一株苯酚降解菌的筛选及其降解特性的初步研究

苯酚是一种严重污染物,目前的化学降解方法存在众多弊端,生物处理方法越来越受到重视。从胜利油田河口采油厂的飞雁滩油田土壤样品中分离,得到一株能够利用并降解苯酚的菌株P2。该菌株能够在以苯酚为唯一碳源和能源的培养基上生长,经BIOLOG细菌自动鉴定系统及16SrDNA鉴定,该菌株为类产碱假单胞菌（Pseudomonas pseudoalcaligenes）。通过苯酚羟化酶特异性引物的设计,从该菌株扩增出苯酚羟化酶大亚基（LmPH）基因,该基因片段编码对苯酚有催化活性的多肽。苯酚降解实验证实,该菌能在30℃192h内完全降解500mg／L的苯酚,Cu^2＋严重抑制该菌株对苯酚的降解,但碱性环境有利于其对苯酚的降解。     

一株苯酚高效降解菌的分离及其分解能力的初步研究

为了寻找能高效降解苯酚的微生物 ,从武汉市某化工厂周围的下水道污泥中 ,筛选分离出一种具有很高苯酚降解能力的菌株PheD1。通过生理生化及外观鉴定[1～ 3] ,将其初步鉴定为假单胞菌 (Pseudomonassp .)。经驯化后发现 ,该菌生长的迟缓期随苯酚浓度的增大而延长 ,但比同类报道的苯酚降解菌要短 ;在 35℃对数生长期时的苯酚降解率超过同类报道[6 ] ,6 0 0mg·L- 1 苯酚浓度的完全降解时间在 2 4h之内 ,比同类报道[4～ 6 ] 苯酚降解菌的分解能力要高。该菌为好氧菌 ,在空气充足的条件下可提高降解能力。对该菌的继续研究可使其在苯酚的生物降解及污水处理等实际运用中起到重要的作用。     

一株苯酚降解菌的分离与鉴定

目的：筛选能高效降解苯酚的微生物,并进行初步鉴定。方法：从某焦化厂排水沟采集污泥,通过逐步驯化筛选苯酚降解菌株;利用形态观察、生理生化检测、16SrDNA序列分析进行初步鉴定。结果：筛选获得1株苯酚降解菌JDM-2—1,该菌能够以苯酚为惟一碳源,耐酚能力高达2200mg／L,在30℃和pH7．0条件下,42h内能将800mg／L的苯酚彻底降解;初步鉴定其为球形芽孢杆菌（Bacillus sphaericus）。结论：菌株JDM-2-1是一株高效降解苯酚的球形芽孢杆菌。     

波茨坦短芽孢杆菌降解苯酚特性及动力学研究

从活性污泥中分离筛选出一株高效苯酚降解菌,经形态特征、生理生化试验及16S rDNA鉴定,该菌株为波茨坦短芽孢杆菌。该菌能以苯酚为唯一碳源和能源,最佳降解条件为:温度30℃,初始pH7.0,摇床转速为160 r/min。苯酚降解试验表明,该菌可在72 h内将初始浓度为1 600 mg/L苯酚完全降解。随着苯酚浓度的增加,底物抑制作用增强。应用Haldane方程对菌株的生长过程进行动力学模拟,拟合曲线与试验测定值相关性良好,各参数分别为μmax(最大比增长率)0.334 h-1,Ks(半饱和常数)14.07 mg/L,Ki(抑制常数)196.89 mg/L,且该菌株苯酚降解动力学与其生长动力学表现出相似的趋势。代谢机制研究表明,苯酚可诱导该菌合成邻苯二酚1,2-加氧酶降解苯酚。     

苯酚降解菌ZJ-1的分离及降解特性研究

目的:筛选苯酚降解菌,用于降解苯酚提高氧化塘处理效率.方法:以苯酚为惟一碳源进行选择性培养.结果:从乌鲁木齐市某炼油厂污水池的活性污泥中分离出一株能以苯酚为惟一碳源培养基上生长的菌株,编号为ZJ-1,该菌株最高可耐受1000mg/L的苯酚.对该苯酚降解菌降解性能研究表明:该菌具有较强的降解能力,在32℃、pH 7左右、接种量1%时,摇床振荡速度120r/min的条件下,该菌株在48h内苯酚降解率可达81%以上.培养液中苯酚浓度在300mg/L、500mg/L时,该菌株的降解率比较明显.当苯酚浓度大于1000mg/L时,则元明显降解效果.结论:ZJ-1菌株对苯酚具有较强的降解能力,具有广阔的应用前景.     

