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1.
微生物絮凝剂产生菌的筛选及培养研究   总被引:11,自引:1,他引:10  
时红  牛志卿  李晋 《生物技术》2003,13(1):25-27
从活性污泥中筛选出3株能产生高效絮凝活性的微生物,对其中1株TJ3进行其最佳培养条件及废水絮凝实验研究。结果表明TJ3的最佳培养条件为:以葡萄糖、蛋白胨作碳,氮源,初始pH值6~7,温度25~30℃,摇床转速120~160r/min,培养时间72h,可产生高絮凝活性的絮凝剂,对高岭土悬浊液絮凝率达92.4%,同时在最佳培养条件下,该菌所产絮凝剂对多种废水净化效果明显,尤其对净化分散兰染液,酵母菌菌液分离最为突出,絮凝率均在95%以上,具有较高的絮凝性能。  相似文献   

2.
絮凝剂产生菌培养条件的研究及在废水处理中的应用   总被引:5,自引:0,他引:5  
通过菌种富集、分离、纯化,从含有大量微生物菌群的土壤和活性污泥中筛选到一株对高岭土悬浊液具有较高絮凝活性的絮凝剂产生菌,将其命名为B23.通过研究该菌株在不同培养时间的生长情况和发酵液的絮凝活性,从而得出发酵液絮凝活性与菌体生长量呈正相关.通过对该菌株培养条件的研究表明,在培养时间为24h、培养温度为30℃、培养基初始pH值为8.0,以葡萄糖为碳源、(NH4)2SO4为氮源时,发酵液絮凝活性最强.用B23菌株所产絮凝剂处理废水后,废水中CODCr的去除率为62.48%,SS的去除率为84.47%,表明该菌株有良好的实际应用前景.  相似文献   

3.
一株絮凝剂产生菌的筛选鉴定及培养条件   总被引:3,自引:0,他引:3  
从淤泥中筛选到1株高效微生物絮凝剂产生菌JX18,经过对其形态特征、生理生化特性、以及16SrRNA序列分析初步鉴定为荧光假单胞菌。该菌培养40h进入稳定期,48h时絮凝活性达到最大。进一步研究表明:菌株JX18最适培养基初始pH值7.0,培养温度30°C,摇床转速160r/min,最佳碳源和氮源分别为葡萄糖和蛋白胨。最适培养条件下,所产絮凝剂对高岭土悬浮液的絮凝活性达到90.56%。  相似文献   

4.
目的:从海口市白沙门污水处理厂活性淤泥中分离微生物絮凝剂产生菌,并对其絮凝特性进行初步研究。方法:稀释平板法进行菌株分离,高岭土悬浊法进行菌株的筛选以及菌株产絮凝剂特性、絮凝剂活性成分和热稳定性的研究;通过形态学和生理生化试验进行菌株的初步鉴定。结果:筛选到2株具有高絮凝活性的产生菌XN-6和XN-8,分别属于乳杆菌属(Lactobacillus sp.)和不动杆菌属(Acinetobater sp.)。菌株XN-6和XN-8发酵液絮凝率最高时,菌株XN-6的最佳pH值、最适温度和最佳转速分别为7、30℃、120r/min;XN-8的最佳pH值、最适温度和最佳转速分别为8、32℃、120r/min;菌株产絮凝剂活性成分热稳定性较差。菌株XN-6和XN-8单独处理污水的絮凝率分别为81.01%和76.78%,联合处理污水的絮凝率为79.08%,基本上不存在协同作用。结论:菌株XN-6和XN-8可作为原始菌株用于开发微生物絮凝剂,有望能应用于污水的处理。  相似文献   

5.
两株微生物絮凝剂产生菌筛选与复合培养研究   总被引:1,自引:0,他引:1  
目的:从土壤中筛选出微生物絮凝剂产生菌株进行复合优化培养得到高效絮凝剂。方法:采用平板划线法分离、纯化和筛选得到生长条件相互匹配的目的菌株,通过单因素和正交实验优化培养件,寻求絮凝活性最佳发酵条件。结果:发现菌株X-3和S-11菌株絮凝活性较高;复合菌株在牛肉膏-蛋白胨培养基中培养,初始pH为8,培养箱温度为35℃的条件下,培养时间72h,产生的分泌物对0.4g/L的高岭土悬浊液加3mg/L CaCl2助凝下絮凝率达到77.15%以上。结论:经鉴定X-3为德克斯氏菌属菌株,S-11为拜叶林克氏菌属菌株,匹配率为85%以上。  相似文献   

