Department of Biosciences, University of Salzburg, Salzburg, Austria.
Central Animal Laboratory, University of Turku, Turku, Finland.
Front Immunol. 2020 Sep 3;11:2118. doi: 10.3389/fimmu.2020.02118. eCollection 2020.
Allergic sensitization to the major allergen Bet v 1 represents the dominating factor inducing a vast variety of allergic symptoms in birch pollen allergic patients worldwide, including the pollen food allergy syndrome. In order to overcome the huge socio-economic burden associated with allergic diseases, allergen-specific immunotherapy (AIT) as a curative strategy to manage the disease was introduced. Still, many hurdles related to this treatment exist making AIT not the patients' first choice. To improve the current situation, the development of hypoallergen-based drug products has raised attention in the last decade. Herein, we investigated the efficacy of the novel AIT candidate BM4, a hypoallergenic variant of Bet v 1, to induce treatment-relevant cross-reactive Bet v 1-specific IgG antibodies in two different mammals, Wistar rats and New Zealand White rabbits. We further analyzed the cross-reactivity of BM4-induced Wistar rat antibodies with the birch pollen-associated food allergens Mal d 1 and Cor a 1, and the functional capability of the induced antibodies to act as IgE-blocking IgG antibodies. Enzyme-linked immunosorbent assay (ELISA) was used to determine the titers of rat IgG1, IgG2a, IgG2b, and IgE, as well as rabbit IgG and IgE antibodies. To address the functional relevance of the induced IgG antibodies, the capacity of rat sera to suppress binding of human IgE to Bet v 1 was investigated by using an inhibition ELISA and an IgE-facilitated allergen-binding inhibition assay. We found that the treatment with BM4 induced elevated Bet v 1-specific IgG antibody titers in both mammalian species. In Wistar rats, high BM4-specific IgG1, IgG2a, and IgG2b titers (10 to 10) were induced, which cross-reacted with wild-type Bet v 1, and the homologous allergens Mal d 1 and Cor a 1. Rat allergen-specific IgG antibodies sustained upon treatment discontinuation. Sera of rats immunized with BM4 were able to significantly suppress binding of human IgE to the wild-type allergens and CD23-mediated human IgE-facilitated Bet v 1 binding on B cells. By contrast, treatment-induced IgE antibody levels were low or undetectable. In summary, BM4 induced a robust IgG immune response that efficiently blocked human IgE-binding to wild-type allergens, underscoring its potential therapeutic value in AIT.
对主要过敏原 Bet v 1 的过敏敏化是导致世界范围内桦树花粉过敏患者出现各种过敏症状的主要因素,包括花粉食物过敏综合征。为了克服与过敏相关的巨大社会经济负担,作为一种治疗策略的过敏原特异性免疫疗法(AIT)被引入。尽管如此,这种治疗方法仍然存在许多障碍,使得 AIT 不是患者的首选。为了改善这种情况,基于低变应原的药物产品的开发在过去十年中引起了关注。在此,我们研究了新型 AIT 候选物 BM4 的疗效,BM4 是 Bet v 1 的低变应原变体,可在两种不同的哺乳动物,Wistar 大鼠和新西兰白兔中诱导与治疗相关的交叉反应性 Bet v 1 特异性 IgG 抗体。我们进一步分析了 BM4 诱导的 Wistar 大鼠抗体与桦树花粉相关的食物过敏原 Mal d 1 和 Cor a 1 的交叉反应性,以及诱导的抗体作为 IgE 阻断 IgG 抗体的功能能力。酶联免疫吸附试验(ELISA)用于测定大鼠 IgG1、IgG2a、IgG2b 和 IgE 以及兔 IgG 和 IgE 抗体的效价。为了解决诱导的 IgG 抗体的功能相关性,通过抑制 ELISA 和 IgE 促进的过敏原结合抑制试验,研究了大鼠血清抑制人 IgE 与 Bet v 1 结合的能力。我们发现,BM4 治疗在两种哺乳动物中均诱导了升高的 Bet v 1 特异性 IgG 抗体效价。在 Wistar 大鼠中,诱导了高 BM4 特异性 IgG1、IgG2a 和 IgG2b 效价(10 至 10),与野生型 Bet v 1 以及同源过敏原 Mal d 1 和 Cor a 1 发生交叉反应。大鼠过敏原特异性 IgG 抗体在治疗停止后持续存在。用 BM4 免疫的大鼠血清能够显著抑制人 IgE 与野生型过敏原的结合以及 CD23 介导的人 IgE 促进的 B 细胞上的 Bet v 1 结合。相比之下,治疗诱导的 IgE 抗体水平较低或无法检测到。总之,BM4 诱导了强大的 IgG 免疫反应,有效地阻断了人 IgE 与野生型过敏原的结合,突显了其在 AIT 中的潜在治疗价值。
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