Enhanced FCGR2A and FCGR3A signaling by HIV viremic controller IgG
Raymond A. Alvarez, … , Viviana Simon, Benjamin K. Chen
Raymond A. Alvarez, … , Viviana Simon, Benjamin K. Chen
Published February 23, 2017
Citation Information: JCI Insight. 2017;2(4):e88226. https://doi.org/10.1172/jci.insight.88226.
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Research Article AIDS/HIV Infectious disease

Enhanced FCGR2A and FCGR3A signaling by HIV viremic controller IgG

Abstract

HIV-1 viremic controllers (VC) spontaneously control infection without antiretroviral treatment. Several studies indicate that IgG Abs from VCs induce enhanced responses from immune effector cells. Since signaling through Fc-γ receptors (FCGRs) modulate these Ab-driven responses, here we examine if enhanced FCGR activation is a common feature of IgG from VCs. Using an infected cell–based system, we observed that VC IgG stimulated greater FCGR2A and FCGR3A activation as compared with noncontrollers, independent of the magnitude of HIV-specific Ab binding or virus neutralization activities. Multivariate regression analysis showed that enhanced FCGR signaling was a significant predictor of VC status as compared with chronically infected patients (CIP) on highly active antiretroviral therapy (HAART). Unsupervised hierarchical clustering of patient IgG functions primarily grouped VC IgG profiles by enhanced FCGR2A, FCGR3A, or dual signaling activity. Our findings demonstrate that enhanced FCGR signaling is a common and significant predictive feature of VC IgG, with VCs displaying a distinct spectrum of FCGR activation profiles. Thus, profiling FCGR activation may provide a useful method for screening and distinguishing protective anti-HIV IgG responses in HIV-infected patients and in monitoring HIV vaccination regimens.

Authors

Raymond A. Alvarez, Ana M. Maestre, Kenneth Law, Natasha D. Durham, Maria Ines Barria, Akiko Ishii-Watabe, Minoru Tada, Manav Kapoor, Mathew T. Hotta, Gabriela Rodriguez-Caprio, Daniel S. Fierer, Ana Fernandez-Sesma, Viviana Simon, Benjamin K. Chen

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Figure 5

IgG from viremic controllers (VCs) and chronically infected patients (CIPs) do not differ in their HIV-1 neutralizing activity.

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IgG from viremic controllers (VCs) and chronically infected patients (CI...
(A and B) Controls for HIV-1 neutralization assay carried out using TZM-bl cells infected with X4-tropic HIV-1 (pNL4-3). Neutralization curve for (A) polyclonal HIV IgG sample or (B) polyclonal HIV+ IgG sample are shown. For HIV-1 neutralization assays, polyclonal IgG were diluted 3-fold starting from a top final concentration of 500 μg/ml in a 10-point titration curve. (C) Maximum neutralization activity of patient-derived IgG comparing noninfected (HIV neg) with VC and CIP. (D) Maximum neutralization activity with VCs split into LTNP and EC subgroups. (E) Neutralization activity as measured by the area under the neutralization curve (AUC) for IgG purified from CIP, VC, and noninfected donors (HIV neg). (F) Neutralization activity (AUC) with VCs split into LTNP and EC subgroups. The mean of 3 experiments for n = 50 IgG is shown.