Immunomodulation of CXCL10 Secretion by Hepatitis C Virus: Could CXCL10 Be a Prognostic Marker of Chronic Hepatitis C?

Chemokine (C-X-C motif) ligand (CXCL)10 and other CXCR3 chemokines are involved in the pathogenesis of acute and “chronic hepatitis C virus (HCV) infection” (CHC). Here, we review the scientific literature about HCV and CXCL10. The combination of circulating CXCL10 and single nucleotide polymorphisms (SNPs) in IL-28B can identify patients with acute HCV infection most likely to undergo spontaneous HCV clearance and those in need of early antiviral therapy. In CHC, the HCV and intrahepatic interferon- (IFN-) γ drive a raised CXCL10 expression by sinusoidal endothelium and hepatocytes, thereby inducing the recruitment of CXCR3-expressing T cells into the liver; thus, CXCL10 plays an important role in the development of necroinflammation and fibrosis. Increased CXCL10 was significantly associated with the presence of active vasculitis in HCV-associated cryoglobulinemia, or with autoimmune thyroiditis in CHC. Pretreatment CXCL10 levels are predictive of early virological response and sustained virological response (SVR) to IFN-α and ribavirin and may be useful in the evaluation of candidates for therapy. The occurrence of SNPs adjacent to IL-28B (rs12979860, rs12980275, and rs8099917), and CXCL10 below 150 pg/mL, independently predicted the first phase viral decline and rapid virological response, which in turn independently predicted SVR. Directly acting antiviral agents-mediated clearance of HCV is associated with the loss of intrahepatic immune activation by IFN-α, associated by decreased levels of CXCL10. In conclusion, CXCL10 is an important marker of HCV clearance and successful therapy in CHC patients. Whether CXCL10 is a novel therapeutic target in CHC will be evaluated.

About 38-76% of CHC patients develop at least one extrahepatic manifestation (EHM) [8]. The term "HCV syndrome" involves hepatic and extrahepatic disorders, and among them, mixed cryoglobulinemic vasculitis can be considered the pathophysiological prototype [9], involving various organs and systems (joints, kidney, nervous system, skin, and eyes). The infected extrahepatic tissues can function as a reservoir for HCV [9] that replicates and expresses viral proteins in extrahepatic tissues, contributing to EHMs. HCV avoids immune elimination, causing the accumulation of circulating immunocomplexes, and autoimmune phenomena [10].
In HCV infection, cytokines and chemokines take part in viral control and liver damage. Chemokine (C-X-C motif) ligand (CXCL)10 and the other CXCR3 chemokines participate in the pathogenesis of acute and "chronic hepatitis C virus (HCV) infection" (CHC).

Cytokines and Chemokines
Cytokines are small proteins, secreted by different types of cells: fibroblasts, immune cells (macrophages, B lymphocytes, and T lymphocytes), endothelial cells, and different epithelial cells. Upon binding to specific receptors, cytokines modulate the balance between cell-based and humoral immune responses and have a key role in host responses to infection, inflammation, immune responses, trauma, cancer, and sepsis [16,17].
The determination of high CXCL10 levels in peripheral liquids is believed to be a marker of host Th1-orientated immune response. Activated Th1 lymphocytes cause an increased IFN-γ and TNF-α production that stimulates the target cells to secrete CXCL10, thus perpetuating the immune cascade [24,25].
Here, we review the scientific literature about HCV infection and CXCL10 [given the complexity of the published data on CXCL10 with other infections, the coinfections (for example, HCV/HIV coinfection) will be excluded].
3. CXCL10 and Acute HCV Infection (Table 1) During acute HCV infection, CXCL9-10-11 induction started 38-53 days and peaked 72-83 days after virus acquisition; a similar pattern was observed for alanine aminotransferase (ALT) levels. The increase of CXCR3-associated chemokines, in the late phase of acute HCV infection, leads to hypothesize a role for cellular immune responses in chemokine secretion [49].