6.
微生物絮凝剂是一类新型的水处理制剂,因其具有高效、无毒、易降解等特点,已成为水处理剂开发的研究热点。为了扩大微生物絮凝剂的种类,本研究从活性污泥和土壤样品中筛选絮凝剂产生菌,最终获得一株具有絮凝活性的菌株,通过16S rDNA鉴定,该菌株为蒙氏假单胞菌(Pseudomonas monteilii),因此命名为P. monteilii YR-1。利用单因素实验和正交试验对该菌株的发酵条件进行了优化,其最佳碳、氮源分别为25 g/L葡萄糖和2 g/L复合氮源(酵母浸粉:尿素:硫酸铵=5:5:2),培养基初始pH值为10,培养温度为28℃,发酵时间为72 h。在最佳培养条件下,其发酵液的絮凝率从37.68%提高到63.52%。这是关于蒙氏假单胞菌产絮凝剂的首次报道。  相似文献   

7.
目的:对分离筛选获得絮凝剂产生菌Sphingomonas sp.X20絮凝特性及培养条件进行研究.方法:采用单因素和正交实验确定最适产絮凝剂培养条件.结果:研究发现,菌株X20的微生物絮凝剂对高岭土悬液具有良好的絮凝效果,在温度为37℃、培养基初始pH7.0、摇床转速为100r/min条件下培养12h获得的絮凝剂絮凝活性最好,絮凝率达92.8%.正交实验结果表明,菌株Sphingomonas sp.X20产絮凝剂最佳培养基的组成:淀粉15g/L,NH4Cl 1.Og/L,KH2P04,2g/L,K2HP04 5g/L,NaC1 O.lg/L,MgS04·7H2O 0.2g/L,pH7.0.结论:菌株X20是一株高效的产絮凝剂菌,具有很好的应用前景.  相似文献   

8.
絮凝剂产生菌的筛选、培养及产物性质研究   总被引:1,自引:0,他引:1  
从活性污泥中筛选出一株高效产絮凝剂菌株,经鉴定为嗜温鞘氨醇杆(Sphingobacterium thalpophilum).采用单因素实验,结果显示该菌产絮凝荆的最适碳源为可溶性淀粉,最适氮源为硫酸铵,最适初始pH值7.0,最适培养温度为30℃.性质研究分析显示,絮凝剂纯品的热稳定性差,其在pH值2.0~8.0的范围内可以保持较高的絮凝活性.  相似文献   

9.
微生物絮凝剂产生菌的选育及絮凝特性研究   总被引:3,自引:0,他引:3  
费文砚  吴涓 《生物技术》2007,17(3):59-63
目的:从土壤中筛选具有良好絮凝活性的菌株进行优化培养并研究其絮凝特性。方法:采用平板划线法分离纯化获得目的菌株,通过单因素和正交实验确定最适培养、絮凝条件,考察该菌的生长及产絮凝剂的周期和絮凝活性分布等特征,及其对次甲基兰的脱色能力。结果:得到絮凝活性较高的菌株C5,其最适产絮条件为:初始pH值7.5,温度36℃,培养时间48h;最适培养基为:葡萄糖10g,KH2PO42g,K2HPO45g,(NH4)2SO40.2g,尿素0.5g,酵母膏0.5g,NaCl0.1g,MgSO4.7H2O0.2g,絮凝率可达92.0%;最适絮凝条件为:2.5mL发酵液,pH6.0,5mL CaCl2溶液;絮凝活性成分主要为多糖和蛋白质,多分布于胞外上清液中;发酵液的絮凝活性与细胞生长量均在培养48h时达最大;对次甲基兰的脱色能力优于硫酸铝和聚丙烯酰胺,2min内脱色率可达97%。结论:菌株C5可产高絮凝活性的絮凝剂,具有良好的应用前景。  相似文献   

10.
从活性污泥中筛选出一株高效的微生物絮凝剂产生菌,鉴定为鲍曼不动杆菌.蚕豆根尖细胞微核试验未显示该菌株所产絮凝剂具有遗传毒性.该菌产絮凝剂的最佳碳源和氮源分别为葡萄糖和酵母浸出汁,培养时间为24 h.在絮凝体系中加入Ca2 能明显提高发酵液的絮凝率.在pH为8.0时对高岭土悬浊液和污水具有良好的絮凝效果.  相似文献   

11.
黑木耳原种胞外酶活性的研究   总被引:1,自引:0,他引:1  
目的:研究黑木耳菌株原种胞外酶活分泌特性,为进行大规模生产用种早期判定提供检测手段。方法:以9个黑木耳栽培菌株的原种为实验材料,分别测定了其胞外漆酶、多酚氧化酶、羧甲基纤维素酶、滤纸维素酶的酶活性变化。结果:胞外漆酶、多酚氧化酶、纤维素酶活性的变化趋势大致相似,酶活随培养时间呈规律性的升高、降低,除个别菌株(3、6)外,不同菌株同种酶活性差别不大,酶活相对较高的菌株有2、3、6、9号。不同菌株酶活高峰出现的时间有差异,较早的出现在培养的第10d,较晚的出现在培养的第70d。结论:被测菌株胞外酶活存在一定的规律性,利用该规律性可检测菌种退化、老化和不利变异。  相似文献   

