Institute for Virology, Johannes-Gutenberg University Mainz, Obere Zahlbacher Straße 67, 55131 Mainz, Germany1
Author for correspondence: Ralf Bartenschlager. Fax +49 6131 393 5604. e-mail bartnsch{at}mail.uni-mainz.de
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Introduction |
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HCV genome organization |
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Virus replication |
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The dynamics of HCV replication can be deduced from the rapid rates of virus production and emergence of mutants. A careful analysis of viral dynamics during antiviral treatment of patients with IFN- revealed a virion half-life of 35 h and a clearance and production rate of ~1012 particles per day (Zeuzem et al., 1998
; Neumann et al., 1998
; Ramratnam et al., 1999
). Although in absolute amounts these numbers are high, they are not with respect to a single cell. Assuming that ~10% of the hepatocytes of a liver are infected and that a liver contains ~2x1011 hepatocytes, this would correspond to a virion production rate of 50 particles per hepatocyte per day (Neumann et al., 1998
).
Another feature of HCV replication is the rapid generation of virus variants. In fact, based on the genomic variability in a small region of NS5B, HCV has been classified into at least six genotypes each with several subtypes (Simmonds et al., 1993 ). Even within a patient HCV does not exist as a single entity but rather as a swarm of microvariants of a predominant master sequence, a phenomenon that has been referred to as quasispecies (for a review see Holland et al., 1992
). The production of such a large number of variants is primarily due to the high error rate of the viral RdRp that, based on analogies with RdRps of other plus-strand RNA viruses, is expected to be in the range of 10-4. This high error rate is reflected by the high mutation rate observed in patients or experimentally inoculated chimpanzees. Using comparative sequence analyses of HCV genomes isolated over intervals of 8 or 13 years a mutation rate of 1·44x10-3 or 1·92x10-3 base substitutions per site per year was found, respectively (Ogata et al., 1991
; Okamoto et al., 1992
). The high variation observed with HCV replication may also account for the fact that a significant fraction of virus genomes appear to be defective (Martell et al., 1992
).
Owing to the lack of a convenient animal model and an efficient cell culture system our current understanding of the molecular mechanisms of HCV replication is based primarily on analogies to the closely related flavi- and pestiviruses and on the characterization of recombinant HCV proteins. Using this limited information the HCV replication cycle can be summarized as follows (Fig. 2): (1) penetration of the host cell and liberation of the genomic RNA from the virus particle into the cytoplasm; (2) translation of the input RNA, processing of the polyprotein and formation of a replicase complex associated with intracellular membranes; (3) utilization of the input plus-strand for synthesis of a minus-strand RNA intermediate; (4) production of new plus-strand RNA molecules which in turn can be used for synthesis of new minus strands, for polyprotein expression or packaging into progeny virions; (5) release of virus from the infected cell.
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Apart from this route, HCV as well as other members of the Flaviviridae family may enter the cell by binding to low-density lipoprotein (LDL) receptors. Based on the observation that HCV particles are associated with beta-lipoproteins (Thomssen et al., 1992 ), Agnello et al. (1999)
analysed whether endocytosis of HCV is mediated by LDL receptors. Using in situ hybridization to determine HCV-RNA-positive cells, a direct correlation between the level of cell surface-expressed LDL receptor and the number of positive cells was found. This result and the finding that HCV does not bind to COS-7 cells unless they have been transfected with the LDL receptor gene (Monazahian et al., 1999
) suggest that HCV particles associated with LDL bind to this receptor. Whether interaction with the LDL receptor or CD81 leads to a productive infection remains to be determined.
