A154:流式细胞术分析抗pd1免疫治疗前或期间黑色素瘤组织活检的免疫反应

E. Shklovskaya, Jenny H. Lee, S. Lim, S. Alavi, J. Thompson, R. Saw, M. Carlino, R. Scolyer, A. Menzies, G. Long, R. Kefford, H. Rizos
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引用次数: 0

摘要

针对程序性细胞死亡蛋白1 (PD-1)免疫检查点的抗体显著提高了晚期转移性黑色素瘤患者的生存率。对抗pd -1治疗的先天和获得性耐药是一个重要的治疗障碍,但耐药机制尚不清楚,难以在细胞水平上建立模型。在这里,我们使用多参数流式细胞术检查了31例III-IV期转移性黑色素瘤患者在(基线,n = 21)或(n = 18)单药抗pd1免疫治疗之前或期间获得的39例肿瘤活检的免疫谱;12名患者对治疗产生了耐药性。样品被酶解并冷冻保存至解冻,并用荧光标记抗体染色,以便对黑色素瘤细胞和肿瘤浸润淋巴细胞(til)进行全面分析。平均黑色素瘤细胞含量为57+4.7%(平均+s.e.m),平均免疫浸润(CD45阳性细胞)为31.5+4.5%。对黑色素瘤细胞抗原呈递分子和PD-1配体表达的分析显示,在基线(9/21,43%)和治疗后肿瘤(10/18,56%)中,HLA-ABC表达频繁下调,包括2/39样本中HLA-ABC完全丧失。在9/39(23%)的肿瘤中观察到HLA-ABC上调。HLA-DR和PD-L1的表达与HLA-ABC的表达密切相关(Spearman r分别为0.68和0.89),提示局部干扰素暴露。与PD-L1不同,PD-L2在活检组织中的黑色素瘤细胞表达较低。相比之下,γ干扰素很容易诱导PD-L2表达,并与分离活检建立的匹配黑色素瘤细胞系中HLA-ABC表达相关(9/39)。我们发现在基线和治疗样本中表征肿瘤细胞免疫特征的参数和TILs之间存在多重相关性。在显著的治疗相关变化中,治疗组携带αβ t细胞受体的常规t细胞比基线高1.4倍(65+2.7% vs 46.2+4.1%), P引用形式:Elena Shklovskaya, Jenny Lee, Su Yin Lim, Sara Alavi, John Thompson, Robyn Saw, Matteo Carlino, Richard Scolyer, Alexander Menzies, Georgina Long, Richard Kefford, Helen Rizos。流式细胞术分析抗pd1免疫治疗前后黑色素瘤组织活检的免疫反应[摘要]。第四届CRI-CIMT-EATI-AACR国际癌症免疫治疗会议:将科学转化为生存;2018年9月30日至10月3日;纽约,纽约。费城(PA): AACR;癌症免疫,2019;7(2增刊):摘要nr A154。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Abstract A154: Flow cytometric analysis of immune responses in the melanoma tissue biopsies before or during anti-PD1 immunotherapy
Antibodies directed against the programmed cell death protein 1 (PD-1) immune checkpoint have significantly improved survival of patients with advanced metastatic melanoma. Innate and acquired resistance to anti-PD-1 treatment represents a significant treatment obstacle, yet the mechanisms of resistance are poorly understood and remain difficult to model at the cellular level. Here we used multiparameter flow cytometry to examine the immune profiles of 39 tumor biopsies obtained from 31 patients with stage III-IV metastatic melanoma prior to (baseline, n = 21) or during (n = 18) single-agent anti-PD1 immunotherapy; twelve patients developed resistance to treatment. Samples were enzymatically dissociated and cryopreserved until thawed and stained with fluorescently labeled antibodies to enable a comprehensive analysis of melanoma cells and tumor infiltrating lymphocytes (TILs). Mean melanoma cell content was 57+4.7% (mean+s.e.m.) while mean immune infiltrate (CD45 positive cells) was 31.5+4.5%. Analysis of melanoma cell expression of antigen presenting molecules and PD-1 ligands revealed frequent downregulation of HLA-ABC expression in both baseline (9/21, 43%) and on-treatment tumors (10/18, 56%), including a complete HLA-ABC loss in 2/39 samples. HLA-ABC up-regulation was observed in 9/39 (23%) tumors. Expression of HLA-DR and PD-L1 strongly correlated with that of HLA-ABC (Spearman r=0.68 and =0.89, respectively), indicative of local interferon exposure. Unlike PD-L1, melanoma cell expression of PD-L2 was low in the biopsied tissue. In contrast, PD-L2 expression was readily induced by gamma interferon and correlated with HLA-ABC expression in matching melanoma cell lines established from the dissociated biopsies (9/39). We found multiple correlations between parameters characterizing the immune profiles of tumor cells and TILs in both baseline and on-treatment samples. Among significant treatment-associated changes, conventional T-cells bearing the αβ T-cell receptor were 1.4-fold higher in the on-treatment group compared to baseline (65+2.7% versus 46.2+4.1%, P Citation Format: Elena Shklovskaya, Jenny Lee, Su Yin Lim, Sara Alavi, John Thompson, Robyn Saw, Matteo Carlino, Richard Scolyer, Alexander Menzies, Georgina Long, Richard Kefford, Helen Rizos. Flow cytometric analysis of immune responses in the melanoma tissue biopsies before or during anti-PD1 immunotherapy [abstract]. In: Proceedings of the Fourth CRI-CIMT-EATI-AACR International Cancer Immunotherapy Conference: Translating Science into Survival; Sept 30-Oct 3, 2018; New York, NY. Philadelphia (PA): AACR; Cancer Immunol Res 2019;7(2 Suppl):Abstract nr A154.
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