Microcystis aeruginosa/Pseudomonas pseudoalcaligenes interaction effects on off-flavors in algae/bacteria co-culture system under different temperatures

We conducted an experiment to study the interaction effects of Microcystis aeruginosa and Pseudomonas pseudoalcaligenes on off-flavors in an algae/bacteria co-culture system at three temperatures(24, 28 and 32℃). Gas chromatography–mass spectrometry was applied to measure off-flavor compounds dimethyl sulfide(DMS), dimethyl trisulfide(DMTS),2-methylisoborneol, geosmin(GEO) and β-cyclocitral. During the lag phase of co-cultured M. aeruginosa(first 15 days), P. pseudoalcaligenes significantly increased the production of DMS, DMTS and β-cyclocitral at all three temperatures. In the exponential phase of co-cultured M. aeruginosa(after 15 days), M. aeruginosa became the main factor on off-flavors in the co-culture system, and β-cyclocitral turned to the highest off-flavor compound. These results also indicated that DMS, DMTS and β-cyclocitral were the main off-flavor compounds in our M. aeruginosa/P. pseudoalcaligenes co-culture system. Univariate analysis was applied to investigate the effects of M. aeruginosa and P. pseudoalcaligenes on the production of off-flavors. The results demonstrated that both M. aeruginosa and P. pseudoalcaligenes could increase the production of DMS and DMTS, while β-cyclocitral was mainly determined by M. aeruginosa. Our results also provide some insights into understanding the relationship between cyanobacteria and heterotrophic bacteria.     

Isolation of Cr(VI) reducing bacteria from industrial e uents and their potential use in bioremediation of chromium containing wastewater

The present study is aimed at assessing the ability of Bacillus sp.JDM-2-1 and Staphylococcus capitis to reduce hexavalent chromium into its trivalent form.Bacillus sp.JDM-2-1 could tolerate Cr(Ⅵ) (4800 μg/mL) and S.capitis could tolerate Cr(Ⅵ) (2800 μg/mL).Both organisms were able to resist Cd2+ (50 μg/mL),Cu2+ (200 μg/mL),Pb2+ (800 μg/mL),Hg2+ (50 μg/mL) and Ni2+ (4000 μg/mL).S.capitis resisted Zn2+ at 700 μg/mL while Bacillus sp.JDM-2-1 only showed resistance up to 50 μg/mL.Bacillus sp.JDM-2-1 and S.capitis showed optimum growth at pH 6 and 7,respectively,while both bacteria showed optimum growth at 37℃.Bacillus sp.JDM-2-1 and S.capitis could reduce 85% and 81% of hexavalent chromium from the medium after 96 h and were also capable of reducing hexavalent chromium 86% and 89%,respectively,from the industrial effluents after 144 h.Cell free extracts of Bacillus sp.JDM-2-1 and S.capitis showed reduction of 83% and 70% at concentration of 10 μg Cr(Ⅵ)/mL,respectively.The presence of an induced protein having molecular weight around 25 kDa in the presence of chromium points out a possible role of this protein in chromium reduction.The bacterial isolates can be exploited for bioremediation of hexavalent chromium containing wastes,since they seem to have the potential to reduce the toxic hexavalent form to its nontoxic trivalent form.     

铜绿假单孢菌AS1.860对紫杉醇的微生物转化

从32株微生物中筛选出对紫杉醇1具有转化能力的4个菌株，并从中挑选出铜绿假单孢菌AS1．860进行放大实验，投入100mg紫杉醇，分离出3个产物，并通过核磁共振谱鉴定了结构，分别为baccatin Ⅲ2、baccatin V3和10—去乙酰baccatin Ⅲ4，其中2和3也是人体代谢的产物。     

芽孢杆菌发酵产碱性果胶酶温度控制策略

采用自行筛选获得一株产碱性果胶酶芽孢杆菌WSH03-09,在小型发酵罐中研究了不同温度对碱性果胶酶分批发酵的影响,结果表明,在恒定39℃条件下,可获得最高酶活5．39u／mL,各温度条件下的菌体干重相差不多,最终均能达11．5g／L左右;在发酵前期,控制温度41℃时最有利于菌体的生长,而在产物合成期,控制37℃有利于获得较高的产物合成比速,在此基础上,提出分阶段温度控制策略,采用此温度控制策略进行碱性果胶酶的发酵,碱性果胶酶酶活达5．99u／mL,比采用单一温度下的最大值提高了11％,其它各项指标也有较大提高．图6表1参6     

A bioaugmentation failure caused by phage infection and weak biofilm formation ability