While the nature of the HCV receptor is not known currently, the major envelope glycoprotein E2 is thought to be responsible for initiating virus attachment to the host cell because E2-specific antisera can block binding to cells (Rosa et al., 1996 ; Zibert et al., 1995
; Farci et al., 1996
). The role of E1 is less clear but the presence of a stretch of hydrophobic amino acids tentatively called the E1 fusion peptide, displaying similarities to the fusion peptides of paramyxovirus and flavivirus suggests that E1 is involved in membrane fusion (Flint et al., 1999
). To study the early steps in the HCV life-cycle, Lagging et al. (1998)
generated vesicular stomatitis virus (VSV) pseudotypes. They expressed chimeric envelope proteins composed of the HCV E1 or E2 ectodomains fused to the transmembrane and cytoplasmic domains of the VSV G protein. As indicated by the formation of plaques, a baby hamster kidney cell line (BHK-21), the human T-cell line MOLT4 and the human hepatoma cell line HepG2 were susceptible to infection with the pseudotypes, but the human cervical carcinoma cell line HeLa and the human embryonic lung cell line L-132 were not. However, only pseudotypes carrying either the E1 or the E2 ectodomain were used, not pseudotypes with both chimeric HCV proteins. This is surprising, because E2 acts as a chaperone for E1, which in the absence of E2 forms misfolded aggregates (Michalak et al., 1997
). Furthermore, E1 and E2 form stable heterodimers that most likely represent the native form found in the HCV envelope (Dubuisson et al., 1994
). Finally, studies with engineered cell surface-expressed E2 glycoproteins folded in a manner comparable to authentic E2 demonstrated that this protein alone did not enable cell fusion (Flint et al., 1999
).
Polyprotein translation and processing
Once inside the cytoplasm the genomic RNA is directly translated. Since HCV most likely does not encode a methyl transferase activity and replicates in the cytoplasm where such cellular enzymes are missing, the genome is not capped. Therefore, translation of the viral RNA is not mediated by a cap-dependent mechanism with ribosomes scanning along the RNA up to the first initiator AUG codon (depending on the isolate there are 45 start codons upstream of the polyprotein translation start site), but rather by an IRES (Tsukiyama-Kohara et al., 1992 ; Wang et al., 1993
). This RNA element residing approximately between nucleotides 40 and 355 forms four highly structured domains. With the exception of one report (Fukushi et al., 1994
) the small domain I, forming a single stemloop between nucleotides 5 and 20, was shown to be dispensable for translation activity and the 5' border of the IRES was mapped between nucleotides 38 and 46 (Honda et al., 1996
; Rijnbrand et al., 1995
; Yoo et al., 1992
). The fact that deletion of the region encompassing domain I stimulates translation suggests a regulatory role of this sequence for polyprotein translation. Because of its 5' proximal position it may also be involved in RNA replication. Two oligopyrimidine tracts are present in the IRES, one in the apical loop of domain III and one between domain III and the small domain II. Domain IV consists of a small stemloop containing the polyprotein start codon at nucleotide position 342 and forms a pseudoknot via base-pairing with a loop in domain III. Since mutagenesis or insertion of AUG initiator codons upstream from the polyprotein start codon have little effect on IRES activity, ribosomes appear to bind in close proximity to the polyprotein initiator AUG with little or no scanning (Reynolds et al., 1996
; Rijnbrand et al., 1996
). The mapping of the actual border of the 3' end of the IRES is still a matter of debate. Most experimental evidence suggests that sequences of the core coding sequence, but not the core protein itself, are required for full IRES activity (Honda et al., 1996
; Reynolds et al., 1995
; Zhao et al., 1999
). However, whether the core-coding sequence is a real component of the IRES or is required to prevent unfavourable base-pairings of the IRES with downstream sequences, disturbing the structure of the 5' NTR, is not known. In agreement with the latter assumption purified 40S ribosome subunits were found to bind to an IRES lacking core-coding sequences (Pestova et al., 1998
). In the same report it was also shown that the HCV IRES binds specifically to the 40S ribosome subunit and does not require any additional translation factors. This property is unique among all eukaryotic RNAs and resembles the interaction of the prokaryotic 30S ribosome subunit with the ShineDalgarno sequence (Pestova et al., 1998
). The IRES elements of picornaviruses require additional cellular factors for binding of the 40S ribosome subunit.
