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An improved helper phage system for efficient isolation of specific antibody molecules in phage display

机译:一种改进的辅助噬菌体系统,可有效分离噬菌体展示中的特定抗体分子

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摘要

Phage display technology has been applied in many fields of biological and medical sciences to study molecular interactions and especially in the generation of monoclonal antibodies of human origin. However, extremely low display level of antibody molecules on the surface of phage is an intrinsic problem of a phagemid-based display system resulting in low success rate of isolating specific binding molecules. We show here that display of single-chain antibody fragment (scFv) generated with pIGT3 phagemid can be increased dramatically by using a genetically modified Ex-phage. Ex-phage has a mutant pIII gene that produces a functional wild-type pIII in suppressing Escherichia coli strains but does not make any pIII in non-suppressing E.coli strains. Packaging phagemids encoding antibody-pIII fusion in F+ non-suppressing E.coli strains with Ex-phage enhanced the display level of antibody fragments on the surfaces of recombinant phage particles resulting in an increase of antigen-binding reactivity >100-fold compared to packaging with M13KO7 helper phage. Thus, the Ex-phage and pIGT3 phagemid vector provides a system for the efficient enrichment of specific binding antibodies from a phage display library and, thereby, increases the chance of obtaining more diverse antibodies specific for target antigens.
机译:噬菌体展示技术已被应用于生物学和医学的许多领域,以研究分子相互作用,尤其是在人类来源的单克隆抗体的产生中。然而,噬菌体表面上抗体分子的极低展示水平是基于噬菌粒的展示系统的固有问题,导致分离特异性结合分子的成功率低。我们在这里显示通过使用基因修饰的Ex-噬菌体可以显着增加用pIGT3噬菌粒产生的单链抗体片段(scFv)的展示。前噬菌体具有一个突变的pIII基因,该基因在抑制大肠杆菌菌株中产生功能性野生型pIII,但在非抑制性大肠杆菌菌株中不产生任何pIII。在包装有F +非抑制性大肠杆菌的Ex-噬菌体中包装编码抗体-pIII融合的噬菌粒可增强重组噬菌体颗粒表面抗体片段的展示水平,与包装相比,抗原结合反应性增加> 100倍与M13KO7辅助噬菌体。因此,Ex-噬菌体和pIGT3噬菌体载体提供了从噬菌体展示文库有效富集特异性结合抗体的系统,从而增加了获得更多特异性针对靶抗原的抗体的机会。

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