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The innate and adaptive immune systems fail to control HCV infection in the majority of infected individuals. HCV is an ssRNA virus, which suggests a role for Toll-like receptors (TLRs) 7 and 8 in initiating the anti-viral response. Here we demonstrate that HCV genomic RNA harbours specific sequences that initiate an anti-HCV immune response through TLR7 and TLR8 in various antigen presenting cells. Conversely, HCV particles are detected by macrophages, but not by monocytes and DCs, through a TLR7/8 dependent mechanism; this leads to chloroquine sensitive production of pro-inflammatory cytokines including IL-1β, while the antiviral type I Interferon response is not triggered in these cells. Antibodies to DC-SIGN, a c-type lectin selectively expressed by macrophages but not pDCs or mDCs, block the production of cytokines. Novel anti-HCV vaccination strategies should target the induction of TLR7/8 stimulation in APCs in order to establish potent immune responses against HCV.
Infection with Hepatitis C virus (HCV) affects 185 million people worldwide, which makes it one of the main public health problems1,2. HCV infection can result in chronic hepatitis with increased risk of progression to cirrhosis and hepatocellular carcinoma (HCC)3. Adaptive immunity in HCV infection is usually delayed, regardless of the outcome of the disease progression, which suggests a lack of proper innate immune responses4,5. This is likely due to the capacity of HCV to evade detection by the innate immune cells4. Different pattern recognition receptors (PRRs) have the capacity to recognize pathogen associated molecular patterns (PAMPs) in HCV and therefore to trigger antiviral and pro-inflammatory innate immune responses6. For this stimulation to take place, HCV has to be recognized by endosomal sensors particularly TLR3, 7 and 8 to detect viral RNA7,8,9,10. Furthermore, the recognition of HCV genomic RNA by the retinoic acid inducible gene-I (RIG-I)11,12,13 upon uncoating of the virus and genomic amplification during HCV infection, can also initiate anti-viral responses. Although poorly understood, the role of TLR3 in the detection of HCV extracellular double stranded RNA (dsRNA) replicative intermediates was reported8,14. TLR7 and TLR8 can detect single stranded RNA (ssRNA) molecules. The potential implication of TLR7 in the innate immune response against HCV was postulated4,15. In this regard, pDCs have been shown to respond to TLR7-ligation in vitro using Huh-7 infected cells16. Moreover, the presence of a GU-rich sequences in the HCV genome was shown to be detected by TLR717. Furthermore, single nucleotide polymorphisms (SNPs) in TLR7 and TLR8 were shown to be associated with a decrease in the magnitude of inflammation and fibrosis in male patients with chronic HCV-infection, and with the response to IFN-α−based therapy as well as the susceptibility to HCV infection18,19,20. However, the underlying mechanisms for the role of TLR-7 in HCV infection are not fully understood. Moreover, little is known about the role of TLR8 in the innate immune responses against HCV. Here we dissect the roles of TLR7 and TLR8 in the detection of specific motifs in the HCV genomic RNA and the differential stimulation of mDCs, pDCs, macrophages and monocytes by HCV particles.
To determine if HCV genome can trigger both TLR7 and TLR8, PBMCs, isolated from healthy donors, were incubated for 24hours with HCV RNA isolated from viral particles; TNF-α production was measured by ELISA. Our results (Fig. 1a) demonstrated that HCV RNA significantly induced TNF-α production following 24h of stimulation (439pg/ml, p<0.0001) compared to control non-stimulated cells. To identify the specific RNA sequences involved in the stimulation of TNF production, we screened the HCV genome and identified 9 new GU-rich sequences (HCVL 1–9) that could potentially trigger TLR7/8 (Supplementary Table S1). Interestingly, three out of these nine sequences (HCVL1, 4 and 8) were able to trigger TNF-α production by PBMCs at levels comparable to those generated upon stimulation with the reference sequence RNA4021 (2,300, 1,800, 2,100 and 3,400pg/ml for HCVL1, 4, 8 and RNA40 respectively, p<0.0001; Fig. 1b). The specificity of stimulation of these sequences was further assessed by introducing mutations (G or U to A) or by treatment with RNase. Both site-directed mutations and RNase treatment completely abrogated the capacity of these sequences to trigger TNF-α production by PBMCs (p<0.0001; Fig. 1c).
