黄芪汤对延缓C离子辐射致大鼠肾组织细胞凋亡的影响及相关机制

目的: 探讨黄芪汤抑制¹²C⁶⁺离子辐射脑模型鼠肾组织细胞凋亡的分子保护机制。方法: 50只SPF级Wistar大鼠随机分为正常对照组,单纯辐射模型组,黄芪汤(高、中、低剂量)组。正常对照组和单纯辐射模型组给予等体积生理盐水灌胃10 ml/(kg·d),黄芪汤治疗组分别灌胃给予黄芪汤18、9、4.5 g/(kg·d),连续给药2周。7 d后除正常对照组外,其余各组大鼠脑组织给予4Gy ¹²C⁶⁺离子束单次照射,辐射后第7日处死各组大鼠。HE染色法观察大鼠肾脏的病理形态变化,ELISA法检测大鼠血清IL-6的含量,实时荧光定量PCR法测定大鼠肾脏Bcl-2、Bax和Caspase-3的基因表达,免疫组化法检测大鼠肾脏Bcl-2、Bax、Caspase-3和NF-κB的蛋白表达。结果: 与正常对照组比较,单纯辐射模型组体重和肾脏指数均显著降低,血清IL-6的含量显著升高,肾脏Bcl-2的基因表达和蛋白表达均显著降低,Bax和Caspase-3的基因表达和蛋白表达均显著升高,NF-κB的蛋白表达也显著升高(P＜ 0.01),单纯辐射组肾小球系膜细胞明显增生,肾小管间质血管明显扩张充血,肾小管管腔狭窄、不规则。与单纯辐射模型组相比,黄芪汤高剂量组体重和肾脏指数均明显升高,黄芪汤各干预组肾脏Bcl-2的基因表达和蛋白表达均显著升高(P＜0.05或P＜0.01);而黄芪汤中、高剂量组Bax和Caspase-3的蛋白表达均显著降低,各干预组血清IL-6的含量显著降低,肾脏Bax和Caspase-3的基因表达均显著降低,肾脏NF-κB的蛋白表达显著下降(P＜0.05或P＜0.01),黄芪汤高剂量组可见肾小球系膜细胞增生情况明显改善,肾小管轮廓清晰。结论: 黄芪汤对¹²C⁶⁺离子辐射脑模型鼠的肾损伤具有一定的防护作用,其作用机制可能与调控Bcl-2/NF-κB信号通路有关。     

基于日光诱导叶绿素荧光的北半球森林物候研究

植被物候是反映植被生长规律的重要指标, 对气候的反馈具有重要意义。日光诱导叶绿素荧光(SIF)通过复杂的能量耗散机制与光合作用相关联, 提供了从空间直接探测大范围植被物候的可能性。为了探究气候变化背景下SIF反演不同森林类型物候的适用性, 该文以北半球35个全球通量网(FLUXNET)森林站点为研究对象, 利用2007-2014年SIF值和总初级生产力(GPP)通过双逻辑生长模型和动态阈值法来估算3种典型森林类型的物候, 并采用相关性分析等方法评价SIF在估算不同森林类型物候时的差异性。主要结果为: 1) SIF对生长季开始时间(SOS)的估算精度高于生长季结束时间(EOS); 2) SIF能够更准确地估算混交林(MF)的SOS, 但是不能精确追踪落叶阔叶林(DBF)和常绿针叶林(ENF)的SOS; 3)春季季前短波辐射是驱动SOS的主要气候因素。综上, 建议在将来的研究中将SIF数据与其他遥感指数整合, 应用于不同植物类型的物候监测。     

