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中子和伽马射线联合辐照对人外周血转录谱的影响。

Effects of Neutron and Gamma Rays Combined Irradiation on the Transcriptional Profile of Human Peripheral Blood.

机构信息

China Institute for Radiation Protection, Taiyuan City, Shanxi Province, China, 030006.

Huazhong University of Science and Technology, Wuhan City, Hubei Province, China, 430074.

出版信息

Radiat Res. 2023 Jul 1;200(1):65-79. doi: 10.1667/RADE-22-00147.2.

Abstract

We studied the effects of neutrons, neutrons and γ rays, and γ rays exposures on the transcription spectrum in human peripheral blood of three healthy adult men. Samples were irradiated with 1.42 Gy 2.5-MeV neutrons, 0.71 Gy neutrons and 0.71 Gy 137Cs γ rays, and 1.42 Gy 137Cs γ rays. Transcriptome sequencing identified 56 differentially co-expressed genes and enriched 26 KEGG pathways. There are 97, 45 and 30 differentially expressed genes in neutron, neutron and γ ray combined treatment, and γ rays, respectively, and 21, 3 and 8 KEGG pathways with significant differences are enriched. Fluorescence quantitative polymerase chain reaction (qPCR) verified differential co-expression of AEN, BAX, DDB2, FDXR, and MDM2. Additionally, irradiation of AHH-1 human lymphocytes with a 252Cf neutron source at 0, 0.14, 0.35, and 0.71 Gy, fluorescence qPCR revealed a dose-response relationship for BAX, DDB2, and FDXR at dose ranges of 0-0.71 Gy, with R2 of 0.803, 0.999, and 0.999, respectively. Thus, neutrons can induce more differentially expressed genes and enrich more pathways. Combined treatment of neutrons and γ-rays may incorporate damage of both high and low LET, the genes activated by neutrons and γ rays combined are almost the combination of genes activated by neutron and γ rays combined treatment. BAX, DDB2 and FDXR are differentially expressed after irradiation by Deuterium-Deuterium (D-D) neutron source and 252Cf neutron source, so they are expected to be molecular targets of neutron damage.

摘要

我们研究了中子、中子和γ射线以及γ射线照射对三名健康成年男性外周血转录谱的影响。样品分别用 1.42 Gy 2.5-MeV 中子、0.71 Gy 中子和 0.71 Gy 137Cs γ 射线以及 1.42 Gy 137Cs γ 射线照射。转录组测序鉴定出 56 个差异共表达基因,并富集了 26 个 KEGG 通路。在中子、中子和γ射线联合处理以及γ射线中,分别有 97、45 和 30 个差异表达基因,有 21、3 和 8 个 KEGG 通路有显著差异。荧光定量聚合酶链反应 (qPCR) 验证了 AEN、BAX、DDB2、FDXR 和 MDM2 的差异共表达。此外,用 252Cf 中子源照射 AHH-1 人淋巴细胞,剂量分别为 0、0.14、0.35 和 0.71 Gy,荧光 qPCR 显示 BAX、DDB2 和 FDXR 在 0-0.71 Gy 剂量范围内存在剂量反应关系,R2 分别为 0.803、0.999 和 0.999。因此,中子可以诱导更多的差异表达基因并富集更多的途径。中子和γ射线的联合处理可能会结合高 LET 和低 LET 的损伤,由中子和γ射线联合处理激活的基因几乎是由中子和γ射线联合处理激活的基因的组合。氘氘 (D-D) 中子源和 252Cf 中子源照射后,BAX、DDB2 和 FDXR 表达差异,有望成为中子损伤的分子靶点。

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