苯甲酸类化合物的微生物降解研究

用富集培养法从工业污水中分离到5个能以苯甲酸为唯一碳源和能源而生长的细苗菌株：不动杆菌（Acinetobactersp.）BJ1,无色杆菌（Achromobactersp.）BY1,假单胞苗（Pseudomonasspp.）SJ1、SY1和SH1、测定了这5个菌株的底物特异性和抗菌素抗性其中BJ1菌株含有1个大质粒和2个小质位在最适培养条件下BJ1菌株对苯甲酸的降解率达98％以上．     

Effect of neem extract against the bacteria isolated from marine fish

Marine ornamental fishes are exceedingly valuable due to their high demand in domestic and international markets. There is a growing global interest to rear the fishes in captivity. But problem due to bacteria and fungi are the major hitch in captive condition. Since, the use of antibiotics is banned, an attempt was made to ascertain in vitro assay of the neem leaves extract against the bacterial pathogens isolated from infected fishes. Bacterial strains isolated from infected regions of the clown fishes Amphiprion sebae and A. ocellaris were identified as Aeromonas hydrophila, Enterobacter sp., E. coli, Pseudomonas aeruginosa, Proteus sp., Streptococcus sp., Vibrio cholerae, V. alginolyticus, V. parahaemolyticus and Yersinia enterocolitica. Ethanol and methanol extracts were highly inhibitory to the bacterial isolates when compared to other solvents. Ethanol extracts exhibited low minimum inhibitory concentration (75-250 microg ml(-1)) as compared to other extracts. The present finding revealed that the neem leaf extract significantly reduces the bacterial pathogens and their infection in marine ornamental fishes.     

Characteristics of culturable endophytic bacteria of Xanthoceras sorbifolia Bunge with tumor roots北大核心CSCD

Xanthoceras sorbifolia Bunge with tumor roots was discovered, and the endophytic bacteria that were isolated from the tumor roots were purified and identified. This paper aimed to study the characteristics of endophytic bacteria. The CAS detection plate, Salkowski colorimetry, phosphate solubilizing circle, and molybdenum antimony spectrophotometry were used to analyze endophytic bacteria ability, which produced siderophores, secreted indole-3-acetic acid (IAA), and dissolved phosphorus. Strains were isolated from the tumor roots through morphological and molecular identification, and they were named XSB1-XSB9, of which 6 strains belonged to Bacillus sp., 2 strains belonged to Brevibacillus sp., and 1 strain belonged to Pseudomonas sp. All 9 strains produced siderophores; strains XSB3, XSB4, XSB8, and XSB9 were extremely high yielding, and strains XSB5 and XSB6 were high yielding. The strains with high yields were XSB3, XSB4, XSB5, XSB6, XSB8, and XSB9 and accounted for 66.7% of the tested strains. Nine strains secreted IAA; the concentration of IAA secreted by the strains that contained tryptophan was between 15-50 mg/L, and the concentration of IAA secreted by the one strain without tryptophan was between 10-35 mg/L. The IAA ability of the XSB2, XSB3, XSB4, XSB5, and XSB9 strains were significantly different (P < 0.05) after adding tryptophan. These results indicate that the synthesis of IAA may be the tryptophan synthesis pathway where tryptophan is used as a precursor. All 9 strains had some ability to dissolve phosphorus. The concentration of phosphate in the solubilizing strains, XSB1, XSB2, XSB4, and XSB5, were significantly higher than that in the other strains (P < 0.01), and the concentration of phosphate solubilizing was between 50-90 mg/L; the ability to dissolve phosphate was increased by 19-29 times. The XSB4 and XSB5 strains, which produced siderophores, secreted IAA and had a strong capacity to dissolve phosphorus, may be candidate strains for promoting growth. This research provides the foundation for the development and utilization of rhizosphere microbes to understand the resistance mechanisms and cultivation level of X. sorbifolia. © 2018 Science Press. All rights reserved.     

