卵巢癌患者血液和腹水中不同细胞毒性细胞亚群的比较研究

Š. Lukešová, V. Vroblová, J. Tošner, J. Kopecký, I. Sedláková, E. Cermakova, D. Vokurková, O. Kopecký
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引用次数: 25

摘要

研究目的许多观察结果表明,免疫系统在上皮性卵巢癌(EOC)患者中起着重要作用。在EOC病例中,肿瘤浸润淋巴细胞的预后意义尚未明确解释。目的是确定细胞毒性T细胞和NK细胞亚群的表型和激活分子,并比较它们在卵巢癌患者恶性腹水和外周血中的表现。材料与方法对53例EOC患者的肘静脉及恶性腹水血样进行细胞毒细胞检测。用流式细胞仪测定其表面和活化特性。外周血淋巴细胞(pbl)和肿瘤浸润淋巴细胞(TILs)的免疫表型多参数分析。结果TILs(75.9%)和pbl(70.9%)以CD3+ T淋巴细胞为主。激活T细胞的数量在TILs中显著增加:CD3+/69+ 6.7% vs. 0.8% (p < 0.001)。(CD3 - /16+56+) NK细胞在TILs中的代表性显著高于前者:11.0% vs. 5.6% (p = 0.041);同样,CD56+细胞的CD56bright和CD-56bright在TILs中也较高(p < 0.001)。激活受体NKG2D存在于45.1%的TILs和32.3%的pbl中(p = 0.034),但我们没有发现TILs和pbl中CD56+/NKG2D+的数量有显著差异。结论腹水/ pbl间室抗肿瘤反应的特点和强度不同。了解效应细胞的表型和功能是了解抗肿瘤免疫应答的基本前提。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Comparative study of various subpopulations of cytotoxic cells in blood and ascites from patients with ovarian carcinoma
Aim of the study A number of observations have indicated that the immune system plays a significant role in patients with epithelial ovarian cancer (EOC). In cases of EOC, the prognostic significance of tumour infiltrating lymphocytes has not been clearly explained yet. The aim is to determine the phenotype and activation molecules of cytotoxic T cell and NK cell subpopulations and to compare their representation in malignant ascites and peripheral blood in patients with ovarian cancer. Material and methods Cytotoxic cells taken from blood samples of the cubital vein and malignant ascites were obtained from 53 patients with EOC. Their surface and activation characteristics were determined by means of a flow cytometer. Immunophenotype multiparametric analysis of peripheral blood lymphocytes (PBLs) and tumour infiltrating lymphocytes (TILs) was carried out. Results CD3+ T lymphocytes were the main population of TILs (75.9%) and PBLs (70.9%). The number of activating T cells was significantly higher in TILs: CD3+/69+ 6.7% vs. 0.8% (p < 0.001). The representation of (CD3–/16+56+) NK cells in TILs was significantly higher: 11.0% vs. 5.6% (p = 0.041); likewise CD56bright and CD–56bright from CD56+ cells were higher in TILs (both p < 0.001). The activation receptor NKG2D was present in 45.1% of TILs vs. 32.3% of PBLs (p = 0.034), but we did not find a significant difference in the numbers of CD56+/NKG2D+ in TILs and PBLs. Conclusions These results prove that the characteristics and intensity of anti-tumour responses are different in compared compartments (ascites/PBLs). The knowledge of phenotype and functions of effector cells is the basic precondition for understanding the anti-tumour immune response.
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