低温高效苯酚降解菌的分离与降解特性

从哈尔滨太平污水厂活性污泥中筛选到7株高效苯酚降解菌,可利用苯酚作为唯一碳源和能源。通过对这7株菌在不同温度、pH值、以及不同苯酚浓度下生长和苯酚降解情况的考察,确定了这7株菌的最适生长温度为10°C,最适pH值为7.5,最大可降解苯酚浓度为3000mg/L。通过对这7株苯酚降解菌降解性能的研究表明:其具有较强的苯酚降解能力,在10°C、pH值为7.5、装液量为50mL、接种量15%、摇床振荡速度160r/min的条件下,反应48h后可使500mg/L的苯酚降解率达90%以上。葡萄糖对菌体的生长及苯酚降解能力均有一定的影响,当葡萄糖浓度是500mg/L时,该菌对苯酚的降解率仍在80%以上。该研究对处理含有其它碳源的含酚废水具有一定的意义。通过DGGE图谱条带的分析表明,其亮度可以说明这些菌在各个系统中均表现为优势菌,且在污水环境中表现出较强的活性,其优势地位能够稳定地存在。其中2、4、24、28条带丰富,表现出它们在污水环境系统中的多样性。     

一株嗜热菌的分离鉴定及其苯酚降解特性

从油田地层水中分离到一株嗜热并高效降解苯酚的BF80菌株,其最适生长和降解苯酚的温度为60℃65℃。利用API50CHB/E系统和16SrDNA序列分析对菌株BF80进行了分类鉴定,该菌株的形态和生理生化特性与Geobacillusthermoglucosidasius基本相同,其16SrDNA序列与GeobacillusthermoglucosidasiusBGSCW95A1(=ATCC43742)的相似性为99·22%。在接种量为1%的条件下,该菌在20h内能完全降解3mmol/L的苯酚;在pH值5·59·0范围内能保持对苯酚良好的降解能力,并在12mmol/L苯酚的无机盐培养基中也能生长和降解苯酚,表明该菌能耐受高浓度苯酚并可用于高温含酚废水的生物处理。     

一株苯酚降解菌的筛选、鉴定及其降解特性

本研究采用逐量分批驯化的方法,从造纸废水中分离得到一株能够以苯酚为唯一碳源生长的苯酚降解菌株F5-1.经形态观察、生理生化特性鉴定及16S rDNA序列分析,将该菌株鉴定为克雷伯菌(Klebsie-lla sp.).该菌株能够在7 h时完全降解初始浓度为100 mg/L的苯酚,降解苯酚主要发生在生长对数期;在pH 5.0～9.0,NaCl浓度0～80 g/L,温度20～40℃范围内,菌株F5-1均可有效降解初始浓度为100～1 200 mg/L的苯酚;能够耐受的最大苯酚浓度为1 500 mg/L.本研究结果表明,F5-1菌株对处理环境条件复杂的含酚废水具有潜在的应用前景.     

一株苯酚降解菌的鉴定及其降解特性

【目的】鉴定从某化工厂附近土样中分离到的一株耐高浓度苯酚的菌株T10,通过优化菌株的培养条件提高菌株对苯酚的降解率。【方法】根据菌株的形态、生理生化鉴定及16S rDNA测序分析确定其种属,以液体摇瓶培养菌株T10对苯酚的降解率为指标,对菌株的生长条件进行优化。【结果】菌株T10属恶臭假单胞菌(Pseudomonas putida)。添加葡萄糖、蛋白胨能有效缩短T10菌的生长周期,并使苯酚的降解率提高1.7倍。在菌体初始接种浓度为10%、温度为30°C、转速为180 r/min条件下,对初始苯酚浓度、pH和装液量的响应面优化结果如下:初始苯酚浓度3 000 mg/L、pH 7.5和装液量80 mL/250 mL,苯酚去除率最高可达到87.56%。【结论】T10菌能够耐受较高浓度的含酚废水,并且对苯酚有较强的降解能力,为下一步利用生物法处理含酚废水提供科学依据。     

两株苯酚降解菌的分离及降解特性的初步研究

从南昌钢铁公司焦化污水处理厂的活性污泥中分离出64株能降解苯酚的细菌,通过耐受性试验从中筛选出2株降解活性较高的苯酚降解菌,编号为F-38和F-64。研究表明:F-38和F-64都为G—菌,苯酚浓度越高,生长延滞期越长;两株菌降解苯酚基本发生在对数期,其对苯酚降解适宜条件为温度30℃,pH值8-9,通气有利于苯酚的降解。     