Arsenic detoxification potential of <Emphasis Type="Italic">aox</Emphasis> genes in arsenite-oxidizing bacteria isolated from natural and constructed wetlands in the Republic of Korea

Arsenic is subject to microbial interactions, which support a wide range of biogeochemical transformations of elements in natural environments such as wetlands. The arsenic detoxification potential of the bacterial strains was investigated with the arsenite oxidation gene, aox genotype, which were isolated from the natural and constructed wetlands. The isolates were able to grow in the presence of 10 mM of sodium arsenite (As(III) as NaAsO₂) and 1 mM of d+glucose. Phylogenetic analysis based on 16S rRNA gene sequencing indicated that these isolated strains resembled members of the genus that have arsenic-resistant systems (Acinetobacter sp., Aeromonas sp., Agrobacterium sp., Comamonas sp., Enterobacter sp., Pantoea sp., and Pseudomonas sp.) with sequence similarities of 81–98%. One bacterial isolate identified as Pseudomonas stutzeri strain GIST-BDan2 (EF429003) showed the activity of arsenite oxidation and existence of aoxB and aoxR gene, which could play an important role in arsenite oxidation to arsenate. This reaction may be considered as arsenic detoxification process. The results of a batch test showed that P. stutzeri GIST-BDan2 (EF429003) completely oxidized in 1 mM of As(III) to As(V) within 25–30 h. In this study, microbial activity was evaluated to provide a better understanding of arsenic biogeochemical cycle in both natural and constructed wetlands, where ecological niches for microorganisms could be different, with a specific focus on arsenic oxidation/reduction and detoxification.     

Assessment of phenol-degrading ability of Acinetobacter sp. B9 for its application in bioremediation of phenol-contaminated industrial effluents

Successful bioremediation of a phenol-contaminated environment requires application of those microbial strains that have acquired phenol tolerance and phenol-degrading abilities. A newly isolated strain B9 of Acinetobacter sp. was adapted to a high phenol concentration by growing sequentially from low- to high-strength phenol. The acclimatised strain was able to grow and completely degrade up to 14?mM of phenol in 136?h. The degradation rates were found to increase with an increase in the phenol concentration from 2.0 to 7.5?mM. The strain preferred neutral to alkaline pH range for growth and phenol degradation, with the optimum being pH 8.0. The optimum temperature for phenol degradation was found to be in the range of 30–35°C. Transmission electron micrographs showed a disorganised and convoluted cell membrane in the case of phenol-stressed cells, showing a major effect of phenol on the membrane. Enzymatic and gas chromatography-mass spectrometry studies show the presence of an ortho-cleavage pathway for phenol degradation. Efficient phenol degradation was observed even in the presence of pyridine and heavy metals as co-toxicants showing the potential of strain in bioremediation of industrial wastes. Application of strain B9 to real tannery wastewater showed 100% removal of initial 0.5?mM phenol within 48?h of treatment.     

不同生境产脂肪酶菌株的筛选及多样性

为发掘不同特性脂肪酶微生物资源,采用纯培养方法从青海高寒草地、雅安山区、成都平原分离得到产脂肪酶菌株54株.通过对菌株的DNA进行ERIC-PCR指纹图谱分析,按聚类树划分为5个操作分类单元.16S rDNA序列测定和聚类分析显示,分离菌株分布于芽孢杆菌属(Bacillus)、克雷伯氏菌属(Klebsiella)、假单胞菌属(Pseudomonas)、葡萄球菌属(Staphylococcus)、肠杆菌属(Enterobacter).多样性分析表明,与青海高寒草地、雅安山区相比,成都平原产脂肪酶菌株遗传多样性更为丰富.在54株菌中都出现了300 bp和1 300 bp两个特异且稳定出现的条带,这两个特异条带可能是产脂肪酶菌株的SCAR标记条带.     

