功能化介孔材料SBA-16对水中碱性橙染料的去除

通过共浓缩法用正硅酸四乙酯(TEOS)、3-巯丙基三乙氧基硅烷(TMMPS)作为硅源,聚醚F127和十六烷基三甲基溴化铵(CTMABr)作为模板剂合成SBA-16,随后将其磺酸基功能化.合成的材料用粉末X射线衍射、氮气吸附脱附和扫描电镜表征.结果表明,n(TEOS)∶n(TMMPS)为3～8时,合成的材料为介孔材料,当n(TEOS)∶n(TMMPS)为7时,该功能化的介孔材料对碱性橙染料的吸附能力最佳;通过不同的pH值下的实验表明,在pH为4～5时,该功能化的介孔材料的吸附能力最好.     

Characterization and catabolic genes detection of three oil-degrading Rhodococcus spp.北大核心CSCD

Oil pollution is one of the major factors causing environmental deterioration. Bioremediation of oil contaminated environments by microorganisms attracts much research attention. This study aimed to screen efficient oil-degrading bacteria from oil contaminated soil and analyze their characteristics and catabolic genes. Oil-degrading bacteria were screened from oil contaminated soil in minimal medium containing crude oil and identified by morphological, physiological and biochemical characteristics and 16S rDNA sequence analysis. Their growth and degradation characteristics were studied with ultraviolet spectroscopy and GC-MS analysis. The surfactant production was studied by adopting culture method. The major oil-degrading related genes were detected by t he PCR a mplification. As a result, t hree oil-degrading bacteria strains named KB1, 2182 and JC3-47 were isolated from the oil contaminated soil samples. The strains could use crude oil as the sole carbon source to degrade oil with a degrading rate of 41.02%, 32.26% and 55.90%, respectively, when cultured in minimal medium containing crude oil for 3 days. The bacteria were identified to belong to genus Rhodococcus. With 100% similarity of 16S rDNA sequences of the three strains with known ones of Rhodococcus, KB1 was preliminarily identified as Rhodococcus erythropolis, 2182 as Rhodococcus equi, and JC3-47 as Rhodococcus qingshengii. They grew well at 10-50 °C, with the initial pH of 3-9 and the NaCl concentration of 0-5%. The optimal temperature for bacterial growth was 35 °C, 35 °C and 30 °C respectively. KB1 and 2182 could grow at pH 2 and 9.0% of NaCl. The bacteria grew well in broth containing different organic substrates as sole carbon source, such as n-dodecane, n-octadecane, benzene, methylbenzene, xylene and naphthaline. KB1 and JC3-47 could grow well in broth containing pyrene. GC-MS analysis revealed that the bacteria could effectively degrade medium- and long-chain alkane components in crude oil. The bacteria produced biosurfactants and decreased the surface tension of the culture broth. They also showed adhesion activities to n-hexadecane. The oil-degrading related genes such as alkane monooxygenase, aromatic-ring-hydroxylating dioxygenase and catechol dioxygenase genes were detected in all the three strains. Besides, biphenyl dioxygenase genes were detected in KB1 and 2182. The isolated Rhodococcus spp. strains could effectively degrade petroleum hydrocarbons with high adaptabilities to extreme environments such as high salt and low temperature. They are supposed to be applied broadly in the bioremediation of oil contaminated soil in such environments.     

Dynamics of bacterial community of Suillus granulatus mushroom shiro in Pine (Pinus tabuliformis) forests北大核心CSCD

