Department of Research and Evaluation, United Kingdom (UK) Health Security Agency, Salisbury, United Kingdom.
Department of Infection Biology, Institute of Infection and Global Health, University of Liverpool, Liverpool, United Kingdom.
Front Immunol. 2022 Apr 12;13:857481. doi: 10.3389/fimmu.2022.857481. eCollection 2022.
The 2013-2016 Ebola virus (EBOV) epidemic in West Africa was unprecedented in case numbers and fatalities, and sporadic outbreaks continue to arise. Antibodies to the EBOV glycoprotein (GP) are strongly associated with survival and their use in immunotherapy is often initially based on their performance in neutralisation assays. Other immune effector functions also contribute to EBOV protection but are more complex to measure. Their interactions with the complement system in particular are comparatively under-researched and commonly excluded from cellular immunoassays. Using EBOV convalescent plasma samples from the 2013-2016 epidemic, we investigated antibody and complement-mediated neutralisation and how these interactions can influence immunity in response to EBOV-GP and its secreted form (EBOV-sGP). We defined two cohorts: one with low-neutralising titres in relation to EBOV-GP IgG titres (LN cohort) and the other with a direct linear relationship between neutralisation and EBOV-GP IgG titres (N cohort). Using flow cytometry antibody-dependent complement deposition (ADCD) assays, we found that the LN cohort was equally efficient at mediating ADCD in response to the EBOV-GP but was significantly lower in response to the EBOV-sGP, compared to the N cohort. Using wild-type EBOV neutralisation assays with a cohort of the LN plasma, we observed a significant increase in neutralisation associated with the addition of pooled human plasma as a source of complement. Flow cytometry ADCD was also applied using the GP of the highly virulent Sudan virus (SUDV) of the species. There are no licensed vaccines or therapeutics against SUDV and it overlaps in endemicity with EBOV. We found that the LN plasma was significantly less efficient at cross-reacting and mediating ADCD. Overall, we found a differential response in ADCD between LN and N plasma in response to various glycoproteins, and that these interactions could significantly improve EBOV neutralisation for selected LN plasma samples. Preservation of the complement system in immunoassays could augment our understanding of neutralisation and thus protection against infection.
2013-2016 年西非爆发的埃博拉病毒(EBOV)疫情在病例数量和死亡人数方面前所未有,且散发性疫情仍在继续出现。针对 EBOV 糖蛋白(GP)的抗体与存活强烈相关,其免疫疗法的应用通常最初基于其在中和测定中的表现。其他免疫效应功能也有助于 EBOV 保护,但更难测量。特别是它们与补体系统的相互作用相对研究较少,通常不包括在细胞免疫测定中。使用 2013-2016 年疫情中的埃博拉康复期血浆样本,我们研究了抗体和补体介导的中和作用,以及这些相互作用如何影响针对 EBOV-GP 及其分泌形式(EBOV-sGP)的免疫反应。我们定义了两个队列:一个与 EBOV-GP IgG 滴度相关的低中和滴度(LN 队列),另一个中和与 EBOV-GP IgG 滴度呈直接线性关系(N 队列)。使用流式细胞术抗体依赖性补体沉积(ADCD)测定,我们发现 LN 队列在介导针对 EBOV-GP 的 ADCD 方面同样有效,但与 N 队列相比,针对 EBOV-sGP 的 ADCD 显著降低。使用含有 LN 血浆的野生型 EBOV 中和测定,我们观察到随着补充人血浆作为补体来源,中和作用显著增加。还使用高毒力苏丹病毒(SUDV)的 GP 进行了流式细胞术 ADCD 测定。目前尚无针对 SUDV 的许可疫苗或治疗方法,且其与 EBOV 流行范围重叠。我们发现 LN 血浆在交叉反应和介导 ADCD 方面的效率明显较低。总体而言,我们发现 LN 和 N 血浆对各种糖蛋白的 ADCD 反应存在差异,并且这些相互作用可以显著提高选定 LN 血浆样本的 EBOV 中和作用。在免疫测定中保留补体系统可以增强我们对中和作用的理解,从而预防感染。
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