苯酚降解菌UW7的鉴定及对苯酚的降解作用

从焦化厂污水处理曝气池泥样中分离出具有降解苯酚能力的UW7菌株,根据形态、生理生化性状初步鉴定为不动杆菌属(Acinetobacter).该菌16S rRNA基因序列(在GenBank中的登录号为GU083586)与多株鲁氏不动杆菌(A.lowffii)的相似性在99%以上.结合形态、生理生化特性,鉴定UW7菌株为鲁氏不动杆菌(A.lowffii UW7),该种细菌具有降解苯酚的特性尚未见报道.该菌株降解苯酚的最适温度为30℃,最适生长pH 7.0,对2.5 g/L浓度的苯酚能够有效降解,对3.5～4.0 g/L浓度的苯酚有较强的耐受能力,是处理高浓度苯酚废水的良好菌种资源.     

乙羧氟草醚降解菌Reudomonas sp.YF1的分离、鉴定与降解特性

从生产乙羧氟草醚工厂的污水处理池污泥中分离到一株乙羧氟草醚降解细菌,命名为YF1.根据表型特征、生理生化特性和16S rDNA序列系统发育分析,将其鉴定为假单胞菌属(Pseudomonas sp.).接种量为5%时,菌株YF1在含200 mg/L乙羧氟草醚的基础盐液体培养基中降解乙羧氟草醚,7 d后降解率约80%.加大接种量和外加营养碳氮源可以促进乙羧氟草醚的降解.该菌株降解乙羧氟草醚的最适pH为7.0,最适温度为30℃.菌株YF1能利用苯酚、邻苯二酚、对苯二酚、苯甲酸、龙胆酸、对硝基苯酚和邻氯苯酚为底物生长,不能利用3-苯氧基苯甲酸为碳源生长,菌株YF1细胞内邻苯二酚1,2-双加氧酶受到乙羧氟草醚或其代谢产物的诱导.图5表1参25     

亚麻温水脱胶液中细菌菌群结构分析

为了探讨实验室条件下模拟的工厂亚麻温水脱胶液中细菌菌群结构,采用纯培养技术和PCR-DGGE技术(Denaturing gradient gel electrophoresis)对细菌菌群结构进行了研究.用纯培养方法分离获得9类菌落,其中假单胞菌属(Pseudomonas)在有氧培养条件下总是处于优势.梭菌属(Clostridium)在厌氧培养过程中总是处于优势.微球菌属(Micrococcus)和葡萄球菌属(Staphylococcus)只有亚麻脱胶初期才有发现.PCR-DGGE指纹图谱显示,亚麻温水脱胶过程中条带数量较少且没有明显种群群落结构演替过程.通过对不同时期沤麻液中16S rDNAV3片段PCR产物d、e两个DGGE条带进行分子克隆、序列测定和Blas份析,发现e条带包含的16S rDNAV3片段除e 35外均属于假单胞菌属.d条带包含着较多不同的16S rDNAV3片段,其中有传统方法没有分离到的泛菌属(Pantoea)细菌、一些NCBI未收录的序列及一些非可培养微生物序列.纯培养技术和PCR-DGGE技术的共同使用,可以更全面准确地提供细菌多样性方面的信息.图4参15     

Arsenite oxidation by <Emphasis Type="Italic">Alcaligenes</Emphasis> sp. strain RS-19 isolated from arsenic-contaminated mines in the Republic of Korea

Arsenite [As(III)]-oxidizing bacteria play important roles in reducing arsenic [As] toxicity and mobility in As-contaminated areas. As-resistant bacteria were isolated from the soils of two abandoned mines in the Republic of Korea. The isolated bacteria showed relatively high resistances to As(III) up to 26 mM. The PCR-based 16S rRNA analysis revealed that the isolated As-resistant bacteria were close relatives to Serratia marcescensa, Pseudomonas putida, Pantoea agglomerans, and Alcaligenes sp. Among the five As-resistant bacterial isolates, Alcaligenes sp. strain RS-19 showed the highest As(III)-oxidizing activity in batch tests, completely oxidizing 1 mM of As(III) to As(V) within 40 h during heterotrophic growth. This study suggests that the indigenous bacteria have evolved to retain the ability to resist toxic As in the As-contaminated environments and moreover to convert the species to a less toxic form [e.g., from As(III) to As(V)] and also contribute the biogeochemical cycling of As by being involved in speciation of As.     