To demonstrate that TLR7/8 triggering was upstream of HCV RNA-mediated stimulation of these cells, we used IRS661, a specific inhibitor of these TLRs22. The capacity of HCVL1, 4 and 8 to stimulate TNF-α production by PBMCs was significantly inhibited when the stimulation was carried out in the presence of IRS661 (Fig. 1d, p<0.0001). To confirm the role of TLR7 and TLR8 in detecting the HCV-encoded sequences, we used HEK cells stably expressing TLR7 or TLR8. These cells were transiently transfected with a plasmid bearing the luciferase-encoding gene under the control of NF-κB-dependent promoter to monitor TLR activation. These cells were exposed to either HCV-encoded sequences or to the CL097 ligand (as a positive control). A significant increase in luciferase activity was observed when cells were exposed to HCV sequences (4-, 2- and 3- fold increase for HCVL-1, 4 and 8, respectively in TLR7 expressing cells, p<0.0001, and 15-, 6- and 3- fold increase, respectively in TLR8 expressing cells, (p<0.0001, Fig. 1e). In contrast, the HCV-encoded sequences were not able to induce any luciferase activity under the same conditions in HEK cells expressing TLR3 alone, which detects dsRNA, while Poly I:C was able to induce luciferase expression in these cells (2.8- fold increase; Fig. 1e). Together, our results showed that the GU-rich sequences, identified herein within the HCV genome, have the capacity to significantly induce cell activation in a TLR7 and TLR8-specifc fashion.
We further assessed the capacity of these three RNA sequences to induce the production of a panel of cytokines and chemokines by different APCs including isolated monocytes, myeloid DCs (mDCs) and plasmacytoid DCs (pDCs) (>98% purified by enrichment). Stimulation of these cells using HCVL1, 4 and 8 induced the production of TNF-α, IL-6, IL-1β, IL-10, IL-12p70, CXCL9 and CXCL10 by these cells to levels comparable to those induced by the chemical ligand of TLR7/8, CL097, as monitored by Cytometric Bead Array (CBA; Table 1). Of note, introduction of G or U to A mutations by site-directed mutagenesis in these sequences also diminished their capacity to stimulate APCs to produce all measured cytokines and chemokines (Table 1). However, the profile of cytokine production was different in monocytes, mDCs, and pDCs. Although, high levels of TNF-α and IL-6 were induced in monocytes, mDC, and pDC upon stimulation, CXCL9 and CXCL10 were mainly produced by pDCs, whereas IL-1β, IL-12p70, and IL-10 were produced by monocytes and mDCs but barely detected in supernatants of stimulated pDCs (Table 1).
Incubation of pDCs, freshly isolated from blood, with HCVL1, 4 and 8 led to the maturation of pDCs as observed by the up-regulation of the surface expression of CD80 (MFI=2,161, 2,267, 2,711 vs control 476, p<0.0001, Fig. 2a) and CD86 (MFI=43,233, 39709, 44,739 vs control 2,739, p<0.0001; Fig. 2b). Moreover, this stimulation induced the production of IFN-α (1,600, 1,500 and 1,700pg/ml respectively, p<0.0001) and IFN-β (1,300, 1,000 and 2,250pg/ml respectively, p<0.0001) by pDCs (Fig. 2c,d respectively).
We next investigated the potential anti-viral activity of cytokines produced by DCs upon stimulation with the HCV-encoded sequences identified in this study. Considering the infiltration of macrophages into the liver of HCV-infected subjects and their contribution to chronicity10, studies were performed in parallel on monocyte-derived macrophages. We infected Huh7.5 cells with HCV in the presence or absence of supernatants from monocytes, pDC, mDCs or macrophages stimulated or not with HCVL1, 4 or 8. Our results showed that the presence of supernatants from monocytes or pDCs stimulated with HCVL1, 4 or 8 reduced HCV replication in Huh7.5 cells by 2 Log10 (p<0.0001), in a way similar to the impact of IFN-α on HCV replication (Fig. 3a,b). In contrast, supernatants from mDCs and macrophages stimulated with HCVL1, 4 or 8 did not have any impact on HCV infection in Huh7.5 cells (Fig. 3c,d). Addition of an anti-IFNR antibody to supernatants from monocytes and pDCs stimulated with HCV RNA abolished their inhibitory effect on HCV infection, thus underlying the role of type I IFN in this mechanism (Fig. 3e,f). Of note, only supernatants from HCV RNA-stimulated monocytes and pDCs induced the phosphorylation of the tyrosine motif Y701 of STAT-1 in PBMCs, which also suggested that this inhibitory activity could be mediated by type I IFNs present in the supernatants of these cells (Supplementary Figure S1).