In six chimpanzees infected with HCV, chemokine induction correlated with intrahepatic type I IFN responses in vivo and was stopped by the neutralization of antibodies against IFN-β in vitro [50].
A study evaluated IL-28B single nucleotide polymorphisms (SNPs) rs12979860 and rs8099917, together with serum CXCL10 levels, reporting that the frequency of IL-28B rs12979860 C/C genotype was higher in patients with spontaneous clearance than those without [51]. The CXCL10 median level was lower among patients with acute HCV infection and spontaneous clearance (764 pg/mL) than those without spontaneous clearance (1481 pg/mL). Considering also the data on CXCL10 levels, the capability of the IL-28B rs12979860 C/C of identifying patients more prone to have spontaneous clearance (83% of those who had a CXCL10 level < 540 pg/mL and 32% of whom with CXCL10 > 540 pg/mL) increased. Combining circulating CXCL10 and SNPs in IL-28B, patients with acute HCV infection who

CXCL10 and acute HCV infection References
Increase of CXCR3-associated chemokines, during the late phase of acute HCV infection [49] An in vivo study showed that despite an early-stage induction of chemokines, the intrahepatic lymphocytic infiltrate increased not earlier than 8 weeks after HCV infection [50] CXCL10 serum levels and SNPs in IL-28B can identify patients with acute hepatitis C who are more prone to undergo spontaneous clearance and those in need of early antiviral therapy [51] Truncated CXCL10 is associated with failure to obtain spontaneous clearance of acute hepatitis C infection [54] Both CXCR3 and CCR2 were overexpressed on HCV-specific CD8+CCR7+CD45RO+ (central memory) cells [55] are more prone to have clearance spontaneously, and those who need an early antiviral therapy, can be identified [51]. These results were confirmed by other studies [52,53]. Moreover, truncated CXCL10 is associated with the lack of spontaneous clearance of acute HCV infection, providing evidence of chemokine antagonism during acute HCV infection [54].
The last study reported that CXCR3 and chemokine receptor (CCR)2 were overexpressed on HCV-specific CD8+CCR7+CD45RO+ (central memory) cells. These results suggested that CXCR3-mediated signals accumulate HCV-specific CD8+ memory T cells in the infected liver [55].

CXCL10 and Chronic CHC (Table 2)
High levels of CXCR3 receptors are expressed by the lymphocytes that infiltrate a hepatitis C-infected liver [56].
CXCL10 and monokine-induced by IFN-γ (Mig)/CXCL9 are upregulated on sinusoidal endothelium. CXCL10 and CXCL9 are secreted by human IFN-γ+TNF-α-stimulated hepatic sinusoidal endothelial cells in vitro, suggesting that in CHC the production of IFN-γ in the liver causes the raised CXCL10 and CXCL9 expression and recruits CXCR3-expressing T cells in the hepatic lobule [56]. CXCR3 ligands are responsible for regional localization of specific lymphocyte subsets in the HCV-infected liver [57][58][59].
Another paper showed that in CHC (but not in other liver disorders), CXCL10 expression was highly correlated with the total transcripts of IFN-γ [60].
HCV can induce CXCL10 in hepatocytes, taking part in the pathogenesis of CHC [61].
Another paper reported that CXCL9 and CXCL10 expression in human hepatocyte-derived cells is upregulated

CXCL10 and chronic CHC References
The intrahepatic production of IFN-γ causes the raised CXCL10 and CXCL9 expression and recruits CXCR3-expressing T cells in the hepatic lobule. [56] CXCR3 ligands are responsible for regional localization of specific lymphocyte subsets in the HCV-infected liver.
[59] Hepatic inflammatory activity was associated more strongly with IFN-γ than with CXCL10.
[60] CXCL10 may be induced by HCV within hepatocytes, resulting to be an important factor in the pathogenesis of CHC.
