(Received for publication, December 4, 1996, and in revised form, March 7, 1997)
From the Division of Infectious Diseases and Immunology, Saint Louis University, St. Louis, Missouri 63110
Our previous results have suggested that the putative core protein of hepatitis C virus (HCV) transcriptionally regulates cellular and viral genes, inhibits cisplatin and c-myc-mediated apoptotic cell death under certain conditions, and transforms primary rat embryo fibroblast cells with a cooperative oncogene. Because HCV appears to cause hepatocellular carcinoma, we evaluated the regulatory role of the HCV core protein on p53, a well known tumor suppressor gene, by an in vitro transfection assay. HCV core protein repressed transcriptional activity of the p53 promoter when tested separately in COS7 and HeLa cells. Deletion mutational analysis of the HCV core gene indicated that the regulatory domain involved in the repression of p53 transcriptional activity is located around amino acid residues 80-122 encompassing a putative DNA binding motif and two major phosphorylation sites. Results from this study suggest that the putative core protein may have an important biological role in the promotion of cell growth by repressing p53 transcription, and this appears to be consistent with certain earlier observations about HCV core moving into the nucleus.
Development of chronic hepatitis and the potential for disease progression to hepatocellular carcinoma (1) are important features of hepatitis C virus (HCV)1 infection in humans. Successful purification of HCV from either infected tissues or cultured cells has not been reported. It is possible that HCV is stringently hepatotropic being restricted to replicate and release only in differentiated hepatocytes, which may have HCV receptors on the cell surface and specific functions that support viral growth (2). Thus it is difficult to study the biological properties and pathogenicity of the virus in the absence of unequivocal evidence for common ancestry of HCV (3). The mechanism of HCV replication at the molecular level so far has depended upon comparative analysis and expression of its partial or entire genome with those of distantly related flaviviruses or pestiviruses (4). The virus genome encodes a single polyprotein precursor of ~3,000 amino acids (5) that is cleaved by both host and viral proteases (6, 7) to generate three putative structural proteins (core, E1, and E2) and at least six nonstructural proteins (NS2, NS3, NS4A, NS4B, NS5A, and NS5B). The structural proteins are located in the amino-terminal one-fourth of the polyprotein. The genomic region encoding the putative core protein is relatively conserved (8). The carboxyl terminus of the core protein has been established at amino acid position 191. The HCV core protein demonstrates diverse biological functions including the regulation of cellular and unrelated viral genes at the transcriptional level (9), suppression of cisplatin and c-myc-induced apoptosis (10), and transformation of REF cells in cooperation with the H-ras oncogene (11).
Hepatocellular carcinoma accounts for over 90% of primary liver cancers and may progress through the inactivation of the p53 gene via mutations (12, 13). Because HCV appears to cause hepatocellular carcinoma, in this study we evaluated the ability of the HCV core protein to regulate the expression of p53 in a cotransfection system. Our results suggested that the HCV core protein caused down-regulation of p53, and this appeared to be consistent with the controversial observations about HCV core moving into the nucleus.
A partial cDNA clone (Blue4/C5p-1) of strain
HCV-1a containing the 5-untranslated region, C, E1, E2, and a portion
of the NS2 region kindly provided by Michael Houghton (Chiron
Corporation, Emeryville, CA) was used as a template for amplification
and cloning of the core genomic region (encompassing amino acids
1-191) into mammalian expression vectors following a similar procedure
described recently (11, 14). Briefly, two synthetic oligonucleotide primers, sense (5
-GTGCTTGCGAATTCCCCGGGA-3
) and antisense
(5
-CGTGGAATTCGCACTTAGTAGG-3
), containing EcoRI restriction
enzyme sites were used for PCR amplification. The amplified DNA was
inserted into the EcoRI site of the pcDNA3 mammalian
expression vector (Invitrogen, San Diego, CA) under the control of the
cytomegalovirus (CMV) early promoter (CMV Core1-191).
