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利用半合成噬菌体抗体文库克隆抗角蛋白人源抗体并进行特性分析。

Cloning and characterization of antikeratin human antibodies using a semisynthetic phage antibody library.

作者信息

Wang Gang, Liu Yu-Feng, Li Chun-Ying, Lu Ning, Gao Tian-Wen, Hua Bing, Wang Yan

机构信息

Department of Dermatology, Xijing Hospital, Fourth Military Medical University, 710032 Xi'an, China.

出版信息

Arch Dermatol Res. 2004 Nov;296(6):270-7. doi: 10.1007/s00403-004-0504-1.

DOI:10.1007/s00403-004-0504-1
PMID:15340746
Abstract

Antikeratin autoantibodies (AK auto Abs) are very important elements of the human immune system. To improve the outcome of studies on AK auto Abs, it is necessary to generate antikeratin human monoclonal antibodies. The purpose of present study was to isolate antikeratin human monoclonal antibodies by panning a phage antibody library. A semisynthetic phage antibody library with capacity of 4.0x10(8) members was previously constructed. Panning of the library was performed against human epidermal keratin extracted from psoriatic scales. At the last round of the panning, individual colonies were grown in culture for expression of phage antibodies. Their binding activities and specificities to keratin were determined by ELISA, and positive clones were analyzed by DNA fingerprinting. The selected clones were induced with IPTG to express soluble Fab fragments, which were further characterized by ELISA, immunohistochemistry and Western blotting. Finally, DNA sequencing of the variable regions was performed. A human antibody clone which was able to express soluble Fab fragments and recognize Mr 46,000 keratin (K17) was isolated. DNA sequencing demonstrated that the VH and VL of the antibody came from the human VH1 and Vkappa2 families, respectively. We conclude that phage antibody library technology is a powerful way to generate human monoclonal antibodies. The antikeratin antibody we isolated in the present study would be useful in the research on AK auto Abs.

摘要

抗角蛋白自身抗体(AK自身抗体)是人类免疫系统的重要组成部分。为了改善关于AK自身抗体的研究结果,有必要制备抗角蛋白人单克隆抗体。本研究的目的是通过淘选噬菌体抗体库来分离抗角蛋白人单克隆抗体。先前构建了一个容量为4.0×10⁸个成员的半合成噬菌体抗体库。利用从银屑病鳞屑中提取的人表皮角蛋白对该文库进行淘选。在淘选的最后一轮,单个菌落进行培养以表达噬菌体抗体。通过ELISA测定它们对角蛋白的结合活性和特异性,并用DNA指纹图谱分析阳性克隆。用IPTG诱导所选克隆表达可溶性Fab片段,再通过ELISA、免疫组织化学和Western印迹进一步鉴定。最后,对可变区进行DNA测序。分离出一个能够表达可溶性Fab片段并识别46000 Mr角蛋白(K17)的人抗体克隆。DNA测序表明该抗体的VH和VL分别来自人VH1和Vκ2家族。我们得出结论,噬菌体抗体库技术是产生人单克隆抗体的一种有效方法。我们在本研究中分离出的抗角蛋白抗体将有助于AK自身抗体的研究。

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