Our results demonstrated that HCV RNA encodes sequences that stimulate APCs and induce anti-viral immune responses. We investigated the capacity of HCV viral particles to trigger such a response in different cellular subsets of APCs. Upon incubation with HCV particles for 24hours, monocytes and DCs did not produce TNF-α. In contrast; these cells produced TNF-α upon incubation with the control CL097 ligand (Fig. 4a,b). Similar results were observed when total PBMCs were exposed to HCV particles (Supplementary Figure S2a). In contrast, both HCV particles, at the same number of RNA copies/ml/cells ratio that was used to stimulate the other APCs, and CL097 induced TNF-α production in macrophages (Fig. 4c). We further validated these observations on a large number of donors (n=20) using a ratio of 20 HCV particles per cell. As expected HCV particles did not induce TNF-α production by monocytes, in contrast macrophages from 19 out of 20 donors responded to HCV stimulation as indicated by TNF-α production (average of 1,517pg/ml, p<0.0001; Supplementary Figure S2b).
We used LPS, CL097 and poly I:C as positive controls to monitor the responsiveness of these APCs in our assay. Both macrophages and monocytes responded to LPS (TLR4 ligand; an average of 2,200pg/ml and 3,000pg/ml, p=0.0069 and 0.0072, respectively), CL097 (TLR7/8 ligand; an average of 3,000pg/ml and 2,100pg/ml, p<0.0001 and p=0.004, respectively) and poly I:C (TLR3 ligand; average of 900pg/ml and 1,300pg/ml, p=0.0054 and 0.015, respectively). However, only macrophages but not monocytes produced TNF-α (2,850pg/ml, p=0.0032) upon stimulation with HCV particles (Supplementary Figure S2c,d), although both macrophages and monocytes were able to produce TNF-α in response to other RNA virus, such as Sendai virus (Supplementary Figure S2e,f). Moreover, HCV particles were able to induce TNF-α production by macrophages in a dose dependent manner, reaching 4,000pg/ml of TNF-α when the ratio of HCV particles to cells were in the range of 50/1 (Fig. 4d). Furthermore, HCV particles stimulated the production of different inflammatory cytokines by macrophages such as IL-6 (2,800pg/ml, p<0.0001), IL-1β (110pg/ml, p<0.0001) and IL-8 (2,950pg/ml, p<0.0001; Fig. 4e). Interestingly, the production of the cytokine IL-12p70, which is crucial for the induction of CD4 T helper (Th1) 1 and CD8 T cell responses, was not induced by HCV particles in macrophages (Fig. 4e).
Macrophages were able to sense HCV particles, however cytokines produced upon this stimulation did not inhibit HCV replication (Fig. 3d) likely due to the absence of the type I interferon. To test this hypothesis, we monitored IFN-β and IFN-stimulated gene expression (IFIT1, OAS1, ISG15) in macrophages after 3hrs incubation with HCV particles, LPS or CL097. Whereas TNF-α levels increased after stimulation with HCV particles, LPS or CL097 (Fig. 5a), the stimulation with the TLR7/8 agonist or HCV particles did not induce IFN-β expression by macrophages (Fig. 5b). To exclude the possibility that macrophages were unable to produce to produce IFN-β, we stimulated these cells with LPS. As shown in Fig. 5b, IFN-β was significantly up-regulated in LPS-stimulated macrophages (an average of 28-fold increase, values were 10, 20 and 56-fold increase in 3 independent donors) thus demonstrating the capacity of macrophages to produce IFN-β under other specific conditions. To further demonstrate the inability of HCV particles to induce the IFN pathway in macrophages, we measured the expression of IFN-stimulated genes (ISGs) at 16hrs after stimulation with HCV particles or LPS. Although LPS induced the up-regulation of IFIT1 (an average of 285-fold increase, values were 90- 480- and 285-fold increase as observed in 3 donors), OAS1 (an average of 30-fold increase, values were 10- 30- and 50-fold increase as observed in 3 donors) and ISG15 (an average of 74.5-fold increase, values were 74- 74.5- and 75-fold increase as observed in 3 donors) in macrophages, the stimulation with HCV particles did not induce the up-regulation of these IFN-stimulated genes (Fig. 5c). Although stimulation of these macrophages with HCV particles or LPS led to the up-regulation of TNF-α expression in macrophages (11- and 13- fold increase respectively (Fig. 5c)). Interestingly, gene expression induced by HCV particles and TLR7/8 ligand CL097 has similar profiles, suggesting HCV likely triggers TLR7/8 in macrophages (Fig. 5a,b).