Activity of the HCV IRES is influenced by several factors. First, the X-tail at the very 3' end of the HCV genome appears to enhance IRES-dependent translation by an as yet unidentified mechanism (Ito et al., 1998 ). Second, several cellular factors have been demonstrated to bind to the HCV IRES and, in most cases, stimulate translation. These include polypyrimidine-tract-binding protein (PTB) (Ali & Siddiqui, 1995
; Kaminski et al., 1995
), the La antigen (Ali & Siddiqui, 1997
), heterogeneous nuclear ribonucleoprotein L (Hahm et al., 1998
) and as yet unidentified proteins with apparent molecular masses of 120, 87 and 25 kDa (Fukushi et al., 1997
; Yen et al., 1995
). The requirements for cellular factors for IRES activity may also explain the dependence on the cell cycle. Using cell lines stably expressing bicistronic reporter constructs with a cap-dependently expressed upstream reporter and a downstream reporter translated from the HCV IRES it was found that IRES-dependent translation was greatest in mitotic and lowest in quiescent (G0) cells (Honda et al., 2000
). One possible explanation would be that HCV translation is regulated by cellular proteins that vary in abundance or activity during the cell cycle.
Directed by the IRES, the polyprotein is translated at the rough endoplasmic reticulum (ER) and cleaved co- and post-translationally by host cell signalases and two viral proteinases. In the last few years a wealth of information regarding the mechanisms of polyprotein processing has been published. It is beyond the scope of this review to summarize all of them and the interested reader is referred to recently published reviews (Bartenschlager, 1999 ; De Francesco et al., 1998
; Reed & Rice, 1998
). As deduced from hydrophobic sequences preceding the cleavage sites and the dependence on microsomal membranes, the CNS2 region is processed by host signal peptidases cleaving at the C/E1, E1/E2, E2/p7, p7/NS2 junctions (Fig. 1
) (Grakoui et al., 1993b
; Hijikata et al., 1991
; Lin et al., 1994a
; Mizushima et al., 1994
). The production of processing intermediates, most notably an E2p7NS2 protein, indicates that not all cleavages within the structural region are cotranslational. Furthermore, a second post-translational cleavage close to the carboxy terminus of the core protein takes place, removing the E1 signal sequence by an as yet unidentified cellular enzyme (Santolini et al., 1994
; Hüssy et al., 1996
). Processing between NS2 and NS3 is a rapid intramolecular reaction and is accomplished by the NS23 proteinase (Grakoui et al., 1993a
; Hijikata et al., 1993a
; Santolini et al., 1995
). Efficient cleavage at this site requires the 130 carboxy-terminal residues of NS2 and the first 180 amino acids of NS3. Within the NS2 sequence His-952 and Cys-993 are essential for enzymatic activity (Grakoui et al., 1993a
; Hijikata et al., 1993a
) and it has been proposed that NS23 is a cysteine proteinase with His-952 and Cys-993 forming a catalytic dyad or, together with Glu-972, a catalytic triad (Gorbalenya & Snijder, 1998
). Alternatively, owing to the activation by zinc and the inhibition by chelating agents like EDTA, the NS23 proteinase might be a zinc-dependent metalloproteinase (Hijikata et al., 1993a
). However, since zinc is required for proper folding of the NS3 proteinase domain it is not known whether zinc is bound by the NS2 domain too or whether the activating effect is due to proper folding of the NS3 domain. Alternatively, the zinc bound by the NS3 domain might play an essential role in catalysis (Wu et al., 1998
).
Processing of the NS35B region is mediated by the NS3 proteinase with the following preferred but not obligatory order of cleavages: NS3/4ANS5A/B
NS4A/B
NS4B/5A (Bartenschlager et al., 1994
; Failla et al., 1995
; Lin et al., 1994b
; Tanji et al., 1994
). Processing at the NS3/4A site is a cotranslational intramolecular reaction whereas cleavage at the other sites can be mediated intermolecularly. However, the HCV proteins most likely form a stable higher-order complex associated with intracellular membranes (Hijikata et al., 1993b
; Ishido et al., 1998
; Koch & Bartenschlager, 1999
; Lin et al., 1997
; Neddermann et al., 1999
). Therefore, even after liberation of NS3 from the polyprotein, the enzyme and its substrate are in very close proximity.
