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一种生产IgG样双特异性抗体的有效途径。

An efficient route to the production of an IgG-like bispecific antibody.

作者信息

Zuo Z, Jimenez X, Witte L, Zhu Z

机构信息

Department of Molecular and Cell Biology, ImClone Systems Incorporated, 180 Varick Street, New York, NY 10014, USA.

出版信息

Protein Eng. 2000 May;13(5):361-7. doi: 10.1093/protein/13.5.361.

DOI:10.1093/protein/13.5.361
PMID:10835110
Abstract

Production of IgG-form bispecific antibody (BsAb-IgG) by co-expressing two antibodies in transfected cells is often inefficient owing to the unwanted pairing between the component heavy and light chains. We have developed an efficient method for the production of a novel IgG-like BsAb by using the natural dimerization mechanism between IgG heavy and light chains. Two single-chain Fv (scFv) of different specificity are fused to the constant domain of human kappa chain (C(L)) and the first constant domain of human heavy chain (C(H1)), to form two polypeptides, (scFv)(1)-C(L) and (scFv)(2)-C(H1)-C(H2)-C(H3), respectively. Co-expression of the two polypeptides in mammalian cells results in the formation of a covalently linked IgG-like hetero-tetramer, Bs(scFv)(4)-IgG, with dual specificity. Our approach yields a homogeneous bispecific IgG-like antibody product with each molecule containing four antigen binding sites, two for each of its target antigens. A Bs(scFv)(4)-IgG was prepared using two scFv antibodies each directed against a different epitope of a vascular endothelial growth factor receptor, the kinase insert domain-containing receptor (KDR). The Bs(scFv)(4)-IgG is capable of simultaneously binding to the two epitopes on the receptor. Further, the Bs(scFv)(4)-IgG also retains the antigen-binding efficacy and biological activity of its component antibodies.

摘要

在转染细胞中共表达两种抗体来生产IgG形式的双特异性抗体(BsAb-IgG),由于组成型重链和轻链之间存在不必要的配对,往往效率不高。我们利用IgG重链和轻链之间的天然二聚化机制,开发了一种高效生产新型IgG样双特异性抗体的方法。将两种不同特异性的单链Fv(scFv)分别与人κ链恒定区(C(L))和人重链第一恒定区(C(H1))融合,形成两条多肽,即(scFv)(1)-C(L)和(scFv)(2)-C(H1)-C(H2)-C(H3)。在哺乳动物细胞中共表达这两条多肽,会形成一种共价连接的IgG样异源四聚体Bs(scFv)(4)-IgG,具有双重特异性。我们的方法产生了一种均一的双特异性IgG样抗体产物,每个分子含有四个抗原结合位点,针对其每个靶抗原各有两个。使用两种分别针对血管内皮生长因子受体激酶插入结构域包含受体(KDR)不同表位的scFv抗体,制备了Bs(scFv)(4)-IgG。Bs(scFv)(4)-IgG能够同时结合受体上的两个表位。此外,Bs(scFv)(4)-IgG还保留了其组成抗体的抗原结合效力和生物学活性。

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