Kil Whoon Jong, Cerna David, Burgan William E, Beam Katie, Carter Donna, Steeg Patricia S, Tofilon Philip J, Camphausen Kevin
Radiation Oncology Branch, National Cancer Institute, Bethesda, Maryland 20892, USA.
Clin Cancer Res. 2008 Feb 1;14(3):931-8. doi: 10.1158/1078-0432.CCR-07-1856.
Temozolomide, a DNA methylating agent, is currently undergoing clinical evaluation for cancer therapy. Because temozolomide has been shown to increase survival rates of patients with malignant gliomas when given combined with radiation, and there is conflicting preclinical data concerning the radiosensitizing effects of temozolomide, we further investigated the possible temozolomide-induced enhancement of radiosensitivity.
The effects of temozolomide on the in vitro radiosensitivity of U251 (a human glioma) and MDA-MB231BR (a brain-seeking variant of a human breast tumor) cell lines was evaluated using clonogenic assay. DNA damage and repair were evaluated using phosphorylated histone H2AX (gammaH2AX), and mitotic catastrophe was measured using nuclear fragmentation. Growth delay was used to evaluate the effects of temozolomide on in vivo (U251) tumor radiosensitivity.
Exposure of each cell line to temozolomide for 1 h before irradiation resulted in an increase in radiosensitivity with dose enhancement factors at a surviving fraction of 0.1 ranging from 1.30 to 1.32. Temozolomide had no effect on radiation-induced apoptosis or on the activation of the G(2) cell cycle checkpoint. As a measure of DNA double strand breaks, gammaH2AX foci were determined as a function of time after the temozolomide + irradiation combination. The number of gammaH2AX foci per cell was significantly greater at 24 h after the combined modality compared with the individual treatments. Mitotic catastrophe, measured at 72 h, was also significantly increased in cells receiving the temozolomide + irradiation combination compared with the single treatments. In vivo studies revealed that temozolomide administration to mice bearing U251 tumor xenografts resulted in a greater than additive increase in radiation-induced tumor growth delay with a dose enhancement factor of 2.8.
These results indicate that temozolomide can enhance tumor cell radiosensitivity in vitro and in vivo and suggest that this effect involves an inhibition of DNA repair leading to an increase in mitotic catastrophe.
替莫唑胺是一种DNA甲基化剂,目前正处于癌症治疗的临床评估阶段。由于已证明替莫唑胺与放疗联合使用时可提高恶性胶质瘤患者的生存率,且关于替莫唑胺的放射增敏作用存在相互矛盾的临床前数据,我们进一步研究了替莫唑胺可能诱导的放射敏感性增强。
使用克隆形成试验评估替莫唑胺对U251(一种人类胶质瘤)和MDA-MB231BR(一种人类乳腺肿瘤的脑靶向变体)细胞系体外放射敏感性的影响。使用磷酸化组蛋白H2AX(γH2AX)评估DNA损伤和修复,并使用核碎裂测量有丝分裂灾难。生长延迟用于评估替莫唑胺对体内(U251)肿瘤放射敏感性的影响。
在照射前将每个细胞系暴露于替莫唑胺1小时导致放射敏感性增加,在存活分数为0.1时剂量增强因子为1.30至1.32。替莫唑胺对辐射诱导的细胞凋亡或G(2)细胞周期检查点的激活没有影响。作为DNA双链断裂的指标,γH2AX焦点根据替莫唑胺+照射组合后的时间确定。与单独治疗相比,联合治疗后24小时每个细胞的γH2AX焦点数量明显更多。在72小时测量的有丝分裂灾难在接受替莫唑胺+照射组合的细胞中也比单一治疗显著增加。体内研究表明,向携带U251肿瘤异种移植物的小鼠施用替莫唑胺导致辐射诱导的肿瘤生长延迟增加大于相加作用,剂量增强因子为2.8。
这些结果表明替莫唑胺可在体外和体内增强肿瘤细胞的放射敏感性,并表明这种作用涉及对DNA修复的抑制,导致有丝分裂灾难增加。
Zotero 插件