Although enzymatically active on its own, proteolytic activity of NS3 is greatly stimulated by NS4A both in transfected cells and in various in vitro assay systems. Coprecipitation studies demonstrated the formation of a detergent-stable complex and the interaction domains have been mapped to the ~30 amino-terminal residues of NS3 and a 12 residue sequence in the centre of NS4A (Bartenschlager et al., 1995 ; Failla et al., 1995
; Lin et al., 1994b
, 1995
; Satoh et al., 1995
; Tanji et al., 1995a
), which can be supplied as a synthetic peptide without loss of activation function (Butkiewicz et al., 1996
; Koch et al., 1996
; Shimizu et al., 1996a
; Steinkühler et al., 1996
; Tomei et al., 1996
). Since mutational ablation of complex formation drastically reduces proteinase activity, it was assumed that interaction of NS4A with NS3 induces conformational changes within the proteinase domain, enhancing enzymatic activity. This hypothesis was confirmed by the resolution of the three-dimensional X-ray structure of the NS3 proteinase (Love et al., 1996
) or NS3 complexed with a synthetic NS4A peptide (Kim et al., 1996
; Yan et al., 1998
). Overall, the enzyme adopts a chymotrypsin-like fold and consists of two
-barrel domains separated by a deep cleft where the amino acid residues forming the catalytic triad are located. The carboxy-terminal domain forms a six-stranded
-barrel and its structural integrity requires a tetrahedrally coordinated zinc ion (De Francesco et al., 1996b
; Stempniak et al., 1997
). In the absence of NS4A the ~30 amino-terminal NS3 residues are flexible and extend away from the protein, whereas in the presence of the cofactor, this region is highly structured and participates in an eight-stranded
-barrel with one strand contributed by NS4A tightly intercalated via several side chains into the NS3 domain. A second structural rearrangement upon NS4A binding leads to an optimization of the geometry of the catalytic triad, accounting most likely for the enhancement of proteinase activity (Love et al., 1998
; Yan et al., 1998
). In addition to serving as a proteinase cofactor, NS4A has two further functions that might contribute to efficient polyprotein cleavage and replication. First, increasing the metabolic stability of NS3 that in the absence of NS4A is degraded very rapidly, and second, anchoring NS3 to intracellular membranes where most of the HCV proteins are located, thereby increasing the local enzyme:substrate concentration and facilitating the formation of a membrane-associated replicase complex (Tanji et al., 1995a
; Wölk et al., 2000
).
A feature conserved in many plus-strand RNA virus families is that proteinase and NTPase/helicase activities reside in a single polypeptide, and the same is found with NS3 of HCV. In fact, two lines of evidence suggest an interdomain coupling.
(1) Although the catalytic efficiencies of the isolated proteinase domain and full-length NS3 are very similar this is not the case with the helicase. A comparison of RNA unwinding activities of a recombinant single chain NS4Afull-length NS3, a full-length NS3 without NS4A and the isolated helicase domain suggests that the presence of the proteinase domain and NS4A enhance helicase activity (Howe et al., 1999 ). This enhancement may be due to, first, a stabilization of the helicase fold in the full-length complex (Yao et al., 1999
) and, second, RNA binding sites in the proteinase domain contributing to helicase substrate binding (Gallinari et al., 1998
).
(2) The resolution of the three-dimensional X-ray crystal structure of a single chain fusion protein of full-length NS3 and the NS4A activator domain revealed that the proteinase and the helicase/NTPase domains are segregated and connected by a flexible single strand (Yao et al., 1999 ). Interestingly, in this molecule the proteinase active site is occupied by the carboxy terminus of NS3. This observation suggests an autoinhibition of the proteinase that may be overcome by interaction with the polyprotein substrate, inducing structural changes and displacing the inhibitor from the active site (Barbato et al., 1999
; Yao et al., 1999
).
