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11.
1IntroductionCadmiumisoneofimportantenvironmentalpolutants.Itisverytoxictobiology(Barber,1994;Colard,1990;Goyer,1995;Nassiri,...  相似文献   
12.
氯代芳香化合物的微生物降解研究   总被引:2,自引:0,他引:2  
生物技术对消除有毒化学品已显示出广阔的应用前景,深入研究有毒化学品微生物降解的生物化学和遗传学,可按照预期目的构建具有更大降解能力的遗传工程菌株,以促使污染物的无害化资源化。本文对纯菌株降解氯代芳香化合物的降解途径、降解性质粒和遗传工程菌株的构建等诸方面进行了综述。  相似文献   
13.
水环境中耐热大肠菌群的抗生素耐药性与质粒谱研究   总被引:5,自引:0,他引:5  
用滤膜法、mFC培养基从5种水体中分离出疑似耐热大肠菌162株,用API微生物分析系统鉴定到种,以Kirby-Bauer法分析其对人畜常用10种抗生素的耐药性,碱裂解法小量制备各菌株质粒DNA做质粒谱分析.结果表明,埃希氏大肠杆菌为优势菌,占分离菌总数的96.3%.除分离自泉水的3株外,其它菌株都对3种及3种以上抗生素耐药,多重耐药率为98.1%.不同水体分离菌株对氧氟沙星、诺氟沙星、庆大霉素、丁胺卡那霉素、链霉素的耐药率有显著性差异(P<0.005).92株菌(56.8%)提取到大小为0.90~158.83kb、数量为1~6个的质粒,有81种质粒谱型.70株(43.2%)未提取到质粒的细菌中有67株为多重耐药.具有相同质粒谱型的菌株耐药谱都不相同.未发现质粒谱与抗生素耐药性间有明显相关性.图1表3参15  相似文献   
14.
The present study was undertaken with the objective of studying repeated batch and continuous degradation of chlorpyrifos (O,O-diethyl O-3,5,6-trichloropyridin-2-yl phosphorothioate) using Ca-alginate immobilized cells of Pseudomonas putida isolated from an agricultural soil, and to study the genes and enzymes involved in degradation. The study was carried out to reduce the toxicity of chlorpyrifos by degrading it to less toxic metabolites. Long-term stability of pesticide degradation was studied during repeated batch degradation of chlorpyrifos, which was carried out over a period of 50 days. Immobilized cells were able to show 65% degradation of chlorpyrifos at the end of the 50th cycle with a cell leakage of 112 × 103 cfu mL?1. During continuous treatment, 100% degradation was observed at 100 mL h?1 flow rate with 2% chlorpyrifos, and with 10% concentration of chlorpyrifos 98% and 80% degradation was recorded at 20 mL h?1 and 100 mL h?1 flow rate respectively. The products of degradation detected by liquid chromatography–mass spectrometry analysis were 3,5,6-trichloro-2-pyridinol and chlorpyrifos oxon. Plasmid curing experiments with ethidium bromide indicated that genes responsible for the degradation of chlorpyrifos are present on the chromosome and not on the plasmid. The results of Polymerase chain reaction indicate that a ~890-bp product expected for mpd gene was present in Ps. putida. Enzymatic degradation studies indicated that the enzymes involved in the degradation of chlorpyrifos are membrane-bound. The study indicates that immobilized cells of Ps. putida have the potential to be used in bioremediation of water contaminated with chlorpyrifos.  相似文献   
15.
为了探讨吡啶降解菌质粒的特性及其与降解的关系,对降解吡啶的2株细菌Paracoccus sp.BW001及Shinellazoogloeoides BC026进行了质粒提取和脉冲电泳实验,确定BW001含有2个190~245kb的大质粒和1个4.5~5.0kb的小质粒,而BC026含有至少3个超过200kb的大质粒.通过高温-SDS法对含有质粒的2株菌进行质粒消除实验,发现质粒消除后的细菌不再降解吡啶,推测降解吡啶的基因可能存在于质粒上.通过电转化将Paracoccus sp.BW001的质粒转入E.coli5α中,发现转化后的菌株具有耐受吡啶的特性.  相似文献   
16.
