法夫酵母生产虾青素发酵条件的研究

方法：分别进行了接种时间、摇床转速、接种量和装液量对法夫酵母细胞生产虾青素摇瓶发酵过程影响的实验,比较了DMSO法、酸热法、碱法和自溶法等破壁方法和提取溶剂之间的差别,测定了法夫酵母生长过程中的生物量、类胡萝卜素产量和培养基中的残糖。结果：确定了最佳的摇瓶发酵条件为：种瓶至发酵摇瓶的接种时间为40h,摇床转速为160r/min,接种量为10%,装液量为50mL;DMSO法和丙酮分别为合适的破壁方法和提取溶剂。结论：初步确定发酵的基本条件,为进行法夫酵母高产虾青素菌种的筛选以及发酵培养基的优化奠定了基础。     

白灵菇液体发酵工艺

以菌丝生物量为指标,探讨了白灵菇最适的液体发酵培养基和培养条件,结果表明:最适培养基为葡萄糖1.0%,玉米粉3.0%,酵母粉0.1%,黄豆粉2.0%,磷酸二氢钾0.15%,硫酸镁0.1%;摇瓶装液量80mL,接种量10%,起始pH为6.5,摇瓶转速160r/min。     

响应面法优化青枯病生防菌Hrp~-菌株的发酵条件

对工程菌Hrp-菌株的摇瓶发酵条件进行优化。首先采用Plackett-Burman设计法对影响Hrp-菌株活菌量的6个因素进行评价,筛选出具有显著效应的2个因素(发酵温度和摇床转速),再用最陡爬坡试验法接近重要因子的最优水平,最后应用中心组合设计确定重要因子的最优水平。确定优化后的发酵条件:初始pH 8.75、装液量为100 mL(500 mL三角瓶)、接种量6.25%、接种龄10 h、温度20℃、摇瓶转速205 r/min。实验结果表明:采用优化后的发酵条件,Hrp-菌株的发酵液菌量由最初的3.30×1010个/mL提高至4.42×1010个/mL,增幅为133.9%。     

海洋红酵母的液体培养

目的探讨提高海洋红酵母的液体高密度培养方法。方法在摇瓶培养条件下,测定温度、pH、装液量、接种量及摇床转速对海洋红酵母BY2菌株生长的影响,进一步放大培养至50L发酵罐,在培养过程流加氨水以控制pH稳定在5.3~5.5的条件下,考察不同葡萄糖浓度对海洋红酵母BY2菌株发酵菌量的影响。结果摇瓶最适培养条件为温度25℃,pH 5.5,接种量8%、装液量40mL/250mL三角瓶、摇床转速200r/min,在此培养条件下,24h时菌量达到8.9×108 CFU/mL;扩大至50L发酵罐,葡萄糖初始浓度为40、60、80、100g/L各罐20~24h时的菌量相应达到26.6×108、29.5×108、47.8×108、66.8×108 CFU/mL。结论提高初始葡萄糖浓度,流加氨水稳定发酵过程的pH,可以显著提高BY2菌株的发酵菌量。     

根霉液态发酵产生纤溶酶的培养条件优化

目的:目前临床使用的溶栓药物疗效肯定,但还存在许多缺陷,而且价格昂贵,因此研制新型溶栓药物的需求迫切。方法:研究了根霉Rhizopus chinensisYY-15液体摇瓶发酵产生纤溶酶的工艺条件。采用单因素试验对液体发酵培养基的碳源、氮源、碳氮比、初始pH进行了优化;采用正交试验对发酵时间、接种量进行了研究。结果:实验范围内菌株液体发酵产纤溶酶的适宜培养基组成为:麸皮水浓度3%(w/v),豆粕浓度5%(w/v),初始培养基pH5.0。适宜培养条件为接种量6%,培养时间72h。优化条件下的摇瓶液体发酵纤溶酶产量平均达98.31 U/ml。     

高生物量富硒酵母的选育及培养条件初步优化

通过筛选、单倍体分离、诱变和原生质体融合,从融合子中选育了一株高生物量富硒酵母菌株（编号为ZFF-28）,其细胞硒总含量分别是原始亲株ZY-67和ZY-198的2.8倍和2.0倍。通过单因素实验和正交试验设计,确定了优化培养条件：6%糖浓度的蔗糖糖蜜,添加0.5% (NH4)2SO4、0.1% H3PO4、60μg/mL Se,pH60～6.5,装液量50mL/250mL三角瓶,接种量10%,培养时间25h。在优化培养条件下,菌株ZFF_28的生物量可达8.2g/L,细胞中硒的含量达2050μg/g,硒总含量达到了16810μg/L,是培养条件优化前的1.3倍。细胞硒含量的91%为有机硒。     

响应面法优化泰乐菌素发酵工艺的研究

以弗氏链霉菌(Streptomyces fradiae)为出发菌株,考察发酵工艺中摇瓶转速、接种量、发酵液初始pH,发酵温度4个因素对泰乐菌素含量的影响。在单因素试验的基础上,采用Box-Behnken响应面设计对各因素进行进一步优化,确定最终发酵条件为:摇瓶转速200r·min-1,接种量7.94%,发酵液初始pH 7.35,温度28.3℃,在此条件下发酵得到的泰乐菌素含量达到13 572μg·mL-1,比优化前提高了19.9%。     

