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511.
硝基甲苯对小鼠睾丸生殖细胞DNA的损伤作用   总被引:1,自引:1,他引:0  
为提供硝基甲苯的环境遗传毒理学依据和建立鱼类生殖细胞的培养方法,采用昆明小鼠睾丸支持细胞/生殖细胞共培养法以及彗星实验,研究了2,4-二硝基甲苯(2,4-DNT)、2,6-二硝基甲苯(2,6-DNT)、对硝基甲苯(4-NT)对小鼠睾丸生殖细胞DNA的损伤作用.结果表明,3种受试硝基甲苯化合物均能够诱导小鼠睾丸生殖细胞DNA单链断裂,而且其受损率与剂量对数具有明显的剂量-效应关系.2,4-DNT、2,6-DNT以及4-NT的各个剂量浓度引起细胞DNA损伤的程度,与对照组相比,均具有显着性差异(p<0.01,p<0.05).受试化合物的毒性顺序为2,6-DNT>2,4-DNT>4-NT,DNA的损伤作用二硝基甲苯大于单硝基甲苯.提示在体外条件下,2,4-DNT、2,6-DNT和4-NT具有生殖毒性,可以引起小鼠睾丸生殖细胞DNA损伤.  相似文献   
512.
硫丹对草鱼Ⅰ相、Ⅱ相酶活性及DNA损伤的影响   总被引:2,自引:0,他引:2  
研究了硫丹对草鱼肝脏Ⅰ相酶氨基比林-N-脱甲基酶(APND)和红霉素-N-脱甲基酶(ERND)、Ⅱ相酶谷胱甘肽-S-转移酶(GST)活性及DNA受损细胞彗星尾长(TL)和尾部DNA含量(%TDNA)的影响。试验共设置0.18、0.36和0.71μg.L-1 3个暴露浓度组和1个空白对照组,分别在试验24、72、120和168 h时取样测定各指标。结果表明,24 h时,0.36和0.71μg.L-1暴露组草鱼肝脏APND活性与对照组相比显著升高(P〈0.05或P〈0.01),72 h时受到显著抑制(P〈0.01);120 h后各暴露组APND活性与对照组相比均表现为受到显著抑制(P〈0.05或P〈0.01)。ERND活性总体表现为受诱导。GST活性总体呈先受诱导后受抑制的变化趋势;0.36和0.71μg.L-1暴露组GST活性均在72 h时达到最高值,之后随暴露时间的延长缓慢降低,并在168 h时表现为受抑制;0.18μg.L-1暴露组在120 h时达到最大值,之后降低,168 h时GST活性与对照组水平相当。经硫丹暴露后,草鱼肝脏细胞DNA明显受损,TL与%TDNA均随硫丹浓度的升高或暴露时间的延长而增加,且相关显著。硫丹可影响草鱼肝脏Ⅰ相、Ⅱ相代谢酶活性,并对肝细胞DNA造成遗传损伤。  相似文献   
513.
Increased education of consumers can be an effective tool for conservation of commercially harvested marine species when product labeling is accurate and allows an informed choice. However, generic labeling (e.g., as white fish or surimi) and mislabeling of seafood prevents this and may erode consumer confidence in seafood product labels in general. We used DNA barcoding to identify the species composition of two types of convenience seafood (i.e., products processed for ease of consumption): fish fingers (long pieces of fish covered with bread crumbs or batter, n = 241) and seafood sticks (long pieces of cooked fish, n = 30). In products labeled as either white fish or surimi, four teleost species were present. Less than 1.5% of fish fingers with species-specific information were mislabeled. Results of other studies show substantially more mislabeling (e.g., >25%) of teleost products, which likely reflects the lower economic gains associated with mislabeling of convenience seafood compared with whole fillets. In addition to species identification, seafood product labels should be required to contain information about, for example, harvesting practices, and our data indicate that consumers can have reasonable confidence in the accuracy of the labels of convenience seafood and thus select brands on the basis of information about current fisheries practice.  相似文献   
514.
PFOA对斑马鱼胚胎发育、行为和DNA损伤的毒性研究   总被引:1,自引:0,他引:1  
全氟辛酸(PFOA)是一种分布广泛的环境持久性有机污染物,在野生动物与人体内普遍被检出。目前PFOA发育毒性的特点和机制尚未阐明,已有的研究显示,PFOA毒性与受试物种及性别密切相关。因此,利用不同物种进行PFOA毒性研究对阐明其毒性机制十分重要。本研究选用了斑马鱼这种理想的脊椎动物模型,考察了PFOA暴露对其胚胎发育的自主运动、心跳、行为、细胞凋亡和DNA损伤的影响。研究发现,始于6hpf的PFOA暴露会导致斑马鱼胚胎自主运动异常,心率降低,且具有一定的剂量依赖性;6~24hpf的高浓度的PFOA暴露(>414.0mg·L-1)会导致胚胎发生显著的细胞凋亡,凋亡主要出现在眼部、头部、心脏和尾部。较高浓度的PFOA暴露(165.6mg·L-1)会使仔鱼的光刺激应激行为模式发生变化。此外,PFOA暴露会致使斑马鱼发生DNA损伤,且损伤程度随PFOA浓度的升高而加重,表明PFOA具有一定的基因毒性。上述结果表明,PFOA对斑马鱼胚胎具有发育毒性,具体表现为自主运动异常,心率降低和行为反应能力变弱,同时伴随畸形、细胞凋亡和DNA损伤。  相似文献   