Purple photosynthetic bacteria from a tropical mangrove environment

Purple photosynthetic bacterial strains were isolated from mud samples collected from the mudflats of Pichavaram mangroves (Tamil Nadu, India) in 1989 and 1990. The presence of two major groups of photosynthetic purple bacteria was recorded, viz., Group 1: purple sulphur bacteria (family Chromatiaceae, strains belonging toChromatium sp.); and Group 2: purple nonsulphur bacteria (family Rhodospirillaceae, strains apparently belonging toRhodopseudomonas sp.).     

As(V)-reduction to As(III) by arsenic-resistant Bacillus spp. bacterial strains isolated from low-contaminated sediments of the Oliveri-Tindari Lagoon,Italy

Five arsenic-resistant bacterial strains designated MT1, MT2, MT3, V1 and V2 were isolated from sediments of the Oliveri-Tindari Lagoon (Italy), which comprises six small lakes whose sediments contain low arsenic concentrations. Phylogenetic analysis of the 16S rRNA gene sequences assigned them to the genus Bacillus. Bacillus sp. strain MT3 showed higher tolerance to As(III) and As(V), as indicated by minimum inhibitory concentrations of 14 and 135 mmol^?1, respectively. Bacillus sp. strain V1 showed growth inhibition at 14 mmol^?1 in the presence of As(III) and at 68 mmol^?1 in the presence of As(V), whereas the arsenic resistance of Bacillus sp. strain MT1 was 10 and 27 mmol^?1 for As(III) and As(V), respectively. The strains Bacillus spp. MT2 and V2 showed low levels of As(III) and As(V) resistance, as it was unable to grow at concentrations>7 and 14 mmol^?1, respectively. The isolated arsenic-resistant Bacillus spp. strains were able to reduce As(V) to As(III), especially Bacillus spp. strain MT3. This study suggests that the isolated bacterial strains play a role in the arsenic biogeochemical cycle of arsenic-poor sediments in the Oliveri-Tindari Lagoon.     

Selection of poly(R)-3-hydroxybutyric acid utilising bacteria by enrichment,optimisation and compatibility testing for consortia development

Bacterial strains with poly-3-hydroxybutyrate (PHB) degradation potential were isolated from waste yard soil samples of selected industrial sites in Uttarakhand, India, and two microbial consortia were developed, i.e. Consortium I comprises Pseudomonas sp. strain Rb10, Pseudomonas sp. strain Rb11 and Bacillus sp. strain Rb18, and Consortium II is composed of Lysinibacillus sp. strain Rb1, Pseudomonas sp. strain Rb13 and Pseudomonas sp. strain Rb19. The current study involved enrichment selection via liquid and semi-solid media, followed by isolation and screening of bacterial strains using PHB pellets and films. Furthermore, the identification and characterisation was done by triphasic approach. The utilisation of PHB by the characterised strains was confirmed by Fourier transform infrared spectroscopy and scanning electron microscopy. Moreover, the minimum inhibitory concentration of solubilised PHB was found to be 2.5?mg/mL, which was detected through ‘clear zone assay’. Further, the selection and biocompatibility testing of potential isolates were performed for the formation of bacterial consortia. Thus, the present work would provide direct and standardised protocol for screening and selection of potential microbiomes for biodegradation of polymers by overcoming the negative effect of organic solvents. Moreover, indigenously developed consortia would be evaluated for their in situ biodegradation potential against various bioplastic films.     

