Discovery and optimization of a novel anti-GUCY2c x CD3 bispecific antibody for the treatment of solid tumors

噬菌体展示 抗体 合理设计 免疫原性 单链可变片段 蛋白质工程 体内 可制造性设计 表位 计算生物学 化学 癌症研究 单克隆抗体 免疫学 生物 生物化学 纳米技术 材料科学 工程类 生物技术 机械工程
作者
Adam Root,Gurkan Guntas,Madan Katragadda,James R. Apgar,Jatin Narula,Chew Shun Chang,Sara R. Hanscom,Matthew T. McKenna,Jason Wade,Caryl Meade,Weijun Ma,Yongjing Guo,Yan Liu,Weili Duan,Claire Hendershot,Amy King,Yan Zhang,Eric Sousa,Amy Tam,Susan Benard,Han-Kwang Yang,Kerry Kelleher,Fang Jin,Nicole Piche‐Nicholas,Sinéad E. Keating,Fernando Narciandi,Rosemary F. Lawrence-Henderson,Mikki Arai,Wayne R. Stochaj,Kristine Svenson,Lidia Mosyak,Khetemcnee Lam,Christopher Francis,Kimberly Marquette,Liliana Wróblewska,Haitao Zhu,Alfredo Darmanin Sheehan,Edward R. LaVallie,Aaron M. D’Antona,Alison Betts,Lindsay King,Edward Rosfjord,Orla Cunningham,Laura Lin,Puja Sapra,Lioudmila Tchistiakova,Divya Mathur,Laird Bloom
出处
期刊:mAbs [Landes Bioscience]
卷期号:13 (1) 被引量:11
标识
DOI:10.1080/19420862.2020.1850395
摘要

We report here the discovery and optimization of a novel T cell retargeting anti-GUCY2C x anti-CD3ε bispecific antibody for the treatment of solid tumors. Using a combination of hybridoma, phage display and rational design protein engineering, we have developed a fully humanized and manufacturable CD3 bispecific antibody that demonstrates favorable pharmacokinetic properties and potent in vivo efficacy. Anti-GUCY2C and anti-CD3ε antibodies derived from mouse hybridomas were first humanized into well-behaved human variable region frameworks with full retention of binding and T-cell mediated cytotoxic activity. To address potential manufacturability concerns, multiple approaches were taken in parallel to optimize and de-risk the two antibody variable regions. These approaches included structure-guided rational mutagenesis and phage display-based optimization, focusing on improving stability, reducing polyreactivity and self-association potential, removing chemical liabilities and proteolytic cleavage sites, and de-risking immunogenicity. Employing rapid library construction methods as well as automated phage display and high-throughput protein production workflows enabled efficient generation of an optimized bispecific antibody with desirable manufacturability properties, high stability, and low nonspecific binding. Proteolytic cleavage and deamidation in complementarity-determining regions were also successfully addressed. Collectively, these improvements translated to a molecule with potent single-agent in vivo efficacy in a tumor cell line adoptive transfer model and a cynomolgus monkey pharmacokinetic profile (half-life>4.5 days) suitable for clinical development. Clinical evaluation of PF-07062119 is ongoing.
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