PO.IM02.06 · 免疫学

LILRB1 antibody targeting the LILRB1/HLA-G axis: Preclinical efficacy, pharmacokinetics, and safety supporting first-in-human trials

海报缩略图:LILRB1 antibody targeting the LILRB1/HLA-G axis: Preclinical efficacy, pharmacokinetics, and safety supporting first-in-human trials
编号 5561 展板 4 时间 4/21 02:00–05:00 区域 Section 7 主讲 Han Byoul Kim, PhD
分会场 Oncogenic Pathways and Cancer Immunity
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作者与单位

Han Byoul Kim, Seok-Joo Kim, Younghoon Kim, Junhaeng Cho, Minsoon Kim, JungA Kim, Suji Hong, Heehang Kim, Shin-Young Kang, Kyungna Ko, Jun-Gyu Park, Hyungjin Cho, Jeeyeon Roh, Young Dok Son, Wooseok Ko

LG Chem, Seoul, Korea, Republic of

摘要 Abstract

Background: LILRB1 is an inhibitory receptor expressed on T cells, B cells, NK cells, and monocytes. It binds to HLA class I molecules, with the highest affinity for HLA-G. This interaction delivers inhibitory signals that allow tumor cells to evade immune surveillance, impairing NK cell, T cell, and macrophage function. Disrupting the LILRB1/HLA-G axis is a promising strategy for restoring anti-tumor immunity. Additionally, LILRB1 may regulate T cell function independently of PD-1, suggesting potential to overcome resistance to PD-1 inhibitors. Methods: Binding affinity and specificity of LG-LILRB1 antibody were assessed via surface plasmon resonance and flow cytometry. Competitive binding assays confirmed blockade of LILRB1/HLA-G interaction. Restoration of immune cell function was evaluated using flow cytometry and western blotting. Anti-tumor efficacy was tested in human LILRB1 transgenic mice. Pharmacokinetics and toxicokinetics were studied in cynomolgus monkeys, and safety was assessed through GLP-compliant toxicology and immunotoxicity studies. Results: LG-LILRB1 antibody showed high-affinity, selective binding to LILRB1 and dose-dependent blockade of HLA-G. Functional assays revealed enhanced T cell proliferation, NK cell cytotoxicity, and macrophage phagocytosis. In vivo, LG-LILRB1 antibody significantly inhibited tumor growth (up to 88.8%) in transgenic mice bearing HLA-G-expressing tumors. Pharmacodynamic analysis showed increased infiltration and activation of CD8⁺ T cells and NK cells. Combination with PD-L1 blockade yielded synergistic anti-tumor effects. In monkeys, LG-LILRB1 antibody exhibited dose-proportional exposure and a long half-life (>12 days). No treatment-related adverse findings were observed in 4-week GLP toxicity studies. Conclusions: LG-LILRB1 antibody, a first-in-class LILRB1 blocker, restored anti-tumor immunity by disrupting the LILRB1/HLA-G axis. It enhanced immune cell function and showed strong efficacy in preclinical models. Favorable pharmacokinetics and safety support its clinical development. Combination with PD-L1 blockade further improved outcomes. These findings support LG-LILRB1 antibody as a promising candidate for cancer immunotherapy, with a Phase 1a trial currently ongoing (NCT06332755).
利益披露 Disclosure
H. Kim, None.. S. Kim, None.. Y. Kim, None.. J. Cho, None.. M. Kim, None.. J. Kim, None.. S. Hong, None.. H. Kim, None.. S. Kang, None.. K. Ko, None.. J. Park, None.. H. Cho, None.. J. Roh, None.. Y. Son, None.. W. Ko, None.

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