RNA replication
As deduced from several coprecipitation studies (Hijikata et al., 1993b ; Ishido et al., 1998
; Lin et al., 1997
), most or all of the HCV polyprotein cleavage products, in particular NS35B, form a replicase complex associated with intracellular membranes that most likely contains cellular proteins too. The formation of such a complex is a feature typical of plus-strand RNA viruses like poliovirus or flaviviruses (Bolten et al., 1998
; Westaway et al., 1997
) and it allows the production of viral proteins and RNA in a distinct compartment. In addition, complex formation permits the tight coupling of functions residing in different polypeptide chains.
The individual steps underlying RNA replication are largely unknown. It is obvious that the NS5B RdRp is the key player catalysing the synthesis of minus- and plus-strand RNA. In vitro the enzyme prefers a primer-dependent initiation of RNA synthesis, either by elongation of a primer hybridized to an RNA homopolymer or via a copy-back mechanism when using heteropolymeric templates (Al et al., 1998 ; Behrens et al., 1996
; Ferrari et al., 1999
; Lohmann et al., 1997
; Yamashita et al., 1998
; Yuan et al., 1997
). In the latter case, sequences at the 3' end fold back intramolecularly and hybridize, generating a 3' end that can be used for elongation, resulting in a product approximately twice the length of the input template. However, at least under certain experimental conditions, HCV NS5B, as well as the RdRp of the closely related pestivirus bovine viral diarrhoea virus (BVDV), can initiate RNA synthesis de novo and it is plausible that this mechanism also operates in vivo (Kao et al., 1999
; Oh et al., 1999
; Luo et al., 2000
; Zhong et al., 2000
). Interestingly, when using high concentrations of GTP or ATP, HCV NS5B can synthesize RNA primer independently from the homopolymeric templates poly(C) and poly(U), respectively, whereas RNA synthesis from poly(I) or poly(A) templates is primer-dependent irrespective of the NTP concentration (Luo et al., 2000
). These results suggest that the enzyme can probably only use GTP or ATP for de novo initiation. It is interesting to note that the 5'-terminal nucleotides of plus- or minus-strand RNA are guanosine or adenine, respectively. The dependence of de novo initiation on high GTP or ATP concentration and the inability of the enzyme to initiate RNA synthesis from poly(A) templates also explains why some groups only observed primer-dependent RNA synthesis with their in vitro assays (Al et al., 1998
; De Francesco et al., 1996a
; Ferrari et al., 1999
; Lohmann et al., 1999a
; Yamashita et al., 1998
).
A still unresolved question is how template specificity is achieved. In most studies NS5B was found to utilize and bind to virtually every RNA (and even DNA) template, albeit with different efficiencies. However, using electrophoretic mobility shift assays and competition experiments, Cheng et al. (1999) provided evidence for a preferential binding of recombinant NS5B to a sequence in the 3' coding region of NS5B. Alternatively, template specificity may be accomplished by the high local concentration of NS5B and the RNA genome from which it is translated, within the replicase complex. A preferential cis-activity of NS5B also would discriminate against RNA genomes containing stop codons or frame-shift mutations introduced by errors of the viral replicase, reminiscent of what has been described for poliovirus (Novak & Kirkegaard, 1994
). While in vitro NS5B is able to copy even a complete full-length HCV genome (Lohmann et al., 1997
), it is very likely that in vivo additional viral or cellular factors are required. Possible viral candidates are the NS3 helicase, by unwinding stable structures in the RNA template and facilitating replication, or the phosphoprotein NS5A. Although the replication function of this protein could not be studied thus far, by analogy to other RNA viruses it is tempting to speculate that NS5A is involved in regulation of RNA replication. For example, in the case of VSV, RNA synthesis occurs only after phosphorylation of the P protein (Barik & Banerjee, 1992
). In the case of the Dengue virus NS5 replicase, subcellular localization and interaction with NS3 are altered by the level of phosphorylation (Kapoor et al., 1995
). Phosphorylation of NS5 or NS5A is a biochemical property conserved in all members of the flaviviruses studied thus far, suggesting that this modification plays an important role in the life-cycle of these viruses (Reed et al., 1998
).