Alcaligenes faecalis subsp. phenolicus subsp. nov. a phenol-degrading, denitrifying bacterium isolated from a graywater bioprocessor

A Gram (-) coccobacillary bacterium, J(T), was isolated from a graywater bioprocessor. 16S rRNA and biochemical analysis has revealed strain J(T) closely resembles Alcaligenes faecalis ATCC 8750T and A. faecalis subsp. parafaecalis DSM 13975T, but is a distinct, previously uncharacterized isolate. Strain J(T), along with the type strain of A. faecalis and its previously described subspecies share the ability to aerobically degrade phenol. The degradation rates of phenol for strain J(T) and reference phenol degrading bacteria were determined by photometrically measuring the change in optical density when grown on 0.1% phenol as the sole carbon source, followed by addition of Gibb's reagent to measure depletion of substrate. The phenol degradation rates of strain J(T) was found to exceed that of the phenol hydroxylase group III bacterium Pseudomonas pseudoalcaligenes, with isolate J(T) exhibiting a doubling time of 4.5 h. The presence of the large subunit of the multicomponent phenol hydroxylase gene in strain J(T) was confirmed by PCR. The presence of the nirK nitrite reductase gene as demonstrated by PCR as well as results obtained from nitrite media indicated denitrification at least to N2O. Based on phenotypic, phylogenetic, fatty acid analysis and results from DNA DNA hybridization, we propose assigning a novel subspecies of Alcaligenes faecalis, to be named Alcaligenes faecalis subsp. phenolicus with the type strain J(T) (= DSM 16503) (= NRRL B-41076).     

Phenol metabolism by two microorganisms isolated from Amazonian forest soil samples

Two microorganisms isolated from Amazonian forest soil samples and identified as Candida tropicalis and Alcaligenes faecalis were capable of degrading phenol (16 and 12 mM, respectively) at high salt concentrations (15% and 5.6%, respectively). Chromatographic and enzymatic studies revealed that each microorganism cleaved phenol at the ortho position with total phenol mineralization. ¹⁴C-phenol mineralization assays showed that both microorganisms assimilated about 30% of the total label. No phenol degradation metabolite (i.e., catechol, cis, cis-muconic acid) was detected in the intercellular medium. The presence of phenol hydroxylase (EC 1.14.13.7) and catechol 1,2-dioxygenase (EC 1.13.11.1) extracellular activity suggested that these microorganisms may secrete these enzymes into the extracellular medium. Journal of Industrial Microbiology & Biotechnology (2000) 24, 403–409. Received 02 November 1999/ Accepted in revised form 08 March 2000     

Salt-tolerant phenol-degrading microorganisms isolated from Amazonian soil samples

Two phenol-degrading microorganisms were isolated from Amazonian rain forest soil samples after enrichment in the presence of phenol and a high salt concentration. The yeast Candida tropicalis and the bacterium Alcaligenes faecoalis were identified using several techniques, including staining, morphological observation and biochemical tests, fatty acid profiles and 16S/18S rRNA sequencing. Both isolates, A. faecalis and C. tropicalis, were used in phenol degradation assays, with Rhodococcus erythropolis as a reference phenol-degrading bacterium, and compared to microbial populations from wastewater samples collected from phenol-contaminated environments. C. tropicalis tolerated higher concentrations of phenol and salt (16 mM and 15%, respectively) than A. faecalis (12 mM and 5.6%). The yeast also tolerated a wider pH range (3-9) during phenol degradation than A. faecalis (pH 7-9). Phenol degradation was repressed in C. tropicalis by acetate and glucose, but not by lactate. Glucose and acetate had little effect, while lactate stimulated phenol degradation in A. faecalis. To our knowledge, these soils had never been contaminated with man-made phenolic compounds and this is the first report of phenol-degrading microorganisms from Amazonian forest soil samples. The results support the idea that natural uncontaminated environments contain sufficient genetic diversity to make them valid choices for the isolation of microorganisms useful in bioremediation.     