To evaluate bacterial community variation in the mushroom shiro of Suillus granulatus during fruiting, we collected soil samples from the mushroom shiro in the pine (Pinus tabuliformis) forest of mountainous area in Beijing from May to November and evaluated the bacterial community using polymerase chain reaction - denaturing gradient gel electrophoresis (PCR-DGGE). Total soil DNA was extracted using a commercial soil DNA isolation kit. PCR amplification and DGGE were performed using bacterial universal primers 338F and 518R. The specific bands were excised from the gel and sequenced. The results revealed that soil bacterial community maintained considerably high level and changed seasonally with the mushroom fruiting. In total, 53 bands of DGGE profiles were sequenced and divided into 5 phyla (Acidobacteria, Actinobacteria, Bacteroidetes, Firmicutes, and Proteobacteria and 22 genera (Acidobacterium, Aminobacter, et al). Species from Proteobacteria and Acidobacteria were the dominant bacterial groups sharing considerably high relative abundance, while class a-Proteobacteria was the most abundant group. The variation of the relative abundance of γ-Proteobacteria species was consistent with the mushroom fruiting season. The relative abundance of Acidobacteria species obviously increased before mushroom flush (in July). The fruiting of S. granulatus and the relative abundance of γ-Proteobacteria were correlated with each other. The present study provided a basis for conservation and domestication of mushroom S. granulatus.     

Isolation,identification and desulfurization mechanism of a sulfur-oxidizing bacterium with salt tolerance北大核心CSCD

Micro-organism with efficient desulfurization performance is a key factor in the biological desulfurization technology. This study aimed to seek such a sulfur-oxidizing strain and understand its desulfurization mechanism. Wastewater in a sewage station of natural gas purification plant was used to screen the sulfide-oxidizing strain, and to identify it based on sequence similarity analysis of 16S rDNA and the morphological characteristics. Thiosulfate was used as substrate for investigating the sulfur oxidation performance and salinity tolerance; the OD600, content change of thiosulfate, sulfate, sulfur, pH and total alkalinity in the cultural system were also investigated. The strain DS-B was found to share the highest sequence similarity with Thioalkalivibrio thiocyanoxidans ARh2, therefore determined as Thioalkalivibrio. At the optimum temperature of 35 °C for growth and degradation, the removal efficiency of thiosulfate could reach 98.7% after 7 days. Strain DS-B had strong resistance to thiosulfate, and the optimal concentration of S2O32- was 2 × 104 mg/L. The analysis for sulfur oxides showed that it could oxidize thiosulfate by the pathway of S2O32-→SO42- / S2O32- → S → SO42-. Therefore the strain DS-B is a sulfur-oxidizing bacterium with great application prospect for its strong salt tolerance and conspicuous removal capability for thiosulfate.     

1株耐冷兼性嗜碱好氧反硝化菌的分离鉴定及反硝化特性

以传统微生物富集分离方法,从垃圾渗滤液活性污泥中筛选到1株高效好氧反硝化菌,通过形态观察、生理生化特征及16S rDNA序列分析,对菌株进行了鉴定,同时对其好氧反硝化特性和异养硝化功能进行了研究.结果表明,筛选到的好氧反硝化菌株为假单胞菌属(Pseudomonas sp.),命名为GL19,GenBank登录号为(KC710974).碳源、C/N、pH及温度对菌株反硝化活性影响较大.在柠檬酸钠为碳源、C/N不低于15、pH 6~10、溶解氧(DO)4.8~7.7 mg·L-1及温度为15~34℃,硝酸盐氮负荷为140 mg·L-1的条件下,硝酸盐去除率均达100%,总氮(TN)平均去除率为96.5%,最终无亚硝酸盐积累;菌株能以亚硝酸盐氮、氨氮为底物进行高效脱氮,20 h内可将140 mg·L-1的亚硝酸盐氮完全去除,28 h内可将280 mg·L-1的氨氮降至3.11 mg·L-1,氨氮去除率达98.9%.显示该菌具有耐冷、高效脱氮特性,可实现同步硝化反硝化,这对南方地区冬季废水处理具有潜在应用价值.     