In addition to viral proteins, cellular components are probably involved in RNA synthesis, too. One candidate is PTB, found to specifically interact with sequences at the 3' NTR (Chung & Kaplan, 1999 ; Ito & Lai, 1997
; Tsuchihara et al., 1997
). Another candidate is glyceraldehyde-3-phosphate dehydrogenase, binding to the poly(U)-sequence in the 3' NTR (Petrik et al., 1999
). Finally, cellular proteins provisionally called p87 and p130 were identified by UV-cross linking experiments with the X-tail sequence, but the nature of these proteins remains to be determined (Inoue et al., 1998
).
Proteins from other viruses may also affect HCV replication. It is interesting to note that the cell lines supporting HCV replication the best are, in most cases, (co-)infected with other viruses like human T-lymphotropic virus type I (in the case of the MT2 T-cell line), a murine retrovirus (in the case of the MOLT4-Ma T-cell line) or EpsteinBarr (EBV) (in the case of the Daudi B-cell line). Furthermore, Sugawara et al. (1999) observed that HCV-positive patients with a hepatocellular carcinoma frequently have a high EBV load, and presented evidence that the enhancement of HCV replication is mediated by EBV nuclear antigen 1. Since this protein is localized in the nucleus, whereas HCV replication occurs in the cytoplasm, the enhancement may be due to an indirect effect, e.g. via activation of transcription of cellular genes, although there is no cellular promoter with an EBV nuclear antigen 1 binding motif known.
Virion assembly and release
In the absence of systems allowing the production of biochemical amounts of virus particles, the assembly of HCV cannot be studied in detail. One potential approach to overcome this limitation is the production of virus-like particles (VLPs) by expression of the structural proteins in heterologous systems, but for HCV this turned out to be very difficult. Thus far there are two reports describing the formation of VLPs. In one report the full-length HCV coding region was transiently expressed with the vaccinia virus T7 hybrid system in HeLa G cells (Mizuno et al., 1995 ). Particles with diameters of ~30 and 45 nm, assumed to correspond to non-enveloped core-like particles and enveloped particles, respectively, were found. In another report, Baumert et al. (1998)
used recombinant baculoviruses to express a region of the HCV genome corresponding to a part of the 5' NTR and the CE2 region in insect cells. They observed VLPs containing selectively encapsidated HCV RNA. Although this report is promising, the efficiency of VLP formation still appears rather low, because the majority of the HCV proteins form aggregates and only a minority assemble to produce VLPs. Furthermore, these particles reside in intracellular membrane vesicles and are not transported out of the cell.
Particle formation may be initiated by core protein interacting with the RNA genome. Although in vitro core protein binds to RNA without detectable specificity, recent evidence indicates a preferential intracellular binding to RNA sequences in the 5' half of the HCV genome (Shimoike et al., 1999 ). Such binding may not only accomplish a selective packaging of the plus-stranded genome but also appears to repress translation from the IRES, suggesting a potential mechanism to switch from translation/replication to assembly (Shimoike et al., 1999
). Whether the core protein forms a distinct nucleocapsid structure or a rather non-structured ribonucleoprotein complex with the RNA genome is not known. Certainly, core protein interacts with itself and the sequences required for this interaction have been mapped to the amino-terminal 115 residues (Matsumoto et al., 1996
). Within this region a tryptophan-rich primary interaction domain was identified between residues 82 and 102 that is masked in the full-length core protein and revealed only under certain experimental conditions (Nolandt et al., 1997
).
A feature typical of the HCV E proteins is their retention in the ER compartment when expressed with various heterologous systems in cell culture (Dubuisson et al., 1994 ). The retention is achieved by signals in the transmembrane domains of E1 and E2 and it has been shown to be a true retention in the ER (Duvet et al., 1999
; Cocquerel et al., 1999
). This observation suggests that viral nucleocapsids acquire their envelope by budding through ER membranes. In this case the virus may be exported via the constitutive secretory pathway. In agreement with this assumption, complex N-linked glycans were found on the surface of partially purified virus particles, suggesting virus transit through the Golgi (Sato et al., 1993
). However, since HCV particles tend to associate with cellular components it remains to be determined whether these glycans are present on the E proteins or on cellular proteins associated with HCV particles.