Impacts of remotely sensed environmental drivers on coral outplant survival

Globally, coral reefs are degrading due to a variety of stressors including climate change and pollution. Active restoration is an important effort for sustaining coral reefs where, typically, coral fragments are outplanted onto degraded reefs. Coral outplants, however, can experience mortality in response to a range of stressors. We pair results of outplant monitoring observations with satellite‐based measurements of multiple oceanographic variables to estimate the relative importance of each driver to coral outplant survival. We find that when considering mean environmental conditions experienced by outplants during the monitoring period, particulate organic carbon (POC) levels are most important in determining outplant survival, with certain levels of POC beneficial for outplants. Sea surface temperature anomalies (SSTA) are also important determinants of outplant survival, where survival is greatest in regions with minimal or slightly negative anomalies. Survival also increases with increasing distance to land, likely due to a reduction in negative ridge‐to‐reef effects on coral outplants. When considering the range (min–max) of environmental conditions experienced during the monitoring period, large fluctuations in photosynthetically active radiation (PAR) and POC are most important in determining outplant survival. Increasing outplant depth can help to counter the negative impacts of large fluctuations in environmental variables. We find that a variety of remotely sensed oceanographic variables have significant impacts on survival and should be considered in coral restoration planning to help evaluate potential restoration sites and ultimately maximize coral outplant survival.     

外源NO对不同UV-B辐射天数处理的小麦叶片总蛋白的影响

研究外源NO对不同UV-B辐射天数处理的小麦叶片总蛋白的影响.采用蒸馏水和0.1 mmol/L 硝普钠（SNP,一种NO供体）浸种24 h,试验设置不同的处理组：CK、CK＋B、SNP、SNP＋B.待幼苗生长7天后取其叶片进行总蛋白的提取及SDS-PAGE凝胶图像的分析.不同处理对叶片总蛋白含量、电泳图谱及电泳条带数目的影响不同;外源NO能显著增加不同UV-B处理天数下小麦叶片总蛋白的含量,且SNP和SNP＋B处理组的电泳条带均较CK和CK＋B处理组的电泳条带变宽且颜色变深.外源NO能显著增加UV-B辐射下小麦叶片的总蛋白含量.同时,不同处理组电泳条带数目的变化反应出一些蛋白的降解和合成,最终也体现了不同处理组蛋白含量的变化.     

Protracted low-dose radiation priming and response of liver to acute gamma and proton radiation

Abstract

This study evaluated liver from C57BL/6 mice irradiated with low-dose/low-dose-rate (LDR) γ-rays (0.01 Gy, 0.03 cGy/h), with and without subsequent exposure to acute 2 Gy gamma or proton radiation. Analyses were performed on day 56 post-exposure. Expression patterns of apoptosis-related genes were strikingly different among irradiated groups compared with 0 Gy (p < 0.05). Two genes were affected in the Gamma group, whereas 10 were modified in the LDR + Gamma group. In Proton and LDR + Proton groups, there were six and 12 affected genes, respectively. Expression of genes in the Gamma (Traf3) and Proton (Bak1, Birc2, Birc3, Mcl1) groups was no longer different from 0 Gy control group when mice were pre-exposed to LDR γ-rays. When each combined regimen was compared with the corresponding group that received acute radiation alone, two genes in the LDR + Gamma group and 17 genes in the LDR + Proton group were modified; greatest effect was on Birc2 and Nol3 (> 5-fold up-regulated by LDR + Protons). Oxygen radical production in livers from the LDR + Proton group was higher in LDR, Gamma, and LDR + Gamma groups (p < 0.05 vs. 0 Gy), but there were no differences in phagocytosis of E. coli. Sections stained with hematoxylin and eosin (H&E) suggested more inflammation, with and without necrosis, in some irradiated groups. The data demonstrate that response to acute radiation is dependent on radiation quality and regimen and that some LDR γ-ray-induced modifications in liver response were still evident nearly 2 months after exposure.     

Calibration of the comet assay for the measurement of DNA damage in mammalian cells

We used X-rays from a linear accelerator and from a low energy therapeutic source to calibrate the single cell gel electrophoresis (comet assay), a widely used method to measure DNA damage. γ-Rays from ⁶⁰Co, with known efficiency in inducing DNA breakage, were used as reference. Human lymphocytes and one murine tumour cell line, F10-M3 cells, were irradiated under different experimental conditions. A similar relationship between radiation dose and induced DNA damage was obtained with γ- and X-rays. A calibration curve was constructed to convert the comet assay raw data into break frequency. The median levels of DNA breaks and oxidative damage in circulating lymphocytes from healthy volunteers were calculated to be 0.76 and 0.80 breaks/10⁹ Da, respectively, (0.50 and 0.52 breaks/10⁶ bp). The values of oxidative DNA damage were in the same order of magnitude as those found by others with HPLC methods.     

