Computational design of N‐linked glycans for high throughput epitope profiling

Author:

Greisen Per Jr.1ORCID,Yi Li2,Zhou Rong3,Zhou Jian3,Johansson Eva2ORCID,Dong Tiantang3,Liu Haimo3,Johnsen Laust B.2,Lund Søren2,Svensson L. Anders2,Zhu Haisun3,Thomas Nidhin1,Yang Zhiru3,Østergaard Henrik4

Affiliation:

1. Digital Science and Innovation Novo Nordisk A/S Seattle USA

2. Global Research Technologies Novo Nordisk A/S Maaloev Denmark

3. Discovery Technology China, Novo Nordisk Research Centre Novo Nordisk A/S Beijing China

4. Global Drug Discovery Novo Nordisk A/S Maaloev Denmark

Abstract

AbstractEfficient identification of epitopes is crucial for drug discovery and design as it enables the selection of optimal epitopes, expansion of lead antibody diversity, and verification of binding interface. Although high‐resolution low throughput methods like x‐ray crystallography can determine epitopes or protein–protein interactions accurately, they are time‐consuming and can only be applied to a limited number of complexes. To overcome these limitations, we have developed a rapid computational method that incorporates N‐linked glycans to mask epitopes or protein interaction surfaces, thereby providing a mapping of these regions. Using human coagulation factor IXa (fIXa) as a model system, we computationally screened 158 positions and expressed 98 variants to test experimentally for epitope mapping. We were able to delineate epitopes rapidly and reliably through the insertion of N‐linked glycans that efficiently disrupted binding in a site‐selective manner. To validate the efficacy of our method, we conducted ELISA experiments and high‐throughput yeast surface display assays. Furthermore, x‐ray crystallography was employed to verify the results, thereby recapitulating through the method of N‐linked glycans a coarse‐grained mapping of the epitope.

Publisher

Wiley

Subject

Molecular Biology,Biochemistry

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