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Model systems to study HCV replication |
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Animal models
The only animal that can be infected with HCV reproducibly is the chimpanzee, but its use is limited by ethical reasons, its scarcity and high maintenance costs. In an attempt to establish a small animal model Xie et al. (1998) experimentally inoculated Tupaias (T. belangeri chinensis), a species shown to be susceptible to infection with the hepatitis B virus (Walter et al., 1996
; Yan et al., 1996
). However, only about one-quarter of the animals became infected with HCV and developed either transient or intermittent viraemia with rather low titres. Recently, two potential alternatives have been described for the propagation of hepatitis B viruses that might be used for HCV as well. Both systems are based on the engraftment of human liver tissue into immunocompromised mice. In the so-called trimera system lethally irradiated mice are rescued with SCID mouse bone marrow cells and used as transplant recipients for human liver pieces infected ex vivo (Ilan et al., 1999
). The other system uses transgenic mice containing the urokinase-type plasminogen activator gene whose expression under control of the liver-specific albumin promoter is hepatotoxic and destroys a high proportion of liver cells. These mice were crossed to mice that due to a recombination activation gene 2 knockout lack mature B and T lymphocytes. Upon transfer of liver cells from an animal susceptible to infection with a hepadnavirus into these mice, the parenchymas of the regenerating mouse livers were composed of up to 90% of the transplanted cells and after infection with the hepadnavirus these mice became highly viraemic (Petersen et al., 1998
). Although both mouse systems have thus far only been used for the propagation of hepadnaviruses, the methodologies might be used for HCV as well.
Infection of cultured cells with HCV
In the last few years several cell culture propagation systems for HCV have been described that are based on the infection of primary cell cultures or cell lines or the cultivation of primary cells from chronically infected patients. However, thus far these systems suffer from poor reproducibility and a low level of HCV replication that can be measured only with highly sensitive techniques. In many cases the minus-strand RNA intermediate that is only formed upon productive replication was measured by strand-specific RTPCR, but owing to false priming during the RTPCR process this assay alone is not really reliable. Several modifications of this method have been developed (Gunji et al., 1994 ; Lanford et al., 1994
), but scepticism remains. Therefore, in addition to minus-strand RNA detection, several other indicators for productive replication have been used, such as an increase of plus-strand RNA during the cultivation period (determined either by b-DNA assay or quantitative RTPCR), the inhibition of replication upon incubation of the cells with IFN-
or antisense oligonucleotides, the transmission of cell-culture-grown HCV to naive cells, the sequence analysis of HCV genomes or genome fragments to demonstrate genomic variability and selection of variants upon infection and cultivation, the detection of viral antigens by immunofluorescence or flow cytometry and the long-term propagation of HCV. A representative selection of these reports is given in Table 1
and only a few will be described in some detail here.
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Since primary cell cultures are not routinely available, most attempts have been undertaken with cell lines of human origin. With respect to hepatoma cell lines, the most detailed results are available for the non-neoplastic cell line PH5CH (Ikeda et al., 1998 ; Kato et al., 1996
). Evidence for HCV replication in these cells is based on (1) the detection of HCV RNA up to 100 days post-infection, (2) the loss of plus-strand RNA upon incubation of the infected cells with IFN-
, and (3) a strong selection for HCV variants in the hypervariable region 1 (HVR1) of the E2 protein, suggesting that only certain variants can bind to or replicate in these cells. A similar decrease of complexity of viral quasispecies has been described for HCV propagated in primary human hepatocytes for up to 3 months (Rumin et al., 1999
).
