key: cord-0002009-6xf4o3oy
authors: Sung, Pil Soo; Shin, Eui-Cheol; Yoon, Seung Kew
title: Interferon Response in Hepatitis C Virus (HCV) Infection: Lessons from Cell Culture Systems of HCV Infection
date: 2015-10-07
journal: Int J Mol Sci
DOI: 10.3390/ijms161023683
sha: d722d17111a045ac6a1427a5ec6967285eea73e0
doc_id: 2009
cord_uid: 6xf4o3oy

Hepatitis C virus (HCV) is a positive-stranded RNA virus that infects approximately 130–170 million people worldwide. In 2005, the first HCV infection system in cell culture was established using clone JFH-1, which was isolated from a Japanese patient with fulminant HCV infection. JFH-1 replicates efficiently in hepatoma cells and infectious virion particles are released into the culture supernatant. The development of cell culture-derived HCV (HCVcc) systems has allowed us to understand how hosts respond to HCV infection and how HCV evades host responses. Although the mechanisms underlying the different outcomes of HCV infection are not fully understood, innate immune responses seem to have a critical impact on the outcome of HCV infection, as demonstrated by the prognostic value of IFN-λ gene polymorphisms among patients with chronic HCV infection. Herein, we review recent research on interferon response in HCV infection, particularly studies using HCVcc infection systems.

Hepatitis C virus (HCV) is a positive-stranded RNA virus in the family Flaviviridae, and it is estimated 130-170 million people are infected with HCV worldwide [1] . Acute HCV infection is spontaneously cured in 20%-30% of patients, but the majority of infected patients fail to clear the virus and develop chronic persistent infection [2] [3] [4] . In addition to a combination regimen of pegylated interferon (IFN)-α and ribavirin, direct acting antiviral drugs (DAAs) against HCV have been developed, and a high rate of sustained virological response (SVR) has been achieved by using these antiviral drugs [5] . However, the high cost of these drugs results in limited access in developing nations where the disease burden is high; therefore, there is still a need for the development of a prophylactic vaccine.

Until now, the pathogenesis of HCV infection has not been clearly elucidated yet. Importantly, the detailed mechanism of innate immune activation by HCV and its implications for viral persistence and treatment response have not been clearly explained. Therefore, understanding HCV-host interactions and immune responses are important novel therapeutics with a higher barrier to viral resistance can be developed [6] . However, there is no established small animal model for the study of the entire life cycle of HCV infection and immunopathogenesis [7] . Severe combined immunodeficiency mice grafted with human hepatocytes are the only small animals that can be infected with HCV, although they cannot exert adaptive immune responses [8] . Recently, genetically-humanized mouse models are being developed to recapitulate the entire life cycle of HCV [9, 10] , but these models have restricted replication of HCV, limiting their utility.

As an experimental tool, development of cell culture-derived HCV (HCVcc) systems has dramatically facilitated HCV research over the last 10 years. Here, we review recent advances in the research on innate immune response in HCV infection and focus primarily on interferon response of host cells.

It was not until 2005, more than 15 years after the discovery of HCV [11] , that the first efficient cell culture model of HCV became available. The identification of a clinical isolate (genotype 2a) that replicates efficiently in Huh-7 hepatoma cells [12] made the first cell culture system possible. This isolate was obtained from a Japanese patient with fulminant HCV infection and was called JFH-1 [13] [14] [15] . Viral particles produced by the transfection of Huh-7 cells with in vitro transcribed JFH-1 RNA could infect naïve cells in cell culture and the liver of chimpanzees in vivo [14] . The HCV virion particles derived from the cell culture system were named "HCVcc" [13] . Until now, only JFH-1 spontaneously replicates in Huh-7 cells without adaptive mutations and releases infectious virus particles [14, 15] .