Alcaligenes faecalis subsp. parafaecalis subsp. nov., a bacterium accumulating poly-beta-hydroxybutyrate from acetone-butanol bioprocess residues

The authors have previously isolated a solvent tolerant bacterium, strain G(T), (T = type strain) capable to convert acetone-butanol bioprocess residues into poly-beta-hydroxybutyrate. Strain G(T) was initially identified as Alcaligenes spp by standard bacteriological tests. In this study the taxonomic position of the bacterium was investigated in detail. The 165 rDNA sequence analysis, the G + C content of DNA (56 mol%) and the presence of ubiquinone Q-8 confirmed strain G(T) as a representative of the genus Alcaligenes. In the polyamine pattern of the bacterium putrescine and cadaverine were detected, but only trace amounts of 2-hydroxyputrescine. The extremely low content of 2-hydroxyputrescine is remarkable, since this unique diamine is a common marker for beta-proteobacteria. Phylogenetic analyses of 16S rDNA demonstrated that Alcaligenes sp. G(T) is most closely related to the species Alcaligenes faecalis (99.6% sequence similarity to A. faecalis HR4 and 98.7% sequence similarity to A. faecalis [ATCC 8750T = DSM 30030T]. On the basis of DNA-DNA relatedness (56% similarity), the unique polyamine pattern, the physiological and biochemical differences strain G(T) could be distinguished from the species A. faecalis. Therefore, a new subspecies for the species Alcaligenes faecalis is proposed; Alcaligenes faecalis subsp. parafaecalis subsp. nov.     

热凝胶的高产策略及功能研究进展

热凝胶（curdlan）又名β-（1→3）-D-葡聚糖,在食品、医药、保健品等领域具有重要的应用潜力。由粪产碱杆菌（Alcaligenes faecalis）或土壤杆菌（Agrobacterium sp．）生物合成的热凝胶以成本低廉、提取与纯化技术成熟而成为研究热点。笔者主要针对提高热凝胶产量的菌株改造和发酵控制策略以及热凝胶生物活性的研究进展和相关专利进行综述。     

假单胞菌诱导筛选菌株PhA苯酚降解动力学及SDS对其影响

为提高苯酚降解速率,由假单胞菌(Pseudonomonas．sp)诱导筛选得到了一株能以苯酚为唯一碳源生长的新菌株Pha,并使其苯酚选择压力从400mg／L逐步提高到了700mg／L。且Pha菌株降解苯酚过程符合一级反应动力学方程。使用十二烷基磺酸钠(SDS)作为增溶剂来促进降解时,发现在SDS浓度为50～150mg／L时,降解苯酚的速率随SDS浓度增加而提高。SDS在低浓度时对其生长影响很小,但浓度达到300mg／L时,对其生长开始有了明显的抑制作用。结果标明PhA菌株有着较高的苯酚耐受浓度,SDS可以显著的提高苯酚的降解速率。SDS的理论最佳投放量为150mg／L。     

新疆艾丁湖中度嗜盐苯酚降解菌多样性研究

高盐含酚废水属于极难处理的废水之一,筛选具有生物学降解能力的嗜盐菌有助于解决这一难题。从新疆艾丁湖盐湖中分离筛选能够降解苯酚的中度嗜盐菌,了解盐湖中度嗜盐苯酚降解菌的多样性组成和降解能力。研究结果表明,10%(质量分数)的盐浓度条件下,分离得到166株嗜盐菌,通过以苯酚为唯一碳源的培养基进行降解活性筛选后得到45株阳性菌,根据细菌16S rRNA基因序列系统进化分析,这45株菌分别归类到3个门,5个科,9个属。其中拟诺卡氏菌属(Nocardiopsis)是优势菌,占总量的68.8%,其余菌分布于Bacillus、Gracilibacillus、Pontibacillus、Halobacillus、Marinococcus和Halomonas属。在含100 mg/L苯酚的液体培养基,经过10 d培养后,这45株菌降解效率为1%~17%。本研究为工业应用提供了嗜盐微生物种质资源,极具进一步发掘和研究价值。     

贯叶连翘总提取物对谷氨酸棒状杆菌和粪产碱杆菌的抗菌作用

报道了经光照和未经光照处理后贯叶连翘总提取物对谷氨酸棒状杆菌和粪产碱杆菌的作用,结果表明,总提取物对谷氨酸状杆菌有强烈的抑菌和杀菌作用,对粪产碱杆菌有抑菌作用,其抑菌或杀菌作用与其浓度有关,且不需光照。     

Microbial metabolism of quinoline and related compounds. IV. Degradation of isoquinoline by Alcaligenes faecalis Pa and Pseudomonas diminuta 7

From sewage and soil isoquinoline-degrading organisms were enriched. Two strains could be isolated which were able to utilize isoquinoline as sole carbon source. The bacteria were tentatively identified as Alcaligenes faecalis and Pseudomonas diminuta with respect to their morphological and physiological characters. When growing on isoquinoline both strains excrete a metabolite into the medium which was identified as 1-oxo-1,2-dihydroisoquinoline. Alcaligenes faecalis was cultivated in continuous culture on 1-oxo-1,2-dihydroisoquinoline to improve growth on isoquinoline and degradative activity.