Biodegradation of phenol by native microorganisms isolated from coke processing wastewater

The present investigation was undertaken to assess the biodegradation of phenol by native bacteria strains isolated from coke oven processing wastewater. The strains were designated ESDSPB1, ESDSPB2 and ESDSPB3 and examined for colony morphology Gram stain characters and biochemical tests. Phenol degrading performance of all the strains was evaluated initially. One of the strains namely ESDSPB2 was found to be highly effective for the removal of phenol, which was used as sole carbon and energy source. From an initial concentration of 200 mg I(-1) it degraded to 79.84 +/- 1.23 mg l(-1). In turn the effect of temperature (20 to 45 degrees C), pH (5-10) and glucose concentration (0, 0.25 and 0.5%) on the rate of phenol degradation by that particular strain was investigated. Observations revealed that the rate of phenol biodegradation was significantly affected by pH, temperature of incubation and glucose concentration. The optimal conditions for phenol removal were found to be pH of 7 (84.63% removal), temperature, 30 degrees C (76.69% removal) and 0.25% supplemented glucose level (97.88% removal). The main significance of the study is the utilization of native bacterial strains from the waste water itself having potential of bioremediation.     

Bioactive potential of seagrass bacteria against human bacterial pathogens

Study of marine organisms for their bioactive potential, being an important part of marine ecosystem, has picked up the rhythm in recent years with the growing recognition of their importance in human life. Investigation was carried out to isolate 32 strains of endo and epiphytic bacteria in 2 seagrass species viz., Syringodium isoetifolium and Cymodocea serrulata. Morphologically different bacterial strains were tested against 5 antibiotic resistant human bacterial pathogens, of which 10 associated bacteria shown inhibitory activity against one or more bacterial pathogens. Minimum inhibitory concentration (MIC) and Minimum bacterial concentration (MBC) determination with extracellular bioactive compounds from the associated bacteria reveals that, the strain ENC 5 showed inhibitory activity against all the bacterial pathogens with the maximum sensitivity against Pseudomonas aeruginosa at the MIC value of 500 microg ml(-1).     

Sequential anaerobic and aerobic treatment of pulp and paper mill effluent in pilot scale bioreactor

In the present study sequential anaerobic and aerobic treatment in two step bioreactor was performed for removal of colour in the pulp and paper mill effluent. In anaerobic treatment, colour 50%, lignin 62%, COD 29%, absordable organic halides (AOX) 25% and phenol 29% were reduced in eight days. The anaerobically treated effluent was separately applied in bioreactor in presence of fungal strain, Paecilomyces sp., and bacterial strain, Microbrevis luteum. Data of study indicated reduction in colour 80%, AOX 74%, lignin 81%, COD 93% and phenol 76 per cent by Paecilomyces sp. where as Microbrevis luteum showed removal in colour 59%, lignin 71%, COD 86%, AOX 84% and phenol 88% by day third when 7 days anaerobically treated effluent was further treated by aerobic microorganisms. Change in pH of the effluent and increase in biomass of microorganism's substantiated results of the study, which was concomitant to the treatment method.     

高产黑色素菌株的分离及鉴定

对从土壤中分离出的321株菌株进行了筛选,得到1株高产胞外黑色素的菌株,比较了其在不同培养基上产黑色素的能力.初步确定该菌株为链霉菌属.该菌黑色素产量高,约为0.70g/L,在产黑色素的微生物中,链霉菌可以作为一类新的菌种资源.图2表1参15     

