Lima G C, Chura-Chambi R M, Morganti L, Silva V J, Cabral-Piccin M P, Rocha V, Medina T S, Ramos R N, Luz D
Laboratory of Bacteriology, Butantan Institute, São Paulo, Brazil.
Biotechnology Center, Institute of Energy and Nuclear Research-CNEN/SP, São Paulo, Brazil.
Front Bioeng Biotechnol. 2023 Jul 31;11:1227212. doi: 10.3389/fbioe.2023.1227212. eCollection 2023.
Microbial systems, such as , as host recombinant expression is the most versatile and the cheapest system for protein production, however, several obstacles still remain, such as recovery of soluble and functional proteins from inclusion bodies, elimination of lipopolysaccharides (LPS) contamination, incomplete synthesis, degradation by proteases, and the lack of post-translational modifications, which becomes even more complex when comes to membrane proteins, because they are difficult not only to produce but also to keep in solution in its active state. T-cell Immunoglobulin and Mucin domain 3 (TIM-3) is a type I transmembrane protein that is predominantly expressed on the surface of T lymphocytes, natural killer (NK) cells, dendritic cells, and macrophages, playing a role as a negative immune checkpoint receptor. TIM-3 comprises a single ectodomain for interaction with immune system soluble and cellular components, a transmembrane domain, and a cytoplasmic tail, responsible for the binding of signaling and scaffolding molecules. TIM-3 pathway holds potential as a therapeutic target for immunotherapy against tumors, autoimmunity, chronic virus infections, and various malignancies, however, many aspects of the biology of this receptor are still incompletely understood, especially regarding its ligands. Here we overcome, for the first time, the challenge of the production of active immune checkpoint protein recovered from bacterial cytoplasmic inclusion bodies, being able to obtain an active, and non-glycosylated TIM-3 ectodomain (TIM-3-ECD), which can be used as a tool to better understand the interactions and roles of this immune checkpoint. The TIM-3 refolding was obtained by the association of high pressure and alkaline pH. The purified TIM-3-ECD showed the correct secondary structure and was recognized from anti-TIM-3 structural-dependent antibodies likewise commercial TIM-3-ECD was produced by a mammal cells system. Furthermore, immunofluorescence showed the ability of TIM-3-ECD to bind to the surface of lung cancer A549 cells and to provide an additional boost for the expression of the lymphocyte activation marker CD69 in anti-CD3/CD28 activated human PBMC. Taken together these results validated a methodology able to obtain active checkpoint proteins from bacterial inclusion bodies, which will be helpful to further investigate the interactions of this and others not yet explored immune checkpoints.
微生物系统,例如,作为宿主的重组表达是最通用且最便宜的蛋白质生产系统,然而,仍然存在一些障碍,例如从包涵体中回收可溶性和功能性蛋白质、消除脂多糖(LPS)污染、合成不完全、被蛋白酶降解以及缺乏翻译后修饰,而对于膜蛋白来说这变得更加复杂,因为它们不仅难以生产,而且难以保持在溶液中的活性状态。T细胞免疫球蛋白和粘蛋白结构域3(TIM-3)是一种I型跨膜蛋白,主要表达于T淋巴细胞、自然杀伤(NK)细胞、树突状细胞和巨噬细胞表面,作为负性免疫检查点受体发挥作用。TIM-3包含一个单一的胞外结构域,用于与免疫系统的可溶性和细胞成分相互作用,一个跨膜结构域和一个胞质尾,负责信号和支架分子的结合。TIM-3通路作为针对肿瘤、自身免疫、慢性病毒感染和各种恶性肿瘤的免疫治疗的潜在治疗靶点,然而,该受体生物学的许多方面仍未完全了解,尤其是关于其配体。在这里,我们首次克服了从细菌细胞质包涵体中生产活性免疫检查点蛋白的挑战,能够获得一种活性且非糖基化的TIM-3胞外结构域(TIM-3-ECD),它可以用作更好地理解这个免疫检查点的相互作用和作用的工具。通过高压和碱性pH的联合作用实现了TIM-3的重折叠。纯化的TIM-3-ECD显示出正确的二级结构,并且与抗TIM-3结构依赖性抗体的识别情况与哺乳动物细胞系统生产的商业TIM-3-ECD相同。此外,免疫荧光显示TIM-3-ECD能够结合肺癌A549细胞表面,并为抗CD3/CD28激活的人外周血单个核细胞中淋巴细胞激活标志物CD69的表达提供额外的促进作用。综上所述,这些结果验证了一种能够从细菌包涵体中获得活性检查点蛋白的方法,这将有助于进一步研究这个以及其他尚未探索的免疫检查点的相互作用。
