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重离子辐射诱导的 DNA 损伤通过 Rpl27a-Rpl5-MDM2-p53/E2F1 信号通路介导小鼠精原细胞凋亡。

Heavy ion radiation-induced DNA damage mediates apoptosis via the Rpl27a-Rpl5-MDM2-p53/E2F1 signaling pathway in mouse spermatogonia.

机构信息

Department of Medical Physics, Institute of Modern Physics, Chinese Academy of Sciences, Lanzhou, 730000, China; Key Laboratory of Heavy Ion Radiation Biology and Medicine of Chinese Academy of Sciences, Lanzhou, 730000, China; Key Laboratory of Basic Research on Heavy Ion Radiation Application in Medicine, Lanzhou, 730000, China; School of Nuclear Science and Technology, University of Chinese Academy of Sciences, Beijing, 100039, China.

Department of Medical Physics, Institute of Modern Physics, Chinese Academy of Sciences, Lanzhou, 730000, China; Key Laboratory of Heavy Ion Radiation Biology and Medicine of Chinese Academy of Sciences, Lanzhou, 730000, China; Key Laboratory of Basic Research on Heavy Ion Radiation Application in Medicine, Lanzhou, 730000, China; School of Nuclear Science and Technology, University of Chinese Academy of Sciences, Beijing, 100039, China.

出版信息

Ecotoxicol Environ Saf. 2020 Sep 15;201:110831. doi: 10.1016/j.ecoenv.2020.110831. Epub 2020 Jun 11.

Abstract

The risk of exposure to ionizing radiation (IR) environments has increased with the development of nuclear technology. IR exposure induces excessive apoptosis of the spermatogonia, which leads to male infertility. Spermatogonia apoptosis may be involved in ribosomal stress triggered by DNA damage following exposure to IR because ribosomal proteins (RPs) directly interact with mouse double minute 2 homolog (MDM2) to induce apoptosis. This study aimed to use comparative proteomics and transcriptomics approach to screen the differential RPs and ribosomal mRNAs in mouse testes following high linear energy transfer (LET) carbon ion radiation (CIR). The expression of ribosomal large subunit protein 27a (Rpl27a) decreased at both protein and mRNA levels in the spermatogonia in vivo. After 6 h of CIR, the immunofluorescence signal of 8-oxo-dG and phosphorylated ataxia-telangiectasia-mutated protein (ATM)/histone H2Ax increased, but that of Rpl27a decreased in the spermatogonia of p53 wild-type and knockout mouse testes. Moreover, the nucleolin was scattered throughout the nucleoplasm after CIR. These results suggested that CIR-induced DNA damage might trigger ribosomal stress, and the reduction in the expression of Rpl27a was associated with DNA damage in the spermatogonia. Similarly, in vitro, the immunofluorescence signal of 8-oxo-dG increased in the GC-1 cells after CIR. Moreover, the expression of Rpl27a was regulated by DNA damage because the co-transfection of ATM and Rpl27a or inhibition of ATM-treated CIR could restore the expression of Rpl27a. Furthermore, the reduction in the expression of Rpl27a led to weakened binding of E2F transcription factor 1 (E2F1) and p53 to MDM2, causing p53 activation and E2F1 degradation in p53 wild-type and knockdown GC-1 cells. This study proposed that heavy ion radiation-induced DNA damage mediated spermatogonia apoptosis via the Rpl27a-Rpl5-MDM2-p53/E2F1 signaling pathway. The results provided the underlying molecular mechanisms of spermatogonia apoptosis following exposure to high LET radiation.

摘要

电离辐射(IR)环境的暴露风险随着核技术的发展而增加。IR 暴露诱导精原细胞过度凋亡,导致男性不育。精原细胞凋亡可能涉及核糖体应激,这种应激是由 IR 暴露后 DNA 损伤引发的核糖体蛋白(RPs)与鼠双微体 2 同源物(MDM2)直接相互作用诱导凋亡引起的。本研究旨在使用比较蛋白质组学和转录组学方法筛选高传能线密度(LET)碳离子辐射(CIR)后小鼠睾丸中差异表达的核糖体蛋白和核糖体 mRNA。体内,Rpl27a 的核糖体大亚基蛋白 27a 在蛋白质和 mRNA 水平上均降低。CIR 后 6 小时,p53 野生型和敲除型小鼠睾丸精原细胞中 8-氧鸟嘌呤-DNA 糖基化酶(8-oxo-dG)和磷酸化 ataxia-telangiectasia-mutated 蛋白(ATM)/组蛋白 H2Ax 的免疫荧光信号增加,而 Rpl27a 的免疫荧光信号减少。此外,CIR 后核仁蛋白在核质中弥散。这些结果表明,CIR 诱导的 DNA 损伤可能引发核糖体应激,Rpl27a 的表达减少与精原细胞中的 DNA 损伤有关。同样,体外,CIR 后 GC-1 细胞中 8-oxo-dG 的免疫荧光信号增加。此外,Rpl27a 的表达受 DNA 损伤调控,因为 ATM 和 Rpl27a 的共转染或抑制 ATM 处理的 CIR 可以恢复 Rpl27a 的表达。此外,Rpl27a 表达的减少导致 E2F 转录因子 1(E2F1)和 p53 与 MDM2 的结合减弱,导致 p53 野生型和敲低 GC-1 细胞中 p53 的激活和 E2F1 的降解。本研究提出,重离子辐射诱导的 DNA 损伤通过 Rpl27a-Rpl5-MDM2-p53/E2F1 信号通路介导精原细胞凋亡。研究结果为高 LET 辐射暴露后精原细胞凋亡提供了潜在的分子机制。

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