活性炭吸附-介质阻挡放电等离子体处理五氯酚

研究了介质阻挡放电(DBD)与活性炭(AC)吸附相结合用于高浓度五氯酚(PCP)废水的处理.含有高浓度的PCP溶液被富集在AC上,通过DBD等离子体降解吸附在AC上的PCP,并且实现AC的循环再利用.主要考察了DBD等离子体作用条件下AC上PCP的降解效果以及3次循环处理后AC吸附等温线的变化.结果表明:随着放电电压和处理时间的增加,AC上PCP的降解效率增加,较高的电源频率有助于PCP的降解,而且经过3次吸附/处理循环后,AC仍然具有较高的吸附能力.     

不同基质体系中白腐茵对喹啉和吲哚的降解

用单基质及混合基质体系,探讨了白腐菌Pleurotus ostreatus BP对氮杂环化合物的降解规律.结果表明,在弱酸性环境下,白腐菌能有效降解喹啉和吲哚.单摹质体系中,喹啉的降解率15 d内能达到89.48%,98.17%的吲哚6 d内被降解;混合基质体系中,基质(喹啉、吡啶、苯酚及氨氮)的加入能促进白腐菌对吲哚的降解,但(吲哚、吡啶、苯酚及氨氮)却抑制了白腐菌对喹啉的降解.不同基质体系中,白腐菌对喹啉和吲哚的降解分别遵循零级和一级反应动力学.相对单基质而言,混合基质的存在对白腐菌生物学特性产生明显影响,可缩短生长周期,提高生长速率和漆酶活性.漆酶在吲哚的降解中起着重要的作用,但不能完全决定喹啉的降解.     

DLL-1菌对甲基对硫磷农药的降解作用及其降解机理

研究了假单胞菌 (DLL - 1)在水溶液介质中降解甲基对硫磷的性能与影响因素及其降解机理。结果表明 ,当菌体浓度为 10 5个·ml-1时 ,即发生快速的降解作用 ,3h时 ,降解率达 88.5 %。在pH为 5 .0、7.0和 9.0条件下 ,DLL - 1菌均产生对甲基对硫磷农药的高效降解作用。采用气相色谱 -质谱联用技术与离子色谱法 ,测定了DLL - 1菌 -甲基对硫磷作用过程产生的中间产物和最终产物 ,表明对硝基苯酚为主要中间产物 ,且DLL - 1菌能将其进一步降解为NO2 -和NO3 -。     

白腐菌对3种含氯二(噁)(口英)类物质的降解作用

探讨了白腐菌射脉侧菌Phlebia radiateI-5-6对3种含氯量不同的二类物质———二苯并呋喃(DF)、2,7-二氯二苯并二(2,7-diCDD)和八氯二苯并呋喃(OCDF)的降解情况,并研究了不同培养条件对二降解的影响.在液体混合培养基中,在培养期内P.radiataI-5-6对3种二类物质的降解量分别为:DF>2,7-diCDD>OCDF;在培养的初始阶段,白腐菌对珠江江水/CEH漂白废水的加入需要一个适应期,然后开始降解这些污染物质.实验表明,在江水/CEH漂白废水处于一定浓度时,污染底物有更大的降解量;选择适当的培养基,可影响白腐菌对二类污染物的降解量.图3表3参17     

多环芳烃降解菌的获得及应用

运用双相(水-硅油)系统可进行有机物降解菌的筛选．本实验用此法获得了多环芳烃(PAHs)的降解菌，降解菌对PAHs有较好的降解作用．堆肥法处理PAHs中接入筛选到的降解菌可以大大加强降解效果．堆肥过程中堆温升高很快，对一些PAHs如荧蒽、芘、苯并[a]芘等可以彻底清除，对更多环的PAHs也可降到很低的浓度．图1表3参4     

白腐真菌降解五氯酚的初步研究

研究了白腐真菌黄孢原毛平革菌在不同营养条件下对五氯酚的降解.采用土豆葡萄糖液体培养基,接种后第2天投加PCP,在胞外木质素降解酶活性极低的真菌反应体系中,五氯酚能够有效降解,4d内10mg·1-1五氯酚降解率达到98%;采用高氮培养基,接种后第6天投加五氯酚,在胞外木质素酶含量极低的真菌反应体系和不含胞外酶的菌丝体反应体系中,五氯酚均能有效降解,1d内降解率分别达到56%和22%;采用低氮培养基,接种后第6天投加五氯酚,在胞外木质素酶含量较高的真菌反应体系、胞外酶液反应体系和不含胞外酶的菌丝体反应体系中,五氯酚均能有效降解,1d内降解率分别达到86%,17%和46%.结果表明,黄孢原毛平革菌在非木质素降解条件下,依赖胞内酶能有效地降解PCP;在木质素降解条件下依赖胞外木质素降解酶和胞内酶降解五氯酚,降解效率高于非木质素降解条件.     