After the discovery of JFH-1-based HCVcc system, other HCV cell culture systems with various genotypes were established. For genotype 2 cell culture systems, J6cc (genotype 2a) [16] and J8cc/DH8cc/DH10cc (genotype 2b) [16, 17] were developed. They replicated and propagated efficiently in Huh-7.5 cells, although they had adaptive mutations to facilitate their replication [16, 17] . The first genotype 1a strain, H77-S, replicated and released infectious particles in Huh-7 cells and immortalized human hepatocytes, although the amount of released virus was lower than JFH-1 [18, 19] . The Con1 (genotype 1b) cell culture system was also reported, but a very low level of replication has also limited its utility [20] . Recently, a new cell culture system of genotype 1a was developed. The TN genome with eight mutations (TNcc) [21] and H77C recombinant harboring 19 mutations (H77Ccc) replicated and spread efficiently in Huh-7.5 cells [22] . Recently, a cell culture system for infectious genotype 3a was also established by introducing adaptive mutations into the S310 strain [23] .

HCVcc system has some limitations that should be considered. The most important limitation is the restricted availability of genotypes established in cell culture models. Currently, HCVcc systems for genotypes 4, 5, and 6 are unavailable. For genotypes 1 and 2, only specific patient clones have been propagated in cell culture systems. It should be noted, however, that a new host factor, SEC14L2 was recently reported to enable replication of non-adapted HCV in hepatoma cells [24] . New cell culture system utilizing SEC14L2-expressing hepatoma cells may overcome the limited availability of HCVcc system. Another limitation of the current HCVcc system is the non-polarized nature of Huh-7-based cells [25, 26] . Hepatocytes are highly polarized in the liver and cell-to-cell transmission takes an important part in the spread of HCV, but the current HCVcc system does not reflect the viral spread occurring in the infected liver. In addition, Huh-7 cells are not fully differentiated [27] and, thus, have a defect in activation of the innate immune response by HCVcc infection [28] .

In primary human hepatocytes (PHHs), replication and virus production by HCVcc infection have been reported [27] , but it is difficult to obtain PHHs for experimental use. Immortalized human hepatocyte was reported to support HCV genome replication, virus assembly, and robust IFN response against the virus [19, [29] [30] [31] and, thus, can be used as an alternative. Differentiated hepatocyte-like cells (DHCs) induced from pluripotent stem cells have also been used for HCVcc infection [32] [33] [34] . DHCs were found to mount an efficient innate immune response after HCVcc infection, including the production of chemokines and type III IFNs [33] . Recently, DHCs from adipose tissue-derived human mesenchymal stem cells (AT-hMSCs) were used for HCVcc infection [35] , and the entry and replication of HCVcc were found to occur efficiently in DHCs from AT-hMSCs.

HCVcc infection systems provide a unique opportunity to study innate immune responses to HCV infection. Here, we focus mainly on recent advances in the study of interferon response in HCV infection.

In HCV-infected cells, viral RNA is sensed by retinoic acid-inducible gene I (RIG-I) and melanoma differentiation-associated protein 5 (MDA-5) in the cytoplasm and Toll-like receptor 3 (TLR3) in the endosome, which leads to downstream signaling that results in the induction of type III and I IFNs and other inflammatory cytokines [28, [36] [37] [38] [39] . Among these receptors, a role of MDA-5 in HCV sensing has remained controversial for several years, and it was recently proven that MDA-5 also participates in HCV sensing in the cytoplasm using HCVcc infection systems [28, 36, 40] .

Intracellular signals from RIG-I, MDA-5, and TLR3 are transmitted via mitochondrial antiviral signaling protein (MAVS) and Toll/IL-1 receptor domain-containing adaptor inducing IFN- (TRIF), respectively, which leads to the interferon regulatory factor-3 (IRF-3)-dependent induction of IFNs and NF-κB activation in HCV-infected cells [38, 39] . Similar to other viruses, HCV uses several mechanisms to interfere with the induction of IFNs, particularly NS3/4A protease. NS3/4A cleaves MAVS, which leads to the impairment of signaling and IFN production in response to HCV RNA [41] . MAVS cleavage by NS3/4A has also been confirmed in HCV-infected liver tissue [42] . NS5A also contributes to immune evasion from the host. IFN-γ expression is inhibited in NS5A-transgenic mice after adenoviral challenge, meaning that NS5A plays an important role toward establishment of chronic HCV infection [43] .