[61] CXCL10 and CXCL9 gene expression in cultured human hepatocyte-derived cells is upregulated by NS5A and core proteins, alone or in combination with cytokines. [62] Hepatocytes in CHC patients participate in CXCL10 production involving TLR2 and CD44.
[66] Nonparenchymal hepatic cells and immune effector cells were recruited in the site of infection by CXCL10. These cells by secreting type I, II, and III IFNs amplify CXCL10 response during the later stages of acute HCV infection. [63] Investigations about the mechanisms of CXCL10 induction in hepatocytes by several factors (such as NF-κB and IRF3). Perpetual inflammation and viral persistence could be arisen because of viral proteins that antagonize with these factors and then interfere with the induction of CXCL10. [64] In the first stage of liver fibrosis, the principal alterations in gene expression affected in particular the IFN-regulated transcriptional network, such as IFN-α/β-inducible genes (STAT1, STAT2, ISGF3G/IRF9, IFI27, G1P3, G1P2, OAS2, and MX1) and IFN-γ-inducible genes (CXCL9, CXCL10, and CXCL11). [67] CXCL10 mRNA expression levels were significantly associated with lobular necroinflammatory grade and HCV genotype 1.
[68] Patients with advanced fibrosis had significantly increased CXCL10 plasma levels.
[69] CXCR3 chemokines are the most strongly expressed chemokines in CHC and presumably have a key role in positioning T cells in the liver. [70,71] CXCL10 is an independent biomarker of the recurrence of significant fibrosis after liver transplantation for HCV infection.
[72] Studies reported that in CHC, CXCL10 can be considered a marker of liver fibrosis.
[73-75] HCV-induced CXCL10 can lead to a raised hepatocyte turnover and the development of cirrhosis, fibrosis, and HCC.
[37] Circulating CXCL10 in many HCV patients is enzymatically processed to produce a CXCL10 antagonist form, introducing a role for chemokine antagonism during HCV infection.
[ [76][77][78] Serum CXCL10 levels were significantly lower in patients with seronegative occult HCV infection than in patients with chronic hepatitis C. [79] The single nucleotide polymorphism CXCL10 rs1439490 G/G is positively associated with occult HCV infection in HCV.
[80] High CXCL10 and TNF-α serum levels were observed in patients with hepatitis C-associated cryoglobulinemia (MC+HCV), and in particular, increased CXCL10 levels were significantly associated with the presence of active vasculitis. [81] In mixed cryoglobulinemia patients, circulating CXCL10 was higher in those with associated autoimmune thyroiditis. [82] by NS5A and core proteins, alone, or in combination, with cytokines [62].
To understand the molecular pathogenesis of the first stage of liver fibrosis (F1-CH-C) in hepatitis C patients, the mRNA expression of 240 selected genes in liver tissue with F1-CH-C was evaluated, compared to the normal liver (NL) [67]. The principal alterations in gene expression affected especially the IFN-regulated transcriptional network, such as IFN-α/β-inducible genes (STAT1, STAT2, etc.) and IFNγ-inducible genes (CXCL9, CXCL10, and CXCL11) [67]. Among the IFN-inducible genes, from fibrosis stage F1 to fibrosis stage F4 (in particular the transition F1-CH-C to F2-CH-C), only the mRNA levels of IFN-γ-inducible genes increased at the limit of the statistical significance, while the expression of the IFN-α/β-inducible genes did not change [67].
A further study showed that in the liver CXCL10 mRNA expression was significantly associated with lobular necroinflammatory grade and HCV genotype 1 [68]. CXCL10 expression increased strongly with a higher stage of fibrosis compared to CXCL9 and CXCL11. The reported data suggested that in CHC, CXCL10 could be determinant in the development of necroinflammation and fibrosis in the liver [68].
