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一种新型的合成原始人抗体文库可用于分离针对癌胚型纤维连接蛋白新表位的抗体。

A novel synthetic naïve human antibody library allows the isolation of antibodies against a new epitope of oncofetal fibronectin.

机构信息

Philochem AG, c/o ETH Zürich, Zurich, Switzerland.

出版信息

MAbs. 2011 May-Jun;3(3):264-72. doi: 10.4161/mabs.3.3.15616. Epub 2011 May 1.

Abstract

Human monoclonal antibodies (mAbs) can routinely be isolated from phage display libraries against virtually any protein available in sufficient purity and quantity, but library design can influence epitope coverage on the target antigen. Here we describe the construction of a novel synthetic human antibody phage display library that incorporates hydrophilic or charged residues at position 52 of the CDR2 loop of the variable heavy chain domain, instead of the serine residue found in the corresponding germline gene. The novel library was used to isolate human mAbs to various antigens, including the alternatively-spliced EDA domain of fibronectin, a marker of tumor angiogenesis. In particular, the mAb 2H7 was proven to bind to a novel epitope on EDA, which does not overlap with the one recognized by the clinical-stage F8 antibody. F8 and 2H7 were used for the construction of chelating recombinant antibodies (CRAbs), whose tumor-targeting properties were assessed in vivo in biodistribution studies in mice bearing F9 teratocarcinoma, revealing a preferential accumulation at the tumor site.

摘要

人源单克隆抗体(mAbs)可常规从噬菌体展示文库中分离得到,针对的是几乎任何具有足够纯度和数量的蛋白质,但文库设计会影响针对目标抗原的表位覆盖。在这里,我们描述了一种新型合成人抗体噬菌体展示文库的构建,该文库在可变重链结构域的 CDR2 环的位置 52 处引入了亲水或带电残基,而不是在相应的胚系基因中发现的丝氨酸残基。该新型文库用于分离针对各种抗原的人源 mAbs,包括纤维连接蛋白的交替剪接 EDA 结构域,该结构域是肿瘤血管生成的标志物。特别是,mAb 2H7 被证明与 EDA 上的一个新表位结合,该表位与临床阶段 F8 抗体识别的表位不重叠。F8 和 2H7 被用于构建螯合重组抗体(CRAbs),并在携带 F9 畸胎瘤的小鼠体内进行了体内分布研究,评估其在肿瘤部位的靶向特性,结果显示在肿瘤部位有优先聚集。

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