Alternatively, the PCR amplified genomic region was inserted into the
mammalian expression vector pBabe/puro bearing the Moloney murine
leukemia virus long terminal repeat (MuLV LTR). A 2.4-kilobase human
p53 promoter sequence (15) fused with the chloramphenicol acetyltransferase (p53-CAT), kindly provided by David Reisman (University of South Carolina), was used as a reporter plasmid to study
the role of the HCV core protein on the p53 promoter.
COS7 and HeLa cells were
obtained from the American Type Culture Collection (Rockville, MD) and
grown in Dulbecco's modified Eagle's medium supplemented with 10%
fetal calf serum. Cells were transfected with the reporter (p53-CAT)
and an effector (HCV core) plasmid using lipofectamine (Life
Technologies, Inc.). Protein extracts were prepared 48 h after
transfection as described previously (9), and cell lysates were assayed
for CAT activity. To test the normalization of transfection efficiency,
duplicate sets of transfections were performed using pSV-gal and a
reporter plasmid, with or without the effector plasmid DNAs. One
transfection set was tested for expression of
-galactosidase by cell
staining with
5-bromo-4-chloro-3-indolyl-
-D-galactopyranoside (9). A
comparable number (15-20% variation) of blue transfected cells expressing
-galactosidase was observed. The other transfection set
was used for CAT assay. The acetylated and nonacetylated forms of
[14C]chloramphenicol were separated by thin layer
chromatography, autoradiographed, and scanned by a Molecular Dynamics
PhosphorImager. The level of CAT activity was calculated as the
percentage of the two acetylated forms of chloramphenicol relative to
the total amount of [14C]chloramphenicol. Duplicate
transfection experiments were repeated at least three times to verify
the reproducibility of the results.
p53 mRNA synthesis, from the
transformed primary REF, was studied by RT-PCR as described previously
(16). Transformed REF cells were prepared by cotransfection with the
core gene construct and the cooperative H-ras oncogene as
described earlier (11). Briefly, cells were fed with fresh culture
medium 2-4 h before transfection. Cells were transfected with HCV core
gene (1 µg) alone or together with H-ras gene (1 µg) and
carrier salmon sperm DNA (18-19 µg) by calcium phosphate
coprecipitation (Bethesda Research Laboratories, Gaithersburg, MD). The
cells were washed with phosphate-buffered saline, fed with fresh medium
at 20 h post-transfection and refed every 4-6 days.
Morphologically transformed cells were separated after 3 weeks
following transfection. For negative control, a plasmid containing the
oncogene alone and the vector or antisense orientation of the HCV core
plasmid were used for comparison. Transformed cells were treated with
acid guanidinium thiocyanate-phenol-chloroform for extraction of the RNA. First strand cDNA was synthesized using random primer and avian myeloblastosis virus-reverse transcriptase. Sense
(5-GAGGCGCTGCCCCCACCATGA-3
, nucleotide positions 734-753) and
antisense (5
-AGCTCTCGGAACATCTCGAAGC-3
, nucleotide positions
1224-1245) synthetic oligonucleotide primers corresponding to the
nucleotide sequence of the p53 gene (17) were used in the RT-PCR for
the amplification of a specific genomic sequence. These selected
primers used in the RT-PCR amplification represent a conserved sequence
of both human and rat p53. A p53 cDNA, kindly provided by Arnold
Levine (Princeton University, NJ), was used as a positive control in
PCR amplification. A PCR amplified ~490-base pair fragment from the
p53 gene plasmid DNA was isolated by 1.2% agarose gel electrophoresis.
The DNA band from p53 plasmid was excised, eluted using an ultra-free
MC column (Millipore Corporation, Bedford, MA), and radiolabeled with
[
-32P]dCTP by random priming with a commercially
available kit (Boehringer Mannheim) for use as a probe. Reaction
products from different cycles of PCR were analyzed by 1.2% agarose
gel electrophoresis followed by Southern blot hybridization. The
autoradiogram was densitometrically scanned (Molecular Dynamics), and
the level of p53 expression in experimental and negative control cells
was compared.
