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树突状细胞/抗原呈递细胞介导提供表达 T 细胞受体 γδ(TCRγδ)的细胞有助于改善体外抗白血病反应。

Dendritic/antigen presenting cell mediated provision of T-cell receptor gamma delta (TCRγδ) expressing cells contributes to improving antileukemic reactions ex vivo.

机构信息

Department of Medicine III, University Hospital of Munich, Munich 81377, Germany.

Department of Orthodontics and Dentofacial Orthopedics, University Hospital, LMU Munich, Munich 80336, Germany.

出版信息

Mol Immunol. 2024 Nov;175:40-54. doi: 10.1016/j.molimm.2024.09.007. Epub 2024 Sep 20.

DOI:10.1016/j.molimm.2024.09.007
PMID:39305847
Abstract

T-cell receptor gamma delta (TCRγδ) expressing T-cells are known to mediate an MHC-independent immune response and could therefore qualify for immune therapies. We examined the influence of dendritic cells(DC)/antigen presenting cell (APC) generated from blast-containing whole blood (WB) samples from AML and MDS patients on the provision of (leukemia-specific) TCRγδ expressing T-cells after mixed lymphocyte culture (MLC). Kit-M (granulocyte-macrophage colony-stimulating factor (GM-CSF) + prostaglandin E1 (PGE1)) or Kit-I (GM-CSF + Picibanil) were used to generate leukemia derived APC/DC (DC)from WB, which were subsequently used to stimulate T-cell enriched MLC. Immune cell composition and functionality were analysed using degranulation- (DEG), intracellular cytokine- (INTCYT) and cytotoxicity fluorolysis- (CTX) assays. Flow cytometry was used for cell quantification. We found increased frequencies of APCs/DCs and their subtypes after Kit-treatment of healthy and patients´ WB compared to control, as well as an increased stimulation and activation of several types of immune reactive cells after MLC. Higher frequencies of TCRγδ expressing leukemia-specific degranulation and intracellularly cytokine producing T-cells were found. The effect of Kit-M-treatment on frequencies of TCRγδ expressing cells and their degranulation could be correlated with the Kit-M-mediated blast lysis compared to control. We also found higher frequencies of TCRγδ expressing T-cells in AML patients´ samples with an achieved remission (compared to blast persistence) after induction chemotherapy. This might point to APC/DC-mediated effects resulting in the provision of leukemia-specific TCRγδ expressing T-cells: Moreover a quantification of TCRγδ expressing T-cells might contribute to predict prognosis of AML/MDS patients.

摘要

T 细胞受体 γδ (TCRγδ) 表达的 T 细胞已知介导 MHC 非依赖性免疫反应,因此有资格进行免疫治疗。我们研究了来自 AML 和 MDS 患者含 blast 的全血 (WB) 样本生成的树突状细胞 (DC)/抗原呈递细胞 (APC) 对混合淋巴细胞培养 (MLC) 后提供 (白血病特异性) TCRγδ 表达 T 细胞的影响。Kit-M(粒细胞-巨噬细胞集落刺激因子 (GM-CSF) + 前列腺素 E1 (PGE1))或 Kit-I(GM-CSF + Picibanil)用于从 WB 生成白血病衍生的 APC/DC (DC),随后用于刺激 T 细胞富集 MLC。使用脱颗粒-(DEG)、细胞内细胞因子-(INTCYT)和细胞毒性荧光水解-(CTX)测定法分析免疫细胞组成和功能。流式细胞术用于细胞定量。与对照相比,我们发现 Kit 处理健康人和患者 WB 后 APC/DC 及其亚型的频率增加,以及 MLC 后几种类型的免疫反应性细胞的刺激和激活增加。发现具有更高频率的 TCRγδ 表达的白血病特异性脱颗粒和细胞内产生细胞因子的 T 细胞。与对照相比,Kit-M 处理对 TCRγδ 表达细胞及其脱颗粒频率的影响可与 Kit-M 介导的 blast 裂解相关。我们还发现诱导化疗后获得缓解(与 blast 持续存在相比)的 AML 患者样本中 TCRγδ 表达 T 细胞的频率更高。这可能指向 APC/DC 介导的效应,导致提供白血病特异性 TCRγδ 表达 T 细胞:此外,TCRγδ 表达 T 细胞的定量可能有助于预测 AML/MDS 患者的预后。

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