Chronic hepatitis C virus (HCV) infection affects over 170 million people worldwide.1 The prevalence of chronic HCV infection in the USA is approximately 1.3%,2 while it is estimated as 1.2-1.5% in Mexico.3,4 Cirrhosis develops in 30-40% of individuals with chronic HCV infection unless the virus is eradicated.5-7 At present, advanced liver disease due to HCV infection is the leading indicator of liver transplantation in the USA and Europe.2 HCV infection is also the most important risk factor for hepatocellular carcinoma (HCC) in Western European and North American populations.8

The standard treatment for HCV infection is based on a combination of PEGylated-interferon alpha (PEG-IFNα) and ribavirin (RBV).5 Pharmacotherapeutic success is evaluated based on viral RNA negativity 24 weeks after completion of the treatment, which is defined as a sustained virological response (SVR).6 Only 40-50% of patients infected with HCV genotype 1 (HCV-1) had SVR after 48 weeks of treatment, whereas 75% of patients infected with HCV genotypes 2 or 3 (HCV-2/ 3) typically achieved SVR after 24 weeks of therapy.9 In HCV-1 cases, additional treatment with protease inhibitors (PI) has improved the SVR rate to about 80%.10

Single nucleotide polymorphisms (SNPs) located close to the coding region of the interleukin 28B (IL28B) gene on chromosome 19 are the most important genetic risk factors associated with SVR in patients infected with HCV.11 Three specific SNPs (rs12979860, rs8099917, and rs8103142) were the strongest predictors of HCV clearance and SVR.9 The aim of this study was to determine the association between the IL28B SNPs, i.e., rs12979860, rs8099917, and rs8103142, and an SVR following treatment based on PEG-IFNa and RBV in a Mexican cohort of HCV-1/2 patients.

Patients were recruited between May 2007 and May 2011 in the Liver Unit of the Fundación Clínica Médica Sur. The protocol was approved by the Institutional Review Boards of the Instituto Nacional de Salud Pública and Fundación Clínica Médica Sur. The cohort provided written consent and they were composed of treatment-naïve patients of both genders who had been diagnosed with HCV-1/2 genotypes, before being treated with PEG-IFNα and RBV therapy, according to the standard protocol.5 The participants completed a written questionnaire to collect socioeconomic, demographic, clinical, and laboratory data.

HCV infection was diagnosed based on the detection of anti-HCV antibodies. The viral load was determined using the COBAS TaqMan HCV test v2.0 (Roche Molecular Systems, Pleasanton, CA) and it was classified as low grade (< 400,000 IU/mL) or high grade (≥ 400,000 IU/mL).

IL28B was genotyped using DNA and mRNA extracted from blood samples with the Ficoll/Trizol method. The purity of the DNA was evaluated spectrophotometrically based on the ratio of the absorbance at 260 nm and 280 nm (A260/280). The DNA integrity was confirmed by agarose gel electrophoresis 0.8%. IL28B genotyping was performed using TaqMan SNP genotyping assays and the cytokine mRNA levels were quantified using TaqMan gene expression assays with a 7900HT Fast Realtime PCR System (Applied Biosystems, Foster City, CA), according to the manufacturer’s instructions. All of the assays were carried out in duplicate. The genotyping quality control used a call rate of 0.99 (i.e., the number of individuals assigned a genotype). All samples with a 0.99 call rate were analyzed by two independent researchers who scored the genotype results using a graphical view (SD 2.4, Applied Biosystems), while all differences were resolved by discussions between the independent researchers, or by rerunning the samples if necessary. If the concordance was < 99.99%, the result was treated as a missing value.

