头颈部晚期鳞状细胞癌患者瘤周注射白细胞介素-2后免疫细胞局部和全身激活的证据。
Evidence for local and systemic activation of immune cells by peritumoral injections of interleukin 2 in patients with advanced squamous cell carcinoma of the head and neck.
作者信息
Whiteside T L, Letessier E, Hirabayashi H, Vitolo D, Bryant J, Barnes L, Snyderman C, Johnson J T, Myers E, Herberman R B
机构信息
Department of Pathology, University of Pittsburgh School of Medicine, Pennsylvania 15213.
出版信息
Cancer Res. 1993 Dec 1;53(23):5654-62.
Interleukin 2 (IL2) was injected peritumorally and intranodally in 36 patients with unresectable squamous cell carcinoma of the head and neck enrolled in an Eastern Cooperative Oncology Group-sponsored phase Ib trial (EST P-Z388). Groups of 6 patients received escalating doses(200, 2 x 10(3), 2 x 10(4), 2 x 10(5), 2 x 10(6), and 4 x 10(6) units) of IL2 daily 5 times/week for 2 weeks. Tumor biopsies were obtained before and after IL2 therapy. Tumor tissue was provided for histology, and the remaining fresh tissue was divided for snap-freezing in -75 degrees C and for separation of tumor-infiltrating lymphocytes (TIL) and tumor cells. Immunophenotyping of TIL performed on cryostat sections of paired pre- and post-IL2 biopsy tissues showed increases after IL2 therapy in the number of T-cells (P = 0.005), natural killer (NK; CD16+) cells (P = 0.0001), CD25+ cells (P = 0.004), and HLA-DR+ cells (P = 0.001) accumulating in the tumor stroma. In the tumor parenchyma, NK cells (P = 0.0001) and HLA-DR+ cells (P = 0.003) were increased after IL2 therapy. The T:NK cell ratios in the tumor stroma and parenchyma were decreased after therapy, suggesting selective accumulation of NK cells. By flow cytometry, TIL recovered from post-IL2 biopsy tissues were enriched (P < 0.05) in CD3-CD56+ (NK) cells. In situ hybridization with [35S] cDNA probes for cytokines and IL2 receptors indicated that the numbers of cells expressing mRNA for IL2, tumor necrosis factor alpha, IL1-beta, gamma-interferon, transforming growth factor beta, and IL2 receptor p55 or p70 were increased in post-IL2 biopsy tissues as compared to pre-IL2 tissues. Cytolytic activity of TIL isolated from post-IL2 tissues was also increased, as determined in 4-h 51Cr release assays against K562 targets (12 +/- 3 mean lytic units/10(7) cells +/- SEM pre-IL2 versus 46 +/- 13 post-IL2; n = 16) and against autologous tumor (13 +/- 8 versus 68 +/- 26; n = 9). Fresh TIL of one clinical responder showed relatively high levels (195 lytic units) of autotumor cytotoxicity after IL2 therapy versus no activity prior to therapy. In the blood, NK and lymphokine-activated killer cell activity, and percentages of CD3-CD56+ NK cells and of activated (CD25+) T-lymphocytes were increased for all doses of IL2.(ABSTRACT TRUNCATED AT 400 WORDS)
在东部肿瘤协作组资助的Ib期试验(EST P-Z388)中,对36例不可切除的头颈部鳞状细胞癌患者进行瘤周和瘤内注射白细胞介素2(IL2)。每组6例患者,每周5次,连续2周,每日接受递增剂量(200、2×10³、2×10⁴、2×10⁵、2×10⁶和4×10⁶单位)的IL2治疗。在IL2治疗前后获取肿瘤活检组织。将肿瘤组织用于组织学检查,其余新鲜组织分为两部分,一部分在-75℃速冻,另一部分用于分离肿瘤浸润淋巴细胞(TIL)和肿瘤细胞。对配对的IL2治疗前后活检组织的低温切片进行TIL免疫表型分析,结果显示,IL2治疗后,肿瘤基质中积聚的T细胞数量增加(P = 0.005)、自然杀伤(NK;CD16⁺)细胞数量增加(P = 0.0001)、CD25⁺细胞数量增加(P = 0.004)以及HLA-DR⁺细胞数量增加(P = 0.001)。在肿瘤实质中,IL2治疗后NK细胞数量增加(P = 0.0001),HLA-DR⁺细胞数量增加(P = 0.003)。治疗后肿瘤基质和实质中的T:NK细胞比值降低,提示NK细胞选择性积聚。通过流式细胞术分析,从IL2治疗后的活检组织中回收的TIL富含(P < 0.05)CD3⁻CD56⁺(NK)细胞。用细胞因子和IL2受体的[³⁵S] cDNA探针进行原位杂交表明,与IL2治疗前的组织相比,IL2治疗后的活检组织中表达IL2、肿瘤坏死因子α、IL1-β、γ-干扰素、转化生长因子β以及IL2受体p55或p70 mRNA的细胞数量增加。从IL2治疗后的组织中分离的TIL的细胞溶解活性也增加,在针对K562靶标的4小时⁵¹Cr释放试验中得到证实(IL2治疗前平均裂解单位/10⁷细胞±SEM为12±3,IL2治疗后为46±13;n = 16),针对自体肿瘤的试验中也得到证实(13±8 vs 68±26;n = 9)。一名临床缓解者的新鲜TIL在IL2治疗后显示出相对较高水平(195裂解单位)的自体肿瘤细胞毒性,而治疗前无活性。在血液中,所有剂量的IL2均可使NK和淋巴因子激活的杀伤细胞活性以及CD3⁻CD56⁺NK细胞和活化(CD25⁺)T淋巴细胞的百分比增加。(摘要截选至400字)
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