白腐菌Trametes hirsute对六氯苯的降解及其条件优化

在液体体系下,筛选了5株白腐菌,对六氯苯进行了降解研究,并优化了白腐菌Trametes hirsute TH对六氯苯的降解条件.结果表明,不同白腐菌均能降解六氯苯,其中白腐菌Trametes sp.TR对六氯苯降解率最高,达90.21%;而白腐菌T.hirsute TH对六氯苯降解率为87.08%,但生物量最高,达3.33 g/L.通过响应面法优化白腐菌T.hirsute TH降解六氯苯的条件,结果显示,转速、接种量和培养时间是影响六氯苯降解的主要因素.优化后的最佳条件为:转速125 r/min,菌丝接种量8%(V/V),培养时间2 d,温度28 ℃,pH为7.在优化条件下,2 d内白腐菌T.hirsute TH对浓度为10 mg/L的六氯苯降解率和降解量分别可达91.52%和2.288 mg L-1 d-1.图2表7参17     

自然水体介质中白腐菌对二英类物质的降解

研究了自然水体介质中白腐菌射脉侧菌(Phlebia radiata)I-5-6对二英类物质2,7-二氯二苯并英(2,7-diCDD)和八氯二苯并呋喃(OCDF)的降解规律.结果显示,在自然河水为介质的培养环境中,2,7-diCDD随着江水加入量的递增,降解率逐步下降,但这种影响随着培养时间的延长而逐步减弱.白腐菌处理OCDF底物的效果并不理想,经过12d处理后,降解率最高只达到36.00%,这很可能是由于OCDF已经高度氧化,再要对它进行氧化降解比较困难.     

施氏假单胞菌N2代谢邻/间/对甲酚的特性研究

本论文以施氏假单胞菌N2为受试菌株,研究了N2菌对邻/间/对甲酚及其混合物的生物降解特性.结果表明,N2菌能以邻/间/对甲酚为唯一碳源和能源生长,但对3种异构体的降解速率各异.完全降解600 mg·L~(-1)的对甲酚仅需6 h,间甲酚则需24 h,但对邻甲酚的降解明显减缓;200 mg·L~(-1)邻甲酚48 h的降解率仅为11.38%.GC-MS结果分析发现,N2菌代谢甲酚途径主要为甲基氧化、芳环羟化,随后脱羧、开环裂解、降解转化至矿化,但3种甲酚的降解途径及酸性代谢产物的形成次序不一致.3种甲酚混合存在时可促进N2菌对其降解,这主要是因为混合碳源的协同作用减少了体系中因产酸过多引起的毒性,从而促进了N2菌对甲酚的降解矿化.     

磺胺类抗生素复合污染降解菌的筛选及其降毒作用

磺胺类抗生素是环境中检测出率较高的一类污染物.微生物降解是一种相对安全、高效且成本低的污染物去除技术,而关于磺胺类抗生素复合污染降解菌对该类抗生素的去除及其降毒能力方面的研究较少.因此,以3种磺胺类抗生素:磺胺吡啶(SP)、磺胺氯哒嗪(SCP)和磺胺二甲嘧啶(SM2)为碳源,从土壤中筛选3种磺胺类抗生素复合污染的降解菌,应用时间毒性微板分析法,测定3种抗生素及其复合污染物在降解前、后对指示生物蛋白核小球藻的毒性效应,并分析降解菌对3种抗生素及其复合物污染物的降毒能力.结果表明,以SP、SCP和SM2为碳源筛选出2株(S1和S2)降解菌,其中,S1菌株对3种抗生素的降解能力优于S2菌株,并初步鉴定S1降解菌为马氏棒杆菌属;S1降解菌的生长状况和降解能力最佳条件:3种抗生素的混合浓度为1 500 mg·L-1,pH=7.0,温度30℃,转速为150 r·min-1以及接种量为2.0％;S1菌株降解后的抗生素及其复合污染物对蛋白核小球藻的毒性明显低于降解前的毒性,降毒率在99％以上;S1降解菌对3种磺胺类抗生素的降解能力为SM2＞SP＞SCP.     

