TY - JOUR
T1 - Expanding the host range of hepatitis C virus through viral adaptation
AU - von Schaewen, Markus
AU - Dorner, Marcus
AU - Hueging, Kathrin
AU - Foquet, Lander
AU - Gerges, Sherif
AU - Hrebikova, Gabriela
AU - Heller, Brigitte
AU - Bitzegeio, Julia
AU - Doerrbecker, Juliane
AU - Horwitz, Joshua A.
AU - Gerold, Gisa
AU - Suerbaum, Sebastian
AU - Rice, Charles M.
AU - Meuleman, Philip
AU - Pietschmann, Thomas
AU - Ploss, Alexander
N1 - Funding Information:
We thank Jade Xiao, Rachael Labitt, Tamar Frilling, and Sabrina Woltemate for excellent technical help and Jenna Gaska, Qiang Ding, and Florian Douam for editing and critical discussions of the manuscript. This study is supported by grants from the National Institutes of Health (R01 AI079031, R01 AI107301, and R21AI117213 to A.P.), a Research Scholar Award from the American Cancer Society (RSG-15-048-01-MPC to A.P.), a Burroughs Wellcome Fund Award for Investigators in Pathogenesis (to A.P.), and a grant from the German Research Foundation (SFB 900/Z1 to S.S.). T.P. was supported by a grant from the European Research Council ERC-2011-StG_281473 (VIRAFRONT) and by a grant from the Helmholtz Association SO-024. M.V.S. is a recipient of a postdoctoral fellowship from the German Research Foundation (Deutsche Forschungsgemeinschaft). This work, including the efforts of Alexander Ploss, was funded by HHS | NIH | National Institute of Allergy and Infectious Diseases (NIAID) (R01 AI079031, R01 AI107301, and R21AI117213). This work, including the efforts of Sebastian Suerbaum, was funded by Deutsche Forschungsgemeinschaft (DFG) (SFB 900/Z1). This work, including the efforts of Markus von Schaewen, was funded by Deutsche Forschungsgemeinschaft (DFG). This work, including the efforts of Thomas Pietschmann, was funded by EC | European Research Council (ERC) (ERC-2011-StG_ 281473-(VIRAFRONT)). This work, including the efforts of Alexander Ploss, was funded by Burroughs Wellcome Fund (BWF). This work, including the efforts of Alexander Ploss, was funded by American Cancer Society (ACS) (RSG-15-048-01-MPC). This work, including the efforts of Thomas Pietschmann, was funded by Helmholtz-Gemeinschaft (Helmholtz Association) (SO-024).
Publisher Copyright:
© 2016 von Schaewen et al.
PY - 2016
Y1 - 2016
N2 - Hepatitis C virus (HCV) species tropism is incompletely understood. We have previously shown that at the level of entry, human CD81 and occludin (OCLN) comprise the minimal set of human factors needed for viral uptake into murine cells. As an alternative approach to genetic humanization, species barriers can be overcome by adapting HCV to use the murine orthologues of these entry factors. We previously generated a murine tropic HCV (mtHCV or Jc1/mCD81) strain harboring three mutations within the viral envelope proteins that allowed productive entry into mouse cell lines. In this study, we aimed to characterize the ability of mtHCV to enter and infect mouse hepatocytes in vivo and in vitro. Using a highly sensitive, Cre-activatable reporter, we demonstrate that mtHCV can enter mouse hepatocytes in vivo in the absence of any human cofactors. Viral entry still relied on expression of mouse CD81 and SCARB1 and was more efficient when mouse CD81 and OCLN were overexpressed. HCV entry could be significantly reduced in the presence of anti-HCV E2 specific antibodies, suggesting that uptake of mtHCV is dependent on viral glycoproteins. Despite mtHCV’s ability to enter murine hepatocytes in vivo, we did not observe persistent infection, even in animals with severely blunted type I and III interferon signaling and impaired adaptive immune responses. Altogether, these results establish proof of concept that the barriers limiting HCV species tropism can be overcome by viral adaptation. However, additional viral adaptations will likely be needed to increase the robustness of a murine model system for hepatitis C. IMPORTANCE At least 150 million individuals are chronically infected with HCV and are at risk of developing serious liver disease. Despite the advent of effective antiviral therapy, the frequency of chronic carriers has only marginally decreased. A major roadblock in developing a vaccine that would prevent transmission is the scarcity of animal models that are susceptible to HCV infection. It is poorly understood why HCV infects only humans and chimpanzees. To develop an animal model for hepatitis C, previous efforts focused on modifying the host environment of mice, for example, to render them more susceptible to HCV infection. Here, we attempted a complementary approach in which a laboratory-derived HCV variant was tested for its ability to infect mice. We demonstrate that this engineered HCV strain can enter mouse liver cells but does not replicate efficiently. Thus, additional adaptations are likely needed to construct a robust animal model for HCV.
AB - Hepatitis C virus (HCV) species tropism is incompletely understood. We have previously shown that at the level of entry, human CD81 and occludin (OCLN) comprise the minimal set of human factors needed for viral uptake into murine cells. As an alternative approach to genetic humanization, species barriers can be overcome by adapting HCV to use the murine orthologues of these entry factors. We previously generated a murine tropic HCV (mtHCV or Jc1/mCD81) strain harboring three mutations within the viral envelope proteins that allowed productive entry into mouse cell lines. In this study, we aimed to characterize the ability of mtHCV to enter and infect mouse hepatocytes in vivo and in vitro. Using a highly sensitive, Cre-activatable reporter, we demonstrate that mtHCV can enter mouse hepatocytes in vivo in the absence of any human cofactors. Viral entry still relied on expression of mouse CD81 and SCARB1 and was more efficient when mouse CD81 and OCLN were overexpressed. HCV entry could be significantly reduced in the presence of anti-HCV E2 specific antibodies, suggesting that uptake of mtHCV is dependent on viral glycoproteins. Despite mtHCV’s ability to enter murine hepatocytes in vivo, we did not observe persistent infection, even in animals with severely blunted type I and III interferon signaling and impaired adaptive immune responses. Altogether, these results establish proof of concept that the barriers limiting HCV species tropism can be overcome by viral adaptation. However, additional viral adaptations will likely be needed to increase the robustness of a murine model system for hepatitis C. IMPORTANCE At least 150 million individuals are chronically infected with HCV and are at risk of developing serious liver disease. Despite the advent of effective antiviral therapy, the frequency of chronic carriers has only marginally decreased. A major roadblock in developing a vaccine that would prevent transmission is the scarcity of animal models that are susceptible to HCV infection. It is poorly understood why HCV infects only humans and chimpanzees. To develop an animal model for hepatitis C, previous efforts focused on modifying the host environment of mice, for example, to render them more susceptible to HCV infection. Here, we attempted a complementary approach in which a laboratory-derived HCV variant was tested for its ability to infect mice. We demonstrate that this engineered HCV strain can enter mouse liver cells but does not replicate efficiently. Thus, additional adaptations are likely needed to construct a robust animal model for HCV.
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U2 - 10.1128/mBio.01915-16
DO - 10.1128/mBio.01915-16
M3 - Article
C2 - 27834208
AN - SCOPUS:85007545186
SN - 2161-2129
VL - 7
JO - mBio
JF - mBio
IS - 6
M1 - e01915-16
ER -