Comparing in vitro affinity measurements of antibodies to TfR1: Surface plasmon resonance versus on-cell affinity

表面等离子共振 化学 亲缘关系 转铁蛋白受体 抗体 分析物 生物物理学 亲和层析 转铁蛋白 生物化学 色谱法 生物 免疫学 纳米技术 纳米颗粒 材料科学
作者
Gillian Bonvicini,Sunitha Bagawath Singh,Patrik Nygren,Mengfei Xiong,Stina Syvänen,Dag Sehlin,Ronny Falk,Karl Andersson
出处
期刊:Analytical Biochemistry [Elsevier]
卷期号:686: 115406-115406 被引量:1
标识
DOI:10.1016/j.ab.2023.115406
摘要

Despite years of utilizing the transferrin receptor 1 (TfR1) to transport large biomolecules into the brain, there is no consensus on how to optimally measure affinity to it. The aim of this study was to compare different methods for measuring the affinities of anti-TfR1 antibodies. Antibodies 15G11, OX26 and 8D3 are known to successfully carry large biologics across the blood-brain barrier in humans, rats, and mice, respectively. The affinity to their respective species of TfR1 was measured with different surface plasmon resonance setups in Biacore and an on-cell assay. When the antibody was captured and TfR1 was the analyte, the dissociation in Biacore was very slow. The dissociation was faster when the antibody was the analyte and TfR1 was the ligand. The Biacore setup with capture of N-terminal FLAG-tag TfR1 yielded the most similar apparent affinities as the cell assay. In conclusion, it is important to evaluate assay parameters including assay orientation, surface capture method, and antibody-format when comparing binding kinetics for TfR1 antibodies. Although it seems possible to determine relative affinities of TfR1 antibodies using the methods described here, both the FLAG-tag TfR1 capture setup and cell assays likely yield apparent affinities that are most translatable in vivo.
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