Research Institute of the McGill University Health Centre Montreal, Montreal, QC, Canada.
Division of Experimental Medicine, McGill University, Montreal, QC, Canada.
Front Immunol. 2020 Sep 30;11:583820. doi: 10.3389/fimmu.2020.583820. eCollection 2020.
Antibody dependent (AD) functions such as AD cellular cytotoxicity (ADCC) were associated with lower viral load (VL) in untreated HIV progressors and protection from HIV infection in the modestly protective RV144 HIV vaccine trial. Target cells used to measure ADCC, AD complement deposition (ADCD), and AD cellular trogocytosis (ADCT) have been either HIV envelope (Env) gp120-coated CEM.NKr.CCR5 cells or HIV infected cell cultures. In HIV infected cell cultures, uninfected bystander cells take up gp120 shed from infected cells. Both gp120-coated and gp120+ bystander cells expose CD4 induced (CD4i) epitopes, which are normally hidden in native trimeric Env expressed by genuinely HIV infected cells since Nef and Vpu downmodulate cell surface CD4. Antibody dependent assays using either of these target cells probe for CD4i Abs that are abundant in HIV plasma but that do not recognize HIV-infected cells. Here, we examined ADCC, ADCD, and ADCT functions using a target cell line, sorted HIV-infected cell line cells, whose HIV infection frequency nears 100% and that expresses HIV Env in a native trimeric closed conformation. Using sorted HIV-infected cells (siCEM) as targets, we probed the binding and AD functions of anti-gp120/Env Abs in plasma from HIV-infected untreated progressor (UTP, = 18) and treated (TP, = 24) subjects, compared to that in Elite controllers (EC, = 37) and Viral Controllers (VC, = 16), which are rare subsets of HIV-infected individuals who maintain undetectable or low VL, respectively, without treatment. Gp120-coated beads were used to measure AD cellular phagocytosis. Equivalent concentrations of input IgG in plasma from UTPs, ECs, and VCs supported higher levels of all AD functions tested than plasma from TPs. When AD activities were normalized to the concentration of anti-gp120/Env-specific Abs, between-group differences largely disappeared. This finding suggests that the anti-gp120/Env Abs concentrations and not their potency determined AD functional levels in these assays. Elite controllers did differ from the other groups by having AD functions that were highly polyfunctional and highly correlated with each other. PCR measurement of HIV reservoir size showed that ADCC activity was higher in ECs and VCs with a reservoir size below the limit of detection compared to those having a measurable HIV reservoir size.
抗体依赖(AD)功能,如 AD 细胞细胞毒性(ADCC),与未经治疗的 HIV 进展者的病毒载量(VL)较低有关,并且在适度保护性 RV144 HIV 疫苗试验中可预防 HIV 感染。用于测量 ADCC、AD 补体沉积(ADCD)和 AD 细胞 trogocytosis(ADCT)的靶细胞是 HIV 包膜(Env)gp120 包被的 CEM.NKr.CCR5 细胞或 HIV 感染的细胞培养物。在 HIV 感染的细胞培养物中,未被感染的旁观者细胞从感染的细胞中摄取 gp120。gp120 包被的和 gp120+旁观者细胞都暴露 CD4 诱导(CD4i)表位,这些表位在由真正感染 HIV 的细胞表达的天然三聚体 Env 中通常是隐藏的,因为 Nef 和 Vpu 下调细胞表面 CD4。使用这两种靶细胞中的任何一种进行的抗体依赖性测定,都可以探测到在 HIV 血浆中含量丰富但不能识别 HIV 感染细胞的 CD4i Abs。在这里,我们使用一种靶细胞系(sorted HIV-infected cell line cells)检查 ADCC、ADCD 和 ADCT 功能,该细胞系的 HIV 感染频率接近 100%,并且以天然三聚体封闭构象表达 HIV Env。使用 sorted HIV-infected cells(siCEM)作为靶细胞,我们探测了来自未经治疗的 HIV 进展者(UTP, = 18)和治疗(TP, = 24)受试者的血浆中和 AD 功能的抗 gp120/Env Abs,与精英控制器(EC, = 37)和病毒控制器(VC, = 16)相比,后者是 HIV 感染者的罕见亚群,分别无需治疗即可维持不可检测或低 VL。gp120 包被珠用于测量 AD 细胞吞噬作用。血浆中输入 IgG 的等效浓度在 UTP、EC 和 VC 中支持比 TP 中的更高水平的所有 AD 功能。当 AD 活性与抗 gp120/Env 特异性 Abs 的浓度归一化时,组间差异基本消失。这一发现表明,在这些测定中,决定 AD 功能水平的是抗 gp120/Env Abs 的浓度而不是其效力。精英控制器与其他组不同,其 AD 功能具有高度多功能性,并且彼此高度相关。HIV 储存库大小的 PCR 测量表明,与具有可测量的 HIV 储存库大小的个体相比,储存库大小低于检测限的 EC 和 VC 中的 ADCC 活性更高。
