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用于生物物理和生物学研究的噬菌体展示筛选Fab片段的克隆、表达及纯化

Cloning, Expression, and Purification of Phage Display-Selected Fab for Biophysical and Biological Studies.

作者信息

Cyr Matthew G, Peng Haiyong, Rader Christoph

机构信息

Department of Immunology and Microbiology, The Herbert Wertheim UF Scripps Institute for Biomedical Innovation & Technology, University of Florida, Jupiter, Florida 33458, USA.

Department of Immunology and Microbiology, The Herbert Wertheim UF Scripps Institute for Biomedical Innovation & Technology, University of Florida, Jupiter, Florida 33458, USA

出版信息

Cold Spring Harb Protoc. 2024 Oct 15. doi: 10.1101/pdb.prot108604.

Abstract

The antigen-binding fragment (Fab) is the ∼50-kDa monovalent arm of an antibody molecule. In the laboratory, the Fab can be produced via either enzymatic digestion or recombinant expression, and its use facilitates the accurate assessment of affinity and specificity of monoclonal antibodies. The high melting temperature of the Fab, together with its low tendency to aggregate and ready conversion to natural and nonnatural immunoglobulin (Ig) formats (without affecting antigen binding properties), have made it a preferred format for phage display, as well as a tool for accurate assessment of affinity, specificity, and developability of monoclonal antibodies. Here, we outline a strategy to clone, express, and purify human or chimeric nonhuman/human Fabs that have previously been selected by phage display. Fabs purified using this approach, which results in milligram amounts, enable a variety of downstream biophysical and biological assays that ultimately inform the success of phage display library generation and selection.

摘要

抗原结合片段(Fab)是抗体分子约50 kDa的单价臂。在实验室中,Fab可通过酶切或重组表达产生,其应用有助于准确评估单克隆抗体的亲和力和特异性。Fab的高熔点,加上其低聚集倾向以及易于转化为天然和非天然免疫球蛋白(Ig)形式(不影响抗原结合特性),使其成为噬菌体展示的首选形式,也是准确评估单克隆抗体亲和力、特异性和可开发性的工具。在此,我们概述了一种克隆、表达和纯化先前通过噬菌体展示筛选出的人源或嵌合非人/人源Fab的策略。使用这种方法纯化得到的Fab产量可达毫克级,可用于多种下游生物物理和生物学检测,最终为噬菌体展示文库的构建和筛选成功提供依据。

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