煤矿污染土壤降解苯并(a)芘微生物多样性及降解能力研究

以苯并(a)芘(50 mg/L)为唯一碳源,对新疆芦草沟煤矿开采区土壤微生物进行3代胁迫培养(每代60 d);采用PCR-DGGE方法了解不同污染程度土样中降解苯并(a)芘的微生物类群和多样性特点;利用高效液相色谱(HPLC)测定胁迫培养每代培养物混合菌群对苯并(a)芘的降解能力。PCR-DGGE结果显示:不同污染程度原始样品与苯并(a)芘胁迫培养第3代培养物的微生物香浓指数(H)、丰度(S)和均匀度(E)有所不同,其中重度污染培养物降解苯并(a)芘的微生物类群最丰富。对优势条带进行克隆,其主要归属于变形菌门(Proteobacteria)、拟杆菌门(Bacteroidetes)和放线菌门(Actinobacteria)。经HPLC检测发现重度污染样品中的群体微生物对苯并(a)芘的降解率明显高于轻度和中度污染样品,达到78.4%。研究表明新疆芦草沟煤矿开采区污染的土壤中可能蕴藏着降解苯并(a)芘的微生物资源。     

新疆石油污染土壤苯并(a)芘降解微生物多样性研究

为研究新疆石油开采区污染土壤中苯并(a)芘降解微生物的群落结构特点,采集克拉玛依石油开采区受污染程度不同的土壤样品, 以苯并(a)芘为唯一碳源、氮源的无机盐培养基五代富集培养, 采用PCR-DGGE 技术对第五代富集培养物的微生物群落结构开展研究, 根据DGGE 指纹图谱分析它们的遗传多样性。研究显示: 三个不同污染样品微生物多样性指数(H) 丰度(S)和均匀度(EH)均有所不同, 重度污染土样降解苯并(a)芘的微生物类群最为丰富, 其次是中度污染土样, 最少的是轻度污染土样; 并且三个样品微生物类群种类差异较大, 菌落相似性低。对 DGGE 的优势条带序列分析, 同源性最高的微生物分别属于变形菌门(Proteobacteria)、拟杆菌门(Bacteroidetes)、放线菌门(Actinobacteria)和厚壁菌门(Firmicutes)。研究表明新疆石油开采区污染程度不同土壤中降解苯并(a)芘的微生物群落结构不同, 提示污染严重的环境里可能蕴藏着高效降解苯并(a)芘的微生物资源。     

苯并[a]芘和镉暴露对食蚊鱼求偶行为的影响

研究苯并[a]芘(BaP)和镉(Cd2+)暴露对雄性食蚊鱼(Gambusia affinis)求偶行为的影响。设对照组和实验组,BaP暴露浓度为0、0.1、100μg/L;Cd2+暴露浓度为0、5、500 nmol/L;分别暴露6和8周。暴露实验结束后,观察雄鱼与雌鱼配对(1∶1)的求偶行为,并作录像记录分析。结果显示,雄鱼在0.1和100μg/L的BaP分别暴露6周后其对雌鱼的求偶行为开始明显降低,并随着暴露浓度的升高和时间的延长而呈现下降趋势;BaP高浓度组(100μg/L)暴露8周后对雄鱼有严重的致死效应。暴露在5和500 nmol/L的Cd2+至8周后雄鱼求偶行为明显降低;雌鱼暴露在低浓度BaP和Cd2+中其对雄鱼的求偶行为无明显影响(P>0.05);但分别在高浓度100μg/L BaP和500nmol/L Cd2+中暴露后,雄鱼对雌鱼的求偶行为显著减少。结果表明,BaP和Cd2+暴露均可降低雄性食蚊鱼的求偶行为。     

