosphate-buffered saline (PBS) at a concentration of 10 mmol/L, and aliquots were stored at -20°C until use. To enhance oligonucleotide uptake, ISIS 2922 or ISIS 26062 was complexed to cationic liposomes DOTAP (Boehringer, Mannheim, Germany) immediately before virus infectivity assay. The pretreatment of the antisense oligonucleotides with DOTAP was performed according to the instructions of the manufacturer.

Virus Infectivity Assay

Confluent cultures of HFF cells were incubated with HCMV infectious strains at a multiplicity of infection (m.o.i.) of 2 or with UV-inactivated samples or with filtered virus-free inocula. After incubation for 1 hour, required for virus adsorption, cells were washed with PBS and incubated in culture medium containing 2% fetal bovine serum. In some experiments, cells incubated with infectious virus were treated with GCV or with oligonucleotides complexed to cationic lipids, including antisense ISIS 2922 or control oligonucleotide ISIS 26062. Cells were treated with ISIS 2922 or ISIS 26062 according to established protocols.^28,29 Briefly, cell monolayers were pretreated with the oligonucleotides overnight in IMDM containing 0.2% fetal bovine serum before infection. After pretreatment, cells were infected with HCMV at a m.o.i. of 2. After 1 hour of incubation, virus was removed and fresh medium containing antisense oligonucleotides was added. For control purposes, cells were incubated with GCV in the same way as described for ISIS 2922 and ISIS 26062. The cell numbers producing HCMV-specific antigens were examined 24 and 72 hours post infection (p.i.) by immunoperoxidase staining using monoclonal antibodies (MAbs; DuPont, Bad Homburg, Germany) directed against 72-kd immediate-early antigen (IEA) and 67-kd late antigen (LA), respectively (described in detail elsewhere).^3,4

Flow Cytometry

To investigate the expression of TSP-1 or p53, 5 x 10⁵ cells were fixed for 10 minutes in 4% buffered formaldehyde. After washing the cells twice in buffer containing 0.5% Tween-20, cells were incubated for 30 minutes with mouse MAbs against TSP-1 (clone 11.4; Dianova, Hamburg, Germany), a MAb specifically detecting mutant p53 (clone PAb 240; Calbiochem, Bad Soden, Germany), or a MAb specifically detecting wild-type p53 (clone PAb 1620; Calbiochem). After washing cell pellets two times in buffer, the fluorescein-isothiocyanate-conjugated goat anti-mouse IgG (Becton Dickinson, Heidelberg, Germany) was added for 30 minutes. Fluorescence intensities were measured by flow cytometry (FACScan, Becton Dickinson). Data collected from 1 x 10⁴ cells were analyzed using Cell Quest software. All experiments were repeated at least three times.

Reverse Transcription-Polymerase Chain Reaction

Total RNA was isolated from mock-infected or infected cells using TRIZOL according to the manufacturer's instructions (Gibco-BRL Life Technologies, Gaithersburg, MD). RNA was reverse transcribed using random hexamer priming. One microgram of total RNA was denaturated at 70°C for 10 minutes and chilled on ice. The denaturated RNA was then co-incubated with 2.5 µmol/L random hexamer oligonucleotides, 1 µmol/L each dNTP, 5 mmol/L MgCl₂, 1 µl of RNAse inhibitor (Boehringer Mannheim), and 1 µl of MuLV reverse transcriptase (Gibco-BRL) in 1X polymerase chain reaction (PCR) buffer II (Perkin-Elmer Corp.) for 1 hour at 37°C. The reverse transcription was inactivated for 5 minutes at 95°C before amplification. TSP-1 primers used were 5'-CGT CCT CTT CCT GAT GCA TG-3' (position 99 to 118) and 5'-GGC AGG ACA CCT TTT TGC AGA-3' (position 1115 to 1135),³⁰ the sequence of GAPDH primers used as control were 5'-TGG GGA AGG TGA AGG TCG GA-3' (position 61 to 81) and 5'-GAA GGG GTC ATT GAT GGC AA-3' (position 151 to 171).³¹ PCR amplification of the cDNA was carried out by adding 0.5 µg of Taq DNA polymerase (Boehringer Mannheim). PCR amplification was done using 26 cycles in a DNA thermocycler as follows: denaturation for 1 minute at 94°C, annealing for 1 minute at 52°C, and extension for 1.5 minutes at 72°C in a Perkin Elmer thermocycler. PCR products were resolved alongside DNA marker on an 8% polyacrylamide gel, stained with silver nitrate, and photographed. The photographs were further analyzed by scanning densitometry using E.A.S.Y. RH system (HeroLab, Wiesloch, Germany), and the ratio of TSP-1/GAPDH band intensity was calculated. To ascertain that TSP-1 transcripts were specifically amplified, sequence analysis of PCR products was performed. Amplified sequences fully matched TSP-1 nucleotide sequence (results not shown).