We compared the capacity of macrophages and monocytes to uptake HCV particles to further investigate the mechanisms leading to their detection by these cells. To measure viral entry, monocytes or macrophages were incubated with HCV for 4hrs followed by treatment with trypsin to remove the viral particles that remained attached to the cell surface. HCV particles bound to the surface of both macrophages and monocytes as we could detect viral RNA in both cell types by RT-PCR following the 4hrs incubation period without trypsin treatment. Upon treatment with trypsin, viral RNA was not detected in monocytes, whereas it was still detected in macrophages (Fig. 6a).
We then investigated the implication of DC-SIGN, known to promote HCV endocytosis, in the specific capacity of macrophages to bind HCV particles. As a control we also monitored the role of CD81 in this process, as CD81 is known to be implicated in HCV entry. Our results showed that whereas macrophages, monocytes, pDCs and mDCs all expressed CD81, DC-SIGN was exclusively expressed by macrophages (Fig. 6b). To assess the potential role of DC-SIGN in the recognition of HCV particles by macrophages, we used a DC-SIGN neutralizing antibody that blocks the interaction of DC-SIGN with HCV envelop protein23. Macrophages were incubated with HCV particles in the presence or absence of the anti-DC-SIGN blocking antibody or with its matched isotype control. TNF-α production by macrophages treated with anti-DC-SIGN was significantly decreased (an average of 90% inhibition, p<0.0001; Fig. 6c), which indicates that DC-SIGN is involved in the uptake of HCV by macrophages. Interestingly, we observed a much higher expression of DC-SIGN on monocytes-derived DCs (MDDCs) as compared to macrophages (an average MFI 40,774 and 4,579 respectively, p=0.0043; Supplementary Figure S3a). However, these MDDCs did not respond to HCV particles as monitored by TNF-α production. In contrast, MDDCs were able to respond to stimulation by CL097 and Sendai virus (Supplementary Figure S3b). Our data showed that DC-SIGN is involved in HCV recognition by macrophages. However, for the stimulation to take place other downstream mechanisms are likely required as MDDCs express high levels of DC-SIGN but are not triggered by HCV particles.
As we described above, TLR7/8 are likely involved in sensing HCV particles. To assess this hypothesis, we tested the capacity of IRS661 and chloroquine, a specific inhibitor of endosomes acidification, to inhibit the stimulation of macrophages by HCV particles. IRS661 inhibited 50% of TNF-α production induced by viral particles (Fig. 6d, p<0.0001), indicating an important role for TLR7/8 in detecting HCV particles by macrophages. Interestingly, chloroquine completely abolished TNF-α production by macrophages exposed to HCV particles (Fig. 6d, p<0.0001), which indicates that this process was mediated by endosomal TLRs.
Together, our data showed that recognition of HCV RNA by monocytes and pDCs mediated anti-HCV functions in an IFN-dependent fashion. However, HCV complete particles, although they were able to stimulate macrophages but not other APCs, failed to induce the production of IFN-β by macrophages; therefore, they were compromised in their antiviral activity.
