Kimura Taiji, Nishida Ai, Ohara Nobutoshi, Yamagishi Daisuke, Horibe Tomohisa, Kikuchi Masakazu
Department of Bioscience and Technology, Faculty of Science and Engineering, Ritsumeikan University, 1-1-1 Noji-higashi, Kusatsu, Shiga 525-8577, Japan.
Biochem J. 2004 Aug 15;382(Pt 1):169-76. doi: 10.1042/BJ20040116.
Polyclonal antibodies that had been raised against particular PDI (protein disulphide-isomerase) family proteins did not cross-react with other PDI family proteins. To evade immune tolerance to the important self-motif Cys-Xaa-Xaa-Cys, which is present in PDI family proteins, we used the phage display library [established by Griffiths, Williams, Hartley, Tomlinson, Waterhouse, Crosby, Kontermann, Jones, Low, Allison et al. (1994) EMBO J. 13, 3245-3260] to isolate successfully the phage antibodies that can cross-react with human and bovine PDIs, human P5, human PDI-related protein and yeast PDI. By measuring the binding of scFv (single-chain antibody fragment of variable region) to synthetic peptides and to mutants of PDI family proteins in a surface plasmon resonance apparatus, we identified clones that recognized sequences containing the CGHC motif or the CGHCK sequence. By using the isolated phage antibodies, we demonstrated for the first time that a lysine residue following the CXXC motif significantly increases the isomerase activities of PDI family proteins. Moreover, we demonstrated that the affinity of isolated scFvs for mutant PDI family proteins is proportional to the isomerase activities of their active sites.
针对特定蛋白质二硫键异构酶(PDI)家族蛋白产生的多克隆抗体不会与其他PDI家族蛋白发生交叉反应。为了规避对存在于PDI家族蛋白中的重要自身基序半胱氨酸-氨基酸-氨基酸-半胱氨酸的免疫耐受,我们使用了[由格里菲思、威廉姆斯、哈特利、汤姆林森、沃特豪斯、克罗斯比、孔特曼、琼斯、洛、艾利森等人(1994年)建立的噬菌体展示文库,《欧洲分子生物学组织杂志》13卷,3245 - 3260页]成功分离出了能与人及牛的PDI、人P5、人PDI相关蛋白和酵母PDI发生交叉反应的噬菌体抗体。通过在表面等离子体共振仪中测量单链抗体片段(scFv)与合成肽以及PDI家族蛋白突变体的结合,我们鉴定出了识别包含CGHC基序或CGHCK序列的克隆。通过使用分离出的噬菌体抗体,我们首次证明CXXC基序后的赖氨酸残基显著提高了PDI家族蛋白的异构酶活性。此外,我们证明了分离出的scFv对突变型PDI家族蛋白的亲和力与其活性位点的异构酶活性成正比。