萘降解质粒pND6的分离和鉴定   总被引:1,自引:1,他引:0  
从工业废水中分离的假单胞菌 (Pseudomonassp .)ND6菌株 ,能以萘为唯一碳源生长 ,使无机盐培养基(MM)中 2g/L的萘在 48h内降解 98% .该菌株含有一个 115kb的大质粒pND6 .DNA杂交实验表明 ,pND6质粒含有与恶臭假单胞菌 (P .putida)G7菌株的NAH7质粒同源的萘降解基因 .图 3表 1参 14  相似文献   
17.
Polymerase chain reaction(PCR)was used to amplify a 600-base pair(bp)sequence of plasmid pGEX-2T DNA bound on soil colloidal particles from Brown soil(Alfisol)and Red soil(Ultisol),and three different minerals(goethite,kaolinite,montmorillonite). DNA bound on soil colloids,kaolinite,and montmorillonite was not amplified when the complexes were used directly but amplification occurred when the soil colloid or kaolinite-DNA complex was diluted,10- and 20-fold.The montmorillonite-DNA complex required at least 100-fold dilution before amplification could be detected.DNA bound on goethile was amplified irrespective of whether the complex was used directly,or diluted 10- and 20-fold.The amplification of mineral-bound plasmid DNA by PCR is,therefore,markedly influenced by the type and concentration of minerals used.This information is of fundamental importance to soil molecular microbial ecology with particular reference to monitoring the fate of genetically engineered microorganisms and their recombinant DNA in soil environments.  相似文献   
18.
The genetic information encoding metabolic pathways for xenobiotic compounds in bacteria often resides on catabolic plasmids. The aim of the present work was to know the location of the genes for degrading 1,2,4-trichlorobenzen. In this paper a 1,2,4-trichlorobenzene-degrading strain THSL-1 was isolated from the soil of Tianjin Chemical Plant using 1,2,4-trichlorobenzene as the sole carbon source. The strain was identified as Pseudomonas stutzeri through morphologic survey and 16S rDNA sequence determination. A plasmid was discovered from strain THSL-1 by using the alkali lysis method. When the plasmid was transformed into E. coli. JM109 by the CaCl2 method, the transformant could grow using 1,2,4-trichlorobenzene as the sole carbon source and had the degradation function of 1,2,4-trichlorobenzene. Therefore, it could be deemed that the plasmid carried the degradative genes of 1,2,4-trichlorobenzene. The average size of the plasmid was finally determined to be 40.2 Kb using selectively three kinds of restricted inscribed enzymes (HindIII, BamHI, and XholI) for single cutting and double cutting the plasmid pTHSL-1, respectively. __________ Translated from China Environmental Science, 2005, 25(4): 385–388 [译自: 中国环境科学]  相似文献   
19.
废弃重组质粒DNA热处理效率的环境影响因素   总被引:1,自引:1,他引:0  
为了解环境因素对质粒DNA热处理效率的影响以及热处理过程的有效性和安全性,以pET-28b质粒为材料,采用定量PCR技术结合质粒转化等方法分析了pH、NaCl、牛血清白蛋白(BSA)及EDTA浓度等因素对质粒DNA热处理的影响.结果表明,NaCl、BSA及EDTA的存在对热处理过程中的质粒DNA具有保护作用,且保护作用依次增强.在纯水中热处理30min后的质粒DNA可扩增的片段数仅是在0.1%的EDTA中热处理30min后质粒DNA可扩增片段数目的1.7%.由于生物实验室废水中通常含有上述有机或无机物质,因此,实际热处理过程中质粒DNA的降解半衰期可能远长于先前报道的2.7~4min,残留的转化活性也可能更高,这必须引起我们高度关注.但是,研究结果也表明,酸性条件下的热处理能加速质粒DNA的失活和降解,因此建议热处理过程可在弱酸性条件下完成,以强化其处理效果.  相似文献   
20.
从实验室的废水生物处理反应器内的活性污泥样本,筛选出来一株以吡啶为唯一碳、氮源的脱氮副球菌(Paracoccus denitrificans),命名为W12;研究了温度、pH值、吡啶初始浓度和投菌量对W12降解吡啶的影响.结果显示,在试验温度范围内高温有利于W12降解吡啶;同时W12降解吡啶的最适pH值范围在7-9;吡啶初始浓度越大降解时间越长,且投菌量越大吡啶降解越快.此外还研究了W12菌上赋存的质粒特性.脉冲场试验表明,W12菌上2个质粒的大小分别为169 kb和182 kb,并通过质粒消除试验证实了质粒参与了编码吡啶降解基因.  相似文献   
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