In the study group of 83 HCV-infected patients, the mean age was 57 ± 11 years. The baseline viral load was 434,955 ± 387,213 IU/mL, and 53% (n = 44) of patients had a high viral load. Genotype 1 was most frequent (70%, n = 58) and the overall SVR was 32% (n = 27) in our population. The SVR was 27% in the HCV-1 group and 44% in the HCV-2 group. After classifying the patients based on their SVR status, we found that patients with SVRs were significantly younger (53 ± 11 vs. 59 ± 11 years, P = 0.048) and they had a significantly lower frequency of high aspartate aminotransferase (AST) levels (18% vs. 82%, P = 0.001) and alanine aminotransferase (ALT) levels (24% vs. 76%, P = 0.001). Furthermore, the alkaline phosphatase (ALP) and gamma-glutamyltranspeptidase (GGT) levels were increased less in patients with SVRs. A high viral load was more frequent in non-SVR patients (77% vs. 23%, P = 0.04) (Table 1).

All SNPs were in Hardy-Weinberg equilibrium and the allelic and genotypic frequencies of all SNPs in this study were similar to other populations (Table 2). The correlation between the observed viral load and treatment response was evaluated directly. The basal viral load was lower (300,377 ± 264,950 copies/mL) in the SVR group than in the non-SVR group (499,840 ± 422,538 copies/mL).

The effects of the IL28B SNPs (rs8099917 G/T, rs12979860 C/T, and rs8103142 T/C) on the treatment response were tested using ORs estimated via logistic regression, which were adjusted for age, gender, body mass index (BMI), and viral load. We found that IL28B rs12979860 C/C had a significant association with the SVR (OR = 4.83, 95% CI = 1.12-20.8, P = 0.033) in the codominant model, while the C/T+T/T genotype had an association in the dominant model (OR = 4.02, 95% CI = 1.11-14.54, P = 0.022). Finally, we found a positive association between the SVR and the log-additive model (OR = 2.12; 95% CI = 1.05-4.26, P = 0.03) (Table 3).

The standard HCV infection therapy is a combination of PEG-IFNα and RBV for 24 or 48 weeks, depending on the HCV genotype.5 The SVR depends on the viral genotype and host factors, particularly gender, age, the presence of insulin resistance, hepatic fibrosis, and the patient’s genetic background. The first attempt to determine the importance of the patient genetic background for the SVR was reported by Ge, et al.7 A genome-wide association study (GWAS) was performed using a cohort of HCV genotype 1-infected patients who were treated with PEG-IFNα and RBV to determine any genomic variations related to SVR. This study showed that the SVR was linked to SNPs located close to the coding region of the interleukin 28B (IL28B) gene on chromosome 19. IL28B belongs to the type III interferon family of cytokines, which contains IL29, IL28A, and IL28B (also known as IFN-λ1, IFN-λ2, and IFN-λ3, respectively).

The effect of the rs12979860 polymorphism on the response to PEG-IFNa and RBV treatment in patients infected with HCV-1 has been demonstrated extensively. Patients who carry the CC polymorphism have SVR rates of > 80%, so this polymorphism is considered to be favorable. By contrast, patients with the TT polymorphism have SVR rates of <40%, so it is considered unfavorable.11 It is clear that genotyping the rs12979860 polymorphism is a strong predictor of the clinical outcome for HCV-infected patients. rs8099917SNP is located in the intergenetic region between IL28A and IL28B and its variations are associated with the PEG-IFNα and RBV therapeutic response, suggesting that the TT genotype is a predictor of a good response whereas the TG/GG genotypes are poor-response indicators.12,13 A third causal variant located in the third exon region of IL28B, i.e., rs8103142, was also found to be important in a GWAS. The polymorphism in this region had a few rare T/C variations, which were strongly associated with SVR in individuals.9,14

The aim of the current study was to determine the association between three IL28B SNPs and SVR after PEG-IFNα and RBV treatment in a Mexican population infected with HCV-1/2. The main finding was that there was an association between rs12979860 CC and SVR in a codominant model (OR = 4.83, 95% CI = 1.12-20.8, P = 0.033). However, there was no statistically significant association between rs8099917 or rs8103142 and SVR. In our population, the overall SVR rate was 32% (n = 27). The SVR rate was 27% in the HCV-1 group and 44% in the HCV-2 group. A previous study of a population from Mexico and Puerto Rico reported an SVR rate of 34% in HCV-1 patients treated with PEG-IFNa and RBV. Thus, these results agreed with those in our study cohort.15

