Yamasaki T, Yamashita J, Handa H, Namba Y, Hanaoka M
No Shinkei Geka. 1984 Feb;12(2):141-50.
The immunoregulatory effects of TCGF (T-cell growth factor) on the generation and growth of syngeneic murine malignant glioma (20-methylcholanthrene-induced 203-glioma)-specific killer T-cell were investigated in C57BL/6 adult mice in order to clarify the immunopotential usefulness for anti-tumor local adoptive immunotherapy against malignant brain tumor. TCGF was prepared and assayed. Briefly, 5 x 10(6) ml mouse spleen cells were cultured with 2 microgram/ml concanavalin A in RPMI-1640 medium supplemented with 2% fetal calf serum for 24 hours. Culture supernatants were concentrated by ammonium sulphate precipitation (55 to 80% saturation) and purified by gel filtration (Sephadex G-100, a molecular weight from 30 to 36,000 daltons) and ion exchange chromatography (DEAE-cellulose, elution with 0.15 M in NaCl at ph 7.4). The purified TCGF had no IFN activity. Assays for TCGF was performed for quantitative analysis using 203-glioma-specific killer T cell clone (G-CTLL), which was obtained by limiting dilution method (0.3 cells/well in 96 well microtiter plate) and maintained for over 6 months in the presence of TCGF. Titer (U/ml) of TCGF was defined as the quantity of TCGF required to obtain one-half of the maximal stimulation of G-CTLL proliferation assay. It was confirmed that the specific killer T-cell against 203-glioma was generated in mice after intracranial as well as subcutaneous inoculation of the tumor cells. The killer T-cell activity of spleen cells, however, began to be severely impaired 2 weeks after intracranial inoculation concurrently with the increased intracranial pressure due to developing the tumor growth. Sensitized lymphocytes obtained from intracranial and subcutaneous tumor-bearing mice were assessed for CTL (cytotoxic T-lymphocyte) activity in MLTC (mixed lymphocyte-tumor cell culture) for 18 hours by microcytotoxicity assay. The specific cytotoxicity against 203-glioma cells was enhanced when sensitized lymphocytes from intracranial and subcutaneous tumor-bearing mice were pre-cultured with optimal TCGF (20 U/ml) for over 5 days. After the treatment of sensitized lymphocytes with anti-Thy-1 monoclonal antibody and complement, however, the specific cytotoxicity of sensitized lymphocytes was eliminated almost completely. Therefore, it was thought that TCGF possesses immunoregulatory effects of enhancement of killer T-cell activity. On the contrary, TCGF had no influence on normal T lymphocytes and the growth of 203-glioma cells in vitro.(ABSTRACT TRUNCATED AT 400 WORDS)
为了阐明针对恶性脑肿瘤的抗肿瘤局部过继性免疫疗法的免疫潜力,在C57BL/6成年小鼠中研究了TCGF(T细胞生长因子)对同基因小鼠恶性胶质瘤(20-甲基胆蒽诱导的203-胶质瘤)特异性杀伤性T细胞的产生和生长的免疫调节作用。制备并检测了TCGF。简要来说,将5×10⁶/ml小鼠脾细胞与2μg/ml伴刀豆球蛋白A在补充有2%胎牛血清的RPMI-1640培养基中培养24小时。培养上清液通过硫酸铵沉淀(55%至80%饱和度)浓缩,然后通过凝胶过滤(葡聚糖G-100,分子量30至36000道尔顿)和离子交换色谱(DEAE-纤维素,在pH 7.4下用0.15M NaCl洗脱)进行纯化。纯化后的TCGF没有IFN活性。使用通过有限稀释法(在96孔微量滴定板中每孔0.3个细胞)获得并在TCGF存在下维持超过6个月的203-胶质瘤特异性杀伤性T细胞克隆(G-CTLL)对TCGF进行定量分析检测。TCGF的效价(U/ml)定义为获得G-CTLL增殖测定最大刺激的一半所需的TCGF量。证实了在颅内和皮下接种肿瘤细胞后,小鼠体内产生了针对203-胶质瘤的特异性杀伤性T细胞。然而,颅内接种后2周,脾细胞的杀伤性T细胞活性开始严重受损,同时由于肿瘤生长导致颅内压升高。通过微量细胞毒性测定法,在混合淋巴细胞-肿瘤细胞培养(MLTC)中对从颅内和皮下荷瘤小鼠获得的致敏淋巴细胞进行18小时的CTL(细胞毒性T淋巴细胞)活性评估。当来自颅内和皮下荷瘤小鼠的致敏淋巴细胞与最佳TCGF(20U/ml)预培养超过5天时,对203-胶质瘤细胞的特异性细胞毒性增强。然而,在用抗Thy-1单克隆抗体和补体处理致敏淋巴细胞后,致敏淋巴细胞的特异性细胞毒性几乎完全消除。因此,认为TCGF具有增强杀伤性T细胞活性的免疫调节作用。相反,TCGF对正常T淋巴细胞和体外203-胶质瘤细胞的生长没有影响。(摘要截短至400字)