515.
为探讨41%草甘膦水溶液(农达)对雄性生殖细胞的毒性及其作用机制以及N-乙酰半胱氨酸(N-acetylcysteine, NAC)的干预效应。以GC-1小鼠精原细胞为受试细胞,设正常对照组、草甘膦染毒组(60、90、120、150、180 mg·L-1)、NAC干预组(10 mmol·L-1 NAC+90 mg·L-1农达)。MTT法检测细胞存活率,Giemsa染色法观察细胞的形态学改变,彗星试验检测细胞DNA损伤,比色法检测细胞培养液乳酸脱氢酶(LDH)以及细胞内超氧化物歧化酶(SOD)、谷胱甘肽(GSH)及丙二醛(MDA)水平的变化。结果显示,随着草甘膦染毒浓度增加,细胞存活率逐渐下降(p<0.01),彗星阳性率逐渐升高(p<0.01);与对照组相比,草甘膦染毒组LDH活性增加(p<0.05,60 mg·L-1组除外),MDA生成量增多(p<0.05),GSH含量降低(p<0.05)和SOD活性降低(p<0.05)。抗氧化剂NAC预处理具有相应的拮抗作用。研究表明,60~180 mg·L-1浓度草甘膦对GC-1细胞有明显的损伤作用,其机制可能是草甘膦诱导氧化应激,导致细胞通透性增加和DNA损伤。抗氧化剂NAC对草甘膦的细胞毒性具有一定保护作用。  相似文献   
516.
为探讨敌百虫致DNA-蛋白质交联作用,以昆明小鼠为受试动物,敌百虫按0、20、40、60 mg·kg-1四个剂量水平,灌胃染毒小鼠两周。第五组以提取的正常小鼠外周血淋巴细胞经50 μmol·L-1的H2O2处理为阳性对照组。采用经改进的彗星试验方法来检测染毒后外周血淋巴细胞DNA-蛋白质交联效应。结果表明,与空白组相比,各敌百虫染毒组都能引起DNA损伤作用(p<0.01)并引起一定程度的DNA-蛋白质交联效应,在较高浓度(40、60 mg·kg-1)时DNA-蛋白质交联尤为明显,存在一定的潜在突变风险。  相似文献   
517.
Following enrichment in its presence, two strains of bacteria, isolated from marine sediments, were shown to degrade the quaternary ammonium surfactant benzyldimethyl hexadecylammonium chloride (BDHAC) in a minimal salts medium. The bacteria identified by 16S ribosomal deoxyribonucleic acid sequencing were shown to belong to several genera and determined to be Bacillus niabensis and Thalassospira sp. Initial investigations demonstrated that the bacteria were capable of degrading BDHAC when it was present at concentrations in the range 2–4 mg mL?1. In media containing BDHAC, up to 90% was degraded within 7 days, but limited growth of the strain was observed at 2 and 4 mg mL?1 BDHAC. Preliminary analysis of samples after degradation experiment by electrospray ionization mass spectrometry/mass spectrometry produced a peak with a parent–daughter ion transition of 136 → 91, corresponding to N,N-dimethylbenzylamine. The presence of this potential metabolite suggests the cleavage of the C-alkyl-N bond as a step in BDHAC catabolism.  相似文献   
518.
Microcystins (MCYST) are the freshwater cyanobacterial toxins, known to induce hepatocellular carcinoma, necrosis, intrahepatic bleeding, as well as human and livestock mortality. Within hepatocytes, MCYST selectively bind to protein phosphatases 1 and 2A, resulting in severe liver damage. The toxicology of MCYST in mice and rats has been well studied, but little is known regarding genotoxicity in aquatic animals. In this study, the zebrafish, Danio rerio was exposed to crude extract of Microcystis aeruginosa bloom. Liver and heart were examined for MCYST-induced toxicity. Light microscopy at 36?h revealed severe, widespread apoptotic necrosis of the majority of hepatocytes, and cytoskeletal deformation in myocardiocytes. Hepatocytes were dissociated with cell shrinkage