高效苯酚降解菌细胞固定化方法与条件的研究

含酚废水是一种难降解有机废水,对环境污染非常严重。目前常利用细菌处理含酚废水。但利用细菌处理含酚废水存在一些缺点,为此将1株高效苯酚降解菌进行细胞固定化。采用正交实验设计方法确定了该菌株固定化的最佳条件,并且考察了该固定化细胞降解苯酚的最佳条件。实验表明:该菌株的固定化细胞降解苯酚能力和耐受苯酚能力均大于游离细胞,经36 h可将1 800 mg/L苯酚降解完全。其降解苯酚的最适温度为30℃,最佳pH值为5~9。     

一株高效苯酚降解真菌的分离鉴定及其菌剂的制备

【背景】含酚废水是普遍存在的有毒、难降解的有机污染物之一,生物法处理含酚废水因成本低、无二次污染而具有广阔的应用前景。可降解苯酚的微生物中,真菌比细菌对恶劣环境的适应性更好。针对液态菌液保存时间较短和运输困难的瓶颈,制备固体菌剂可以提高菌体存活率和储藏稳定性。【目的】筛选一株能够高效降解苯酚的真菌,优化其降酚性能并选择合适的载体制备菌剂。【方法】通过逐级驯化和纯化分离降酚菌,筛选得到降酚性能较强的真菌并通过ITS r DNA基因测序进行种属鉴定,通过参数优化进一步提高菌株降解苯酚的性能;以不同材料为载体制备菌剂,通过稀释平板计数法和苯酚降解实验探究菌剂在不同温度下的保存效果。【结果】分离筛选得到一株高效降解苯酚真菌QWD1,通过鉴定证明其属于Magnusiomyces capitatus,其最适降解条件:(NH_4)_2SO_4为氮源,接种量为15%,pH为7.0,温度为35°C,氮源浓度为14 mmol/L。在此条件下,28 d内对1 600 mg/L苯酚去除率可以达到97.15%;制备菌剂最合适载体为谷糠,适宜保存温度为4°C,保存时间可达到90 d甚至更长,活菌数高达2.5×10~8 CFU/g左右,降解苯酚效果良好。【结论】筛选得到了一株高效降解苯酚真菌,优化其降解性能并将其制备成菌剂,为处理含酚废水提供了新菌种和理论支持。     

苯酚降解菌F6的筛选鉴定及降解特性

本研究利用逐级驯化的方法,从广西某工厂的废水中分离得到一株能利用苯酚作为唯一碳源生长的高效苯酚降解菌F6。采用16S r DNA序列分析的方法,将菌株F6鉴定为芽孢杆菌(Bacillus sp.)。F6菌株在8 h内几乎完全降解100 mg/L的苯酚,降解率达99.9%,该菌株的菌体生长与苯酚降解呈同步趋势,主要在对数生长期降解苯酚。F6最高耐受苯酚浓度为1 800 mg/L,在温度25~40℃,p H值6.0~9.0,盐度0~40 g/L范围内,F6菌株均能保持对苯酚良好的降解能力。菌株F6的降解底物具有广谱性,除了能够利用苯酚作为唯一碳源,还可以利用邻苯二酚、间苯二酚、对苯二酚、连苯三酚、甲苯、氯苯等酚类化合物为其生长代谢提供碳源和能源。综上所述,菌株F6在应用于处理成分复杂、含酚浓度较高的废水中将具有很大的潜力。     

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.     