12.
The lysozyme activity of 354 lysozyme-positive and 100 lysozyme-negative (by the results of qualitative test) staphylococcus strains were studied quantitatively. The method was based on titration of the lysozyme in the culture fluid of 48-hour broth cultures of the strains under study. The quantitative method proved to be more sensitive than the qualitative one, and permitted to reveal the lysozyme production in 71% of the strains which were formerly considered to be lysozyme-negative. There were distinct species differences between the lysozyme-positive staphylococci: the mean lysozyme level in the S. aureus was significantly greater then in the S. epidermis. There was no regular association between the lysozyme activity, staphylococcus origin, bacteriophage reference and the antibiotic resistance.  相似文献   

13.
Although enrichment culture is typically employed to isolate cellulolytic microbes, this approach tends to favor fast-growing species and discriminates against all others. Therefore, efforts to prevent the overgrowth of fast-growing species are necessary to isolate novel cellulase-producing strains. In this study, we developed a simple culture method for isolating hitherto-uncultured microbes that possess cellulase activity, particularly exocellulase. In this method, the microbial source (a forest soil) was suspended in sterilized water and inoculated onto a mineral salts agar medium, which was then overlaid with filter paper to sandwich the microbial suspension between the agar surface and paper. The filter paper fibers served to immobilize the microbial cells and were the dominant carbon source. Following cultivation at 30°C for 2 weeks, emerging colonies were isolated based on their morphology and were then subjected to phylogenetic and enzyme analyses. Using this method, 2,150 CFUs/g dry soil were obtained, and the ratio of fungal to bacterial isolates was approximately 4:1. Phylogenetic analyses revealed that most fungal and bacterial isolates belong to ten and two genera, respectively. Notably, all isolates possessed exocellulase activity, and several strains showed strong activity that was comparable to Trichoderma cellulase. Many isolates also exhibited cellulase and xylanase activity, and several strains possessed laccase activity. It is expected that the culture method described here will be useful for the isolation of hitherto-uncultured cellulolytic microbes and the identification of novel cellulases.  相似文献   

14.
Luminescent method for the detection of antibacterial activities   总被引:1,自引:0,他引:1  
A new rapid and sensitive method for the detection of antibacterial activities was based on luminescent indicator strains. Listeria innocua 8811 and Enterococcus faecalis 32 were transformed with plasmid carrying bacterial luciferase genes. Subsequent strains became capable to emit light during the exponential growth phase. The addition of bacteriocin containing culture supernatants to such cultures induced a drop of their light emission which was correlated to the combined antibacterial activity of acid stress and bacteriocin. The detection of antagonistic activity is independent of its mode of action, i.e. bactericidal or bacteriostatic. This method allowed to directly visualize the antagonistic activity of bacteriocin producer strains toward target strains in coculture experiments. However, a control co-culture with non-producing bacteriocin mutant was necessary in order to distinguish between nutrients competition and bacteriocin activity. Finally, five class IIa bacteriocins were purified from culture supernatants of eight strains detected in 3 days from a 120 lactic acid bacteria collection.  相似文献   

15.
The present study was conducted to screen microorganisms that produce phospholipase D (PLD), and we especially focused on the strains having high transphosphatidylation activity. Eighty bacterial strains were isolated from soil samples by a screening method utilizing a preliminary selection medium with phosphatidylcholine (PC) as the sole carbon source. The culture supernatants were then assayed for PLD activity. The finding of dual PLD activities in cultures revealed that the hydrolytic and transphosphatidylation activities were correlated. Consequently, six strains were selected as stably producing PLD enzyme(s) during continuous subcultures. The culture supernatants of selected strains synthesized phosphatidylglycerol, phosphatidylserine and phosphatidylethanolamine from PC with high conversion rates. These isolated strains will be made available to carry out phospholipid modification through the efficient transphosphatidylation activity of the PLD that they produce.  相似文献   

