Human Interferon Regulatory Factor 2 Gene Expression is Induced in Chronic Hepatitis C Virus Infection-A Possible Mode of Viral Persistence

Rathindra M Mukherjee; Budhapriyavilas Bansode; Puja Gangwal; Aparna Jakkampudi; Panyala B Reddy; Padaki N Rao; Rajesh Gupta; D Nageshwar Reddy

doi:10.1016/S0973-6883(12)60080-2

Human Interferon Regulatory Factor 2 Gene Expression is Induced in Chronic Hepatitis C Virus Infection-A Possible Mode of Viral Persistence

J Clin Exp Hepatol. 2012 Mar;2(1):27-34. doi: 10.1016/S0973-6883(12)60080-2. Epub 2012 Apr 12.

Authors

Rathindra M Mukherjee¹, Budhapriyavilas Bansode¹, Puja Gangwal¹, Aparna Jakkampudi¹, Panyala B Reddy¹, Padaki N Rao², Rajesh Gupta², D Nageshwar Reddy²

Affiliations

¹ Asian Health Care Foundation, Somajiguda - 500082, Hyderabad, AP, India.
² Asian Institute of Gastroenterology, Somajiguda - 500082, Hyderabad, AP, India.

Abstract

Background: The interferon regulatory factors (IRFs) are a family of transcription factors known to be involved in the modulation of cellular responses to interferons (IFNs) and viral infection. While IRF-1 acts as a positive regulator, IRF-2 is known to repress IFN-mediated gene expression. The increase in the IRF-1/IRF-2 ratio is considered as an important event in the transcriptional activation of IFN-α gene toward development of the cellular antiviral response.

Objective: This study was performed to assess the expression of IRF mRNAs along with the expression level of IFN-α, its receptor (IFNAR-1), and the signal transduction factor (STAT-1) in treatment naive hepatitis C virus (HCV)-infected subjects.

Materials: Thirty-five chronically infected (CHC) patients and 39 voluntary blood donors as controls were included in the study. Quantification of HCV-RNA (ribonucleic acid) and genotyping were done by real-time polymerase chain reaction (PCR) and hybridization assays, respectively, using patient's serum/plasma. In both controls and patients, the serum level of IFN-α and IFN-α was measured by flow cytometry. Target gene expressions were studied by retro-transcription of respective mRNAs extracted from peripheral blood mononuclear cells (PBMCs) followed by PCR amplification and densitometry. Minus-strand HCV-RNA as a marker of viral replication in PBMCs was detected by an inhouse PCR assay.

Results: Both IRF-1 and IRF-2 genes were significantly enhanced in CHC than in control subjects (P < 0.001). A significant positive correlation (r (2) = 0.386, P <0.01) was obtained between higher IRF-2 gene expression and increasing level of HCV-RNA. Chronically infected subjects (13%) harboring replicating HCV in PBMCs showed no significant differences in gene expressions than the subjects without HCV in PBMCs.

Conclusion: Our findings indicate that HCV modulates host immunity by inducing IRF-2 gene to counteract IRF-1-mediated IFN-α gene expression. Since the IRF-2 gene is known to encode oncogenic protein, the role of IRF-2 in CHC patients developing hepatocellular carcinoma warrants further studies.

Keywords: CHC, chronic hepatitis C; CLD, chronic liver disease; Gene expression; HBV, hepatitis B virus; HBsAg, hepatitis B virus surface antigen; HCC, hepatocellular carcinoma; HCV, hepatitis C virus; IFN, interferon; IRES, internal ribosomal entry site; IRF, interferon regulatory factors; PBMC, peripheral blood mononuclear cells; PCR, polymerase chain reaction; SVR, sustained virological response; VCAM, vascular cell adhesion molecule; hepatitis C virus; interferon regulatory factor 2; interferon-alfa; peripheral blood mononuclear cells.