In the current study we identified novel HCV-encoded RNA sequences that can elicit TLR7/8-mediated innate immune responses. We show here that the presence of GU-rich sequences in HCV ssRNA are essential but not sufficient to stimulate immune responses as 6 out of the 9 GU-rich ssRNA sequences identified in our study did not induce detectable responses. This suggests that other parameters might also participate in determining the capacity of viral ssRNA to trigger TLR7/8. Moreover, other sequences with the capacity to stimulate TLR7/8 might also exist in HCV genome. HCV-encoded RNA sequences that we identified here stimulated inflammatory cytokines and chemokines, as well as type I IFN-dependent anti-HCV responses by primary APCs, particularly monocytes, mDCs and pDCs. These responses could not be initiated by HCV particles as monocytes and DCs were defective in their capacity to sense HCV particles. Only macrophages were able to sense HCV particles, however, this induced a pro-inflammatory environment, which is prevalent in HCV infected subjects as it was previously shown to be associated to disease progression24,25. Importantly, HCV particles failed to induce the production of type I IFN, thus allowing HCV to escape the intrinsic antiviral innate immune response.
The lack of DC and monocyte activation by HCV is in line with earlier reports showing a deficiency in virus uptake by these cells26,27. Our results suggest that this is likely a result of a blockade at the entry step, which might be due to the lack of DC-SIGN expression in primary DCs and monocytes. DC-SIGN plays a key role in the uptake of HCV as previously shown in vitro by monocyte-derived DCs23,28 and further confirmed by our current data; we demonstrated that macrophage activation by HCV particles is DC-SIGN-dependent. Although, DC-SIGN is not expressed by peripheral DCs29,30, it is expressed on dermal DCs, ‘monocytoid’ DCs in the lymph nodes and macrophages in the liver31,32,33,34,35, which suggests that these cells could sense HCV in its target tissue. DC-SIGN expression does not warrant optimal responses upon recognition of HCV since we show that monocyte-derived DCs, although expressing high levels of DC-SIGN, did not respond to HCV particles. This lack of response was specific to HCV as these same cells strongly responded to Sendai virus, which is another RNA virus. In line with this hypothesis, earlier reports have shown that immature DCs can readily uptake HCV particles through DC-SIGN-mediated internalization into a non-lysosomal compartment, where virus escapes the detection by TLRs28,36.
The lack of detection of HCV particles did not apply to all innate APCs as we showed here that macrophages could indeed recognize HCV particles through a DC-SIGN-dependent interaction, which leads to the triggering of TLR7/8 signaling, as confirmed by the use of TLR antagonists, and the production of pro-inflammatory cytokines. Whether the differentiation of monocytes into macrophages in vitro have impacted their activation profile, and consequently enhanced their potential to detect HCV particles remains unknown and deserves further investigations. However, the in vitro differentiation of monocytes to MDDCs did not render them sensitive to the stimulation with HCV particles, which suggests that the ability to detect HCV particles required monocytes differentiation into macrophages.
Moreover, type I IFN and IFN-stimulated genes, i.e. IFIT1, OAS1, and ISG15 gene expression signature, which are key mediators of viral inhibition37,38,39,40, were not induced upon stimulation of macrophages by HCV particles. The biased IFN signal in response to HCV in macrophages is not likely specific to HCV but rather reflects an altered type I IFN response upon triggering of TLR7/8 in these cells. For instance, activation of macrophages with chemical ligands of TLR7/8, i.e. CL097, did not induce any significant interferon production by these cells. However, upon activation with LPS, which triggers TLR4, the same macrophages produced IFN-β. Those results suggest that activation of TLR7/8 pathway in macrophages does not lead to type I IFN production.
One of these potential mechanisms that could explain the lack of type I interferons production by these cells could involve NLRX-1, an inhibitor of mitochondrial antiviral immunity, which is known to prevent the induction of antiviral response in macrophages41,42. Moreover, alternatively activated STAT1 has been shown to negatively regulate TLR7/8 signaling in macrophages, especially prevent type I IFN production43. The antagonist effects of IL-1β may also contribute in the absence of IFN production in macrophages as IL-1β inhibits IFN-β synthesis44. IL-1βinhibits type I IFN responses by directly promoting IFN receptor turnover45 and antagonize STAT1 activity46. Moreover, the absence of type I IFN production by macrophages upon stimulation with HCV particles might be due to the fact that TGF-β and IL-10, which are produced by macrophages themselves, have the capacity to negatively regulate TLRs-induced type I IFN production47,48; this possibility remains to be investigated in future studies.