A cotransfection assay was used to investigate the role of the HCV
core gene product on the transcription of the human p53 gene. COS7
cells were cotransfected with the plasmid encompassing the human p53
promoter linked to a reporter CAT gene (p53-CAT) and increasing amounts
of CMV Core1-191 plasmid DNA. The vector alone was also
used as a negative control in the cotransfection assay. A
representation of the CAT assay result is shown in Fig.
1A. Results from this experiment suggested that the core protein inhibits p53 promoter activity in a
dose-dependent manner. The CAT activity decreased
(20-85%) as the quantity of CMV Core1-191 plasmid DNA
was increased in the transfection of cells (Fig. 1A,
lanes 1-5). A similar effect was observed utilizing the
MuLV LTR-driven HCV core gene in a transfection with the human p53 promoter reporter construct in the transient transfection assay (Fig.
1B). An in vitro transient assay using a mouse
p53-CAT construct and the CMV Core1-191 plasmid DNAs was
also performed. HCV core protein displayed repressor activity on the
mouse p53 promoter (data not shown). Taken together, these results
suggested that repression of p53 promoter activity may be attributed to
the exogenous expression of the HCV core protein.
To determine whether HCV core protein-mediated p53 transcriptional regulation is cell type-specific or may be influenced by the endogenous expression of integrated E6 from human papilloma virus 18, we chose to use human cervical carcinoma (HeLa) cells. A CAT assay was performed by transfection of p53-CAT and different doses of the HCV core gene. The mean results from at least three independent experiments are shown in Table I. The results indicated that the inhibition of p53 promoter activity by the HCV core protein was not limited to a specific function in COS7 cells. The inhibition of p53 promoter activity by the core protein might be due to a phenomenon called squelching (18), where high levels of cotransfected activator proteins have been shown to repress expression of certain genes through sequestration of coactivators away from the promoter. To exclude the possibility of squelching in the inhibition of p53 promoter activity by HCV core protein, the core-mediated activation of the c-myc promoter was tested. Under the same conditions, the core protein stimulated the human c-myc promoter (>400% as the index) and inhibited p53 promoter (68% as the index) activity in COS7 cells (data not shown). Additionally, the dose-dependent regulation of p53 promoter activity (Fig. 1A) suggested that the suppression is not due to squelching.
|
To identify the domain responsible for suppression of p53 promoter
activity, a full-length clone and deletion mutants of the core gene
encompassing different lengths of amino acids (amino acids 1-55,
1-80, 1-122, and 80-191) were used in a CAT assay. The core gene
deletion mutants were tested for protein expression by an in
vitro transient expression. The CAT assay results of transcriptional regulation of the p53 promoter by the full-length and
HCV core gene deletion mutants and vector DNA are shown in Fig.
2. The results indicated that the core protein domain
required for the majority of p53 repression is located between amino
acid positions 80 and 122.
To determine whether the endogenous p53 gene is repressed by the HCV core gene in HCVcore/H-ras transformed REF cells, the p53 mRNA level was measured by semiquantitative RT-PCR. The level of p53 mRNA present in the primary REF cells and HCV core transformed REF cells appeared to be similar. This observation is inconsistent with the CAT assay results presented here. However, it is possible that the level of the HCV core protein expression is different in HCV core/ras transformed REF cells than in an in vitro transient assay. HCV core protein-mediated repression of p53 may be an early event that precedes cellular transformation. Therefore p53 expression is no longer relevant in the transformed REF cells. Because p53 maintains the genetic integrity of cells by controlling progression through the cell cycle, the loss of p53 function appears therefore to be associated with increased genetic instability and the accumulation of mutations, which likely precede oncogenic transformation (19). Together, our observations suggest that the HCV core protein may exert a biological role for the promotion of cell growth by repression of p53 transcription during persistent infection. However, we did not observe a clear relationship between p53 and HCV core protein expression at this time, and the in vivo function of the core protein remains unclear.
