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合成噬菌体展示Fab文库的设计与构建。

Design and construction of synthetic phage-displayed Fab libraries.

作者信息

Bostrom Jenny, Fuh Germaine

机构信息

Department of Antibody Engineering, Genentech Inc., South San Francisco, CA 94080, USA.

出版信息

Methods Mol Biol. 2009;562:17-35. doi: 10.1007/978-1-60327-302-2_2.

Abstract

Diversity-the variability carried by the amino acid sequences of a synthetic antibody library-can be generated by synthetic degenerate oligonucleotides. One can experiment with different diversity designs in the variable domains of light and heavy chains (V(H) and V(L)) to generate antibody libraries with different properties. The ability to precisely define the final diversity of a library facilitates the process of isolating, characterizing, and optimizing an antibody lead. Here we describe detailed protocols for the design and construction of phage-displayed synthetic antibody libraries in which diversity is generated in the complementarity determining regions (CDRs) of the V(H) of a single humanized bivalent Fab scaffold. The example used in the protocol provides a general methodology for generation of libraries with engineered CDR diversity that can be applied to a template antibody sequence of choice.

摘要

多样性——由合成抗体文库的氨基酸序列携带的变异性——可通过合成简并寡核苷酸产生。人们可以在轻链和重链的可变结构域(V(H)和V(L))中试验不同的多样性设计,以产生具有不同特性的抗体文库。精确界定文库最终多样性的能力有助于分离、表征和优化抗体先导物的过程。在此,我们描述了噬菌体展示合成抗体文库设计和构建的详细方案,其中多样性在单一人源化二价Fab支架的V(H)互补决定区(CDR)中产生。方案中使用的示例提供了一种用于产生具有工程化CDR多样性文库的通用方法,该方法可应用于所选的模板抗体序列。

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