The impact of the rs12979860 polymorphism on SVR has been extensively demonstrated in HCV-1 patients treated with PEG-IFNα and RBV. However, the IL28B genotype is less relevant to PEG-IFNα and RBV treatment of patients with HCV genotypes 2 and 3, in whom the CC variant was correlated with an SVR rate of 87.4%, while the CT and TT genotypes were correlated with SVR rates of 70.7% and 73.1%, respectively.16 A cross-analysis of the rs12979860 CC variant and additional genotyping of the rs8099917 SNP had no effect on the response prediction, whereas those with the rs12979860 TT variant had an improved SVR prediction after additional genotyping of rs8099917 SNPs.17

It is known that the prevalence of rs12979860 CC varies greatly among ethnic groups, i.e., 23.1% to 97.9%.18 In this study, the rs12979860 polymorphisms CC, CT, and TT were present in 24%, 41%, and 35% of patients, respectively. The prevalence of the C allele in the Mexican Pima population is 55.5%.18 In another Mexican cohort containing 205 HCV-1-infected patients, the frequencies were 18.5%, 19.5%, and 62.0% for the CC, CT, and TT variants, respectively.19 The reference SNP cluster report for rs12979860 in the HapMap Project reported a CC prevalence of 28.6%.20

In the present study, we tested the effects of age, the levels of ALT, AST, ALP, and GGT, and the viral load on SVR. Other reported baseline predictors of the SVR with interferon-based therapies include patient body weight, insulin resistance, steatosis, and fibrosis stage.21,22 In previously untreated patients, the SVR predictors include a low baseline viral load (OR = 11.6), IL28B genotype (rs12979860 CC vs. TT or CT; OR = 2.6, OR = 2.1), absence of cirrhosis (OR = 4.3), HCV 1b subtype (OR = 2.0), non-black race (OR = 2.0), and BMI (< 30 vs. > 30; OR = 1.6).23

Understanding the associations between different IL28B polymorphisms and SVR after treatment with PEG-IFNα and RVB is an important issue, because there is a debate over whether all untreated patients should receive triple therapy given the increased costs and possible adverse effects. In countries such as Mexico, an analysis of proposed strategies based on IL28B rs12979860 and SVR could be very useful in terms of cost-effectiveness. This analysis could also provide benefits related to adverse effects, treatment tolerance, and the induction of viral drug resistance.

At present, the possible effects of IL28B on available direct-acting antiviral (DAA) therapies, such as PI, are not clear. However, a comparison was made to test the benefits of dual therapy (PEG-IFNα and RVB) relative to the current triple therapy (PEG-IFNα, RVB, and PI) in untreated HCV-1 patients. The treatment strategies were guided by the rapid viral response (RVR) and the IL28B genotype, which made it possible to avoid PI exposure in 25-33% of patients, thereby reducing costs and risks and improving benefits. Based on this, it is recommended to use free PI strategies as a first-line therapy in patients with the IL28B CC genotype or those with an RVR.24 Patients with rs12979860 CT or TT benefit from the addition of DAAs and their SVR rates increased twofold with boceprevir or telaprevir to 55-70% in the treatment naïve.25

In the Mexican HCV-1-infected population, patients with favorable characteristics such as rs12979860 CC and a low viral load, or younger patients without major disturbances in liver function tests, could benefit from dual therapy with peg-IFNα and RVB. Several factors are associated with the treatment response, but we argue that predicting a failure to respond to therapy is the most useful parameter for clinical management.

In conclusion, the frequencies of the rs12979860 alleles CC, CT, and TT in the study population were 24%, 41%, and 35%, respectively. rs12979860 CC was the best positive predictive of SVR, whereas SVR was not associated with the SNPs rs8099917 or rs8103142.

The authors declare no competing interests.

This work was supported by the following grant: CONACyT SALUD-2008-01-87267. We would like to thank all the researchers and all the personnel from Instituto Mexicano de Salud Pública and Dirección de Investigación Biomédica of Fundación Clínica Médica Sur. Special Acknowledgement to the patients who accept participate in this study