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通过链改组工程 Fab 对 SDM 抗原的性别特异性。

Engineering the male-specificity of Fab against SDM antigen by chain shuffling.

机构信息

College of Veterinary Medicine, Hunan Agricultural University, Changsha, Hunan Province, PR China.

出版信息

Theriogenology. 2013 May;79(8):1162-70. doi: 10.1016/j.theriogenology.2013.02.012. Epub 2013 Apr 3.

Abstract

High-titer serologically detected male (SDM) antibody fragments are essential for specific binding to the SDM antigen and promoting its application. The A8 clone previously obtained from an original phage antibody library was further affinity-matured by light- and high-chain shuffling respectively, to generate the end product B9 clone. The binding capacity of B9 phage Fabs to male splenocytes doubled the value of its parental A8 clone (determined using ELISA). Based on immunofluorescent staining, B9-Fabs mainly bound to the surface antigen of male splenocytes and recognized testicular cells. The resulting B9-Fabs detected a single protein (approximately 40 kDa determined using Western blot analysis of male splenocytes and testis); its high SDM antigen binding ability might have been because of mutation sites and varied lengths of the amino acid sequences in the complementarity determining regions-3 of the κ and Fd chains. The new recombinant clones of Fab that were phage-enhanced using chain shuffling were candidate molecules for investigating molecular mechanisms of SDM antigens specific binding and applications.

摘要

高滴度血清学检测的雄性(SDM)抗体片段对于与 SDM 抗原的特异性结合和促进其应用至关重要。先前从原始噬菌体抗体文库中获得的 A8 克隆通过轻链和重链改组分别进行亲和力成熟,产生最终产物 B9 克隆。B9 噬菌体 Fab 与雄性脾细胞的结合能力是其亲本 A8 克隆的两倍(通过 ELISA 确定)。基于免疫荧光染色,B9-Fab 主要与雄性脾细胞的表面抗原结合,并识别睾丸细胞。所得 B9-Fab 检测到一种单一的蛋白质(通过对雄性脾细胞和睾丸的 Western blot 分析确定为约 40 kDa);其具有高 SDM 抗原结合能力,可能是由于互补决定区-3 中的突变位点和 κ 链和 Fd 链的氨基酸序列长度不同。使用链改组增强的 Fab 的新型重组克隆是研究 SDM 抗原特异性结合和应用的分子机制的候选分子。

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引用本文的文献

1
Sexing murine embryos with an indirect immunofluorescence assay using phage antibody B9-Fab against SDM antigen.
J Vet Med Sci. 2015 Jun;77(6):711-4. doi: 10.1292/jvms.14-0650. Epub 2015 Feb 8.

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