根源信号参与调控气孔行为的机制及其农业节水意义

在土壤干旱情况下,根源信号一方面向植物地上部分的长距离传输,为地上部分提供了土壤水分获取能力的测度,另一方面调控气孔开度,抑制蒸腾作用并提高植物的水分利用效率．文中综述了根源信号参与调控植物水分利用的生理机制和理论模型,指出该模型与根系吸水模型、气孔导度模型耦合,能够更好地反映植物叶片对土壤干旱以及大气干旱的响应、评述了在根源信号参与调控植物水分关系的基础上发展的调亏灌溉(RDI)、部分根系干旱(PRD)和控制性交替灌溉(CAI)等有效灌溉手段,有助于合理配置根系层供水量,通过根土相互作用和信号物质的传输,降低蒸腾和提高水分利用效率、另外,根源信号在调控根系生长发育、延缓地上部分生长以调节根冠比例,优化资源分配以利于生殖生长等方面均有所为,为全面提高农田水分利用效率提供节水生理基础。     

苯并(a)芘诱导的肺细胞癌变过程中时间异质性的拉曼光谱分析

目的 肺癌在生物学特性、基因组变异、增殖速度及化疗响应方面的时间异质性,构成了对有效治疗的显著阻碍。肺癌时间异质性的复杂性,结合其空间异质性,为研究带来了极大挑战。本文将为肺癌研究开辟新的方向,有助于更深入地理解肺癌的时间异质性,从而提升对肺癌的治疗成功率。方法 应用拉曼光谱显微技术作为监测肺癌细胞生物分子组成实时变化的有力工具,揭示了疾病的时间异质性。通过拉曼光谱与多元统计分析的结合,对苯并(a)芘处理后人类肺上皮细胞的生物分子变化进行了细致观察。结果 随时间推移,核酸、脂质、蛋白质及类胡萝卜素含量呈现下降趋势,而葡萄糖浓度上升。这些变化模式暗示,苯并(a)芘可导致遗传物质结构损伤、促进脂质过氧化、干扰蛋白质代谢、降低类胡萝卜素生成,并改变葡萄糖代谢路径。运用拉曼光谱技术,以实时、无侵入性、非破坏性的方式监控肺癌细胞内的生物分子动态,进而阐明其关键分子特性。结论 本项研究深化了对肺癌演进的认识,并为发展个性化治疗策略提供支持,助力提升患者的临床治疗效果。     

苯并(a)芘对鲫鱼肝脏EROD活性的影响

研究了典型多环芳烃类有机污染物苯并(a)芘(BaP)对鲫鱼(Carassius auratus)肝脏7-乙氧基-3-异吩唑酮-脱乙基酶(EROD)活性的影响。结果表明,注射后96 h,10和100 mg.kg-1处理组肝脏EROD活性被明显诱导,分别为对照组的2.3(P<0.05)和3.1倍(P<0.01)。肝脏EROD活性随着时间延长继续升高,至注射后14 d,1 mg.kg-1处理组鲫鱼肝脏EROD活性为对照的3.0倍(P<0.001),而100 mg.kg-1处理组则高达5.8倍(P<0.001)。鲫鱼肝脏EROD活性可作为反映BaP暴露水平的生物标志物。BaP对鲫鱼的最低效应浓度为1 mg.kg-1(鱼体重)。     

苯并[a]芘对小鼠肝脏和肾脏中丙二醛和过氧化氢酶的影响

目的探讨苯并[a]芘（B（a）P）对小鼠肝脏和肾脏脂质过氧化及抗氧化能力的影响。方法采用B（a）P口腔灌胃连续染毒3 d后,取肝、肾组织作匀浆,采用TBA比色法测定鼠肝脏和肾脏内的丙二醛（MDA）的含量,钼酸铵比色法测定鼠肝脏和肾脏内的过氧化氢酶（CAT）的含量。结果肝中各剂量染毒组的MDA含量增加,其中5 mg/kg、10 mg/kg剂量组与油剂对照组比较差异有显著性（P〈0.05）。肾脏中各剂量染毒组的MDA含量均有所增加,其中10 mg/kg剂量组与对照组比较差异有显著性（P〈0.05）。肝脏中各剂量染毒组的CAT的含量低剂量增加高剂量减少,肾脏中各剂量染毒组的CAT的含量增加。结论B（a）P可引起MDA含量增加诱导小鼠肝肾的脂质过氧化损伤。     