Despite HCV interference with the induction of IFNs, IFNs are endogenously produced by HCV-infected cells [28, 29, [44] [45] [46] . Both genotype 2a [28, 29, [44] [45] [46] and genotype 1a [29] were reported to activate intracellular interferon signaling pathways. IFNs are currently classified into three major classes: type I, type II, and type III. Among them, type I and III IFNs are considered innate immune response IFNs. Among type I IFNs, there are 13 IFN-αs, in addition to IFN-β, IFN-ω, IFN-ε, and IFN-κ [47] . IFN-λs (IFN-1 or IL-29; -2 or IL-28A; and -3 or IL-28B) are a new family of IFNs that have been designated as type III IFNs. Since the discovery of IFN-λs in 2003, their functions have been considered to overlap with type I IFNs because signaling via the IFN- receptor is similar to that via the IFN-α/β receptor. After binding to their receptors, type I and III IFNs initiate a signaling cascade through the Janus kinase (JAK)-signal transducer and activator of transcription (STAT) pathways. The cellular actions are then mediated by the induction of interferon-stimulated genes (ISGs) that have antiviral and/or immunomodulatory activity [48, 49] .

Recently, it was demonstrated that IFN-s are major IFNs produced by HCV-infected cells [28, [44] [45] [46] . IFN-s activate the same JAK-STAT pathway as type I IFNs [48] [49] [50] , thereby inducing a similar set of ISGs. Although the exact source of IFN-s in HCV-infected liver remains to be clarified, it seems that the production of IFN-s by HCV-infected hepatocytes results in the expression of ISGs, presumably through autocrine and/or paracrine signaling via the IFN-λ receptor [28, [44] [45] [46] .

Although HCV interferes with the induction of IFNs, continuous ISG up-regulation in HCV-infected liver has been demonstrated in chimpanzee models [51, 52] and HCV-infected patients [53, 54] . Interestingly, HCV RNA and ISG mRNA are detected simultaneously in hepatocytes from patients with chronic HCV infection [55] . This finding suggests that HCV infection potently stimulates the production of endogenous IFNs, which leads to ISG up-regulation in infected liver [55] , and that HCV survives under the ISG up-regulation perhaps due to the protein kinase R (PKR)-mediated suppression of ISG protein translation [56, 57] .

As a rapid response to type III and I IFNs, IFN stimulated gene factor 3 (ISGF3), which consists of tyrosine-phosphorylated STAT1 (PY-STAT1), tyrosine-phosphorylated STAT2 (PY-STAT2), and IRF9, mediates the induction of numerous ISGs, including STAT1, STAT2, and IRF9 themselves [47] . Recently, it was demonstrated that prolonged induction of a set of ISGs is mediated by unphosphorylated ISGF3 (U-ISGF3), which is composed of unphosphorylated STAT1 (U-STAT1), unphosphorylated STAT2 (U-STAT2), and IRF9 [58, 59] . The U-ISGF3 level is increased by sustained exposure to IFNs, and U-ISGF3 leads to enhanced expression of a set of ISGs (U-ISGF3-downstream ISGs, U-ISGs) [58] . In other words, there appear to be two phases of ISG expression following type III or I IFN stimulation. The initial rapid response is driven by the classical phosphorylated form of ISGF3, which is followed by a second, more prolonged response driven by U-ISGF3 [58] .

In line with this report, we recently demonstrated that endogenous production of type III and I IFNs by HCV infection increases the levels of U-ISGF3, composed of U-STAT1, U-STAT2, and IRF9 proteins [60] . Using HCVcc infection systems with immune-competent liver cells such as PHHs and TLR3-transfected Huh7 cells, we demonstrated that U-ISGF3 induces the expression of U-ISGs [60] .

As mentioned above, ISGs induced by endogenous type III or I IFNs are up-regulated in HCV-infected liver [53, 54, [60] [61] [62] . Representative ISGs that are maintained at high levels of expression include ISG15, IFI27, IFI44, Mx1, and OAS-1 [53, 54, [60] [61] [62] . These ISGs are regulated not only by ISGF3 but also by U-ISGF3, and they are mainly antiviral [58, 60] . We recently found that increased levels of U-STAT1, U-STAT2, and IRF9 are able to inhibit HCV RNA replication without exogenous IFN treatment [60] . This finding suggests that the sustained expression of ISGs by U-ISGF3 has antiviral activity against HCV in the infected liver but is insufficient to clear the virus.