Moreover, patients with advanced fibrosis had significantly increased CXCL10 plasma levels. The reported data suggested that in patients with HCV genotype 1 CXCR3associated chemokines are promising noninvasive markers of hepatic fibrosis [69][70][71].
After liver transplantation (LT) for HCV infection, the recurrence of liver fibrosis can lead to graft loss and patient mortality [72]. One, 3, 5, and 7 years after LT, routine protocol biopsy was conducted, to evaluate the graft inflammation and fibrosis. In the first year upon LT, CXCL10 levels were highly associated with early fibrosis recurrence, regardless of other risk confounders, suggesting that after LT, CXCL10 is an independent biomarker of recurrent significant fibrosis for HCV infection [72].
Moreover, it has been shown that HCV-induced CXCL10 can lead to a raised hepatocyte turnover and the development of cirrhosis, fibrosis, and HCC [38].
In many HCV patients, circulating CXCL10 is enzymatically processed to produce a CXCL10 antagonist form, introducing a role for chemokine antagonism during HCV infection [76][77][78].
Patients with seronegative "occult HCV infection" (OCI) are anti-HCV and serum HCV-RNA negative but have viral RNA in the liver and altered levels of liver enzymes [79]. A study examined if the rs12979860 polymorphism of IL-28B and serum CXCL10 levels are different between chronic and seronegative OCI. The IL-28B CC genotype was significantly more prevalent in seronegative OCI (52.5%) than in CHC (24.6%; P < 0 0001) or healthy controls (32.5%; P = 0 039). Patients with seronegative OCI had significantly lower mean serum CXCL10 levels than CHC patients [79].
CHC is associated with HCV-EHM. Several studies demonstrated elevated CXCL10 and TNF-α circulating levels in patients with HCV-associated cryoglobulinemia (MC+HCV) and raised CXCL10 significantly associated with the presence of active vasculitis [81], particularly in the presence of AT [82,83].

HCV Therapy and CXCL10
In the first study, CXCL10 serum levels were significantly (P < 0 02) higher in patients with chronic hepatitis C (509 8 ± 365 4 pg/mL, mean ± s d ) than in healthy controls (30 8 ± 20 0 pg/mL, mean ± s d ). Serum CXCL10 was gradually reduced by IFN therapy, and after the successful treatment of CHC, circulating CXCL10 reached the same levels of healthy controls [59,84].
In 29 HCV genotype 1-infected patients, CXCL10 and CXCL9 were high and decreased after an antiviral therapy with a good outcome [85]. The CXCL10 level measured before starting the antiviral treatment was greater in patients with HCV who then became nonresponders (NR) to therapy (P = 0 002), indicating that CXCL10 plasma levels can predict nonresponsiveness or responsiveness to antiviral therapy with pegylated IFN (PEG-IFN), in the presence/absence of ribavirin (RBV) [85].
CHC patients treated with PEG-IFN with sustained viral response (SVR) had significantly lower pretreatment circulating CXCL10 than NR patients (332.4 vs. 476.8 pg/mL). A significant decrease of serum CXCL10 was shown in patients with SVR but not in NR. Pretreatment serum CXCL10 levels and baseline viral load were reported to be predictive factors of SVR in HCV genotype 1 patients [86].
Another study investigated circulating CXCL10 in 265 HCV-infected patients, before, during, and after PEG-IFNα 2a plus RBV treatment [87]. CXCL10 levels declined after the therapy, remaining low in patients with a SVR. On the contrary, at the end of the therapy, CXCL10 plasma levels rebounded in patients who had detectable HCV RNA. Using cut-off CXCL10 levels of 150 and 600 pg/mL to predict a SVR in HCV genotype 1-infected patients gave a specificity and sensitivity of 81% and 95%, respectively [87].