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

 
Effects of HCMV Infection on TSP-1 and p53 Expression

To study the effects of HCMV infection on TSP-1 and p53 expression, both HFF and U373MG cells were infected with HCMV AD169 and Hi91 strains at a m.o.i. of 2. Both human fibroblasts and U373MG represent fully permissive cell types for HCMV replication in cell culture,³² which was confirmed by immunoperoxidase staining against HCMV-specific IEA and LA as controls for each experiment. In both HFF- and U373MG-infected cultures more than 99% of cells stained positively for HCMV IEA and more than 98% and 92% of cells stained positively for LA, respectively (data not shown).

The levels of cell-associated TSP-1 were evaluated by flow cytometry at different times after virus inoculation and compared with those of mock-infected HFF and U373MG cells. Although at 4 hours p.i. no HCMV-mediated modulation of TSP-1 could be detected within the infected HFF cell populations, significant differences were observed 24 and 72 hours p.i. Infection of HFF with AD169 strain decreased TSP-1-specific fluorescence intensity to 51% after 24 hours and to 21% after 72 hours p.i of the mock-infected control. Similar results were obtained when HFF cells were infected with the HCMV-Hi91 strain (Figure 1A) .

View larger version (21K): [in this window] [in a new window]   Figure 1. Time course of TSP-1 protein expression in HFF (A) and U373MG (B) cells. TSP-1 was measured by flow cytometry in mock-infected or AD169- or Hi91-infected cells 4, 24, and 72 hours after infection p.i. The results are expressed as relative mean fluorescence intensity units. Data are depicted as means ± SD from one representative experiment performed in triplicate. Statistically significant differences were found between virus-infected and mock-infected cultures (P < 0.05) after 24 and 72 hours as determined by Student's t-test.

View larger version (22K): [in this window] [in a new window]   Figure 2. Time course of p53 protein expression in HFF (A) and U373MG (B) cells. p53 was measured by flow cytometry in mock-infected or AD169- or Hi91-infected cells 4, 24, and 72 hours p.i. The results are expressed as relative mean fluorescence intensity units. Data are depicted as means ± SD from one representative experiment performed in triplicate. Statistically significant differences were found between virus-infected and mock-infected HFF cultures (P < 0.05) after 24 and 72 hours as determined by Student's t-test.

Additional experiments were performed to determine whether HCMV-specific viral gene expression was responsible for changes in TSP-1 and/or p53 expression. In four independent experiments, it was found that neither ultrafiltrated supernatants from virus-infected cells nor UV-inactivated virus affected TSP-1 or p53 protein expression in HFF or U373MG cells as determined by flow cytometry (data not shown).

Effects of HCMV on TSP-1 mRNA Expression

To study whether HCMV-mediated reduction of TSP-1 protein levels were due to impaired mRNA synthesis, TSP-1 mRNA levels in HFF and U373MG cells infected with strain AD169 at different times after virus inoculation were measured by reverse transcription PCR. Reverse transcription was carried out using specific primers for TSP-1 and GAPDH. As shown, HCMV infection resulted in the reduction of TSP-1 mRNA levels similarly in both cell types already at 4 hours p.i. (Figure 3A) . Densitometric analyses of TSP-1-specific bands revealed that HCMV infection but not treatment with UV-inactivated virus or virus-free filtrates (not shown) resulted in inhibition of the respective mRNA to 60% of the mock-infected cultures. TSP-1 mRNA was found to be further reduced to 25% and 5% of the mock-infected cultures at 24 and 72 hours p.i., respectively (Figure 3B) .

View larger version (25K): [in this window] [in a new window]   Figure 3. Time course of TSP-1 mRNA expression in mock-infected (-) and AD169-infected (+) HFF cells. Total RNA was isolated 4, 24, or 72 hours p.i. Reverse transcription PCR was done using specific primers for TSP-1 and GAPDH, and products were visualized by staining with silver nitrate on polyacrylamide gel (A). The bands were analyzed by densitometry. Relative density values of TSP-1 mRNA are depicted as the mean of three experiments ± SD (B).

