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A Cassette Vector System for the Rapid Cloning and Production of Bispecific Tetravalent Antibodies

机译:快速克隆和生产双特异性四价抗体的盒式载体系统

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Bivalent single chain (sc)Fv-Fc antibodies have been used for years as recombinant alternatives of natural immunoglobulins. We have extended this approach to the scFv-Fc-scFv antibody format to obtain tetravalent antigen binding and the possibility to generate bispecific antibodies. We developed a mammalian expression vector system to construct tetravalent scFv-Fc-scFv antibodies with two NcoI+NotI compatible cloning sites flanking the Fc gene fragment. We demonstrated direct cloning from single chain antibody gene libraries and tested various scFv combinations. Transient production of scFv-Fc-scFv antibodies in human embryonic kidney (HEK) 293T cells achieved volumetric yields of up to 10 mg/L. However, expression levels were strongly dependent on the carboxyterminal scFv and the scFv combination. All scFv-Fc-scFv antibodies exclusively formed disulfide-linked homodimers. Antigen binding studies revealed dual specificity for all scFv-Fc-scFv employing different scFv fragments. Comparison of C-reactive protein (CRP) specific monovalent scFv LA13-IIE3, bivalent scFv-Fc and Fc-scFv LA13-IIE3, and tetravalent scFv-Fc-scFv (scFv LA13-IIE3 in combination with scFvs LA13-IIE3, TOB4-B11, or TOB5-D4) revealed an up to 500-fold increased antigen binding. This novel scFv-Fc-scFv antibody expression system allows simple and fast testing of various scFv combinations.
机译:二价单链(sc)Fv-Fc抗体已被用作天然免疫球蛋白的重组替代品多年。我们已经将此方法扩展到scFv-Fc-scFv抗体形式,以获得四价抗原结合和生成双特异性抗体的可能性。我们开发了哺乳动物表达载体系统,以构建具有两个位于Fc基因片段​​两侧的NcoI + NotI兼容克隆位点的四价scFv-Fc-scFv抗体。我们展示了从单链抗体基因库直接克隆并测试了各种scFv组合。在人胚胎肾(HEK)293T细胞中短暂生产scFv-Fc-scFv抗体可实现高达10 mg / L的体积产率。然而,表达水平强烈依赖于羧基末端scFv和scFv组合。所有scFv-Fc-scFv抗体都仅形成二硫键连接的同型二聚体。抗原结合研究揭示了对采用不同scFv片段的所有scFv-Fc-scFv的双重特异性。 C反应蛋白(CRP)特异性单价scFv LA13-IIE3,二价scFv-Fc和Fc-scFv LA13-IIE3和四价scFv-Fc-scFv(scFv LA13-IIE3与scFvs LA13-IIE3,TOB4-的比较) B11或TOB5-D4)显示最多增加500倍的抗原结合。这种新颖的scFv-Fc-scFv抗体表达系统可以轻松快速地测试各种scFv组合。

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