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开发一种体外检测方法,用于筛选犬类程序性死亡受体-1/程序性细胞死亡配体 1 单克隆抗体治疗药物。

Development of an in vitro assay for screening programmed death receptor-1/programmed cell death ligand 1 monoclonal antibody therapy in dogs.

机构信息

Laboratory of Molecular Diagnostics and Therapeutics, Joint Graduate school of Veterinary Medicine, Yamaguchi University, 1677-1 Yoshida, Yamaguchi 753-8515, Japan.

Nippon Zenyaku Kogyo Co., Ltd., Koriyama, Fukushima, Japan.

出版信息

Vet Immunol Immunopathol. 2024 Aug;274:110792. doi: 10.1016/j.vetimm.2024.110792. Epub 2024 Jun 13.

DOI:10.1016/j.vetimm.2024.110792
PMID:38878679
Abstract

Immunomodulatory antibody drugs that modulate the function of immune checkpoint molecules, such as programmed death receptor-1 (PD-1) and programmed cell death ligand 1 (PD-L1), have been established as new cancer treatments in human medicine. In recent years, there have also been reports on antibodies that inhibit immune checkpoint molecules in dogs, and clinical trials using such antibodies for canine cancer have been gradually increasing in number. Because inhibitory antibodies restore T-cell function by inhibiting the binding of PD-1 on T cells and its ligand PD-L1, the quality of antibody function has been evaluated using activated T cells or peripheral blood mononuclear cells isolated from healthy dogs; however, the assays and dogs used significantly vary. Therefore, in the present study, we developed a reporter gene assay using reporter cells (Jurkat/NFATluc/cPD1) and effector cells (CTAC/OKT3/cPDL1). Jurkat/NFATluc/cPD1 were generated by introducing both of the NFAT-responsive luciferase gene as a marker of T-cell signaling and canine PD-1, into a human T lymphoid cell line, Jurkat. CTAC/OKT3/cPDL1 were generated by introducing single-chain FV (scFV) of anti-human CD3 antibody (OKT3) and canine PD-L1 into a canine thyroid carcinoma cell line, CTAC. Ligation of PD-1 on Jurkat/NFATluc/cPD1 via binding of PD-L1 on CTAC/OKT3/cPDL1 suppressed NFAT luciferase activity induced by CD3 ligation by scFV of OKT3. The addition of anti-canine PD-1 and PD-L1 antibodies, both of which were previously developed in our laboratory, restored this suppression with high sensitivity, although the anti-human PD-L1 antibody atezolizumab induced a very weak restoration. This assay is an useful method for functionally evaluating the inhibition of canine PD-1 and PD-L1 binding.

摘要

免疫调节抗体药物调节免疫检查点分子的功能,如程序性死亡受体-1(PD-1)和程序性细胞死亡配体 1(PD-L1),已被确立为人类医学中的新型癌症治疗方法。近年来,也有关于在狗中抑制免疫检查点分子的抗体的报道,并且使用此类抗体治疗犬癌症的临床试验数量逐渐增加。由于抑制性抗体通过抑制 PD-1 在 T 细胞上与其配体 PD-L1 的结合来恢复 T 细胞功能,因此使用来自健康狗分离的激活 T 细胞或外周血单核细胞来评估抗体的功能质量;然而,所用的测定和狗有很大的不同。因此,在本研究中,我们使用报告细胞(Jurkat/NFATluc/cPD1)和效应细胞(CTAC/OKT3/cPDL1)开发了一种报告基因测定法。Jurkat/NFATluc/cPD1 通过将 NFAT 反应性荧光素酶基因作为 T 细胞信号的标志物和犬 PD-1 引入人 T 淋巴细胞系 Jurkat 中而产生。CTAC/OKT3/cPDL1 通过将抗人 CD3 抗体(OKT3)的单链 FV(scFV)和犬 PD-L1 引入犬甲状腺癌细胞系 CTAC 中而产生。通过 CTAC/OKT3/cPDL1 上的 PD-L1 与 Jurkat/NFATluc/cPD1 上的 PD-1 结合,抑制 Jurkat/NFATluc/cPD1 上的 PD-1 抑制由 OKT3 的 scFV 诱导的 NFAT 荧光素酶活性。我们实验室先前开发的抗犬 PD-1 和 PD-L1 抗体的添加以高灵敏度恢复了这种抑制作用,尽管抗人 PD-L1 抗体 atezolizumab 诱导了非常弱的恢复作用。该测定法是一种用于功能评估犬 PD-1 和 PD-L1 结合抑制的有用方法。

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