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利用酵母展示和新一代测序技术进行表位作图

Epitope Mapping Using Yeast Display and Next Generation Sequencing.

作者信息

Van Blarcom Thomas, Rossi Andrea, Foletti Davide, Sundar Purnima, Pitts Steven, Melton Zea, Telman Dilduz, Zhao Lora, Cheung Wai Ling, Berka Jan, Zhai Wenwu, Strop Pavel, Pons Jaume, Rajpal Arvind, Chaparro-Riggers Javier

机构信息

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

23andMe Inc., South San Francisco, CA, USA.

出版信息

Methods Mol Biol. 2018;1785:89-118. doi: 10.1007/978-1-4939-7841-0_7.

Abstract

Monoclonal antibodies are the largest class of therapeutic proteins due in part to their ability to bind an antigen with a high degree of affinity and specificity. A precise determination of their epitope is important for gaining insights into their therapeutic mechanism of action and to help differentiate antibodies that bind the same antigen. Here, we describe a method to precisely and efficiently map the epitopes of multiple antibodies in parallel over the course of just several weeks. This approach is based on a combination of rational library design, yeast surface display, and next generation DNA sequencing and provides quantitative insights into the epitope residues most critical for the antibody-antigen interaction. As an example, we will use this method to map the epitopes of several antibodies that neutralize alpha toxin from Staphylococcus aureus.

摘要

单克隆抗体是治疗性蛋白质中最大的一类,部分原因在于它们能够以高度的亲和力和特异性结合抗原。精确确定其表位对于深入了解其治疗作用机制以及区分结合相同抗原的抗体很重要。在这里,我们描述了一种方法,可在短短几周内并行精确且高效地绘制多种抗体的表位图谱。这种方法基于合理的文库设计、酵母表面展示和下一代DNA测序的组合,并提供了对抗体 - 抗原相互作用最关键的表位残基的定量见解。例如,我们将使用这种方法来绘制几种中和金黄色葡萄球菌α毒素的抗体的表位图谱。

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