Previously, it was demonstrated that patients with high levels of ISGs in their liver at baseline respond poorly to combined therapy with pegylated IFN- and ribavirin [53, 54, [60] [61] [62] [63] [64] . Moreover, it has been shown that increased ISG expression at baseline is a stronger predictor of a poor response to pegylated IFN-/ribavirin therapy than is the IL28B genotype [53] . Some reports have emphasized USP18 as a critical factor conferring unresponsiveness to exogenous IFN-α treatment by suppressing intracellular signaling [65] [66] [67] [68] . However, the mechanism underlying the increase and maintenance of USP18 protein levels in HCV-infected liver has not been clearly elucidated. Recently, we found that prolonged exposure to IFN- up-regulates U-ISGF3 and U-ISGs, including ISG15, and that ISG15 causes the refractoriness to exogenous IFN- treatment by stabilizing USP18 protein [60] .

In 2013, the gene IFNL4 was first described [69] . IFNL4 expression is influenced by a germline dinucleotide frameshift variant located in exon 1 of IFNL4 [69] . The IFNL4-∆G allele generates the full-length IFN-λ4 protein, whereas the IFNL4-TT allele does not create IFN-λ4 due to a premature stop [69] . The IFNL4-∆G allele is associated with a poor response to pegylated IFN-α/ribavirin therapy [69, 70] , and a recent study concluded that the IFNL4-∆G/TT genotype is the primary polymorphism underlying poor treatment response in HCV-infected patients [71] . Another study showed that IFNL4-∆G genotype is associated with high levels of ISGs and that hepatic levels of ISG15 in chronic hepatitis C are strongly associated with IFN-λ4 expression, suggesting that IFN-λ4 contributes to induction of ISGs in HCV-infected liver [72] . Forced expression of IFNL4 gene up-regulates ISGs in PHHs and HepG2 cells [69, 73] , and has antiviral effects against HCV [74] . Recombinant IFN-λ4 protein activates the JAK-STAT pathway through binding to the IFN-λ receptor [75] , evokes similar gene expression pattern to IFN-λ3 [76] . Future study using HCVcc infection systems will explain the mechanism of IFN-λ4 induction in HCV-infected cells and the effects of endogenous IFN-λ4 on both ISG induction and the response to exogenous IFN-α treatment.

After HCV infection, the expression of some genes is down-regulated, and the expression of those genes tends to be further down-regulated in the liver of non-responders to IFN treatment [61, 77] . One of the genes down-regulated in HCV-infected liver is dual specificity phosphatase 1 (DUSP1), a mitogen-activated protein kinase phosphatase (MKP) that de-phosphorylates mitogen-activated protein kinases (MAPKs) [78] . We demonstrated that silencing DUSP1 expression inhibits HCV replication in HCVcc-infected cells and HCV replicon cells by up-regulating antiviral ISGs [77] . DUSP1 silencing enhances the nuclear translocation of STAT1 and causes the induction of ISGs [77] . Although the detailed mechanism of DUSP1 down-regulation in HCV-infected liver remains to be elucidated, this serves as an example of how hosts regulate the expression of ISGs and restrict viral infection while bypassing endogenous IFN production.

In virus-infected cells, viral peptides are processed and loaded onto major histocompatibility complex (MHC) class I molecules and presented to viral peptide-specific CD8 + cytotoxic T cells [79] . Recently, we demonstrated using an HCVcc system that IFN-induced up-regulation of MHC class I molecules is attenuated by HCV infection [57] . HCV RNA activates PKR, which phosphorylates the translation initiation factor eIF2α to block the translation of proteins, including ISGs [56] and MHC class I [57] . The attenuated expression of MHC class I by HCV infection causes a reduction of the effector functions of HCV-specific CD8 + T cells [57] . Before our study, several studies had investigated the effect of HCV proteins on MHC class I expression with conflicting results. The expression of MHC class I was not affected by overexpression of HCV proteins in one study [80] , whereas another study showedup-regulation of MHC class I expression by the HCV core [81] . By using an HCVcc model, we were able to evaluate the effect of the whole life cycle of HCV infection on MHC class I expression, and we demonstrated the attenuation of IFN-induced MHC class I expression by HCVcc infection.