一株菲降解菌的特性及相关降解基因的克隆

从石油污染土壤中分离到一株菲降解菌2F5-2.根据该菌株生理生化特征和16S rDNA序列相似性分析,将其初步鉴定为鞘氨醇杆菌属(Sphingobium sp.).该菌株在10 h内对100 mg/L的菲的降解率为100%.降解菲的最适温度为30℃,最适pH为7.对降解途径的初步研究显示,该菌株通过水杨酸途径降解菲.克隆了编码芳香烃双加氧酶α亚基的基因phdA,它与菌株Sphingomonas sp.P2、Sphingobium yanoikuyae B1、Sphingomonas sp.ZP1中phdA的同源性分别为97.9%、98%和100%,表明该基因具有保守性.图6参16     

耐热石油烃降解混合菌的筛选及其群落结构分析

对克拉玛依采集的部分石油污染土壤进行了筛选,得到了5组石油烃高效降解混合菌,其中混合菌KL9-1在45℃的条件下,通过7 d的降解,稀油的降解率达到43.27%,稠油的降解率达到20.09%。混合菌KL9-1经过多次分离纯化后,获得3株具有石油烃降解能力的优势单菌,3株单菌对稀油的降解率都在30%以上。结合分离单菌株的形态、生理生化特征和16S rDNA基因序列的分析结果,初步鉴定KL9-1-1为Pseudomonas putida,KL9-1-2和KL9-1-3为Pseudomonas sp.。     

Biodegradation kinetics of cymoxanil in aquatic system

A potential method to detoxify pesticides in aquatic system is using bioremediation. In this study, four microorganisms (Pseudomonas sp (EB11), Streptomyces sp. (EB12), Aspergillus niger (EB13) and Trichoderma viride (EB14) were isolated from cucumber leaves previously treated with cymoxanil using enrichment technique. These strains were evaluated for their potential to detoxify cymoxanil in aquatic system at the concentration level of 5×10^?4M. The effect of pH and temperature on the growth ability of the tested strains was also investigated by measuring the intracellular protein and mycelia dry weight for bacterial and fungal strains, respectively. Moreover, the remaining toxicity of cymoxanil after 28 days of incubation with tested strains was evaluated to confirm the complete removal of any toxic materials (cymoxanil and its metabolites). The results showed that the optimum pH for the growth of cymoxanil degrading strains (bacteria and fungi) was 7. A temperature of 30°C appears to be the optimum for the growth of either fungal or bacterial strains. Pseudomonas sp. (EB11) was the most effective strain in cymoxanil degradation followed Streptomyces sp (EB12), Trichoderma viride (EB14) and Aspergillus niger (EB13), with half-lives of 4.33, 9.5, 17.3 and 24.7 days, respectively. The degradation of cymoxanil by bacterial strains was much faster than fungal one. There is no remaining toxicity of cymoxanil detected in aqueous media previously treated with Pseudomonas sp. (EB11) for 28 days. The results suggest that bioremediation by Pseudomonas sp. (EB11) are promising for the detoxification of cymoxanil in aqueous media.     

杀虫单降解菌的筛选分离与降解特性研究

从农药厂废水排放沟污泥中分离到一株对杀虫单有较强降解能力的菌株LY－4,经鉴定为巨大芽孢杆菌（Bacillus megaterium)。其生长的最适pH为7,最适温度为30℃。该菌对杀虫单有很强的耐受性,在杀虫单浓度ρ＝5000mg/L时,仍能较好地生长并发挥降解作用。当杀虫单初始浓度高于一定值时,一定量的菌剂对杀虫单的降解率随底物浓度的提高而降低,而绝对去除量则随底物浓度的提高而提高。与不加菌的对照相比,加入LY－4后,可使杀虫单浓度在很短的时间内降到很低的水平。图5表1参6     

Identification of two alkane hydroxylases involved in long-chain n-alkane degradation by Dietzia sp. DQ12-45-1b北大核心CSCD

The aim of this study was to identify genes involved in long-chain alkane degradation in Dietzia sp. DQ12-45-1b. Functional genes were annotated by genome analysis. Induction of alkane hydroxylase genes by C28 n-alkane was analyzed by using quantitative real-time PCR in wild-type Dietzia sp. DQ12-45-1b and its alkW1 gene knockout mutant strain M 5-5. From the genome of Dietzia sp. DQ12-45-1b, two homologues, G1 and G2 genes were annotated, which showed 50% amino acid sequence similarity with AlmA from Acinetobacter sp. DSM17874, and 48% amino acid sequence similarity with LadA from Geobacillus thermodenitrificans NG80-2, respectively. In addition, G1 showed 71% amino acid sequence similarity with G1a, and G2 showed 34% and 87% amino acid sequence similarities with G2a and G2ß, respectively, which were annotated from Dietzia sp. E1 genome. In addition, the alkW1 gene knockout strain M 5-5 could grow with C28 n-alkane as the sole carbon source, indicating the presence of potential long-chain alkane hydroxylase gene(s) other than alkW1 in Diezia sp. DQ12-45-1b. Accordingly, induction of G1 and G2 genes was observed when Dietzia ap. DQ12-45-1b and alkW1 knockout mutant strain M 5-5 grew with C28 n-alkane as sole carbon source. The results indicated that G1 and G2 genes are mostly responsible for the degradation of long-chain alkanes in Dietzia sp. DQ12-45-1b, which has unique multiple alkane hydroxylase systems.     