and margination of nuclear chromatin. Laddering of genomic DNA from the liver and heart of the exposed fish in an increment of 180–200?bp was consistent with apoptosis. Fluorimetric analysis of DNA unwinding was carried out to determine the DNA strand breakage. After 36?h exposure, the % double-stranded DNA was significantly reduced in hepatocytes and myocardiocytes. In conclusion, the results obtained in this study indicate that, the extract of M. aeruginosa bloom is genotoxic to fish. The DNA damage observed in this study may be attributed to the activation of DNA endonucleases. This model of DNA damage may contribute for identifying novel molecular mechanisms of interest for therapeutic application.  相似文献   
519.
The use of aquatic organisms to monitor for contamination is well-established. Therefore, this study was designed to assess the adverse effects of titanium dioxide nanoparticles (TiO2NP) in freshwater snail Lymnea luteola L. (L. luteola). For TiO2NPs ecotoxicity tests, snails were exposed for seven days. A dose and time-response relationship was observed for TiO2NP-induced genotoxicity. Induction of oxidative stress in digestive gland was observed by a decrease in glutathione and gluthathions-S-transferase levels accompanied by elevated malondialdehyde levels at TiO2NP (9 and 28 µg/mL). Superoxide dismutase activities were markedly reduced at TiO2NP (9 and 28 µg/mL) at days 1 and 3, but not at day 7. Catalase activities were decreased at days 1 and 3 but increased at higher concentration of TiO2NP at day 7. DNA fragmentation occurring in L. luteola due to ecotoxic impact TiO2NP was further substantiated by alkaline single-cell gel electrophoresis assay and expressed in terms of percent tail DNA and olive tail moment. The results indicate that the interaction of these TiO2NP with snail influences the toxicity, which is mediated by oxidative stress in a dose- and time-dependent manner. The measurement of DNA integrity in L. luteola thus provides an early warning signal of contamination of the aquatic ecosystem by TiO2NP. Data suggest the freshwater snail L. luteola is a potential biomonitor organism.  相似文献   
520.
  1. No binding of chromium was detected after incubation of calf thymus nuclei with hexavalent chromium up to 0.5 mM.

  2. Chromium was readily taken up and tightly bound after incubation with trivalent chromium.

  3. In a DNA‐filter binding assay, increasing amounts of chromium and DNA were bound with increasing chromium trichloride concentrations incubated with the nuclei.

  4. Treatment with proteinase K abolished the increase in DNA retention induced by trivalent chromium.

  5. It is concluded that trivalent chromium is the ultimate genetoxic agent after chromate uptake by living cells.

  相似文献   
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