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硒蛋白 P 抑制辐射诱导的晚期活性氧积累和正常细胞损伤。

Selenoprotein P inhibits radiation-induced late reactive oxygen species accumulation and normal cell injury.

机构信息

Free Radical and Radiation Biology Division, Department of Radiation Oncology, University of Iowa, Iowa City, Iowa.

出版信息

Int J Radiat Oncol Biol Phys. 2013 Nov 1;87(3):619-25. doi: 10.1016/j.ijrobp.2013.06.2063.

Abstract

PURPOSE

Radiation is a common mode of cancer therapy whose outcome is often limited because of normal tissue toxicity. We have shown previously that the accumulation of radiation-induced late reactive oxygen species (ROS) precedes cell death, suggesting that metabolic oxidative stress could regulate cellular radiation response. The purpose of this study was to investigate whether selenoprotein P (SEPP1), a major supplier of selenium to tissues and an antioxidant, regulates late ROS accumulation and toxicity in irradiated normal human fibroblasts (NHFs).

METHODS AND MATERIALS

Flow cytometry analysis of cell viability, cell cycle phase distribution, and dihydroethidium oxidation, along with clonogenic assays, were used to measure oxidative stress and toxicity. Human antioxidant mechanisms array and quantitative real-time polymerase chain reaction assays were used to measure gene expression during late ROS accumulation in irradiated NHFs. Sodium selenite addition and SEPP1 overexpression were used to determine the causality of SEPP1 regulating late ROS accumulation and toxicity in irradiated NHFs.

RESULTS

Irradiated NHFs showed late ROS accumulation (4.5-fold increase from control; P<.05) that occurs after activation of the cell cycle checkpoint pathways and precedes cell death. The mRNA levels of CuZn- and Mn-superoxide dismutase, catalase, peroxiredoxin 3, and thioredoxin reductase 1 increased approximately 2- to 3-fold, whereas mRNA levels of cold shock domain containing E1 and SEPP1 increased more than 6-fold (P<.05). The addition of sodium selenite before the radiation treatment suppressed toxicity (45%; P<.05). SEPP1 overexpression suppressed radiation-induced late ROS accumulation (35%; P<.05) and protected NHFs from radiation-induced toxicity (58%; P<.05).

CONCLUSION

SEPP1 mitigates radiation-induced late ROS accumulation and normal cell injury.

摘要

目的

辐射是癌症治疗的常见方式,但由于正常组织毒性,其疗效往往受到限制。我们之前已经表明,辐射诱导的晚期活性氧(ROS)的积累先于细胞死亡,这表明代谢氧化应激可能调节细胞的辐射反应。本研究的目的是研究硒蛋白 P(SEPP1)——组织中硒的主要供应者和抗氧化剂——是否调节辐照正常人类成纤维细胞(NHF)中晚期 ROS 的积累和毒性。

方法和材料

采用流式细胞术分析细胞活力、细胞周期相分布和二氢乙啶氧化,以及集落形成试验,以测量氧化应激和毒性。使用人类抗氧化机制阵列和定量实时聚合酶链反应(PCR)分析,测量辐照 NHF 中晚期 ROS 积累过程中的基因表达。添加亚硒酸钠和过表达 SEPP1,以确定 SEPP1 是否调节辐照 NHF 中晚期 ROS 的积累和毒性。

结果

辐照 NHF 显示晚期 ROS 积累(比对照增加 4.5 倍;P<.05),发生在细胞周期检查点途径激活之后,先于细胞死亡。CuZn-和 Mn-超氧化物歧化酶、过氧化氢酶、过氧化物酶 3 和硫氧还蛋白还原酶 1 的 mRNA 水平增加了约 2-3 倍,而冷休克结构域 E1 和 SEPP1 的 mRNA 水平增加了 6 倍以上(P<.05)。在辐照前添加亚硒酸钠可抑制毒性(45%;P<.05)。过表达 SEPP1 可抑制辐照诱导的晚期 ROS 积累(35%;P<.05)并保护 NHF 免受辐照诱导的毒性(58%;P<.05)。

结论

SEPP1 减轻了辐照诱导的晚期 ROS 积累和正常细胞损伤。

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