Cesano A, Visonneau S, Cioé L, Clark S C, Santoli D
Wistar Institute, Philadelphia, PA 19104, USA.
Cancer Immunol Immunother. 1995 Mar;40(3):139-51. doi: 10.1007/BF01517345.
The TALL-104 cell line, originally derived from a patient with T cell leukemia, can be maintained indefinitely in culture in the presence of interleukin-2 (IL-2) and is endowed with a highly potent major-histocompatibility-complex (MHC)-non-restricted tumoricidal activity both in vitro and in animal models. The present study analyzes in detail the short- and long-term effects of irradiation and cyclosporin A (CsA) treatment on the growth and tumoricidal function of this T cell clone as compared to polyclonal lymphokine-activated killer (LAK) cell preparations from healthy donors. DNA and RNA syntheses by both TALL-104 and LAK cells were irreversibly arrested a few hours after irradiation with 40 Gy. However, 4-h 51Cr-release assays, performed on different days (day 1 to day 7) after irradiation, showed that the cytotoxic efficiency of TALL-104 cells against hematopoietic and solid tumor targets was only modestly reduced, whereas that of LAK cells was severely inhibited. Moreover, the cytotoxic responses to recombinant human IL-2 and IL-12, measured 18 h after irradiation and cytokine addition, were normal in the case of TALL-104 cells but were abolished in the case of LAK cells. Co-culture of IL-2- or IL-12-preactivated TALL-104 cells with a tumor target for 5 days in the absence of cytokines resulted in a lower efficiency of lysis, as compared to the non-irradiated effectors, especially if the initial stimulus was IL-12. These findings suggest the requirement of multiple cytokine stimulation for optimal expression of tumoricidal activity by lethally irradiated TALL-104 cells. CsA, while abrogating TALL-104 cell proliferation at the low dose of 0.5 microgram/ml, inhibited their cytotoxic function marginally only at high doses (100 micrograms/ml). By contrast, CsA reduced dose-dependently the cytotoxicity of LAK cells starting at very low doses (0.5 microgram/ml). CsA did not impair the ability of TALL-104 and LAK cells to produce interferon (IFN) gamma, tumor necrosis factor (TNF) alpha, and granulocyte/macrophage-colony-stimulatory factor (GM-CSF) in response to IL-2, IL-12, or tumor targets. Irradiation reduced drastically IFN gamma production by LAK, but not TALL-104 cells; release of TNF alpha and GM-CSF by either type of effector was inhibited by 10%-50%, depending on the stimulus. The high resistance and immunosuppressive drugs renders tis immortal T cell clone a potentially safe and effective reagent for new adoptive-transfer approaches to cancer in MHC-incompatible recipients.
TALL-104细胞系最初源自一名T细胞白血病患者,在白细胞介素-2(IL-2)存在的情况下可在培养中无限期维持,并在体外和动物模型中具有高效的主要组织相容性复合体(MHC)非限制性杀瘤活性。本研究详细分析了与来自健康供体的多克隆淋巴因子激活的杀伤(LAK)细胞制剂相比,照射和环孢素A(CsA)处理对该T细胞克隆的生长和杀瘤功能的短期和长期影响。用40 Gy照射后数小时,TALL-104细胞和LAK细胞的DNA和RNA合成均被不可逆地阻断。然而,在照射后不同天数(第1天至第7天)进行的4小时51Cr释放试验表明,TALL-104细胞对造血和实体瘤靶标的细胞毒性效率仅略有降低,而LAK细胞的则受到严重抑制。此外,在照射和添加细胞因子18小时后测量的对重组人IL-2和IL--12的细胞毒性反应,TALL-104细胞正常,但LAK细胞则被消除。在无细胞因子的情况下,将IL-2或IL-12预激活的TALL-104细胞与肿瘤靶标共培养5天,与未照射的效应细胞相比,裂解效率较低,尤其是当初始刺激为IL-12时。这些发现表明,致死性照射的TALL-104细胞的杀瘤活性的最佳表达需要多种细胞因子刺激。CsA在0.5微克/毫升的低剂量时可消除TALL-104细胞增殖,但仅在高剂量(100微克/毫升)时才略微抑制其细胞毒性功能。相比之下,CsA从非常低的剂量(0.5微克/毫升)开始就剂量依赖性地降低LAK细胞的细胞毒性。CsA不会损害TALL-104细胞和LAK细胞响应IL-2、IL-12或肿瘤靶标产生干扰素(IFN)γ、肿瘤坏死因子(TNF)α和粒细胞/巨噬细胞集落刺激因子(GM-CSF)的能力。照射可大幅降低LAK细胞而非TALL-104细胞的IFNγ产生;取决于刺激因素,两种效应细胞释放TNFα和GM-CSF均被抑制10%-50%。这种高抗性和免疫抑制药物使这种永生T细胞克隆成为MHC不相容受体中癌症新的过继转移方法的潜在安全有效试剂。
