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Selection of recombinant anti-SH3 domain antibodies by high-throughput phage display

机译:高通量噬菌体展示技术筛选重组抗SH3结构域抗体

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摘要

Antibodies are indispensable tools in biochemical research and play an expanding role as therapeutics. While hybridoma technology is the dominant method for antibody production, phage display is an emerging technology. Here, we developed and employed a high-throughput pipeline that enables selection of antibodies against hundreds of antigens in parallel. Binding selections using a phage-displayed synthetic antigen-binding fragment (Fab) library against 110 human SH3 domains yielded hundreds of Fabs targeting 58 antigens. Affinity assays demonstrated that representative Fabs bind tightly and specifically to their targets. Furthermore, we developed an efficient affinity maturation strategy adaptable to high-throughput, which increased affinity dramatically but did not compromise specificity. Finally, we tested Fabs in common cell biology applications and confirmed recognition of the full-length antigen in immunoprecipitation, immunoblotting and immunofluorescence assays. In summary, we have established a rapid and robust high-throughput methodology that can be applied to generate highly functional and renewable antibodies targeting protein domains on a proteome-wide scale.
机译:抗体是生化研究中必不可少的工具,并且在治疗中起着越来越重要的作用。尽管杂交瘤技术是抗体生产的主要方法,但噬菌体展示是一种新兴技术。在这里,我们开发并采用了高通量管线,可以并行选择针对数百种抗原的抗体。使用针对110个人类SH3结构域的噬菌体展示的合成抗原结合片段(Fab)文库进行结合选择,产生了靶向58种抗原的数百种Fab。亲和力测定表明代表性Fab与它们的靶标紧密结合且特异性结合。此外,我们开发了一种适用于高通量的有效亲和力成熟策略,该策略可以显着提高亲和力,但不会影响特异性。最后,我们在常见的细胞生物学应用中测试了Fab,并在免疫沉淀,免疫印迹和免疫荧光测定中确认了对全长抗原的识别。总而言之,我们已经建立了一种快速而强大的高通量方法,该方法可用于在蛋白质组范围内产生针对蛋白质结构域的功能强大且可再生的抗体。

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