两株高效苯酚降解菌的筛选、鉴定及生物强化-DTRO组合工艺初步验证

【目的】从煤化工废水中分离、筛选苯酚高效降解微生物,初步考察微生物与DTRO技术联用,构建含酚废水生物强化处理工艺的可行性。【方法】采用苯酚浓度梯度培养基对苯酚降解微生物进行分离和筛选;根据菌体形态电子显微镜观察、菌株生理生化特性考察和16S r RNA基因系统发育树构建,对菌株进行初步生物学鉴定;将筛选出的高效苯酚降解菌制备成相应的菌剂与碟管式反渗透(DTRO)技术组合形成"生物强化-DTRO"工艺,并试用于含酚废水的处理。【结果】共获得7株纯化细菌,其中Phe-03和Phe-05为高效苯酚降解菌;该2株菌均可以苯酚为唯一碳源生长。经鉴定Phe-03为壤霉菌属(Agromyces)菌株;Phe-05为棒杆菌属(Corynebacterium)菌株。到目前为止,壤霉菌属(Agromyces)菌株降解苯酚尚未见报道。在初始苯酚浓度达到1 300 mg/L条件下,Phe-03和Phe-05菌株44 h内对苯酚降解率均达到70%以上;76 h后苯酚降解率均超过90%。组合形成的"生物强化-DTRO"工艺不仅可以有效去除废水中的酚类化合物,而且还能减少反渗透膜污染,以及增加膜的通透性。【结论】研究表明微生物技术可与DTRO技术联用,构建含酚废水生物强化处理工艺,可为含酚废水处理技术研究提供一种选择思路。     

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。     

3-苯氧基苯甲酸降解菌Sphingomonas sp. SC-1降解苯酚环境条件及其降解中间产物的研究

【目的】探究高效降解3-苯氧基苯甲酸(3-Phenoxybenzoic acid,3-PBA)的鞘氨醇单胞菌(Sphingomonas sp.) SC-1对苯酚的降解特性。【方法】采用HPLC测定微生物降解体系中苯酚残留量,考察环境条件对菌株SC-1降解苯酚的影响;分析不同培养时间苯酚降解体系混合样品的HPLC谱图,确定其降解中间产物。【结果】菌株SC-1能在基础盐培养基中以苯酚为唯一碳源和能源生长,在初始pH 7.0、30 °C条件下,24 h可完全降解100 mg/L苯酚;Cu2+、Ba2+、Mn2+等对其降解苯酚有不同程度的抑制作用;HPLC谱图分析,初步确定邻苯二酚是菌株SC-1降解苯酚的中间产物,且该菌株可在48 h内完全降解100 mg/L邻苯二酚。【结论】菌株SC-1对苯酚及邻苯二酚均有较强的降解能力,为完善3-PBA的降解途径及污染3-PBA或含酚废水或含酚农药残留的降解提供了数据参考。     

苯酚降解菌红球菌(Rhodococcus sp.) P1的鉴定及其在焦化废水中的应用

摘要:【目的】酚类物质的去除是焦化废水处理的关键问题,目的是从焦化废水中分离高效的苯酚降解细菌。【方法】以苯酚为唯一碳源筛选纯化降解苯酚细菌,菌株鉴定采用菌落形态和16S rRNA 序列分析方法,并研究其苯酚降解特性和在焦化废水中的除酚作用。【结果】菌落形态和16S rRNA序列比对分析表明分离的P1菌株为红球菌属(Rhodococcus sp.)细菌;其耐酚浓度高达1400 mg/L,苯酚降解的最适条件为32℃－42℃、pH 7.0和0－4%盐;苯酚降解动力学曲线符合Haldane动力学模型,qmax=0.517/h,Ks=77.487 mg/L,Ki=709.965 mg/L;不同重金属对红球菌P1菌株的苯酚降解抑制作用不同,Zn2+、Mn2+和低浓度的Pb2+对菌株降酚没有影响,Cu2+、Ni2+、Cd2+均抑制菌株对酚的降解;红球菌P1菌株2d内可完全降解1/3焦化原水中的279.9 mg/L酚类物质。【结论】P1菌株是1株高效的苯酚降解菌,具有生物处理焦化废水酚类物质的潜力。     

一株高效苯酚降解菌的选育及降酚性能研究

从一绝缘材料厂的污水中分离得到一株可高效降解苯酚的菌株JY01, 该菌株的形态和理化特征与Bacillus基本相同, 其16S rDNA序列与Bacillus simplex (AM9216370)的相似性为99.01%。在接种量为2%的条件下, 该菌在pH为6.0~9.0和温度为18°C~36°C的范围内保持对苯酚良好的降解能力; 30 h内, 当苯酚浓度为1100 mg/L和1300 mg/L时, 其降解率分别为99.16%和74.76%。这将为进一步采用生物法处理含酚废水提供了可靠的控制条件。     