Two biological aerated filters (BAF) were setup for ammonia removal treatment of the circulation water in a marine aquaculture. One of the BAFs was bioaugmented with a heterotrophic nitrifying bacterium, Lutimonas sp. H10, where the ammonia removal was not improved and the massive inoculation was even followed by a nitrification breakdown from day 9 to 18. The nitrification was remained stable in control BAF operated under the same conditions. Fluorescent in situ hybridization (FISH) with rRNA-targeted probes and cultivable method revealed that Lutimonas sp. H10 almost disappeared from the bioaugomented BAF within 3 d, and this was mainly due to the infection of a specific phage as revealed by flask experiment, plaque assay and transmission electron observation. Analyses of 16S rRNA gene libraries showed that bacterial groups from two reactors evolved di erently and an overgrowth of protozoa was observed in the bioaugmented BAF. Therefore, phage infection and poor biofilm forming ability of the inoculated strain are the main reasons for bioaugmentation failure. In addition, grazing by protozoa of the bacteria might be the reason for the nitrification breakdown in bioaugmented BAF during day 9–18.     

一株高效十四烷降解菌的筛选及降解条件优化

采集某炼油厂废水处理车间的回流污泥,以十四烷作为唯一碳源筛选分离到一株高效十四烷降解菌。经形态学观察和生理生化特征研究,鉴定为布兰汉氏球菌(Branhamella sp.)。对其降解十四烷的条件进行了优化,实验结果表明,最适降解条件为接种量0.5%,温度35℃,初始pH=7,碳氮摩尔比为0.4:1,在最佳条件下,当十四烷的初始浓度约为50mg/L时,在12h内降解率高达98%以上。     

Degradation of o-chloronitrobenzene as the sole carbon and nitrogen sources by Pseudomonas putida OCNB-1

A bacterial strain that utilized o-chloronitrobenzene(o-CNB) as the sole carbon,nitrogen and energy sources was isolated from an activated sludge collected from an industrial waste treatment plant. It was identified as Pseudomonas putida based on its morphology,physiological,and biochemical characteristics with an automatic biometrical system and the 16S rRNA sequence analysis. Microcosm study showed that the biodegradation of o-CNB was optimized at culture medium pH 8.0 and 32°C. At these conditions,the st...     

4株邻苯二甲酸二丁酯降解菌的分离鉴定及其相关降解基因的克隆

从土壤中分离纯化出4株能降解邻苯二甲酸二丁酯(DBP)的菌株,分别命名为JDC-1、JDC-8、JDC-9、JDC-12,并对其进行了形态学、生理生化及分子生物学鉴定.菌株革兰氏染色阳性,16S rDNA序列分析显示4株菌均与节杆菌属(Arthrobacter sp.)有99%以上的序列相似性,初步判断这4株菌为Arthrobacter sp..通过PCR扩增及克隆,均获得了1个约900 bp的DNA片段,测序结果显示该片段与Arthrobacter keyseri的邻苯二甲酸3,4-双加氧酶基因的核苷酸序列相似性为96%以上.对4株菌的最适生长条件及对DBP的降解能力进行了分析,结果显示,4株菌的最适生长条件为pH 7.0~8.5,温度30~35℃.以DBP作为目标测试物,在适宜条件下测试了4株菌的降解能力,显示这4株菌均为高效降解菌,效率最高的JDC-1能在28 h内将500 mg/L的DBP降解完全,最慢的JDC-8经40 h能将500 mg/L的DBP降解完全,本研究对于DBP降解机制的研究及微生物资源的开发都具有重要意义.     

铜绿假单胞菌增强型绿色荧光蛋白标记的研究

根据增强型绿色荧光蛋白(EGFP)基因设计了上下游引物P1和P2,通过对铜绿假单胞菌菌株X3绿色荧光蛋白标记研究,构建了铜绿假单胞菌标记系统,获得带有EGFP标记的基因工程菌X9,为进行相关的跟踪研究创造了条件.该菌株绿色荧光标记性能稳定.通过转化子基因组DNAPCR和斑点杂交检测,外源EGFP基因存在于转化子染色体上. 图 6参 14     

几种诱导子对青霉PT95菌株固态发酵产生类胡萝卜素的影响

分别用粗糙脉孢菌(Neurosporacrassa)、紫红曲霉(Monascuspurpureus)、掷孢酵母(Sporobolomycesroseus)、深红酵母(Rhodotorularubra)、诺卡氏菌(Nocardiasp. )N89和游动放线菌(Actinoplanessp. )A05的细胞壁制成6种诱导子.当在玉米培养基中添加适量诱导子进行诱导培养时,青霉PT95菌株的菌核生物量和菌核中积累的类胡萝卜素含量有了显著的提高(P<0. 01),从而提高了PT95菌株的类胡萝卜素产率.其中, 4种真菌诱导子的效果明显好于另外2种放线菌诱导子,紫红曲霉诱导子的效果最好.当培养基中紫红曲霉诱导子的质量分数为100μg/g时,每百克玉米的类胡萝卜素产率达到14 446μg,比对照提高176%.除紫红曲霉诱导子外,其余5种诱导子都能显著提高总色素中的β-胡萝卜素百分含量(P<0. 01). 表4参9