Isolation and characterization of an Arthrobacter sp. strain HB-5 that transforms atrazine

A bacterial strain (HB-5) capable of utilizing atrazine as sole carbon and nitrogen source for growth was isolated from an industrial wastewater sample by enrichment culture. The isolate was identified as Arthrobacter sp. according to its phenotypic features, physiologic and biochemical characteristics, and phylogenetic analysis. The strain exhibited faster atrazine degradation rates in atrazine-containing mineral media than the well-characterized atrazine-degrading bacteria Pseudomonas sp. ADP. The broad optimum pH and temperature ranges observed for strain HB-5 indicate that it has potential for remediation of atrazine-contaminated sites. Strain HB-5 first metabolizes atrazine to yield hydroxyatrazine. Then, the bacterium metabolizes hydroxyatrazine to cyanuric acid, but could not mineralize atrazine.     

氯氰菊酯降解菌的筛选鉴定及其降解特性研究

从农药厂废水排放口附近的污泥中分离到1株能降解氯氰菊酯的细菌LQ-3.根据其形态、生理生化特征和16S rDNA(GenBank Accession No.FJ222585)序列分析,将该菌株鉴定为Starkeya sp..LQ-3菌株只能以共代谢方式降解氯氰菊酯,在有酵母粉、蛋白胨、葡萄糖等营养物质存在的条件下,5 d内对20 mg·L-1氯氰菊酯的降解率达到72.1%.LQ-3菌株降解氯氰菊酯的最适温度为30 ℃左右,pH值为7～8.LQ-3菌株还能降解功夫菊酯、甲氰菊酯、联苯菊酯和溴氰菊酯.酶的定域试验表明,LQ-3菌株降解氯氰菊酯的酶属于胞外酶.     

Methylobacterium sp. YAL-2对乙酰甲胺磷的降解特性

从有机磷生产厂家的下水道污泥中分离出一株对高浓度和低浓度乙酰甲胺磷都具有高效降解能力的寡营养菌YAL-2,根据形态、生理生化和16S rRNA基因系统发育分析,将菌株YAL-2鉴定为Methylobacterium sp.降解特性实验表明,菌株YAL-2能利用乙酰甲胺磷为唯一碳源生长和降解;在添加了甲醇的无机盐培养基中,84 h可完全降解300mg L-1乙酰甲胺磷,24 h将50 mg L-1和10 mg L-1乙酰甲胺磷降至非检测水平;4 d能完全去除100 mg L-1甲胺磷,5 d分别降解58.4%和40.6%的100 mg L-1乐果、敌敌畏.小青菜农药残留去除实验显示,菌株YAL-2可在7 d内将乙酰甲胺磷和甲胺磷将至限量水平.结果表明,将菌株YAL-2应用于保证果蔬等食品的食用安全是可行的.     

Effect of pH on biologic degradation of Microcystis aeruginosa by alga-lysing bacteria in sequencing batch biofilm reactors

In this paper, the effect of pH on biological degradation of Microcystis aeruginosa by alga-lysing bacteria in laboratory-scale sequencing batch biofilm reactors (SBBRs) was investigated. After 10 d filming with waste activated sludge, the biological film could be formed, and the bioreactors in which laid polyolefin resin filler were used to treat algal culture. By comparing the removal efficiency of chlorophyll a at different aerobic time, the optimum time was determined as 5 h. Under pH 6.5, 7.5, and 8.5 conditions, the removal rates of Microcystis aeruginosa were respectively 75.9%, 83.6%, and 78.3% (in term of chlorophyll a), and that of Chemical Oxygen Demand (COD_Mn) were 30.6%, 35.8%, and 33.5%. While the removal efficiencies of ammonia nitrogen (NH ₄ ⁺ - N) were all 100%. It was observed that the sequence of the removal efficiencies of algae, NH ₄ ⁺ - N and organic matter were pH 7.5>pH 8.5>pH 6.5. The results showed that the dominant alga-lysing bacteria in the SBBRs was strain HM-01, which was identified as Bacillus sp. by Polymerase Chain Reaction (PCR) amplification of the 16S rRNA gene, Basic Local Alignment Search Tool (BLAST) analysis, and comparison with sequences in the GenBank nucleotide database. The algicidal activated substance which HM-01 strain excreted could withstand high temperature and pressure, also had better hydrophily and stronger polarity.