南京市黑臭河流水体中细菌多样性的研究

以南京市城南河为研究对象,分别提取上中下游的水体样本,分析水质中的氮、磷、COD等水质指标,并利用变性梯度凝胶电泳技术(DGGE)分析了城南河不同位置的细菌多样性。结果表明:城南河水体中的平均总氮为30.06 mg/L,总磷为6.14 mg/L,COD为42.03 mg/L,均超过国家V类水质标准。结合外观,城南河属于严重污染的典型黑臭河流。DGGE分析的结果表明:城南河具有较高的细菌多样性,优势菌群主要是变形菌门和拟杆菌门2大类群,且不同取样点细菌种类差别不大。     

降解纤维素产甲烷的四菌复合系

自然环境中通常是微生物群落协同完成纤维素的降解,构建可降解纤维素的混菌体系是认识微生物相互作用的关键.利用富集培养法,结合变性梯度凝胶电泳(DGGE)指纹检测技术以及厌氧滚管技术,建立了一种筛选简单降解纤维素产甲烷复合菌系的方法.利用此方法从青藏高原若尔盖高寒湿地分离到一个由4株菌构成的降解纤维素产甲烷的稳定菌系.结果表明,该复合菌系由纤维素水解菌Clostridium glycolicum、非纤维素水解菌Trichococcus flocculiformis和Parabacteroides merdae、产甲烷古菌Methanobacterium subterraneum等具有不同功能的4种菌株组成,且在这4株菌的共同作用下可将纤维素直接转化为CH4.该简单复合系的获得为今后纤维素转化甲烷复合菌系的代谢控制和遗传改造提供了一个平台.     

DGGE及T-RFLP分析光照下电位对细菌群落的影响

电位和光照能影响生物电化学系统中产电光合微生物的富集和生长,为了明确电位对细菌多样性的影响,采用变性梯度凝胶电泳(denaturing gradient gel electrophoresis,DGGE)和末端限制性片段长度多态性(terminal restriction fragment length polymorphism,T-RFLP)两种方法分析光照条件下电位对电极生物膜细菌群落多样性的影响,实验设置0、0.2、0.4、0.6 V(vs.Ag/AgCl)4个电位.结果表明,0.6 V(vs.Ag/AgCl)下电极生物膜细菌DGGE条带数量较其他处理明显降低,对条带的测序结果显示不同电位下电极生物膜细菌主要属于α-变形菌纲(α-Proteobacteria)、β-变形菌纲(β-Proteobacteria)和梭菌纲(Clostridia).而0.2 V(vs.Ag/AgCl)处理下末端限制性片段(terminal restriction fragment,T-RF)的数量最高,片段数量随电压进一步升高呈现降低趋势.虽然DGGE和T-RFLP两种方法分析结果有一定差异,但都能反映电位对电极生物膜细菌群落多样性影响显著,高电位降低了细菌多样性.     

高效氨氧化菌群富集、驯化及其动态变化规律分析

利用选择性培养基对氨氧化菌群进行了连续驯化,得到了氨氮去除效率稳定的氨氧化菌群。采用平板菌落计数法结合聚合酶链式反应-变性梯度凝胶电泳(PCR-DGGE)技术考察了氨氧化菌群在连续传代过程中数量及群落结构的动态变化,并考察了pH值、碳源(HCO3-)浓度和氨氮浓度等因素对氨氧化菌群去除氨氮效率的影响。结果表明,通过连续驯化,氨氧化菌的比例由最初的1.8%提高到了31.3%。在碳源浓度为1.5 mg/L,NH4+-N初始浓度为200 mg/L,pH值为8的条件下,菌群对氨氮的去除率达99%以上。     

DGGE、T-RFLP 、LH-PCR对两种活性污泥的微生物种群多样性分析的比较

采用基于PCR扩增的分子生态技术DGGE、T-RFLP和LH-PCR，对2种典型污水处理系统中的活性污泥（生活污泥、焦化污泥）进行微生物种群多样性分析；并以此比较3种技术的优劣，提出不同应用条件下研究方法的选择依据。根据实验结果：DGGE得到的条带较多，但误差来源也最多；T-RFLP技术较为灵敏，但需要选择适当的内切酶，严格控制酶切条件，并且文库比对误差较大；而LH-PCR操作简单，结果稳定性较高。虽然目前尚无法判断3种方法的准确性，但LH-PCR在活性污泥的微生物种群多样性分析中已显示出潜在优势。     

Structural changes in soil communities after triclopyr application in soils invaded by Acacia dealbata Link

Triclopyr is a commonly used herbicide in the control of woody plants and can exhibit toxic effects to soil microorganisms. However, the impact on soils invaded by plant exotics has not yet been addressed. Here, we present the results of an 18-month field study conducted to evaluate the impact of triclopyr on the structure of fungal and bacterial communities in soils invaded by Acacia dealbata Link, through the use of denature gradient gel electrophoresis. After triclopyr application, analyses of bacterial fingerprints suggested a change in the structure of the soil bacterial community, whereas the structure of the soil fungal community remained unaltered. Bacterial density and F:B ratio values changed across the year but were not altered due to herbicide spraying. On the contrary, fungal diversity was increased in plots sprayed with triclopyr 5 months after the first application. Richness and diversity (H´) of both bacteria and fungi were not modified after triclopyr application.     