污染土壤中苯并(a)芘的微生物降解途径研究进展

苯并(a)芘(BaP)是一种具有强致癌、致畸和致突变的多环芳烃(PAHs)。为了修复BaP污染的土壤,探索其降解途径是很重要的。为此,综述了国内外有关污染土壤中苯并(a)芘的微生物降解情况,对不同真菌、细菌降解苯并(a)芘的能力、代谢途径、共代谢底物以及环境影响因素进行了介绍和比较,提出了苯并(a)芘中间代谢产物的累积及其环境毒性方面的研究是修复苯并(a)芘污染土壤的重要方向。     

苯并[a]芘暴露对三疣梭子蟹鳃、肝胰腺组织毒理学指标的影响

本文研究了三疣梭子蟹(Portunus trituberculatus)在对苯并[a]芘(BaP)富集(15 d)、释放(15d)过程中其鳃和肝胰腺组织的4种毒理学指标的响应.4种毒理学指标分别为7-乙氧基异吩噁唑酮-脱乙基酶(EROD)、谷胱甘肽硫转移酶(GST)、超氧化物歧化酶(SOD)和脂质过氧化(LPO).设置了0.05 μg/L和0.45 μg/L两个实验组以及海水和丙酮对照组.结果显示,在富集阶段,与海水对照组相比,第1天时0.05 μg/L和0.45μg/L实验组鳃、肝胰腺组织的各毒理指标均显著受到诱导(P＜0.05),诱导程度随BaP暴露浓度的增加而增大.而后鳃、肝胰腺组织的EROD、GST活性以及鳃组织的SOD活性达到峰值后下降,肝胰腺组织的SOD活性以及鳃、肝胰腺组织的丙二醛(MDA)含量则持续增加.鳃组织的EROD、GST、SOD活性到达峰值时间早于肝胰腺组织,其活性以及MDA含量也低于肝胰腺组织.在释放阶段,0.45pg/L实验组鳃组织的SOD活性,0.05μ-g/L和0.45 μg/L两个实验组肝胰腺组织的SOD活性均依然显著高于同期海水对照组水平(P＜0.05),其余各浓度实验组鳃、肝胰腺组织均能恢复到同期海水对照组水平(P＞ 0.05).实验结果表明,三疣梭子蟹的鳃组织对于BaP暴露响应时间比肝胰腺组织更早,但均具有一定的恢复能力.     

Modulation of aortic protein phosphorylation by benzo(a)pyrene: Implications in PAH-induced atherogenesis

The toxicity of polycyclic aromatic hydrocarbons such as benzo(a)pyrene, 7,12-dimethylbenz(a)anthracene, and 3-methylcholanthrene has been associated with alterations in the proliferation of vascular smooth muscle cells and the development of lesions of mesenchymal origin. Because phosphorylation of endogenous substrates plays a central role in the regulation of smooth muscle cell growth, the present studies were conducted to evaluate the phosphorylation pattern of medial aortic protein upon repeated in vivo exposure of Japanese quail to benzo(a)pyrene (BaP). Medial aortic homogenates from quail treated for 10 weeks with 10 mg/kg benzo(a)pyrene or vehicle were processed for in vitro measurements of protein phosphorylation. In vitro phosphorylation of endogenous or exogenous proteins stimulated in vitro by phorbol myristate acetate/phosphatidyl-serine or cyclic AMP, known activators of protein kinase C and cyclic AMP-dependent protein kinase, respectively, was examined in the cytosolic and particulate fractions of homogenates from control and treated animals. Benzo(a)pyrene treatment significantly enhanced the basal phosphorylation of Mr 113, 35, and 23 kDa proteins in the cytosolic fraction. Modest increases in the phosphorylation of Mr 71, 52, and 38 kDa were also observed under basal conditions. No changes in the basal phosphorylation of particulate proteins were observed. Phosphorylation of endogenous protein substrates by protein kinase C in the cytosolic fraction was not altered by benzo(a)pyrene treatment. In contrast, inhibition of C-kinase-mediated phosphorylation of endogenous Mr 272, 72, and 45 kDa proteins was observed in the particulate fraction of aortic homogenates from benzo(a)pyrene-treated quail relative to controls. Exogenous histone phosphorylation by PKC in the particulate, but not cytosolic fraction, was decreased by benzo(a)pyrene treatment. The effects of benzo(a)pyrene on the C-kinase system were specific, since cAMP-mediated phosphorylation of endogenous proteins, as well as exogenous histone, was not altered by benzo(a)pyrene. Interestingly, benzo(a)pyrene treatment was associated with a selective increase of Mr 200, 80, and 67 kDa proteins in the cytosolic fraction. Collectively, these data are consistent with the hypothesis that medial protein phosphorylation is a significant molecular target of benzo(a)pyrene within the vascular wall.     

