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用于从噬菌体展示文库中生成抗体的微孔板自动淘选和筛选程序。

Automated panning and screening procedure on microplates for antibody generation from phage display libraries.

作者信息

Turunen Laura, Takkinen Kristiina, Söderlund Hans, Pulli Timo

机构信息

VTT Technical Research Centre of Finland, Espoo, Finland.

出版信息

J Biomol Screen. 2009 Mar;14(3):282-93. doi: 10.1177/1087057108330113. Epub 2009 Feb 17.

DOI:10.1177/1087057108330113
PMID:19224869
Abstract

Antibody phage display technology is well established and widely used for selecting specific antibodies against desired targets. Using conventional manual methods, it is laborious to perform multiple selections with different antigens simultaneously. Furthermore, manual screening of the positive clones requires much effort. The authors describe optimized and automated procedures of these processes using a magnetic bead processor for the selection and a robotic station for the screening step. Both steps are performed in a 96-well microplate format. In addition, adopting the antibody phage display technology to automated platform polyethylene glycol precipitation of the enriched phage pool was unnecessary. For screening, an enzyme-linked immunosorbent assay protocol suitable for a robotic station was developed. This system was set up using human gamma-globulin as a model antigen to select antibodies from a VTT naive human single-chain antibody (scFv) library. In total, 161 gamma-globulin-selected clones were screened, and according to fingerprinting analysis, 9 of the 13 analyzed clones were different. The system was further tested using testosterone bovine serum albumin (BSA) and beta-estradiol-BSA as antigens with the same library. In total, 1536 clones were screened from 4 rounds of selection with both antigens, and 29 different testosterone-BSA and 23 beta-estradiol-BSA binding clones were found and verified by sequencing. This automated antibody phage display procedure increases the throughput of generating wide panels of target-binding antibody candidates and allows the selection and screening of antibodies against several different targets in parallel with high efficiency.

摘要

抗体噬菌体展示技术已得到充分确立并广泛用于筛选针对所需靶标的特异性抗体。使用传统的手动方法,同时用不同抗原进行多次筛选非常费力。此外,手动筛选阳性克隆需要付出很多努力。作者描述了这些过程的优化和自动化程序,使用磁珠处理器进行筛选,使用机器人工作站进行筛选步骤。两个步骤均以96孔微孔板形式进行。此外,将抗体噬菌体展示技术应用于自动化平台时,无需对富集的噬菌体库进行聚乙二醇沉淀。对于筛选,开发了一种适用于机器人工作站的酶联免疫吸附测定方案。该系统以人γ-球蛋白作为模型抗原建立,用于从VTT天然人单链抗体(scFv)文库中筛选抗体。总共筛选了161个γ-球蛋白选择的克隆,根据指纹分析,13个分析克隆中有9个不同。使用相同文库,以睾酮牛血清白蛋白(BSA)和β-雌二醇-BSA作为抗原对该系统进行了进一步测试。总共从两种抗原的4轮筛选中筛选了1536个克隆,发现了29个不同的睾酮-BSA结合克隆和23个β-雌二醇-BSA结合克隆,并通过测序进行了验证。这种自动化抗体噬菌体展示程序提高了生成大量靶标结合抗体候选物的通量,并允许高效地并行筛选针对几种不同靶标的抗体。

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