Another study reported significantly lower CXCL10 levels in patients with a rapid viral response (RVR) (P < 0 0001) and in patients obtaining a SVR (P = 0 0002) [88]. In multivariate logistic regression analyses, a low CXCL10 value independently predicted RVR and SVR. A baseline cut-off CXCL10 value of 600 pg/mL evidenced a negative predictive value (NPV) of 79% for patients with HCV genotype 1, similar to the one obtained using a reduction in HCV-RNA by at least 2 logs after 12 weeks of therapy (NPV 86%) [88].
Thyroid autoimmunity is a frequent side effect of IFN-α therapy for CHC [89,90].
Both thyroid autoimmunity and dysfunction are common side effects of IFN-α therapy for CHC, being thyroid autoantibodies the main predisposing factor for the development of thyroid dysfunctions. A paper evaluated prospectively the thyroid status in patients in treatment with 2 distinct preparations of recombinant IFNs [91]. Most patients developing thyroid autoimmunity during the IFN treatment showed a destructive thyroiditis in short temporal relationship to the appearance of thyroid autoantibodies [91].
Pretreatment mean circulating CXCL10 was significantly higher in patients who did not develop thyroid antibody positivity or dysfunctions (Group I) compared to those who showed the appearance of serum thyroid antibodies and later clinically overt thyroid dysfunction (Group II). The two groups had different rates of favourable response to IFN-α treatment (33 and 90%, respectively) [89].
In a further study, CD8+ cells were increased in the liver and correlated with inflammation [92]. Patients with CHC showed high serum concentration of CXCL10/CCL3 (vs. healthy subjects). After PEG-IFN-α-2b plus RBV therapy, CCR5(high)/CXCR3(high)-expressing CD8+ cell frequency raised in the peripheral blood, while CXCL10/CCL3 serum concentration decreased. The obtainment of viral control was linked to a rise in CXCR3(high)-expressing CD8+ cells during the therapy [92].
Another study showed that in patients with CHC, low levels of intrahepatic and systemic CXCL10 predict a good first-phase decline of HCV RNA during PEG-IFN and RBV therapy [93].
In patients with a sufficient first response to PEG-IFN, RBV ameliorates the kinetics of the early response to therapy [94], and at 12 hours, serum CXCL10 was higher than that present in patients treated with PEG-IFN alone (7.6-vs. 3.8-fold; P = 0 01) [94].
Serum CXCL10 levels were significantly lower in responders and are considered a predictor for SVR also in patients with HCV 4 genotype [100,101].
In CHC patients treated with PEG-IFN and RBV, IL-28B gene polymorphisms are strongly associated with SVR [102]. CXCL10 was assessed in the pretreatment serum of 115 NR and 157 sustained responders. Mean CXCL10 was lower in sustained responders compared to NR (437 ± 31 vs. 704 ± 44 pg/mL, P < 0 001). The PPV of low CXCL10 levels (<600 pg/mL) for SVR was 69%, while the NPV of elevated CXCL10 levels (>600 pg/mL) was 67%. The three IL-28B genotypes (in particular rs12979860) CC, TT, and CT were reported in 30%, 21%, and 49% of patients, and the relative SVR rates were 87%, 39%, and 50%, respectively. The circulating CXCL10 levels within the IL-28B genotype groups gave more information regarding the probability of SVR (P < 0 0001). In patients with CT, CC, and TT genotypes, a higher SVR rate was reported in those with low CXCL10 levels versus those with high CXCL10 (CT, 64% versus 24%; CC, 89% versus 79%; and TT, 48% versus 20%). The combination of IL-28B genotype and pretreatment serum CXCL10 levels leads to a significantly higher predictive value to discriminate between SVR and nonresponse, especially in non-CC genotypes [102].
A second study confirmed that the occurrence of SNPs adjacent to IL-28B (rs12979860, rs12980275, and rs8099917), and CXCL10 below 150 pg/mL, independently predicted the first phase viral decline and RVR, which in turn independently predicted SVR [103].