T- and B-cells selected for high HCV replication have been derived from the T-cell lines MT-2 and MOLT-4 and the B-cell line Daudi. For example, an MT-2C cell clone was described that supports HCV replication for up to 198 days post-infection (Mizutani et al., 1996b ). By comparing the complete sequence of the HCV genome replicating in these cells with the sequences present in the inoculum it was found that only a limited virus population replicates in MT-2C cells (Sugiyama et al., 1997
), suggesting the selection of certain variants particularly adapted to these cells. Long-term propagation of HCV for more than 1 year has been described for the human T- and B-cell lines HPBMa10-2 and Daudi (Nakajima et al., 1996
), and virus could be transmitted several times to naive cells by cocultivation (Shimizu & Yoshikura, 1994
). To demonstrate infectivity of cell-culture-grown HCV in an animal, Shimizu et al. (1998)
inoculated a chimpanzee with ~103 genome equivalents present in the culture supernatants from Daudi cells that had been infected with HCV for 58 days. After ~5 weeks HCV RNA became detectable in the serum of the animal and vanished after week 25. Interestingly, the major HVR1 sequence in the serum of the animal corresponded to the predominant variant in the patient serum used for infection of Daudi cells. However, in PBMCs of the chimpanzee the major variant corresponded to the dominant variant found in Daudi cells and this variant was not found in the inoculum patient serum. These results suggest the selection of a lymphotropic HCV variant during cell culture passage.
Transfection of cell lines with cloned HCV sequences
Compared to the infection of cell lines with HCV-containing patient material, the introduction of cloned virus genomes is superior because the inoculum is well defined and can be generated in high quantities. Most importantly, the genome can be manipulated at will, permitting a detailed genetic analysis of viral functions. Although the production of infectious virus from cells transfected with cRNA (RNA generated by in vitro transcription of a cloned DNA copy of the viral genome) has been described for several plus-strand RNA viruses (Boyer & Haenni, 1994 ), this approach turned out to be very difficult for HCV. Up to now only two reports have been published describing the replication of a transfected HCV genome in the human hepatoma cell lines Huh-7 or HepG2 (Dash et al., 1997
; Yoo et al., 1995
). However, in both studies truncated HCV genomes were used that lacked the authentic 3' NTR. The replication competence of such genomes contradicts the finding that the highly conserved sequence at the very 3' end of the genome is essential for replication in vivo (Yanagi et al., 1999
; Kolykhalov et al., 2000
) and in cells transfected with selectable HCV replicons (unpublished results; see below). A clarification of this issue awaits the sequence analysis of the recloned 3' truncated RNAs and the successful infection of chimpanzees with culture medium from these cells.
Recently we have developed selectable subgenomic HCV RNA molecules replicating to high levels after transfection into the human hepatoma cell line Huh-7 (Lohmann et al., 1999b ). Based on the assumption that high expression levels of the structural proteins might be cytotoxic (Moradpour et al., 1998
) and the observation that for several plus-strand RNA viruses like alpha-, flavi- and pestiviruses the structural proteins are not required for RNA replication (Behrens et al., 1998
; Khromykh & Westaway, 1997
; Liljestrom & Garoff, 1991
), the sequences of the structural proteins were deleted. To allow selection for only those cells in which HCV will efficiently replicate, the gene encoding the neomycin phosphotransferase, conferring resistance to the antibiotic G418, was introduced downstream of the HCV IRES (Fig. 3
). A second IRES element was included to allow translation of the HCV NS proteins. Since we did not know whether NS2 was required for replication, two variants were generated spanning the NS25B or the NS35B region. Upon transfection of these bicistronic RNAs and selection of the cells with G418, only those supporting replication of these RNAs amplified the neo gene and developed resistance, whereas non-transfected cells and cells unable to support replication died. With this approach cell clones could be established with both the NS25B and the NS35B replicon, albeit with low efficiency. Surprisingly, these selected cells carried large amounts of HCV RNAs detectable by Northern blot, or after metabolic radiolabelling with 3[H]uridine, providing formal proof that these RNAs were actively replicating in the cells. Using these techniques we detected 10005000 RNA molecules per cell, which is several orders of magnitude higher compared to infection systems (Blight & Gowans, 1995
). As expected for a replicative intermediate, minus-strand RNA was present in ~10-fold molar lower amounts compared to plus-strand RNA. HCV proteins could be detected by immunoprecipitation after metabolic radiolabelling with 35[S]methionine (Lohmann et al., 1999 b
) or Western blot (K. Kurpanek & R. Bartenschlager, unpublished results) and were confined to the cytoplasm.
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Concluding remarks |
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Acknowledgments |
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References |
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