16.
【目的】从牡丹(Paeonia suffruticosa Andr.)根部组织中分离鉴定内生细菌,测定拮抗菌株脂肽类活性物质的体外抑菌活性。【方法】采用平板对峙法筛选出对牡丹灰霉病菌(Botrytis paeoniae Oadem)、牡丹炭疽病菌(Gloeosporium sp.)、牡丹黑斑病菌(Altenaria sp.)、牡丹黄斑病菌(Phyllosticta commonsii)有拮抗作用的内生细菌。基于形态特征、生理生化特性和16S rRNA基因序列同源性鉴定拮抗菌株。根据脂肽类抗菌物质合成相关基因序列对拮抗菌株进行基因扩增检测,采用酸沉淀法提取拮抗菌株的脂肽类物质,平板对峙法测定脂肽类物质的体外抑菌活性。【结果】从牡丹根部组织中共分离获得62株内生细菌,其中菌株Md31和Md33对4种病原菌均有较明显的抑制作用。Md31和Md33被鉴定为解淀粉芽孢杆菌(Bacillus amyloliquefaciens)。通过对菌株Md31和Md33进行5个脂肽类合成功能基因bmyB、fenD、ituC、srfAA和srfAB的检测,序列同源性分析,表明两个菌株具有合成脂肽类物质的能力。菌株Md31和Md33的脂肽类粗提物对所测试的牡丹病原真菌均具有不同程度的抑制作用。【结论】获得了2株对牡丹病原菌有良好抑制效果的解淀粉芽孢杆菌Md31和Md33,两个菌株的脂肽类粗提物也具有较强的体外抑菌活性,该研究为牡丹内生细菌的进一步开发应用奠定了基础。  相似文献   

17.
目的:从新疆石河子盐碱地菊芋生长根际土壤中分离筛选高产菊粉酶活力菌株。方法:通过稀释平板涂布法分离微生物;利用^60Co诱变选育,96孔板筛选突变菌株;采用3,5-二硝基水杨酸比色法测定菊粉酶酶活。结果:分离到12株具有菊粉酶活力的菌株,复筛得到1株高产菊粉酶活力菌株,将其命名为G-60;以此菌株为出发菌株进行^60Co诱变,利用96孔板对诱变菌株进行筛选,经摇瓶发酵酶活测定,得到1株高产菊粉酶酶活的突变株,酶活达46.62U/mL,是未诱变菌株酶活的2.72倍。结论:经诱变得到1株高产菊粉酶活力的突变菌株。  相似文献   

18.
The gamete activity of compatible mating strains of the isogamous, heterothallic species Chlamydomonas eugametos was investigated. Gamete activity was optimum within 4 h after flooding of agar slants and was maintained over a 24-h period. When male and female mating strains were mixed in proportions of 1:4, 2:3, 1:1, 3:2, and 4:1, the results based on zygote yield, indicated the strains exhibited different degrees of gamete activity. The male strain consistently showed less gamete activity than the female strain in a variety of culture conditions.  相似文献   

19.
目的从云南传统发酵豆豉中分离乳酸菌,并从中筛选具有高抑菌活性的菌株,进一步研究其抑菌谱,并初步分析其抑菌机制,为新型生物防腐剂的开发提供理论依据。方法应用传统纯培养技术及spot-on-lawn法从云南传统发酵豆豉中筛选得到具有抑菌作用的乳酸菌40株,并从中筛选得到1株具有高效抑菌活性的植物乳杆菌YM-4-3菌株。通过HPLC和紫外分光对其主要抑菌物质进行分析与抑菌试验。结果 YM-4-3菌株是1株具有新型生物防腐剂应用潜力的乳酸菌菌株。结论初步推测YM-4-3菌株抑菌机制为有机酸主导,细菌素和其他化学抑菌物质协同作用。  相似文献   

20.
采用研磨法从健康大花黄牡丹的根、茎、叶柄、叶和种子中进行菌种分离,依据其形态、培养特征及其他生物学特性对菌株进行初步鉴定;采用平板对峙法对分离的内生菌进行拮抗试验研究,并对强活性菌株进行16S rD-NA序列鉴定,以明确大花黄牡丹内生菌的种类,筛选对农作物病害有抑制作用的菌株.结果表明:(1)获得内生真菌188株,鉴定为10个属,以短蠕孢属(50%)、青霉孢属(18.6%)和曲霉孢属(12.3%)为优势种群.获得内生放线菌145株,以链霉菌属(98.6%)为优势种群.表明大花黄牡丹内生菌在数量和种类上存在极丰富的多样性,同时在不同组织存在一定的差异性.(2)抑菌试验结果显示,21.6%真菌对指示菌有抑菌作用,抑菌圈直径最大为10mm;27.8%放线菌对指示菌有抑菌作用,其中菌株PND31的抑菌活性较强,抑菌谱较广.(3)16S rDNA序列鉴定显示,菌株PND31与链霉菌属聚在一起,初步归为链霉菌属一个种.  相似文献   

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