Variations of Bacterial Community Structure in Flooded Paddy Soil Contaminated with Herbicide Quinclorac

The denaturing gradient gel electrophoresis (DGGE) method was applied to determine the relative genetic complexity of microbial communities in flooded paddy soil treated with herbicide quinclorac (3,7-dichloro-8-quinoline-carboylic acid). The results obtained showed a significant effect of quinclorac on the development of bacterial populations in soils contaminated with different concentrations of the herbicide at the early time after application. In general, however, the number of populations of the same soil sample treated with the same concentration of the quinclorac differed obviously with increasing incubation time within the early 8 weeks. The scale of differences in banding patterns-showed that the microbial community structures of the quinclorac-treated and non-quinclorac-treated soils were not significantly different after 21 weeks of incubation. Quantification, as demonstrated in this paper, was studied by establishing dose-response relationships. Significant pattern variations were quantified. Prominent DGGE bands were excised, cloned and sequenced to gain insight into the identities of predominant bacterial populations. The majority of DGGE band sequences were related to bacterial genera Clostridium, Sphingobacterium, Xanthomonas and Rhodococcus.     

Combined use of molecular biology taxonomy, Raman spectrometry, and ESEM imaging to study natural biofilms grown on filter materials at waterworks

DNA-based population analysis was applied in combination with Raman spectrometry and Environmental Scanning Electron Microscopy for the characterisation of natural biofilms from sand and activated carbon filters operated for a long term at a municipal waterworks. Whereas the molecular biology polymerase chain reaction combined with denaturing gradient gel electrophoresis approach provides a deeper insight into the bacterial biofilm diversities, Raman spectrometry analyses the chemical composition of the extracellular polymer substances (EPS), microorganisms embedded in EPS as well as other substances inside biofilm (inorganic compounds and humic substances). Microscopy images the spatial distribution of biofilms on the two different filter materials. In addition, bacterial bulk water populations were compared with biofilm consortia using the molecular fingerprint technique mentioned.Population analysis demonstrated the presence of more diverse bacterial species embedded in a matrix of EPS (polysaccharides, peptides, and nucleic acids) on the sand filter materials. In contrast to this, activated carbon granules were colonised by reduced numbers of bacterial species in biofilms. Besides α-, β-, and γ-Proteobacteria, a noticeable specific colonisation with Actinobacteria was found on activated carbon particles. Here, the reduced biofilm formation came along with a decreased EPS synthesis. The taxonomy profiles of the different biofilms revealed up to 60% similarity on the same filter materials and 32% similarity of different materials. Similarity of adherent communities from filter materials and bulk water populations from the filter effluent varied between 36% and 58% in sand filters and 6–40% in granular activated carbon filters.The biofilm investigation protocols are most crucial to subsequent acquisition of knowledge on biofilm dynamics and bacterial contributions to transformation or adsorption processes in waterworks facilities.     

Bacterial diversity in paclobutrazol applied agricultural soils

The aim of this study was to investigate the bacterial communities on paclobutrazol [(2RS, 3RS)-1-(4-Chlorophenyl)-4, 4-dimethyl-2-(1H-1,2,4-triazol-1-yl) pentan-3-ol]–applied agricultural soils by denaturing gradient gel electrophoresis (DGGE) of polymerase chain reaction (PCR) amplified 16S rDNA gene fragments. Three different agricultural soil samples were collected from paclobutrazol applied mango and waxapple orchards, peanut fields and untreated rice fields as a control for DGGE analysis. The DGGE pattern of PCR- generated 16S rDNA gene fragments indicated that the bacterial populations from four paclobutrazol–applied soils of peanut fields were closely related to each other and two paclobutrazol–applied soils of mango and waxapple orchards harbored closely related bacterial communities. But, paclobutrazol–free agricultural soils comprised relatively a different bacterial group. However, the bacterial populations of mango and waxapple orchard are completely different from the bacterial communities of peanut field. Further purification and sequence analysis of 40 DGGE bands followed by phylogenetic tree assay showed similar results that soil bacteria from paclobutrazol applied mango and waxapple orchard are phylogenetically related. Based on the phylogenetic analysis, the clone M-4 was clad 100 % (bootstrap value) with Mycobacterium sp. The Mycobacterium sp. has been proved to degrade the phenolic compounds such as phenol, 4-chlorphenol, 2,4-dichlorophenol and paclobutrazol molecule containing chlorobenzene ring.     

碱预处理污泥产酸效果及其生物群落研究

为了提高污泥水解酸化过程中的挥发酸产量,获取污水脱氮除磷所需的内碳源,以深圳市罗芳污水厂的二沉池污泥为研究对象,采用不同的碱量对其进行预处理。通过测定碱预处理污泥水解酸化过程中的挥发酸浓度,并采用聚合酶链式反应-变性梯度凝胶电泳(polymerase chain reaction denature gradient gel electrophoresis,PCR-DGGE)技术对参与碱预处理污泥水解酸化产酸过程的主要微生物种群进行分析,结果表明,当碱投加量为0.20 g NaOH/g VSS时,初始溶出的蛋白浓度为1 780 mg/L;水解酸化15 d时,挥发酸总量达到3 473 mg/L;参与产酸的主要细菌属于Firmicutes、Proteobacteria、Bacteroidetes三个门类。