The cysteine 34 residue of A1M/α1-microglobulin is essential for protection of irradiated cell cultures and reduction of carbonyl groups

Abstract

α₁-microglobulin (A1M) is a 26 kDa plasma and a tissue protein belonging to the lipocalin family. The reductase and free radical scavenger A1M has been shown to protect cells and extracellular matrix against oxidative and irradiation-induced damage. The reductase activity was previously shown to depend upon an unpaired cysteinyl side-chain, C34, and three lysyl side-chains, K92, 118, and 130, located around the open end of the lipocalin pocket. The aim of this work was to investigate whether the cell and matrix protection by A1M is a result of its reductase activity by using A1M-variants with site-directed mutations of the C34, K92, K118, and K130 positions. The results show that the C34 side-chain is an absolute requirement for protection of HepG2 cell cultures against alpha-particle irradiation-induced cell death, upregulation of stress response and cell cycle regulation genes. Mutation of C34 also resulted in loss of the reduction capacity toward heme- and hydrogen peroxide-oxidized collagen, and the radical species 2,2´-azino-bis (3-ethyl-benzo-thiazoline-6-sulphonic acid) (ABTS). Furthermore, mutation of C34 significantly suppressed the cell-uptake of A1M. The K92, K118, and K130 side-chains were of minor importance in cell protection and reduction of oxidized collagen but strongly influenced the reduction of the ABTS-radical. It is concluded that antioxidative protection of cells and collagen by A1M is totally dependent on its C34 amino acid residue. A model of the cell protection mechanism of A1M should be based on the redox activity of the free thiolyl group of the C34 side-chain and a regulatory role of the K92, K118, and K130 residues.     

Epicatechin ameliorates ionising radiation-induced oxidative stress in mouse liver

Abstract

The current study was intended to evaluate the hepatoprotective effect of Epicatechin (EC) against radiation-induced oxidative stress, in terms of inflammation and lipid peroxidation. Swiss albino mice were administered with EC (15 mg/kg body weight) for three consecutive days before exposing them to a single dose of 5-Gy ⁶⁰Co gamma (γ) irradiation. Mice were necropsied and livers were taken for immunohistochemistry, western blot analysis and biochemical tests for the detection of markers of hepatic oxidative stress. Nuclear translocation of nuclear factor kappa B (NF-κB) and lipid peroxidation were increased whereas the activities of superoxide dismutase (SOD) and catalase (CAT), reduced glutathione (GSH) content and ferric reducing antioxidant power (FRAP) were diminished upon radiation exposure compared to control. Translocation of NF-κB from cytoplasm to nucleus and lipid peroxidation were found to be inhibited whereas an increase in SOD, CAT, GSH and FRAP was observed in the mice treated with EC prior to irradiation. Thus, pre-treatment with EC offers protection against γ-radiation induced hepatic alterations.     

Relationship between serum reactive oxidative metabolite level and skin reaction in an irradiated rat model

Abstract

Purpose. Ionizing radiation generates free radicals and reactive oxygen species that induce DNA damage in vivo. This study aimed to determine the relationship between serum reactive oxygen metabolite (ROM) levels and skin reaction after irradiation in a rat model. Methods and materials. I. Female Wistar rats were classified into 0 Gy (control), 2 Gy, and 30 Gy groups; serum ROM levels were measured in the very acute phase. II. Other female Wistar rats were classified into 0 Gy (control), 30 Gy, 50 Gy, and 70 Gy groups; serum ROM levels were measured before and 3, 7, 16, 24, 31, and 38 days after irradiation. Skin reaction was evaluated according to the SRS (0–5) twice every week. Results. Serum ROM levels in the subacute phase were significantly higher in the 50 and 70 Gy groups than in the 0 and 30 Gy groups [p = 0.029, repeated-measure analysis of variance (ANOVA)]. As expected, SRSs increased in the order of the 0 Gy, 30 Gy, 50 Gy, and 70 Gy groups and differed significantly among these groups (p < 0.001, repeated-measure ANOVA). Peak serum ROM levels were observed 16 days after irradiation in all irradiated groups and corresponded with the appearance of visible skin reaction after irradiation. Conclusions. Serum ROM levels may be useful for evaluating radiation damage in mammals. Further investigations are required to investigate changes in intracellular metabolism after irradiation at gene and protein levels.