The isolation of the JFH-1 clone and the establishment of HCVcc infection systems made it possible to perform various studies on host-virus interactions and innate immune responses against HCV infection. Now is the era of DAAs, and HCVcc systems have greatly contributed to the advent of the DAA era. However, much remains to be resolved. Above all, the precise mechanism of interferon response and its paradoxical contribution to viral persistence should be elucidated. Novel cell culture models that closely mimic host responses with various clinical strains are the prerequisite for understanding the pathogenesis of HCV infection and clarifying the mechanism of viral persistence.

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Hepatitis C virus-induced hepatocellular carcinoma

Hepatitis C virus and hepatocarcinogenesis

CD8(+) T-Cell responses in acute hepatitis C virus infection

Current and future therapies for hepatitis C virus infection

Antiviral resistance and direct-acting antiviral agents for HCV

Animal models for the study of hepatitis C virus infection and related liver disease

Hepatitis C virus replication in mice with chimeric human livers

Completion of the entire hepatitis C virus life cycle in genetically humanized mice

Murine models of hepatitis C: What can we look forward to?

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Efficient replication of the genotype 2a hepatitis C virus subgenomic replicon

Complete replication of hepatitis C virus in cell culture

Production of infectious hepatitis C virus in tissue culture from a cloned viral genome

Robust hepatitis C virus infection in vitro

Robust full-length hepatitis C virus genotype 2a and 2b infectious cultures using mutations identified by a systematic approach applicable to patient strains

Highly efficient infectious cell culture of three hepatitis C virus genotype 2b strains and sensitivity to lead protease, nonstructural protein 5A, and polymerase inhibitors

Production of infectious genotype 1a hepatitis C virus (Hutchinson strain) in cultured human hepatoma cells

Generation of infectious hepatitis C virus in immortalized human hepatocytes

Production of infectious genotype 1b virus particles in cell culture and impairment by replication enhancing mutations

Highly efficient full-length hepatitis C virus genotype 1 (strain TN) infectious culture system

Efficient infectious cell culture systems of the hepatitis C virus (HCV) prototype strains HCV-1 and H77

Development of hepatitis C virus genotype 3a cell culture system

SEC14L2 enables pan-genotype HCV replication in cell culture

The HCV life cycle: In vitro tissue culture systems and therapeutic targets

Hepatitis C virus envelope components alter localization of hepatocyte tight junction-associated proteins and promote occludin retention in the endoplasmic reticulum

Production of infectious hepatitis C virus in primary cultures of human adult hepatocytes

HepG2 cells mount an effective antiviral interferon-lambda based innate immune response to hepatitis C virus infection

Hepatitis C virus infection induces the beta interferon signaling pathway in immortalized human hepatocytes

Hepatitis C virus genotype 1a growth and induction of autophagy

Hepatitis C virus infection impairs IRF-7 translocation and Alpha interferon synthesis in immortalized human hepatocytes

Human pluripotent stem cell-derived hepatocytes support complete replication of hepatitis C virus

Modeling hepatitis C virus infection using human induced pluripotent stem cells

Productive hepatitis C virus infection of stem cell-derived hepatocytes reveals a critical transition to viral permissiveness during differentiation

MicroRNA-27a modulates HCV infection in differentiated hepatocyte-like cells from adipose tissue-derived mesenchymal stem cells

MDA5 plays a critical role in interferon response during hepatitis C virus infection

Control of temporal activation of hepatitis C virus-induced interferon response by domain 2 of nonstructural protein 5A

Regulation of hepatic innate immunity by hepatitis C virus

Immune responses to HCV and other hepatitis viruses

EFTUD2 is a novel innate immune regulator restricting hepatitis C virus infection through the RIG-I/MDA5 pathway

