Functional Analysis of a Novel Complement C5a Receptor 1-Blocking Monoclonal Antibody

单克隆抗体 阻塞(统计) 补语(音乐) C5a受体 补体受体 受体 补体成分5 阻断抗体 化学 补体系统 抗体 生物 免疫学 生物化学 计算机科学 表型 基因 计算机网络 互补
作者
Leon Cyranka,Ida Mariegaard,Mikkel-Ole Skjødt,Rafael Bayarri‐Olmos,Tom Eirik Mollnes,Peter Garred,Anne Rosbjerg
出处
期刊:Journal of Innate Immunity [S. Karger AG]
卷期号:15 (1): 836-849 被引量:3
标识
DOI:10.1159/000535084
摘要

The complement system anaphylatoxin C5a is a critical player in inflammation. By binding to complement C5a receptor 1 (C5aR1/CD88), C5a regulates many cellular functions, mainly as a potent pro-inflammatory inducer. We describe the generation and selection of a potent antagonistic C5aR1 mouse monoclonal antibody (mAb). Initial C5aR1 hybridoma clone selection was performed with a cell-binding study in human whole blood. In-house C5aR1 mAb assessment for C5aR1 inhibition was done via the iLite® C5a assay. C5aR1 mAb specificity was investigated on C5aR1his- and C5aR2his-expressing Flp-In™-CHO cells. Physiological C5aR1 inhibition was assessed via a C5a-driven calcium flux assay and stimulation assay based on isolated polymorphonuclear leukocytes (PMNs) and a whole blood model stimulated with Escherichia coli. The supernatant of hybridoma clones targeting the N-terminal section of C5aR1 displayed efficient binding to C5aR1 in whole blood, which was confirmed for purified mAbs. The C5aR1 mAb 18-41-6 was selected following the assay of in-house C5aR1 mAbs via the iLite® C5a assay. The mAb 18-41-6 was specific for C5aR1. Full-size and/or F(ab')2 preparations of mAb 18-41-6 were found to efficiently abrogate C5a-induced calcium flux in neutrophils and to significantly reduce the upregulation of the activation markers CD11b (neutrophils, monocytes) and CD66b (neutrophils). Our results demonstrate that mAb 18-41-6 is a valuable tool for investigating the C5a-C5aR1 axis and a potential therapeutic candidate for inflammatory disease treatment.

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