Technology center, LenioBio GmbH, Dusseldorf, Germany.
Laboratory of Nematology, Wageningen University, Wageningen, Netherlands.
Front Immunol. 2023 Jan 26;14:1088852. doi: 10.3389/fimmu.2023.1088852. eCollection 2023.
Several vaccine platforms have been developed to fight pathogenic threats, with Virus-Like Particles (VLPs) representing a very promising alternative to traditional platforms. VLPs trigger strong and lasting humoral and cellular immune responses with fewer safety concerns and higher stability than other platforms. The use of extensively characterized carrier VLPs modified with heterologous antigens was proposed to circumvent the viral complexity of specific viruses that could lead to poor VLP assembly and yields. Although carrier VLPs have been successfully produced in a wide variety of cell-based systems, these are limited by low protein yields and protracted clone selection and optimization workflows that limit VLP screening approaches. In response, we have demonstrated the cell-free protein synthesis (CFPS) of several variants of the hepatitis B core (HBc) carrier VLP using a high-yielding tobacco BY-2 lysate (BYL). High VLP yields in the BYL system allowed in-depth characterization of HBc variants. Insertion of heterologous sequences at the spike region of the HBc monomer proved more structurally demanding than at the N-terminus but removal of the C-terminal domain allowed higher particle flexibility and insert acceptance, albeit at the expense of thermal and chemical stability. We also proved the possibility to scale the CFPS reaction up to 1L in batch mode to produce 0.45 grams of the native HBc VLP within a 48-hour reaction window. A maximum yield of 820 µg/ml of assembled VLP particles was observed at the 100µl scale and most remarkably the CFPS reaction was successfully scaled from 50µl to 1L without any reduction in protein yield across this 20,000-fold difference in reaction volumes. We subsequently proved the immunogenicity of BYL-derived VLPs, as flow cytometry and microscopy clearly showed prompt recognition and endocytosis of fluorescently labelled VLPs by human dendritic cells. Triggering of inflammatory cytokine production in human peripheral blood mononuclear cells was also quantitated using a multiplex assay. This research establishes BYL as a tool for rapid production and microscale screening of VLP variants with subsequent manufacturing possibilities across scales, thus accelerating discovery and implementation of new vaccine candidates using carrier VLPs.
已经开发出几种疫苗平台来对抗致病威胁,其中病毒样颗粒 (VLPs) 是一种非常有前途的替代传统平台的方法。VLPs 引发强烈且持久的体液和细胞免疫反应,比其他平台具有更少的安全问题和更高的稳定性。使用经过广泛表征的载体 VLPs 进行修饰,使其带有异源抗原,被提议用于规避特定病毒的病毒复杂性,这可能导致 VLPs 组装和产量不佳。尽管载体 VLPs 已经在多种基于细胞的系统中成功生产,但这些系统受到低蛋白产量和延长的克隆选择和优化工作流程的限制,这些限制了 VLPs 的筛选方法。作为回应,我们使用高效的烟草 BY-2 裂解物 (BYL) 展示了乙型肝炎核心 (HBc) 载体 VLP 的几种变体的无细胞蛋白质合成 (CFPS)。在 BYL 系统中,VLPs 的高产量允许对 HBc 变体进行深入表征。在 HBc 单体的刺突区域插入异源序列比在 N 末端更具结构挑战性,但去除 C 末端结构域允许更高的颗粒灵活性和插入接受度,尽管以热和化学稳定性为代价。我们还证明了在批处理模式下将 CFPS 反应扩大到 1L 的可能性,以便在 48 小时的反应窗口内生产 0.45 克天然 HBc VLP。在 100µl 规模下观察到组装的 VLP 颗粒的最大产量为 820µg/ml,最显著的是,CFPS 反应成功地从 50µl 扩大到 1L,而在反应体积相差 20000 倍的情况下,蛋白质产量没有任何降低。随后,我们证明了 BYL 衍生的 VLPs 的免疫原性,因为流式细胞术和显微镜清楚地显示了荧光标记的 VLPs 被人树突状细胞快速识别和内吞。使用多重分析也定量了人外周血单核细胞中炎症细胞因子产生的触发。这项研究确立了 BYL 作为一种快速生产和微尺度筛选 VLP 变体的工具,随后在各个规模上进行制造,从而加速了使用载体 VLPs 发现和实施新疫苗候选物的进程。
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