Differential Alterations in Metabolic Pattern of the Spliceosomal UsnRNAs during Pre-Malignant Lung Lesions Induced by Benzo(a)pyrene: Modulation by Tea Polyphenols

The differential alterations of the spliceosomal UsnRNAs (U1, U2, U4, U5, and U6) were reported to be associated with cellular proliferation and development. The attempt was made in this study to analyze the metabolic pattern of the spliceosomal UsnRNAs during the development of pre-malignant lung lesions induced in experimental mice model system by benzo(a)pyrene (BP) and also to see how tea polyphenols, epigallocatechin gallate (EGCG) and epicatechin gallate (ECG), modulate the metabolism of these UsnRNAs during the lung carcinogenesis. No significant changes in the level of the UsnRNAs were seen in the inflammatory lung lesions at 9th week due to treatment of BP. However, there was significant increase in the level of U1 (∼2.5 fold) and U5 (∼47%) in the hyperplastic lung lesions at 17th week. But in the mild dysplastic lung lesions at 26th week, the level of UsnRNAs did not change significantly. Whereas, in the dysplastic lung lesions at 36th week there was significant increase in the level of the U2 (∼2 fold), U4 (∼2.5 fold) and U5 (∼2 fold). Due to the EGCG and ECG treatment the lung lesions at 9th week appeared normal and in the 17th, 26th, and 36th week it appeared as hyperplasia. The level of the UsnRNAs was significantly low in the lung lesions at 9th week (only U2 and U4 by EGCG), at 17th week (only U1 by EGCG/ECG), at 26th week (U1 by ECG; U2, U4 and U5 by EGCG/ECG) and at 36th week (U1 by ECG, U2 and U4 by EGCG/ECG). Whereas, there was significant increase in the level of U5 (by EGCG/ECG) and U6 (by EGCG only) in the lung lesions at 36th and 26th week respectively. This indicates that the metabolism of the spliceosomal UsnRNAs differentially altered during the development of pre-malignant lung lesions by BP as well as during the modulation of the lung lesions by the tea polyphenols.     

用EROD研究苯并芘和六氯苯的联合毒性作用

用7-乙氧基异叻唑酮-脱乙基酶(EROD)检测的方法,研究了苯并芘和六氯苯对日本青鳉肝脏EROD酶的比活力的影响。结果表明,苯并芘和六氯苯对EROD酶的比活力均有激活作用,在实验浓度范围内,EROD酶的比活力与两者浓度之间存在剂量-效应关系。苯并芘和六氯苯表现为一定的协同作用。实验同时发现日本青鳉在六氯苯和苯并芘中暴露后,EROD酶的比活力开始有一个短暂的降低,然后持续升高。对六氯苯和苯并芘暴露的最佳时间进行了探讨。     

苯并（a）芘对大弹涂鱼肝脏过氧化氢酶活性的影响

过氧化氢酶 (ＣＡＴ)是生物体内一种含巯基 ( -ＳＨ)的抗氧化酶 ,可与谷胱甘肽过氧化物酶一起 ,清除超氧化物歧化酶歧化超氧阴离子自由基(Ｏ2 - )产生的过氧化氢 (Ｈ2 Ｏ2 ) ,进而阻断可产生活性极高的羟自由基 (ＯＨ)的Ｈａｂｅｒ Ｗｅｉｓｓ反应 :Ｍ Ｏ2 - Ｈ2 Ｏ2 →Ｍ2 ＯＨ ＯＨ Ｏ2 (Ｍ 为金属离子 ) ,因而在生物体的抗氧化防御系统中占有重要地位[1 2 ] 。研究表明 ,包括ＣＡＴ在内的抗氧化防御系统的成分可由于氧化污染的胁迫而发生改变 ,尝试以这些抗氧化防御系统成分的变化作为氧化胁迫的生物指标的研究正在成为毒理学研究的…     

