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针对绿色荧光蛋白的鲨鱼源单域抗体的筛选、鉴定及晶体结构

Selection, identification and crystal structure of shark-derived single-domain antibodies against a green fluorescent protein.

机构信息

College of Ocean Food and Biological Engineering, Jimei University, Xiamen 361021, China.

Institute of Health and Medicine, Hefei Comprehensive National Science Center, CAS Key Laboratory of Innate Immunity and Chronic Disease, Division of Life Sciences and Medicine, University of Science & Technology of China, Hefei 230007, China.

出版信息

Int J Biol Macromol. 2023 Aug 30;247:125852. doi: 10.1016/j.ijbiomac.2023.125852. Epub 2023 Jul 17.

DOI:10.1016/j.ijbiomac.2023.125852
PMID:37460076
Abstract

Shark variable domain of new antigen receptors (VNARs) are the smallest naturally occurring binding domains with properties of low complexity, small size, cytoplasmic expression, and ease of engineering. Green fluorescent protein (GFP) molecules have been analyzed in conventional microscopy, but their spectral characteristics preclude their use in techniques offering substantially higher resolution. Besides, the GFP molecules can be quenched in acidic environment, which makes it necessary to develop anti-GFP antibody to solve these problems. In view of the diverse applications of GFP and unique physicochemical features of VNAR, the present study aims to generate VNARs against GFP. Here, we identified 36 VNARs targeting eCGP123, an extremely stable GFP, by phage display from three immunized sharks. These VNARs bound to eCGP123 with affinity constant K values ranging from 6.76 to 605 nM. Among them, two lead VNARs named aGFP-14 and aGFP-15 with nanomolar eCGP123-binding affinity were selected for in-depth characterization. aGFP-14 and aGFP-15 recognized similar epitopes on eCGP123. X-ray crystallography studies clarified the mechanism by which aGFP14 interacts with eCGP123. aGFP-14 also showed cross-reaction with EGFP, with K values of 47.2 nM. Finally, immunostaining analyses demonstrated that aGFP-14 was able to bind effectively to the EGFP expressed in both cultured cells and mouse brain tissues, and can be used as a fluorescence amplifier for EGFP. Our research demonstrates a feasible idea for the screening and production of shark-derived VNARs. The two high-affinity VNARs developed in the study contribute to the diversity of GFP sdAbs and may enhance the applications of GFP.

摘要

鲨鱼新型抗原受体(VNAR)的可变域是自然界中最小的天然结合域,具有低复杂度、小尺寸、细胞质表达和易于工程化的特点。绿色荧光蛋白(GFP)分子已在常规显微镜下进行了分析,但由于其光谱特性,限制了其在提供更高分辨率的技术中的应用。此外,GFP 分子在酸性环境中会被猝灭,因此需要开发抗 GFP 抗体来解决这些问题。鉴于 GFP 的广泛应用和 VNAR 独特的物理化学特性,本研究旨在生成针对 GFP 的 VNAR。在这里,我们从三只免疫鲨鱼中通过噬菌体展示技术,鉴定出 36 种针对 eCGP123 的 VNAR,eCGP123 是一种非常稳定的 GFP。这些 VNAR 与 eCGP123 的亲和力常数 K 值范围为 6.76-605 nM。其中,两种具有纳米级 eCGP123 结合亲和力的先导 VNAR,分别命名为 aGFP-14 和 aGFP-15,被选中进行深入表征。aGFP-14 和 aGFP-15 识别 eCGP123 上相似的表位。X 射线晶体学研究阐明了 aGFP14 与 eCGP123 相互作用的机制。aGFP-14 还与 EGFP 发生交叉反应,K 值为 47.2 nM。最后,免疫染色分析表明,aGFP-14 能够有效地与培养细胞和小鼠脑组织中表达的 EGFP 结合,并且可以作为 EGFP 的荧光增强剂。我们的研究为鲨鱼衍生 VNAR 的筛选和生产提供了一个可行的思路。本研究开发的两种高亲和力 VNAR 丰富了 GFP sdAbs 的多样性,可能增强 GFP 的应用。

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