Grimm E A, Bruner J M, Carinhas J, Köppen J A, Loudon W G, Owen-Schaub L, Steck P A, Moser R P
Department of Tumor Biology, University of Texas, M.D. Anderson Cancer Center, Houston 77030.
Cancer Immunol Immunother. 1991;32(6):391-9. doi: 10.1007/BF01741334.
Outgrowth of tumor-infiltrating lymphocytes (TIL) from the human primary brain tumor glioblastoma multiforme was achieved by OKT3 initiation (10 ng/ml), followed by sustained expansion by interleukin-2 (IL-2; 200 U/ml). Tumor-infiltrating lymphocyte (TIL) initiation by this process was performed in parallel with the standard "IL-2-only" method. Of ten tumors, seven yielded TIL in response to OKT3/IL-2, whereas only three of these seven grew after initiation with IL-2 alone. On the basis of cell doubling times, at least 60 doublings, resulting in (hypothetically) up to 10(23) TIL from as few as 2 x 10(5) cells in tumor suspensions, could be achieved using OKT3/IL-2. OKT3-initiated TIL proliferated in culture for as long as 288 days, although senescence of some cultures occurred at as early as 73 days. Significant heterogeneity of lymphocytes infiltrating the fresh tumors and heterogeneity of resultant TIL phenotype and function were apparent, yet several common trends were noted. In all cases after OKT3 initiation, significant net growth was not apparent until approximately 14 days. In contrast, in the three samples that grew in response to IL-2 alone, log-phase growth was always observed earlier. During the early phase of the cultures, all TIL expressed some killing activity toward a broad spectrum of tumors, including the autologous tumor. No consistent preference of TIL for lysis of autologous tumor was observed. Glioblastoma multiforme TIL cultures contained a mixture of CD8+ and CD4+ cells, with few CD16+ or NKH-1+. Of the six TIL examined in detail for population phenotype in relationship to time in culture, four eventually became exclusively CD4+. Further analysis of these CD4+ TIL indicated that all were of the helper-inducer class, 4B4+ and 2H4-. Concurrent with the decline in CD8+ cells, a decline in the cytolytic activity of these TIL cultures occurred. Furthermore, in two TIL that remained CD8+, a decline in the cytolytic activity also occurred. Therefore, loss of killing activity was not merely a reflection of the major cell phenotype changes. These results indicate that the OKT3/IL-2 process provides an alternative to IL-2 alone for TIL initiation and growth, as well as providing a novel system for further analysis of tumor-derived lymphocyte and accessory cell functional potential.
通过OKT3启动(10纳克/毫升),随后用白细胞介素-2(IL-2;200单位/毫升)持续扩增,成功实现了从人原发性脑肿瘤多形性胶质母细胞瘤中培养肿瘤浸润淋巴细胞(TIL)。通过该方法启动肿瘤浸润淋巴细胞(TIL)的培养与标准的“仅用IL-2”方法同时进行。在10个肿瘤样本中,7个对OKT3/IL-2有反应产生了TIL,而这7个样本中只有3个在仅用IL-2启动培养后生长。根据细胞倍增时间,使用OKT3/IL-2,至少可实现60次倍增,(假设)从肿瘤悬液中少至2×10⁵个细胞可产生多达10²³个TIL。OKT3启动的TIL在培养中可增殖长达288天,尽管有些培养物早在73天就出现了衰老。浸润新鲜肿瘤的淋巴细胞存在显著异质性,以及所得TIL的表型和功能也存在异质性,但也注意到了一些共同趋势。在所有经OKT3启动后的病例中,直到大约14天才有明显的净生长。相比之下,在仅对IL-2有反应而生长的3个样本中,对数期生长总是更早出现。在培养的早期阶段,所有TIL对包括自体肿瘤在内的多种肿瘤都表现出一定的杀伤活性。未观察到TIL对自体肿瘤裂解有一致的偏好。多形性胶质母细胞瘤TIL培养物包含CD8⁺和CD4⁺细胞的混合物,很少有CD16⁺或NKH-1⁺细胞。在详细检查的6个TIL群体表型与培养时间关系的样本中,4个最终完全变成了CD4⁺。对这些CD4⁺TIL的进一步分析表明,它们均为辅助诱导型,4B4⁺和2H4⁻。随着CD8⁺细胞数量的减少,这些TIL培养物的细胞溶解活性也出现下降。此外,在两个仍为CD8⁺的TIL中,细胞溶解活性也下降了。因此,杀伤活性的丧失不仅仅是主要细胞表型变化的反映。这些结果表明,OKT3/IL-2方法为TIL的启动和生长提供了一种替代仅用IL-2的方法,同时也为进一步分析肿瘤来源的淋巴细胞和辅助细胞的功能潜力提供了一个新系统。
