Shaw Stephen M, Middleton Jenny, Wigglesworth Kim, Charlemagne Amber, Schulz Oliver, Glossop Melanie S, Whalen Giles F, Old Robert, Westby Mike, Pickford Chris, Tabakman Rinat, Carmi-Levy Irit, Vainstein Abi, Sorani Ella, Zur Arik A, Kristian Sascha A
Agalimmune Ltd., Sandwich, Kent, UK.
BioLineRx Ltd, Modi'in-Maccabim-Re'ut, Israel.
Cancer Cell Int. 2019 Dec 19;19:346. doi: 10.1186/s12935-019-1059-8. eCollection 2019.
Treatments that generate T cell-mediated immunity to a patient's unique neoantigens are the current holy grail of cancer immunotherapy. In particular, treatments that do not require cumbersome and individualized ex vivo processing or manufacturing processes are especially sought after. Here we report that AGI-134, a glycolipid-like small molecule, can be used for coating tumor cells with the xenoantigen Galα1-3Galβ1-4GlcNAc (α-Gal) in situ leading to opsonization with pre-existing natural anti-α-Gal antibodies (in short anti-Gal), which triggers immune cascades resulting in T cell mediated anti-tumor immunity.
Various immunological effects of coating tumor cells with α-Gal via AGI-134 in vitro were measured by flow cytometry: (1) opsonization with anti-Gal and complement, (2) antibody-dependent cell-mediated cytotoxicity (ADCC) by NK cells, and (3) phagocytosis and antigen cross-presentation by antigen presenting cells (APCs). A viability kit was used to test AGI-134 mediated complement dependent cytotoxicity (CDC) in cancer cells. The anti-tumoral activity of AGI-134 alone or in combination with an anti-programmed death-1 (anti-PD-1) antibody was tested in melanoma models in anti-Gal expressing galactosyltransferase knockout (α1,3GT) mice. CDC and phagocytosis data were analyzed by one-way ANOVA, ADCC results by paired t-test, distal tumor growth by Mantel-Cox test, C5a data by Mann-Whitney test, and single tumor regression by repeated measures analysis.
In vitro, α-Gal labelling of tumor cells via AGI-134 incorporation into the cell membrane leads to anti-Gal binding and complement activation. Through the effects of complement and ADCC, tumor cells are lysed and tumor antigen uptake by APCs increased. Antigen associated with lysed cells is cross-presented by CD8α+ dendritic cells leading to activation of antigen-specific CD8+ T cells. In B16-F10 or JB/RH melanoma models in α1,3GT mice, intratumoral AGI-134 administration leads to primary tumor regression and has a robust abscopal effect, i.e., it protects from the development of distal, uninjected lesions. Combinations of AGI-134 and anti-PD-1 antibody shows a synergistic benefit in protection from secondary tumor growth.
We have identified AGI-134 as an immunotherapeutic drug candidate, which could be an excellent combination partner for anti-PD-1 therapy, by facilitating tumor antigen processing and increasing the repertoire of tumor-specific T cells prior to anti-PD-1 treatment.
能够产生针对患者独特新抗原的T细胞介导免疫的治疗方法是目前癌症免疫治疗的圣杯。特别是,那些不需要繁琐且个性化的体外处理或制造过程的治疗方法尤其受到追捧。在此我们报告,一种类糖脂小分子AGI-134可用于在肿瘤细胞原位包被异种抗原α-半乳糖(Galα1-3Galβ1-4GlcNAc,简称α-Gal),从而导致其被预先存在的天然抗α-Gal抗体(简称抗Gal)调理,进而触发免疫级联反应,产生T细胞介导的抗肿瘤免疫。
通过流式细胞术检测在体外利用AGI-134用α-Gal包被肿瘤细胞后的各种免疫效应:(1)抗Gal和补体的调理作用;(2)自然杀伤细胞(NK细胞)介导的抗体依赖性细胞毒性(ADCC);(3)抗原呈递细胞(APC)的吞噬作用和抗原交叉呈递。使用活力检测试剂盒检测AGI-134介导的癌细胞补体依赖性细胞毒性(CDC)。在表达抗Gal的半乳糖基转移酶敲除(α1,3GT)小鼠的黑色素瘤模型中检测单独使用AGI-134或与抗程序性死亡-1(抗PD-1)抗体联合使用时的抗肿瘤活性。采用单因素方差分析分析CDC和吞噬作用数据,配对t检验分析ADCC结果,Mantel-Cox检验分析远端肿瘤生长情况,Mann-Whitney检验分析C5a数据,重复测量分析分析单个肿瘤的消退情况。
在体外,通过将AGI-134掺入细胞膜实现肿瘤细胞的α-Gal标记,可导致抗Gal结合和补体激活。通过补体和ADCC的作用,肿瘤细胞被裂解,APC摄取肿瘤抗原增加。与裂解细胞相关的抗原由CD8α+树突状细胞交叉呈递,从而导致抗原特异性CD8+T细胞激活。在α1,3GT小鼠的B16-F10或JB/RH黑色素瘤模型中,瘤内注射AGI-134可导致原发性肿瘤消退,并具有强大的远隔效应,即它可防止未注射的远端病变的发展。AGI-134与抗PD-1抗体联合使用在预防继发性肿瘤生长方面显示出协同效益。
我们已确定AGI-134为一种免疫治疗候选药物,通过促进肿瘤抗原加工并在抗PD-1治疗前增加肿瘤特异性T细胞库,它可能是抗PD-1治疗的优秀联合搭档。
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