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从鲨鱼合成文库中快速分离IgNAR可变单域抗体片段。

Rapid isolation of IgNAR variable single-domain antibody fragments from a shark synthetic library.

作者信息

Shao Cui-Ying, Secombes Chris J, Porter Andrew J

机构信息

Department of Molecular and Cell Biology, Foresterhill, School of Medical Sciences, University of Aberdeen, Aberdeen AB25 2ZD, UK.

出版信息

Mol Immunol. 2007 Jan;44(4):656-65. doi: 10.1016/j.molimm.2006.01.010. Epub 2006 Feb 24.

Abstract

The immunoglobulin isotype IgNAR (Novel Antigen Receptor) was discovered in the serum of the nurse shark (Ginglymostoma cirratum) and wobbegong shark (Orectolobus maculates) as a homodimer of two protein chains, each composed of a single variable domain (V) domain and five constant domains. The IgNAR variable domain contains an intact antigen-binding site and functions as an independent domain able to react to antigen with both high specificity and affinity. Here we describe the successful construction of a synthetic phage-displayed library based upon a single anti-lysozyme clone HEL-5A7 scaffold, which was previously selected from an immune IgNAR variable domain library. The complementarity-determining region 3 (CDR3) loop of this clone was varied in both length and composition and the derived library was used to pan against two model proteins, lysozyme and leptin. A single anti-lysozyme clone (Ly-X20) and anti-leptin clone (Lep-12E1) were selected for further study. Both clones were shown to be functionally expressed in Escherichia coli, extremely thermostable and bind to corresponding antigens specifically. The results here demonstrate that a synthetic IgNAR variable domain library based on a single framework scaffold can be used as a route to generate antigen binders quickly, easily and without the need of immunization.

摘要

免疫球蛋白同种型IgNAR(新型抗原受体)在护士鲨(长吻锯鲨)和斑纹须鲨的血清中被发现,它是由两条蛋白质链组成的同二聚体,每条链由一个可变结构域(V)和五个恒定结构域组成。IgNAR可变结构域包含一个完整的抗原结合位点,作为一个独立结构域发挥作用,能够以高特异性和亲和力对抗原作出反应。在此,我们描述了基于单个抗溶菌酶克隆HEL-5A7支架成功构建合成噬菌体展示文库的过程,该克隆先前是从免疫IgNAR可变结构域文库中筛选出来的。该克隆的互补决定区3(CDR3)环在长度和组成上均有所变化,所得文库用于筛选两种模型蛋白,即溶菌酶和瘦素。筛选出了一个抗溶菌酶克隆(Ly-X20)和一个抗瘦素克隆(Lep-12E1)用于进一步研究。结果表明,这两个克隆均能在大肠杆菌中功能性表达,具有极高的热稳定性且能特异性结合相应抗原。此处结果表明,基于单个骨架支架的合成IgNAR可变结构域文库可作为一种无需免疫就能快速、轻松地生成抗原结合物的途径。

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