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首页> 外文期刊>Tissue antigens. >The isolation and characterisation of human monoclonal HLA-A2 antibodies from an immune V gene phage display library.
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The isolation and characterisation of human monoclonal HLA-A2 antibodies from an immune V gene phage display library.

机译:从免疫V基因噬菌体展示文库中分离和鉴定人单克隆HLA-A2抗体。

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摘要

Molecular cloning techniques and V gene phage display have revolutionised the production of human monoclonal antibodies. Antibodies of a defined specificity can be obtained by selecting phage display libraries on antigen in a process known as panning. We have applied these techniques to the isolation of three HLA-A2-specific single chain variable domain fragments (scFv) from a patient alloimmunised by blood transfusion. Analysis of specificity with cells of HLA genotyped donors revealed the following: i) in addition to the major reactivity with HLA-A2, cross-reactivity with the HLA-A28 epitope; and ii) inhibition of scFv binding to the antigen by the patients' antibodies. The heavy chain variable genes of all three were derived from the germline gene Cos-3, carry the hallmarks of somatic hypermutation, and are most likely derived from clonally related B cells. The light chain variable domains were encoded by DPK1 and DPK8 from the VkappaI family. These data show that phage display can be used to clone HLA-specific alloantibodies that recognise the native antigen from alloimmunised patients.
机译:分子克隆技术和V基因噬菌体展示彻底改变了人类单克隆抗体的生产。可以通过在淘选过程中选择抗原上的噬菌体展示文库来获得具有特定特异性的抗体。我们已将这些技术应用于从通过输血同种免疫的患者中分离出三个HLA-A2特异性单链可变域片段(scFv)。对HLA基因型供体细胞的特异性分析显示:i)除了与HLA-A2的主要反应性之外,还与HLA-A28表位具有交叉反应性; ii)通过患者的抗体抑制scFv与抗原的结合。这三个基因的重链可变基因均来自种系基因Cos-3,带有体细胞超突变的特征,最有可能源自克隆相关的B细胞。轻链可变域由来自VkappaI家族的DPK1和DPK8编码。这些数据表明噬菌体展示可用于克隆识别来自同种免疫患者的天然抗原的HLA特异性同种抗体。

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