石化废水生物处理塔内生物膜不同菌系生态关系的研究（Ⅰ）

本实验以石油化工废水生物处理塔中生物膜为材料,分离得三株苯酚降解菌和一株石油解菌。分别测定了它们对酚的降解和耐受能力、适宜的生长温度、Ｐ＾Ｈ和氯化钠浓度。证明三株酚降解菌不仅可以苯灵唯一碳源,而且可耐受４００毫克／升浓度的苯酚。     

Enhancement of phenol biodegradation by Ochrobactrum sp. isolated from industrial wastewaters

Ochrobactrum sp., was tested with regard to its phenol degradation capacity at different pH levels, and with different carbon sources (mineral salt medium with glucose (MSG) and the same medium with 0.5%, 1%, and 2% (v/v) molasses (MSM)) and phenol concentrations. The highest degradation was in mineral salt medium with 1% (v/v) molasses (45.9%), while degradation was 21.1% in mineral salt medium with 5 g l⁻¹ glucose. These data show that the addition of molasses to mineral salt medium enhanced phenol degradation by Ochrobactrum sp. The bacterium can be used effectively to treat wastewaters containing phenol.     

一株油脂降解菌的筛选鉴定及降解效果分析

为了筛选分离得到一株具有油脂降解能力的菌株,同时探究菌株的特性和降解能力。以屠宰场污染土作为菌源,通过梯度驯化法最终筛选分离得到能够将橄榄油作为单一碳源生长的降解菌。随后通过形态特征观察、Biolog生理生化测试以及16S rRNA基因序列比对分析鉴定,实验菌株为革兰氏阴性菌,属于无色杆菌属（Achromobacter sp.）,在构建的系统发育树上与Achromobacter pulmonis聚为一支。综合运用紫外分光光度法和高效液相色谱法检测,测得实验菌株培养4~5 d时对橄榄油的降解率可以达到90%,同时测得菌株降解油脂的最适pH和最适温度分别为7.5和35 ℃,该菌株在盐浓度低于40 g·L-1环境中降解率较高。此外实验结果表明,实验菌株对各类型油脂均具有较高的降解效率,具有广泛的应用前景。     

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。     

Isolation, identification and characterization of a novel Ralstonia sp. FD-1, capable of degrading 4-fluoroaniline

A gram-negative strain, designated as FD-1, isolated from aerobic activated sludge was capable of metabolizing 4-fluoroaniline (4-FA) as its sole carbon and nitrogen source and energy supply. According to the Biolog GNIII detection method 17 of 71 carbon substrates were easily utilized, while 12 of 23 substrates did not inhibit strain FD-1. The 16S rDNA sequence from strain FD-1 was 99 % similar to Ralstonia sp., suggesting that it belonged to the genus Ralstonia. The optimal conditions for growth and 4-FA degradation were pH 7 and 30 °C. The tolerance to 4-FA were 1,250 mg/L, while the tolerance to salinity was 15 g/L. Catechol 2,3-dioxygenase activity was detected and degradation intermediates were analyzed by liquid chromatography mass spectrometry leading to a proposed degradation pathway and suggesting that extradiol cleavage was involved in 4-FA degradation. This is the first report on the degradation of 4-FA by a bacterium from the Ralstonia genus.     

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。     

Rate of Biodegradation of Phenol by Klebsiella oxytoca in Minimal Medium and Nutrient Broth Conditions

The rate of biodegradation of phenol by Klebsiella oxytoca strain was studied in the nutrient broth and M9 minimal medium. It was found that K. oxytoca degrade phenol at elevated phenol concentration where 75% of initial phenol concentration of 100 ppm will degrade within 72 h. This rate was increased with increasing the initial cell densities, increasing the aeration rate and increasing the time required for complete degradation. At phenol concentration above 400 ppm, the cells were unable to degrade the substrate efficiently due to the increasing concentration of phenol in the medium. The culture conditions were also showed a significant impact on the ability of these cells to remove phenol. The optimum solution pH and temperature were 6.8 and 37°C, respectively. The growth of these cells in the presence and absence of phenol was modeled and it was found that the Recatti equation best fit the growth in the absence of phenol whereas the Voltera equation accounted for the history of the cell population in the presence of phenol.     

