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利用可移除的SpyCatcher/SnoopCatcher单元通过重链和轻链之间的特异性配对构建双特异性抗体。

Construction of bispecific antibodies by specific pairing between the heavy chain and the light chain using removable SpyCatcher/SnoopCatcher units.

作者信息

Yoshida Jyunna, Kato Yuki, Isogawa Ai, Tanaka Yoshikazu, Kumagai Izumi, Asano Ryutaro, Nakanishi Takeshi, Makabe Koki

机构信息

Graduate School of Science and Engineering, Yamagata University, 4-3-16 Jyonan, Yonezawa, Yamagata, 992-8510, Japan.

Department of Biotechnology and Life Science, Graduate School of Engineering, Tokyo University of Agriculture and Technology, 2-24-16 Naka-cho, Koganei, Tokyo, 184-8588, Japan.

出版信息

J Biol Eng. 2024 Oct 14;18(1):57. doi: 10.1186/s13036-024-00454-z.

Abstract

During the production of bispecific antibodies (bsAbs), nonspecific pairing results in low yields of target bsAb molecules, an issue known as the "mispairing problem." Several antibody engineering techniques have been developed to overcome mispairing issues. Here, we introduce "bsAb by external pairing and excision" (BAPE), a novel chain pairing method that induces specific chain pairing by fusing external SpyCatcher/Tag and SnoopCatcher/Tag units. These tags are then removed via protease cleavage. In this study, we applied this method to force the correct pairings of heavy and light chains while the heavy-chain pairing was achieved by the Knobs-into-Holes mutation. We then confirmed the formation of interchain bridges with covalent isopeptide bonds. Both anti-CD3/anti-Her2 and anti-CD3/anti-EGFR bsAbs displayed satisfactory target binding activities and in vitro cell-killing activity with activated T-cells.

摘要

在双特异性抗体(bsAb)的生产过程中,非特异性配对会导致目标bsAb分子产量低下,这一问题被称为“错配问题”。已经开发了几种抗体工程技术来克服错配问题。在此,我们介绍“通过外部配对和切除产生bsAb”(BAPE),这是一种新型的链配对方法,通过融合外部的SpyCatcher/Tag和SnoopCatcher/Tag单元诱导特异性链配对。然后通过蛋白酶切割去除这些标签。在本研究中,我们应用该方法强制重链和轻链正确配对,同时通过Knobs-into-Holes突变实现重链配对。然后我们证实了共价异肽键的链间桥的形成。抗CD3/抗Her2和抗CD3/抗EGFR双特异性抗体均表现出令人满意的靶向结合活性以及与活化T细胞的体外细胞杀伤活性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/08e2/11476941/16d97af87eba/13036_2024_454_Fig1_HTML.jpg

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