The IFN-free direct antiviral agent (DAA) therapy has changed radically antiviral therapy in HCV infection, so that a successful treatment can be reached to practically all patients irrespective of their comorbidity [108]. Actually, 3 classes of DAAs are available, and they differ according to the specific viral protein they target: NS3/4A protease inhibitors (voxilaprevir, simeprevir, glecaprevir, grazoprevir, and paritaprevir); NS5A inhibitors (ombitasvir, ledipasvir, velpatasvir, elbasvir, pibrentasvir, and daclatasvir); and NS5B polymerase inhibitors that block replication of viral RNA (dasabuvir and sofosbuvir) [109]. During DAA treatment, the inhibition of HCV replication leads to reversal of NK cells and phenotypic and functional shifts of CD4 and CD8 T cells typical of CHC, triggering viral reactivation in patients with chronic hepatitis B and recurrence of HCC in some patients with earlier effective cancer treatment [109].
Danoprevir is a powerful and selective DAA, targeting the protease activity of HCV NS3/4A [112]. During the treatment with danoprevir, changes in the CXCL10 plasma level were associated with categorical changes in HCV RNA concentration at days 7 and 14. Hepatic inflammation can be reduced by an effective treatment with a DAA and patients with an elevated baseline CXCL10 level have a higher firstphase HCV RNA decline during treatment with an NS3/4A protease inhibitor [112].
Actual therapeutic strategies are derived from the combination of PEG-IFN, RBV, and (only for patients with genotype 1 infection) a protease inhibitor. HCV treatment is developing fast from IFN-α-based therapies to IFN-α-free regimens consisting of DAAs that have an increased efficacy and tolerability in clinical trials. Virologic relapse after DAA therapy is a common cause of treatment failure, even if the reason of such relapse or whether some patients are more likely to recurrent viremia is still unknown. Circulating CXCL10 decreases with HCV clearance by DAA therapy.
Another study measured CXCL10 in 428 patients at baseline, week 1, and week 2 of oral treatment for HCV infection, suggesting that CXCL10 could be considered a surrogate marker of the rate of intracellular viral replication complex decay [113].
Peripheral and liver CXCL10 levels were evaluated in 15 patients administered with TVR/PEG-IFN/RBV, showing that CXCL10 identified very RVR in patients treated with DAAs [114].
It was investigated whether the elimination of HCV with DAAs normalizes the expression of IFN-stimulated genes and NK cell function, from the liver and blood of 13 HCVinfected patients who did not respond to treatment with PEG-IFN and RBV, during treatment with daclatasvir and asunaprevir [115]. DAA-mediated clearance of HCV was associated with the loss of intrahepatic immune activation by IFN-α, indicated by decreased levels of CXCL10 and CXCL11 and normalization of NK cell phenotype and function [115].
The treatment of CHC with DAAs results in a fast decline in viral load and circulating CXCL10 that were followed by a SVR [116].
Another paper evaluated the role of the immune system and miRNA levels in acquiring a SVR after DAA therapy in CHC patients with/without prior RG-101 (anti-miR-122) dosing [117]. Twenty-nine patients with HCV genotype 1 (n = 11), 3 (n = 17), or 4 (n = 1) were administered with sofosbuvir and daclatasvir ± ribavirin. Eighteen patients were treated earlier with RG-101. All patients had an SVR12. CXCL10 levels decreased during treatment, but remained high 24 weeks after the treatment in comparison to healthy subjects (median 53.82 and 39.4 pg/mL, P = 0 02). The reported data showed that the effective treatment of CHC patients with/without prior RG-101 dosing reduces broad immune activation and normalized miR-122 levels [117].