Characterization of a salt-tolerant bacterium Bacillus sp. from a membrane bioreactor for saline wastewater treatment

High salt concentrations can cause plasmolysis and loss of activity of cells, but the salt-torlerant bacterium can endure the high salt concentrations in wastewater. In this research 7 salt-torlerant bacteria, which could survive in dry powder products and could degrade organic contaminants in saline wastewater, were isolated from a membrane bioreactor. The strain NY6 which showed the fastest growth rate, best property for organic matter degradation and could survive in dry powder more than 3 months was selected and characterized. It was classified as Bacillus aerius based on the analysis of the morphological and physiological properties as well as the 16 S rRNA sequence and Neigh borjoining tree. The strain NY6 could survive in the salinity up to 6% and the optimal growth salinity is2%; it belongs to a slightly halophilic bacterium. The capability of its dry powder products for COD removal was 800 mg COD/(g·day) in synthesized saline wastewater with salinity of 2%. According to salt-tolerant mechanism research, when the salinity was below 2%, the stain NY6 absorbed K+and Na+to maintain osmotic equilibrium, and when the salinity was above 2%, the NY6 kept its life by producing a large amount of spores.     

不同16SrDNA靶序列对DGGE分析活性污泥群落的影响

为探讨不同通用引物扩增16S rDNA靶序列对活性污泥微生物群落分析的影响,更合理的利用变性梯度凝胶电泳(DGGE)技术分析活性污泥样品.从连续流搅拌槽式反应器(CSTR)中获取活性污泥,以3对通用引物341f/534r、968f/1 401r和341f/926r扩增16S rDNA序列,用DGGE分离PCR扩增产物.研究表明采用不同引物对进行DGGE分析时,群落多样性和动态存在显著的差异.341f/534r和968f/1 401r的靶序列分离效果较好,341f/926r的靶序列分离效果较差.引物341f/534r和341f/926r DGGE图谱显示S2和S3相似性高,引物968f/1 401r DGGE图谱显示S1和S2相似性高.由此可见采用不同引物对进行DGGE分析时,群落结构之间的相似性和动态是不一致的.341f/534r的DGGE图谱中条带丰富,多样性最好,968f/1 401r的DGGE图谱次之,341f/926r DGGE图谱条带最少,多样性也较差.因此,在利用DGGE分析活性污泥样品时采用引物341f/534r和968f/1 401r是比较适宜的.     

根据具体情况优化EPA8310中色谱分离条件

运用Agilent（安捷伦）1200系列高效液相色谱和多环芳烃专用柱ZORBAX Eclipse PAH（4.6×250mm、5μm,P.N.959990-918,S.N.USPAB01066）,对16种多环芳烃化合物混合溶液进行分析,根据具体实验条件优化EPA8310中色谱分离条件并得到了更节省时间、分离效率更好的流动相梯度变化程序。     

16Mn钢疲劳过程中的声发射特性研究

根据有关标准,设计加工了16Mn钢试样,并运用LOCAN320声发射仪、MTS810疲劳实验机和声发射传感器,用3种不同的试验方案,采集16Mn钢材料疲劳过程中的声发射(AcousticEmission,AE)信号特征参数,用于分析其疲劳过程中的声发射特性。重点探讨了16Mn钢材料在低周疲劳全过程中释放的声发射信号特征参数变化规律,得出声发射技术可用来评估16Mn钢材料的损伤程度,进而预测其疲劳寿命的结论。此外,充分利用试验中得到的不同疲劳载荷条件下试样的疲劳寿命,根据成组法修正了矩形截面试样16Mn钢材料的S-N曲线,经验证与实际结果吻合性较好。     

Bacterioplankton Community Structure and Dynamics in Enclosures During Bioremediation Experiments in an Acid Mining Lake

In an acid mining lake (pH 2.6) enclosure experiments wereperformed with the addition of different concentrations oforganic carbon, nitrogen and phosphorus. SSCP-communityfingerprints, based on 16S rRNA gene amplicons, were performed tomonitor changes in the structure of the total bacterialcommunity and the sulfate reducing bacteria (SRB) in themesocosms. Total bacterial cell counts, as assessed byepifluorescence microscopy, were increased in the mesocosmsamended with organic carbon. The addition of carbon alsoincreased the number of abundant bacterial taxa substantiallyalong depth. Sulfate reducing bacteria (SRB) could be detected inall enclosures and all parts of the water column. These SRBbelonged to genus Desulfobacter as indicated bycoroborating molecular data.