To study the mechanism involved in the HCMV-mediated effects on TSP-1 and p53 expression, HCMV-infected cells were treated with two anti-HCMV agents. GCV, a drug clinically used for treatment of HCMV disease, targets HCMV DNA synthesis and does not prevent immediate-early or early virus gene expression.^33,34 In contrast, the antisense oligonucleotide ISIS 2922 specifically blocks the function of HCMV IE mRNA and thus prevents the de novo synthesis of viral IE proteins before viral DNA replication occurs.²⁸ The antiviral effects of both agents were determined in infected cultured HFF and U373MG cells by quantification of numbers of cells carrying HCMV-specific IEA and LA by means of immunoperoxidase staining technique. The number of HCMV IEA/LA-positive cells detected after treatment with either drug was compared with those detected in the untreated controls (Figure 4) .

View larger version (26K): [in this window] [in a new window]   Figure 4. Effects of antiviral drugs GCV and ISIS 2922 on HCMV IEA (•) and LA () expression in HFF cultures (A and C) and U373MG cultures (B and D) infected with AD169. The numbers of HCMV IEA- and LA-positive cells were determined by means of immunoperoxidase staining and counted 24 hours (IEA) and 72 hours (LA) p.i. The results are expressed as percentage of IEA/LA-positive cells of infected controls without drug treatment. In control cultures, more than 98% and 92% of cells stained positive for IEA or LA, respectively. Data are shown representative of three independent experiments.

Next, the effects of GCV and ISIS 2922 on TSP-1 and p53 expression in HCMV (AD169)-infected HFF and U373MG cells were compared. Expression of these proteins was assessed by means of flow cytometry at 3 days p.i. The relative mean fluorescence intensity values obtained by histogram analyses of populations stained with MAb 11.4 (recognizing TSP-1), MAb Pab 240 (recognizing mutant p53), and MAb Pab 1620 (recognizing wild-type p53) are depicted in Tables 1 and 2 , respectively. The results showed that HCMV-mediated down-regulation of TSP-1 (as indicated by the reduced MAb 11.4-related fluorescence intensity) was prevented by ISIS 2922 but not by GCV in HFF (Table 1) . Moreover, GCV treatment had no influence on the HCMV-mediated enhancement of MAb Pab 1620-specific fluorescence intensity in infected HFF. In contrast, the values obtained for ISIS 2922-treated infected HFF did not differ from mock-infected control values, suggesting that ISIS 2922 completely prevented wild-type p53 up-regulation. Neither GCV nor ISIS 2922 modified the expression of mutant p53 in U373MG cells (Table 2) .

View larger version (27K): [in this window] [in a new window]   Figure 5. TSP-1 mRNA expression in mock-infected (-) and AD169-infected HFF (+) cells without treatment, after treatment with GCV or after treatment with ISIS 2922. Reverse transcription PCR was done using specific primers for TSP-1 and GAPDH (standard control). Products were visualized by staining with silver nitrate on polyacrylamide gel. The bands were analyzed by densitometry (A). Relative density values of TSP-1 mRNA are depicted as the mean of three experiments ± SD (B).

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

Based on its effects on tumor and endothelial cell behavior, TSP-1 has attracted attention as a possible negative regulator of tumor growth and metastasis. In addition to its direct effects on tumor cells, TSP-1 reduces tumor growth by inhibition of angiogenesis possibly through an indirect mechanism induced by infected fibroblasts.^23,36 Initial studies have confirmed that increased TSP-1 expression suppressed growth and metastasis of some tumors in vivo and inhibited angiogenesis.^37-39 In the present study HCMV infection of both fibroblasts and astrocytoma cells resulted in down-regulation of TSP-1. Therefore, it is conceivable that the infection of stromal and/or tumor cells, frequently observed in patients with different malignancies,^1,4 stimulates angiogenesis due to an imbalance between positive and negative regulators. Although the exact role of HCMV in tumorigenesis is unclear, angiogenic properties resulting from HCMV infection could be responsible for tumor progression in these patients.