Cardif is an adaptor protein in the RIG-I antiviral pathway and is targeted by hepatitis C virus

Cleavage of mitochondrial antiviral signaling protein in the liver of patients with chronic hepatitis C correlates with a reduced activation of the endogenous interferon system

Inhibition of intrahepatic gamma interferon production by hepatitis C virus nonstructural protein 5A in transgenic mice

Hepatitis C virus induces interferon-lambda and interferon-stimulated genes in primary liver cultures

IL-29 is the dominant type III interferon produced by hepatocytes during acute hepatitis C virus infection

HCV infection induces a unique hepatic innate immune response associated with robust production of type III interferons

Interferons at age 50: Past, current and future impact on biomedicine

IFN-lambdas mediate antiviral protection through a distinct class II cytokine receptor complex

IL28B inhibits hepatitis C virus replication through the JAK-STAT pathway

Interleukin-29 uses a type 1 interferon-like program to promote antiviral responses in human hepatocytes

Genomic analysis of the host response to hepatitis C virus infection

Stealth and cunning: hepatitis B and hepatitis C viruses

Interferon-induced gene expression is a stronger predictor of treatment response than IL28B genotype in patients with hepatitis C

Interferon signaling and treatment outcome in chronic hepatitis C

Simultaneous detection of hepatitis C virus and interferon stimulated gene expression in infected human liver

Hepatitis C virus blocks interferon effector function by inducing protein kinase R phosphorylation

Hepatitis C virus attenuates interferon-induced major histocompatibility complex class I expression and decreases CD8+ T cell effector functions

IFNβ-dependent increases in STAT1, STAT2, and IRF9 mediate resistance to viruses and DNA damage

Unphosphorylated STAT1 prolongs the expression of interferon-induced immune regulatory genes

Roles of unphosphorylated ISGF3 in HCV infection and interferon responsiveness

Hepatic gene expression discriminates responders and nonresponders in treatment of chronic hepatitis C viral infection

Cell-type specific gene expression signature in liver underlies response to interferon therapy in chronic hepatitis C infection

Hepatic gene expression during treatment with peginterferon and ribavirin: Identifying molecular pathways for treatment response

Hepatic ISG expression is associated with genetic variation in interleukin 28B and the outcome of IFN therapy for chronic hepatitis C

Protein ISGylation modulates the JAK-STAT signaling pathway

Silencing of USP18 potentiates the antiviral activity of interferon against hepatitis C virus infection

interferon induces long-lasting refractoriness of JAK-STAT signaling in the mouse liver through induction of USP18/UBP43

Interferon-β and interferon-λ signaling is not affected by interferon-induced refractoriness to interferon-α in vivo

A variant upstream of IFNL3 (IL28B) creating a new interferon gene IFNL4 is associated with impaired clearance of hepatitis C virus

IFN-λ4: The paradoxical new member of the interferon lambda family

Comparison of functional variants in IFNL4 and IFNL3 for association with HCV clearance

Hepatic expression levels of interferons and interferon-stimulated genes in patients with chronic hepatitis C: A phenotype-genotype correlation study

Prokunina-Olsson, L. Expression of interferon λ 4 is associated with reduced proliferation and increased cell death in human hepatic cells

Interferon-lambda4 is a cell-autonomous type III interferon associated with pre-treatment hepatitis C virus burden

Interferon λ 4 signals via the IFNλ receptor to regulate antiviral activity against HCV and coronaviruses

Transcriptome analysis reveals a classical interferon signature induced by IFNlambda4 in human primary cells

Suppression of dual specificity phosphatase I expression inhibits hepatitis C virus replication

Dual-specificity phosphatases: Critical regulators with diverse cellular targets

MHC class I antigen presentation: Learning from viral evasion strategies

Expression of hepatitis C virus proteins does not interfere with major histocompatibility complex class I processing and presentation in vitro

Upregulation of major histocompatibility complex class I on liver cells by hepatitis C virus core protein via p53 and TAP1 impairs natural killer cell cytotoxicity

The authors declare no conflict of interest.