饲料中添加壳聚糖季铵盐对凡纳滨对虾生长及非特异免疫的影响

实验研究壳聚糖季铵盐对凡纳滨对虾生长性能及非特异性免疫能力的影响。在饲料中分别添加0、0.05%、0.10%、0.15%和0.20%的壳聚糖季铵盐, 制成5组等氮等能饲料。将900尾[初体质量(3.820.34) g]健康的凡纳滨对虾随机分成5组(45尾4平行), 养殖时间56d。结果表明:饲料中添加壳聚糖季铵盐显著影响凡纳滨对虾的生长, 0.15%实验组凡纳滨对虾的增重率和特定生长率最佳(P0.05)。饲料中添加壳聚糖季铵盐0.1%、0.15%和0.20%能显著提高凡纳滨对虾血清溶菌酶和碱性磷酸酶及酚氧化酶的活性(P0.05)。饲料中添加壳聚糖季铵盐可显著提高凡纳滨对虾抗副溶血弧菌感染的能力(P0.05), 0.15%组的保护效果最好, 其相对免疫保护率为33.24%。壳聚糖季铵盐能显著提高凡纳滨对虾的生长性能和抗病能力, 本实验条件下适宜的添加量为0.15%。     

Phenol degradation performance by isolated Bacillus cereus immobilized in alginate

Phenol degradation by Bacillus cereus AKG1 MTCC9817 and AKG2 MTCC 9818 was investigated and degradation kinetics are reported for the free and Ca-alginate gel-immobilized systems. The optimal pH for maximum phenol degradation by immobilized AKG1 and AKG2 was found to be 6.7 and 6.9, respectively, while 3% alginate was optimum for both the strains. The degradation of phenol by free as well as immobilized cells was comparable at lower concentrations of phenol (100–1000 mg l⁻¹). However, the degradation efficiency of the immobilized strains was higher than that of the free strains at higher phenol concentrations (1500–2000 mg l⁻¹), indicating the improved tolerance of the immobilized cells toward phenol toxicity. More than 50% of 2000 mg l⁻¹ phenol was degraded by immobilized AKG1 and AKG2 within 26 and 36 days, respectively. Degradation kinetics of phenol by free and immobilized cells are well represented by the Haldane and Yano model.     

Degradation of 2,4,6-trichlorophenol by Azotobacter sp. strain GP1.

A bacterium which utilizes 2,4,6-trichlorophenol (TCP) as a sole source of carbon and energy was isolated from soil. The bacterium, designated strain GP1, was identified as an Azotobacter sp. TCP was the only chlorinated phenol which supported the growth of the bacterium. Resting cells transformed monochlorophenols, 2,6-dichlorophenol, and 2,3,6-trichlorophenol. Phenol and a number of phenolic compounds, including 4-methylphenol, all of the monohydroxybenzoates, and several dihydroxybenzoates, were very good carbon sources for Azotobacter sp. strain GP1. The organism utilized up to 800 mg of TCP per liter; the lag phase and time for degradation, however, were severely prolonged at TCP concentrations above 500 mg/liter. Repeated additions of 200 mg of TCP per liter led to accelerated degradation, with an optimum value of 100 mg of TCP per liter per h. TCP degradation was significantly faster in shaken than in nonshaken cultures. The optimum temperature for degradation was 25 to 30 degrees C. Induction studies, including treatment of the cells with chloramphenicol prior to TCP or phenol addition, revealed that TCP induced TCP degradation but not phenol degradation and that phenol induced only its own utilization. Per mol of TCP, 3 mol of Cl- was released. 2,6-Dichloro-p-benzoquinone was detected in the resting-cell medium of Azotobacter sp. strain GP1. By chemical mutagenesis, mutants blocked in either TCP degradation or phenol degradation were obtained. No mutant defective in the degradation of both phenols was found, indicating separate pathways for the dissimilation of the compounds. In some of the phenol-deficient mutants, pyrocatechol was found to accumulate, and in some of the TCP-deficient mutants, 2,6-dichlorohydroquinone was found to accumulate.