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无标记表位分组分析单克隆抗体能够鉴定抗原异质性。

Label-free epitope binning assays of monoclonal antibodies enable the identification of antigen heterogeneity.

机构信息

Rinat-Pfizer Inc, South San Francisco, CA 94080, USA.

出版信息

J Immunol Methods. 2012 Aug 31;382(1-2):101-16. doi: 10.1016/j.jim.2012.05.010. Epub 2012 May 17.

DOI:10.1016/j.jim.2012.05.010
PMID:22609372
Abstract

Label-free biosensors are often used in the discovery of therapeutic antibodies to characterize the epitope binding regions of a panel of monoclonal antibodies that target a specific antigen, thus facilitating their organization into epitope groups or "bins". When tested in a pairwise combinatorial manner, two antibodies that compete with one another for binding to a specific antigen may be grouped into the same epitope bin - that is, they recognize similar or overlapping epitopes - whereas two antibodies that bind simultaneously to the antigen are placed into different epitope bins. However, depending on the assay format used, results from such experiments can sometimes contradict one another. Here, we provide two examples that illustrate how antigen heterogeneity, either inherent in an antigen sample, or induced by the assay conditions, can confound the interpretation of epitope binning results and, in some cases, lead to erroneous conclusions. We highlight why assays that employ solution antigen are often more reliable than those that employ immobilized antigen and, by corroborating our binning results with assays that utilize native antigen, we determine which subpopulations of our heterogeneous antigen samples are biologically relevant and thus improve the correlation between epitope bins and functional activity. Furthermore, we provide recommendations for performing definitive binning assays and a diagnostic assay procedure that can be followed when antigen heterogeneity is suspected.

摘要

无标记生物传感器常用于治疗性抗体的发现中,以鉴定针对特定抗原的单克隆抗体的表位结合区域,从而将其组织成表位组或“bin”。当以成对组合的方式进行测试时,两种相互竞争与特定抗原结合的抗体可能被归为同一表位 bin,即它们识别相似或重叠的表位,而同时与抗原结合的两种抗体则被归入不同的表位 bin。然而,根据所用的测定方法,这些实验的结果有时可能相互矛盾。在这里,我们提供了两个示例,说明抗原异质性如何(无论是抗原样品固有的,还是由测定条件诱导的)会混淆表位 bin 结果的解释,并在某些情况下导致错误的结论。我们强调了为什么使用溶液抗原的测定方法通常比使用固定化抗原的测定方法更可靠,并且通过将我们的 bin 结果与使用天然抗原的测定方法进行验证,我们确定了我们的异质抗原样品的哪些亚群具有生物学相关性,从而提高了表位 bin 与功能活性之间的相关性。此外,我们还提供了进行明确 binning 测定的建议以及在怀疑抗原异质性时可以遵循的诊断测定程序。

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