Department of Chemistry, Indiana University, 800 East Kirkwood Avenue, Bloomington, Indiana 47405, United States.
Laboratory of Bacteriology, National Institute of Allergy and Infectious Diseases, 903 South 4th Street, Hamilton, Montana 59840, United States.
ACS Appl Bio Mater. 2021 Dec 20;4(12):8205-8214. doi: 10.1021/acsabm.1c00718. Epub 2021 Nov 10.
Ligands of the tumor necrosis factor superfamily (TNFSF) are appealing targets for immunotherapy research due to their integral involvement in stimulation or restriction of immune responses. TNFSF-targeted therapies are currently being developed to combat immunologically based diseases and cancer. A crucial determinant of effective TNFSF receptor binding and signaling is the trimeric quaternary structure of the ligand. Additionally, ligand multivalency is essential to propagate strong signaling in effector cells. Thus, designing a synthetic platform to display trimeric TNFSF ligands in a multivalent manner is necessary to further the understanding of ligand-receptor interactions. Viral nanocages have architectures that are amenable to genetic and chemical modifications of both their interior and exterior surfaces. Notably, the exterior surface of virus-like particles can be utilized as a platform for the modular multivalent presentation of target proteins. In this study, we build on previous efforts exploring the bacteriophage P22 virus-like particle for the exterior multivalent modular display of a potent immune-stimulating TNFSF protein, CD40 ligand (CD40L). Using a cell-based reporter system, we quantify the effects of tunable avidity on CD40 signaling by CD40L displayed on the surface of P22 nanocages. Multivalent presentation of CD40L resulted in a 53.6-fold decrease of the half maximal effective concentration (EC) compared to free CD40L, indicating higher potency. Our results emphasize the power of using P22-based biomimetics to study ligand-receptor interactions within their proper structural context, which may contribute to the development of effective immune modulators.
肿瘤坏死因子超家族(TNFSF)的配体由于它们在刺激或限制免疫反应中的整体参与,是免疫治疗研究的有吸引力的靶标。目前正在开发 TNFSF 靶向疗法来治疗免疫相关疾病和癌症。有效 TNFSF 受体结合和信号传导的关键决定因素是配体的三聚体四级结构。此外,配体的多价性对于在效应细胞中传播强信号是必不可少的。因此,设计一个能够以多价方式展示三聚体 TNFSF 配体的合成平台对于进一步了解配体-受体相互作用是必要的。病毒纳米笼具有结构,适合对其内部和外部表面进行遗传和化学修饰。值得注意的是,病毒样颗粒的外表面可被用作模块化多价呈现靶蛋白的平台。在这项研究中,我们基于以前的研究,探索了噬菌体 P22 病毒样颗粒,用于在 P22 纳米笼表面外部分子模块多价展示有效的免疫刺激 TNFSF 蛋白,CD40 配体(CD40L)。使用基于细胞的报告系统,我们通过 CD40L 在 P22 纳米笼表面上的展示来量化可调节亲和力对 CD40 信号的影响。与游离的 CD40L 相比,CD40L 的多价展示导致半最大有效浓度(EC)降低了 53.6 倍,表明其效力更高。我们的结果强调了使用基于 P22 的仿生学来研究配体-受体相互作用在其适当的结构背景下的力量,这可能有助于开发有效的免疫调节剂。