A paper by Yamagiwa et al. investigated the importance of pretreatment serum CXCL10 levels and IL-28B genotyping in predicting SVR to TVR-based triple therapy in patients with HCV 1 genotype [118]. The median CXCL10 levels were significantly lower in rapid virologic response (RVR) (343 pg/mL in RVR vs. 593 pg/mL in non-RVR patients, P < 0 01) or SVR (359 pg/mL in SVR vs. 566 pg/mL in non-SVR patients, P < 0 05) in the IL-28B non-TT genotype group. RVR rates were significantly lower in the group with higher serum CXCL10 levels (>450 pg/mL). In the non-TT IL-28B genotype group, RVR and SVR rates were significantly lower in the group with higher CXCL10 levels. SVR rates in the group with lower CXCL10 levels (<450 pg/mL) raised to 82% for those showing RVR, but decreased to 27% in the group with higher CXCL10 levels for those not showing RVR. The paper showed that the determination of serum CXCL10 levels before treatment could be useful to predict an effective virologic response to TVR-based triple therapy, particularly in patients with IL-28B non-TT genotype [118].
A study explored the dynamic gene expression profile of PBMCs collected from 27 HCV-infected patients undergoing DAA therapy [119]. The pretreatment expression level of IFN-induced protein 44 (IFI44) and CXCL10 correlated with the pretreatment expression level of IFN-β. After DAA treatment, a significant decrease (P < 0 05) in the expression levels of IFN-β, IFI44, and CXCL10 was observed in the PBMCs. These data showed that pretreatment activation of IFN-β response is rapidly normalized after DAA treatment [119].

Conclusion
CXCL10 and the other CXCR3 chemokines are chemoattractants for leukocytes, especially Th1 lymphocytes, and are involved in the pathogenesis of acute and "chronic hepatitis C virus (HCV) infection" (CHC). The combination of the serum level of CXCL10 and SNPs in IL-28B can identify patients with acute HCV infection who are most likely to have clearance spontaneously and those in need of early antiviral therapy.
In CHC, the HCV and intrahepatic production of IFN-γ drive a raised CXCL10 and CXCL9 expression by sinusoidal endothelium, and by hepatocytes, and thereby promote the continuing recruitment of CXCR3-expressing T cells into the hepatic lobule. CXCL10 plays a key role in the development of necroinflammation and fibrosis in the liver parenchyma in CHC; furthermore, plasma levels of CXCL10 are significantly higher in patients with advanced fibrosis. In MC+HCV patients, increased CXCL10 levels were significantly associated with the presence of active vasculitis. Furthermore, in CHC and MC patients, CXCL10 circulating levels were higher in those with associated AT.
After the successful IFN therapy of CHC, the circulating CXCL10 levels declined to the same level as in a healthy volunteer. Pretreatment CXCL10 levels were predictive of both EVR and SVR to IFN-α and RBV and may be useful to evaluate candidates for therapy. The occurrence of SNPs adjacent to IL-28B (rs12979860, rs12980275, and rs8099917), and low circulating CXCL10, independently predicted the first phase viral decline and RVR, which in turn independently predicted SVR.
Actual therapeutic strategies are derived from the combination of PEG-IFN, RBV, and (only for patients with genotype 1 infection) a protease inhibitor (as telaprevir or boceprevir). Several molecules are under clinical evaluation for their potential to bypass the disadvantages of the actual available treatments [120].
The abovementioned studies underline the importance of CXCL10 as a marker of HCV clearance and successful therapy in CHC patients.
The above reported data indicate that in HCV-infected patients, antibodies able to block the interaction between CCR5/CXCR3 and their ligands could decrease chronic liver inflammation. Since HCV is not directly cytopathic, if the migration of nonspecific T cells to the infected liver is impaired, liver damage will be reduced. This strategy could be evaluated in patients without a SVR after current standard treatment [71].
Virtually, some chemokines and their receptors are prognostic tools to predict anti-HCV treatment responses, and if this could be confirmed, these predictors could be added to daily clinical practice. Moreover, the blocking of chemokines (CXCL10) and chemokine receptors (CXCR3) is a therapeutic strategy to be evaluated in the future for nonresponders to current anti-HCV therapy [71].

Conflicts of Interest
The authors have nothing to declare.