无苯酚培养基分离到的降酚菌多样性的分子分析

用3种不含苯酚的培养基(YPG、10%YPG和LB)从上海焦化厂废水处理系统(A2/O法)好氧池的悬浮污泥分离到24株降酚菌株.通过16SrDNAPCR扩增产物的限制性酶切分析(amplifiedribosomalDNArestrictionanalysis,ARDRA)、ERICPCR指纹图谱分析、多组分苯酚羟化酶大亚基(thelargestsubunitofthemulticomponentphenolhydroxylase,LmPH)基因的PCR扩增及16SrRNA基因测序的方法对这些降酚菌株进行表征.通过ARDRA分型,将这24株降酚菌株分为8个类型;利用ERICPCR可以将这24个菌株分为17种类型,说明同一ARDRA类型内菌株具有多样性.对17个ERIC类型代表菌株的16SrDNA扩增产物进行克隆并测序,测序结果在GenBank和RDP中进行比对.结果表明,与这17个代表菌株同源性最高的菌中,有6株是未见报道具有降酚功能的菌株.在这24株降酚菌中,有19株在苯酚含量为200mg/L的MP培养基中培养5d,苯酚降解率为20%左右,其余5株苯酚降解率达到100%,且均属于Rhodococcus属.本研究在降酚菌生物多样性上作了有益的探索.图2表1参20     

ERIC-PCR:一种快速鉴别环境细菌菌株的方法

以 Ｅ Ｒ Ｉ Ｃ（ 肠杆菌基因间共有重多序列） 序列设计的特异引物对３ 株大肠杆菌、３ 株软腐欧氏杆菌、２ 株草生欧氏杆菌、１ 株梨火疫欧氏杆菌、１ 株催娩克氏菌、１ 株阴沟肠杆菌和９ 株具有降酚能力的细菌等２０ 种细菌的基因组 Ｄ Ｎ Ａ 进行 Ｐ Ｃ Ｒ 分析．每种菌株均存在数目不等的各自独特的带型,能够区分同一种类中极为相近的菌株．经多次重复,各特异性扩增的主要带型能重复稳定出现．聚类分析的结果表明,供试菌株多数按照分类地位归到相应的组中．９ 种具有降酚能力的细菌中,２ 种分离自处理焦化废水池活性污泥,７ 种来自土壤样品． Ｅ Ｒ Ｉ Ｃ Ｐ Ｃ Ｒ 指纹图显示,前２ 种属于一类,都有一条大小约１ ．１ ｋｂ 的主带,其它７ 种土壤中分离出来的细菌除其中１ 种有１ 条约１ ．２ ｋｂ 大小的主带外,其余６ 种都有１ 条大小约１ ．４ ｋｂ 的带．聚类分析将从土壤中分离出来的细菌归为３ 种不同的类型． Ｅ Ｒ Ｉ Ｃ Ｐ Ｃ Ｒ 可以从分子水平对细菌基因组进行快速指纹图分析,在对环境细菌分离物进行快速鉴定和归类等方面具有实用价值     

Strengthening effects of ammonia nitrogen on the harmless biological treatment of oily sludge

To improve the efficiency of oil degradation and strengthen the harmless treatment of oily sludge, three dominant strains identified as Chryseomicrobium sp. YL2, Gordonia sp. YL3 and Acinetobacter sp. YL5 were isolated from soil near a refinery, and the effects on the bioremediation of the oily sludge from the refinery were investigated. The results showed that the efficiency of oil degradation increased by 31.5% compared with the control when the dominant strains were added to the treatment of oily sludge. Furthermore, the dominant strains could use oil as a carbon source for heterotrophic nitrification–aerobic denitrification. The addition of ammonia nitrogen resulted in a large number of remaining microbes and heightened dehydrogenase activity in the oily sludge, further accelerating oil degradation, mainly for C₁₁ to C₂₅ saturated hydrocarbons, and the oil degradation efficiency increased by 40.8%. After 120 days of bioremediation, the biotoxicity of oily sludge, which was expressed by the equivalent phenol concentration, decreased by 40.0% compared with that of the control, indicating that the addition of ammonia nitrogen enhanced the biodegradation of oil. This method can be used to strengthen the harmless treatment of oily sludge in practical engineering applications.