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首页> 外文期刊>Journal of Immunological Methods >Development of a multi-product leached protein A assay for bioprocess samples containing recombinant human monoclonal antibodies.
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Development of a multi-product leached protein A assay for bioprocess samples containing recombinant human monoclonal antibodies.

机译:多种产品浸出蛋白的开发,用于包含重组人单克隆抗体的生物过程样品的测定。

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摘要

The detection of low level of protein A leached from monoclonal antibody downstream purification process is often interfered by the presence of excess amount of product antibody. In order to prevent this interference, we developed a new multi-product leached protein A assay that used acidification to completely dissociate the IgG-ProteinA complex, followed by neutralization under selected condition to prevent re-formation of the IgG-ProteinA complex. The amount of protein A was then determined by a sandwich immunoassay using Meso Scale Discovery technology. The assay takes approximately 3h to complete for one 96-well plate of samples, and this has been successfully applied to samples containing different monoclonal antibody products examined so far. The data demonstrates that this assay is robust and efficient in determining leached protein A contamination during purification of recombinant monoclonal antibodies.
机译:从单克隆抗体下游纯化过程中浸出的低水平蛋白A的检测通常会受到过量产物抗体的存在的干扰。为了防止这种干扰,我们开发了一种新的多产品浸出蛋白A分析方法,该方法使用酸化作用将IgG-ProteinA复合物完全解离,然后在选定条件下进行中和,以防止IgG-ProteinA复合物重新形成。然后使用Meso Scale Discovery技术通过夹心免疫测定法确定蛋白A的量。对于一个96孔板样品,该测定大约需要3小时才能完成,目前已成功应用于包含不同单克隆抗体产物的样品。数据表明,该测定在确定重组单克隆抗体纯化过程中确定淋溶的A蛋白污染方面既可靠又有效。

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