Culture of adult rat lung cells: Benzo(a)pyrene metabolism and mutagenesis

Summary A method is described for obtaining and culturing large numbers of lung cells from normal adult male rats. The lungs were perfused in situ to remove blood cells and then perfused via the trachea with a trypsin-collagenase solution to initiate tissue digestion. The tissue was further digested in the enzyme solution and approximately 2×10⁸ viable lung cells were obtained per animal. Primary cultures contained a mixed cell population. Through eight subcultures about 70% of the cell population possessed an epithelial-like morphology, whereas the remaining 30% was fibroblast-like. Three clones of epithelial-like cells were isolated at the fourth subculture. The mass culture lung cells and the epithelial-like clone that was studied retained a normal karyotype and did not grow in soft agar. Both the mass culture cells and the epithelial clone metabolized the lung carcinogen benzo(a)pyrene (BP) to water-soluble products. Furthermore, the mass culture lung cells metabolized BP to intermediate(s) which mutated Chinese hamster V79 cells from ouabain sensitivity to ouabain resistance. These lung cell cultures have potential use in cell transformation, mutation and carcinogen metabolism studies. Visiting scientist from Hungary. This research was supported by Grant 5 R01 CA20022 and Public Health Service Contract N01 CP33278 from the Division of Cancer Cause and Prevention, National Cancer Institute, National Institutes of Health.     

城市污泥和土壤中苯并（a）芘的初步研究

应用GC／MS技术对我国11个城市污泥和4种土壤中的苯并（a)芘进行研究,探讨苯并（a)芘在城市污泥和土壤中的含量和分布特征,结果表明,城市污泥中苯并（a)芘的含量在0．007－0．578mg.kg^-1之间,平均为1．272mg/kg^-1,绝大部分低于1．0mg/kg^-1,但在珠海和北京污泥中超过我国农用污泥的控制标准,褐土,水稻土和石灰性土中苯并（a)芘的含量分别为2．138,0．782和0．664mg.kg^-1,在赤红壤中未检出,城市污泥中苏并（a)芘含量与污水来源,污水处理方式和污泥类型等因素有关,土壤中苯并（a)芘含量与母质,大气污染,污水灌溉,污泥农用等因素有关。     

熏烤肉制品中苯并芘的危害及控制措施

本文从食品安全的角度出发,对熏烤肉制品中的有害物质苯并(a)芘的产生,对人体的危害作用,以及控制熏烤肉制品中苯并(a)芘残留的方法进行了初步的研究.这对提高熏烤肉制品品质和对苯并(a)芘进行深入的研究具有重要意义.     

Ubiquitin Protein Ligase Ring2 Is Involved in S‐phase Checkpoint and DNA Damage in Cells Exposed to Benzo[a]pyrene

Previous studies in our laboratory demonstrated that Ring2 may affect DNA damage and repair through pathways other than through regulating the expression of the nucleotide excision repair protein. In a series of experiments using wild‐type cell (16HBE and WI38) and small interfering RNA (siRNA) Ring2 cells exposed to benzo[a]pyrene (BaP), we evaluated the cell cycle and DNA damage. The benzo(a)pyrene‐7,8‐dihydrodiol‐9,10‐epoxide (BPDE–DNA) adduct assay demonstrated that in vitro exposure to BaP increased DNA damage in a time‐ and dose‐dependent manner in wild‐type and siRNA Ring2 cells. Analysis of covariance showed that a decrease of Ring2 caused DNA hypersensitivity to BaP. Flow cytometry results and proliferating cell nuclear antigen levels indicated that inhibition of Ring2 attenuated the effect of BaP on S‐phase arrest. Taken together, these data implied that the lower proportion of cells in the S phase induced by inhibition of Ring2 may play an important role in DNA hypersensitivity to BaP.