HCV particles selectively activated macrophages to induce pro-inflammatory cytokines, such as IL-1β, TNF-α and IL-8, which have been shown to be up-regulated in chronically HCV-infected individuals and correlate with HCV-driven fibrogenesis10,25,49,50,51. This may further suggest that activation of macrophages by HCV can potentially contribute to disease progression in infected patients by this virus. In line with this hypothesis, resident hepatic macrophages, Kupffer cells (KCs), in HCV-infected subjects were shown to be the primary cellular source of liver inflammation as they produce significantly high levels of IL-1β upon exposure to HCV10. The production of IL-1β, also observed in our experiments, indicates the capacity of HCV particles to activate the inflammasome in macrophages10. While macrophages sensed HCV particles, this did not trigger IL-12p70 production and consequently this detection might not be sufficient to prime potent Th1 and CD8 T cell responses. Hence our results indicate that macrophage sensing of HCV particles triggers a pro-inflammatory response that does not include the pathways and cytokines required for the development of a protective adaptive cellular immune response. Liver macrophages are stimulated during chronic HCV infection, however their profile suggests that they do not support the induction of proper T cell responses52. The capacity of resident and infiltrating macrophages in the liver to detect HCV particles and produce anti-viral type-I IFNs remains to be investigated as these cells might have some differences compared to monocytes-derived macrophages. Of note, HCV core protein (HCVc) has been found to be able to block TLR3-mediated secretion of IFN-α, IFN-β by human KC53.
In conclusion, in this study we have shown that innate immune responses mediated by HCV particles were limited to macrophages as neither monocytes, mDCs nor pDCs have the potential to detect HCV viral particles. However, activation of macrophages by HCV is not optimal and does not trigger anti-viral responses but rather induces a pro-inflammatory response. Thus, the development of an anti-HCV vaccine should consider strategies that lead to a proper stimulation of TLR7/8 in monocytes, mDCs and pDCs in order to improve the quality of the immune response against HCV54,55. Our results thus pave the way for a better understanding of the essential innate immune responses to HCV, which are key elements for the development of an effective anti-HCV vaccine.
Hepatoma Huh7.5 cell line (provided by Dr. Charles Rice, Rockefeller University) and Huh7.5–20 producing JFH1 HCV (provided by Dr. T. Jake Liang, National Institutes of Health) were cultured in DMEM-based complete growth medium. The 293HEK cell line expressing TLR3, TLR7 or TLR8, and the plasmid pNiFty2-Luc were obtained from Invivogen (USA). The pNiFty2-Luc plasmid contains a reporter gene expression cassette that allows firefly luciferase production under the control of NF-κB. Nine sequences within the HCV genome containing around 65% GU were selected and synthesized (Integrated DNA Technologies, Canada). TLR7/8 agonist RNA40, CL097 and TLR3 agonist poly I:C were obtained from Invivogen. DC-SIGN blocking antibody and matched isotype control were obtained from R&D Systems.
The following Abs were used for flow cytometry: CD80-FITC, CD86-PE, CD14-Pacific blue, Linage-Alexa700 (CD3, CD19, CD16), HLA-DR-APC-cy7, CD11c-APC, CD123-FITC, CD81-PE (BD Bioscience, USA), DC-SIGN-PE (R&D Systems, USA). A viability dye (Molecular Probes® LIVE/DEAD® Fixable Dead Cell Stain Kits, Invitrogen) was used to exclude dead cells. Cells were stained and analyzed by FACS using the BD LSRII cytometer and FlowJo software.
Human peripheral blood mononuclear cells (PBMCs) were isolated from leukapheres using ficoll density centrifugation. Enrichment kits for monocytes, plasmacytoid dendritic cells (pDCs) and panDC separation were obtained from STEMCELL Technologies Inc. Myeloid DCs (mDCs) were isolated from PBMCs using the CD1c+ Dendritic Cell Isolation Kit (Miltenyi Biotec, USA). Typically, the purity of cell fractions was >98% as determined by staining with anti-CD14-PB Abs for monocytes, and with lineage-Alexa700 (CD3, CD14, CD19, CD16), HLA-DR-APC-Cy7, CD11c-APC and CD123-PE Abs for DCs. To prepare macrophages, monocytes were cultured in the X-VIVOTM 15 medium (lonzabio, USA) for 6 days in the presence of GM-CSF (50ng/ml; R&D Systems, USA). To obtain monocyte-derived DCs (MDDCs), monocytes were cultured for 6 days in the X-VIVOTM 15 medium supplemented with GM-CSF (50ng/ml) and IL-4(20ng/ml). Informed consent was obtained from all the donors and the project was approved by the Institutional Review Boards (IRB) of the Centre Hospitalier de l′Université de Montréal Research Center, Vaccine & Gene Therapy Institute of Florida.