The down-modulation of TSP-1 mRNA and protein expression could be due to inactivation of tumor suppressor proteins in HCMV-infected fibroblasts. Previous studies demonstrated that accumulation of tumor suppressor proteins, including wild-type p53 and Rb in HCMV-infected cells, was associated with loss of their function.^7-9,11 These effects of HCMV result mainly from the binding of tumor suppressor proteins by HCMV IE proteins reminiscent of the effects of oncoproteins of small DNA tumor viruses.^7-9,11 It was initially suggested that inactivation of p53 in HCMV-infected cells represents a major mechanism in down-modulation of TSP-1 expression as this tumor suppressor gene is involved in the positive regulation of TSP-1.^23,40 In patients with Li-Fraumeni syndrome inactivation of p53 due to lack or mutation of p53 alleles was associated with reduced expression of TSP-1.²³ Indeed, we observed that decreased TSP-1 amounts in HCMV-infected fibroblasts were paralleled by increased levels of wild-type p53 in the cytoplasm of the cells. However, in U373MG cells that express a mutated variant of p53²⁵ TSP-1 was similarly reduced on HCMV infection whereas the level of p53 remained unaltered. In a glioblastoma cell line (U87MG) carrying wild-type p53²⁵ the level of TSP-1 was similar to the level in U373MG cells (not shown). Unfortunately, we were not able to determine the effects of HCMV infection on the expression of TSP-1 in U87MG because these cells have a low permissivity for HCMV (<1%). Moreover, it has been reported that induction of wild-type p53 in glioblastoma cells did not alter TSP-1 levels.⁴¹ These findings support our results indicating that the HCMV-mediated modulation of the TSP-1 expression may occur via intracellular pathways independent of p53. Rb, a different tumor suppressor protein, was also shown to be involved in the positive regulation of TSP-1 gene expression.^23,40 As HCMV has been shown to functionally inhibit Rb,^8,9 it is conceivable that this mechanism could contribute to reduced expression of TSP-1.

In addition to tumor suppressor proteins, cellular transcription factors may also influence TSP-1 gene expression.¹⁶ In the human and mouse, TSP-1 promoter potential binding sites for different transcription factors are present.^42-45 It has been shown that HCMV activates cellular metabolism in a manner similar to growth factors and hormones,^46-48 resulting in activation of different proto-oncogenes and transcription factors.^46-47 For example, both mitogenic stimuli and HCMV infection induce expression of proto-oncogenes such as c-jun, c-fos, and c-myc.⁴⁹ In particular, the Jun proto-oncogene product was shown to repress thrombospondin expression in rat embryo fibroblasts.⁵⁰ It is known that cellular proto-oncogenes can be induced by transactivating HCMV IE proteins but also by inactivated HCMV particles within minutes after infection independent of HCMV gene expression.⁵¹ Our results demonstrate that HCMV-induced proto-oncogene activation before HCMV gene expression does not play a major role in TSP-1 regulation. And TSP-1 expression was not modified either by inactivated HCMV or by HCMV-induced nonspecific soluble factors present in cell culture supernatants. Thus, it is likely that effects on TSP-1 gene expression stem from transcription activity of HCMV IE proteins. For example, HCMV IE gene expression controls activation transcription factor-1/c-AMP responsive element binding protein (ATF-1/CREB)⁵² that in turn negatively regulates TSP-1 expression.⁴⁵ This negative regulation may occur either directly by binding of ATF-1 to a negative regulatory site in the TSP-1 promoter or indirectly by negative regulation of Rb via an ATF binding site in the promoter of Rb.^45,53 Our results demonstrate that HCMV-mediated TSP-1 down-regulation is due to HCMV IE gene expression, which can be prevented by specific inhibition of HCMV IE mRNA with the antisense oligonucleotide ISIS 2922 but not by inhibition of HCMV DNA replication with GCV.

Recently, we and others suggested that HCMV IE gene expression plays an important role in HCMV-associated pathogenicity.^27,33,34 Evidence has been presented in this report that GCV or related drugs are not sufficient in this regard,^33,34 although drugs suppressing the HCMV IE phase may be of more relevance.³⁴ In this report it was shown that ISIS 2922 specifically blocks HCMV IE mRNA, which resulted in complete inhibition of HCMV-mediated down-regulation of TSP-1. In summary, the inhibition of HCMV IE gene products provides an important approach for the treatment of HCMV-associated angiogenesis involved in various pathogenic conditions such as tumor growth or inflammation.

	Acknowledgements

 
We are grateful to Gabi Bauer for microphotographs and Sandra Dujardin and Gesa Meincke for technical assistance.

	Footnotes

 
Address reprint requests to Dr. Jindrich Cinatl, Institut für Medizinische Virologie, Zentrum der Hygiene, Klinikum der Johann Wolfgang Goethe-Universität, Sandhofstrasse 2–4, D-60528 Frankfurt am Main, Germany. E-mail: cinatl{at}em.uni-frankfurt.de

Supported by the foundations Hilfe für krebskranke Kinder Frankfurt, e.V., and Frankfurter Stiftung für krebskranke Kinder.

Accepted for publication March 20, 1999.

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