Interaction between complement receptor gC1qR and hepatitis C virus core protein inhibits T-lymphocyte proliferation
David J. Kittlesen, … , Thomas J. Braciale, Young S. Hahn
David J. Kittlesen, … , Thomas J. Braciale, Young S. Hahn
Published November 15, 2000
Citation Information: J Clin Invest. 2000;106(10):1239-1249. https://doi.org/10.1172/JCI10323.
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Interaction between complement receptor gC1qR and hepatitis C virus core protein inhibits T-lymphocyte proliferation

Abstract

Hepatitis C virus (HCV) is an important human pathogen that is remarkably efficient at establishing persistent infection. The HCV core protein is the first protein expressed during the early phase of HCV infection. Our previous work demonstrated that the HCV core protein suppresses host immune responses, including anti-viral cytotoxic T-lymphocyte responses in a murine model. To investigate the mechanism of HCV core-mediated immunosuppression, we searched for host proteins capable of associating with the core protein using a yeast two-hybrid system. Using the core protein as bait, we screened a human T cell–enriched expression library and identified a gene encoding the gC1q receptor (gC1qR). C1q is a ligand of gC1qR and is involved in the early host defense against infection. Like C1q, HCV core can inhibit T-cell proliferative responses in vitro. This core-induced anti–T-cell proliferation is reversed by addition of anti-gC1qR Ab in a T-cell proliferation assay. Furthermore, biochemical analysis of the interaction between core and gC1qR indicates that HCV core binds the region spanning amino acids 188 to 259 of gC1qR, a site distinct from the binding region of C1q. The inhibition of T-cell responsiveness by HCV core may have important implications for HCV persistence in humans.

Authors

David J. Kittlesen, Kimberly A. Chianese-Bullock, Zhi Qiang Yao, Thomas J. Braciale, Young S. Hahn

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Figure 6

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Cell-surface expression of gC1qR on human PBMCs and MOLT-4 cell lines. C...
Cell-surface expression of gC1qR on human PBMCs and MOLT-4 cell lines. Cell-surface expression of gC1qR in MOLT-4 T-cell line (a), and human PBMCs (b). MOLT-4 T-cell line or human PBMCs were incubated with media alone (left panel) or anti-gC1qR Ab, 74.5.2 (right panel), and stained cells were examined for FACS analysis. Value (%) represents the cell population gated with gC1qR-positive cells. (c) Analysis of surface-biotinylated gC1qR. Cell-surface proteins of human PBMCs were biotinylated. Solubilized membrane proteins were subjected to SDS-PAGE before (lane 1) or after (lane 2) immunoprecipitation with anti-gC1qR mAb 60.11 and 74.5.2. The separated proteins were transferred to PVDF membranes and developed using streptavidin. MFI, mean fluorescence intensity; 1°, primary; 2°, secondary.