TNF-α production was measured using the Human TNF alpha ELISA Ready-SET kit (eBioscience, USA). In parallel, cytokines (IL-1β, IL-6, IL-10, IL-12p70 and TNF-α) and chemokines (CXCL9, CXCL10) were measured by Cytometric Bead Array (CBA) using the Human Inflammatory Cytokine Kit and Human Chemokine Kit (BD Biosciences, USA). Type I IFN was measured using the Human Interferon alpha ELISA kit and the Human Interferon Beta ELISA Kit (PBL Interferon Source, USA).
RNA was extracted using RNeasy Mini Kit (QIAGEN, USA). The expression of mRNA for TNF-α and IFN-β, together with the mRNA for the IFN-stimulated genesIFIT1, OAS1 and IAS15, was measured using predesigned primers and probe sets (Roche-Applied-Science) and the LightCycler® 480 Probes Master(ROCHE, USA). Real-time RT-PCR (Qiagen) was carried out in a LightCycler 480 II (Roche) according to manufacturer’s recommendations. The expression of each gene in different samples was normalized relative to GAPDH mRNA levels.
The Huh7.5–20 cells stably producing HCV particles were cultured in DMEM-based complete growth medium for 4 days. The cell culture supernatant was harvested and filtered through a 0.45μm filter to remove cell debris (Sarstedt, Germany). To concentrate the virus, supernatant containing HCV particles was passed through an Amicon ultra-15 centrifugal filter-100 (Millipore, USA). Filters were sterilized with 70% alcohol and rinsed with PBS before use. Concentrated viral aliquots were stored at −80°C for further use. The viral titer was quantified by real-time RT-PCR. Briefly, RNA was extracted from cell culture supernatant using the QIAamp Viral RNA Mini Kit (QIAGEN, USA). Real time PCR was performed as described above using the specific forward primer 5′-CGGGAGAGCCATAGTGG-3′, reverse primer 5′-AGTACCACAAGGCCTTT-3′, and the probe 5′-/56-FAM/CTGCGGAACCGGTGAGTACAC/3IABlkFC (IDT, USA).
This study was approved by the Institutional Review Boards (IRB) of the Centre Hospitalier de l′Université de Montréal Research Center, Vaccine & Gene Therapy Institute of Florida and at all participating sites’ IRBs. All experiments were performed in accordance with the guidelines and regulations approved by the ethic committees from CRCHUM, VGTIFL and all IRBs. Study participants provided written informed consent for the use of their plasma and cells for the current research investigation.
Statistical analyses were performed using the GraphPad Prism 5. Details are included in Figure legends. Actual p-value is showed in the main text when it is available.
How to cite this article: Zhang, Y. et al. HCV RNA Activates APCs via TLR7/TLR8 While Virus Selectively Stimulates Macrophages Without Inducing Antiviral Responses. Sci. Rep. 6, 29447; doi: 10.1038/srep29447 (2016).
We would like first to thank all the study participants for their generous collaboration. We thanks Dr. Charles Rice kindly provided Hepatoma Huh7.5 cell line and Dr. T. Jake Liang provided Huh7.5–20 cell line producing JFH1 HCV virus. We also thank Dr. Naglaa Shoukry and Dr. Joumana Zeidan for their reading of the manuscript and help with editing.
Author Contributions Y.Z. designed and performed experiments, analysed data and wrote the manuscript. M.E.F. and P.A. helped with analysis and wrote the manuscript. F.P.D. and Z.H. performed DC. separation and cytokine/chemokine detection by Cytometric Bead Array. F.P.D. and M.S.A.-H. optimized the method for HCV quantification. Z.H. helped with viral production and infection in vitro. Y.S. helped with flow cytometric analysis. E.K.H. provided experiment advice. E.A.S. and R.-P.S. designed and supervised the project, and wrote the manuscript.