Viral proteins may influence cellular genes, which in turn may be involved in the negative regulation of oncogenes or tumor suppressor genes. Inactivation of cellular genes may be a mechanism for the disruption of normal cell growth (20). Additionally, host factor has been identified as an important component for modulation of RNA virus replication (21). The HCV core protein is highly basic (isoelectric point 12.05) and could in principle show affinity toward nucleic acids and translocate to the nucleus during the mitotic phase, when the nuclear membrane is absent (22). Regions responsible for RNA and ribosome binding activities are probably located in the amino-terminal portion of the putative core protein (23). However, the presence of a putative DNA-binding motif, nuclear localization signals, phosphorylation sites, and the appearance of the core protein in the nucleus suggest its possible function as a gene regulatory protein (9, 24-27). Three different core protein products of ~21 (p21), 19 (p19), and 16 kDa (p16) have been reported (26). Both p21 and p19 displayed a cytoplasmic localization, whereas p16 shows localization to the nucleus. In regard to HCV genotype 1a, the production of the truncated p16 was associated with an amino acid substitution at codon 9 to a lysine residue. In contrast, the core protein of genotype 1b has been shown to lack nuclear localization (4, 26). Whether the difference in nuclear localization of the core protein is genotype-specific or cell type/cell cycle-specific or whether p16 is synthesized during virus replication in the infected cells remains to be examined. It is also not clear at this time if translocation of the putative core protein into the nucleus is affected by the expression of other HCV-associated proteins. HCV core protein exhibits promoter-specific differences in its mode of action. However, the mechanism by which the core protein regulates transcription remains to be elucidated.
Repression of the endogenous human p53 gene may have a biological implication in the development of hepatocellular carcinoma. The p53 gene encodes a tumor suppressor protein involved in maintaining the genetic integrity of the cell. Consistent with this, somatic mutations that are strongly implicated in the etiology of sporadic human malignancies, and germ line mutations in p53 are associated with a number of inherited cancers (19). A large number of patients with hepatocellular carcinoma are exposed to hepatitis B and/or hepatitis C virus, and a p53 mutation is found in a significant number of these patients (28). Reduced or inactivated p53 in HCV-infected cells would thus lead to the suppression of cell cycle arrest, leading to rapid progression through the requisite DNA damage repair cycle prior to genomic replication. Several DNA tumor viruses have been shown to interact with the p53 protein, functionally disabling p53 in the infected cells and possibly contributing to virus-dependent transformation (29-31). Recent studies suggest that retroviruses may differ from DNA tumor virus by influencing p53 transcription rather than directly interacting with p53 protein. Human immunodeficieny virus transactivator protein Tat transcriptionally represses p53 expression in T-cells, suggesting that Tat-mediated repression may contribute to human immunodeficieny virus-associated pathologies (32). Similarly, human T-cell leukemia virus type 1 Tax protein may promote malignant transformation through the repression of p53 transcription (33).
Cancer is a multi-step process that requires a cumulative effect altering both positive and negative regulators of cell proliferation and cell survival (34, 35). Inactivation of p53 is an important event in human cancer (19, 36). However, with the exception of functional inactivation of the p53 protein by viral proteins (33, 37), products of the MDM2 gene (38, 39) and PAX (40) and all previously reported examples of p53 inactivation in human tumors have been due to mutations within the p53 gene or gross chromosomal rearrangement within the p53 locus. Inhibition of p53 transcription by the core protein of HCV may serve as an important factor in this multi-step process. In addition, it is conceivable that the inappropriate expression of core protein (in the absence of viral morphogenesis) may contribute to malignancy by activating specific target genes, as well as by inactivating other inhibitory genes in addition to p53. Indeed, further study is necessary to correlate the expression level of p53 and core protein in HCV-mediated hepatocellular carcinoma.
We thank Robert B. Belshe for helpful discussions, Michael Houghton for providing the HCV cDNA (Blue4/C5p-1), Arnold Levine for p53 cDNA, David Reisman for the p53-CAT construct, and Kathy Banker for preparation of the manuscript.