万古霉素产生菌发酵培养基及发酵条件的优化

通过单因素分析和正交试验,对万古霉素产生菌的发酵培养基和发酵条件进行了研究,确定最佳的发酵培养基配方为葡萄糖2.0%,淀粉3.0%,豆粕1.8%,大豆粉2.2%,氯化钠0.2%,碳酸钙0.2%,与原培养基配方相比,优化后万古霉素的摇瓶发酵效价提高了11.2%。同时优化了部分发酵条件,即二级种接种量为10%,溶氧为摇床转速220 r/min时250 mL摇瓶装液量为25 mL。将优化后的发酵工艺进罐验证,其保持了较高的适应性和连续性。     

杆菌JSM1601发酵产核酸的研究

确定了杆菌（Brevibacterium ammoniagenes）JMS1601发酵产核酸的最佳发酵培养基：葡萄糖12％,酵母浸膏1．5％,磷酸二氢钾0．3％。最佳摇瓶培养条件：温度32℃,摇床转速160r／min,接种量（v／v）5％,装液量100ml／500ml。     

高富硒酵母的筛选及富硒强化研究

富硒酵母在医学保健和制药产业中有着重要的应用,高富硒酵母是富硒酵母产品开发的基础。以新疆富硒土壤为样品来源,通过马丁培养基的初筛和富硒能力的复筛,筛选到一株富硒量相对较高的黏红酵母菌株Rhodotorula glutinis X-20。优化了菌株的富硒培养条件,结果显示,利用2%甘油为碳源可显著提高酵母中硒的累积,培养12 h时添加50μg/m L的亚硒酸钠能够保证酵母较高的硒累积量和生物量,添加0.4 mmol/L的磷酸盐可以有效地促进硒的转运和累积,最终使Rhodotorula glutinis X-20富硒量达到5 009μg/g。     

黄粉虫幼虫对硒的生物积累

在饲料中添加含硒化合物喂养黄粉虫Tenebrio molitor L.幼虫,测定幼虫硒含量、粪便硒含量和体重的变化,计算黄粉虫幼虫特定生长率及幼虫对硒生物积累系数,分析黄粉虫有效积累硒的条件。结果表明,饲料硒含量在15~20mg/kg时,幼虫硒含量明显提高,对硒的生物积累系数高于其它试验组水平,饲料硒含量过高,幼虫硒含量降低,正常生长受到抑制。黄粉虫幼虫特定生长率、取食量、排粪量、干物质含量随着饲料硒含量的增加而降低,死亡率、粪便硒含量随着饲料硒含量的增加而增大。饲料硒含量为15～20mg/kg时黄粉虫幼虫对硒的生物积累效果最好。     

Inulinase production by the marine yeast Cryptococcus aureus G7a and inulin hydrolysis by the crude inulinase

The marine yeast strain G7a isolated from sediment of China South Sea was found to secrete a large amount of inulinase into the medium. This marine yeast strain was identified to be a strain of Cryptococcus aureus according to the results of routine yeast identification and molecular methods. The crude inulinase produced by this marine yeast showed the highest activity at pH 5.0 and 50 °C. The optimal medium for inulinase production was artificial seawater containing inulin 4.0% (w/v), K₂HPO₄ 0.3% (w/v), yeast extract 0.5% (w/v), KCl 0.5% (w/v), CaCl₂ 0.12% (w/v), NaCl 4.0% (w/v) and MgCl₂·6H₂O 0.6% (w/v), while the optimal cultivation conditions for inulinase production were pH 5.0, a temperature of 28 °C and a shaking speed of 170 rpm. Under the optimal conditions, over 85.0 U/ml of inulinase activity was produced within 42 h of fermentation at shake flask level. This is very high level of inulinase activity produced by yeasts. A large amount of monosaccharides and oligosaccharides were detected after inulin hydrolysis by the crude inulinase.     

多拷贝毕赤酵母重组菌表达GCL摇瓶优化和高密度发酵

目的:构建高效表达白地霉脂肪酶的毕赤酵母重组菌株,并对筛选得到的菌株进行摇瓶发酵条件优化和分批补料高密度发酵工艺研究。方法:将诱导型表达载体pPIC9K-gcl电转化至毕赤酵母GS115。通过橄榄油-罗丹明B平板和摇瓶发酵筛选高脂肪酶活力的重组菌株,运用基于TaqMan探针的实时荧光定量PCR 法确定其拷贝数,并对菌株进行摇瓶发酵条件优化。在此基础上,研究重组菌在3L 发酵罐中的高密度发酵工艺。结果:筛选得到一株具有3 个白地霉脂肪酶基因拷贝的菌株GS115/pPIC9K-gcl 78#,初始酶活力为220 U/ml。当摇瓶发酵条件为甲醇诱导96 h,每24 h甲醇添加量1 %,接种量2 %,培养基初始pH 7.0,500 ml摇瓶装液量50 ml,甲醇诱导温度25℃ 时酶活力达735 U/ml。3L 发酵罐高密度发酵176.5 h,酶活力达到3360 U/ml,总蛋白含量达到4.30 g/L,且发酵过程中细胞活性一直保持在96 % 以上。结论:基因拷贝数与重组菌株的产酶水平呈正相关,摇瓶优化可显著提高重组菌株的产酶能力,为白地霉脂肪酶的工业化生产奠定了技术基础。     

Protozoan biomass relation to nutrient and chemical oxygen demand removal in activated sludge mixed liquor

The relationship between biomass concentration to nutrient and chemical oxygen demand (COD) removal in mixed liquor supplemented with sodium acetate was investigated, using three protozoan isolates and three different initial biomass concentrations (10(1), 10(2) and 10(3) cells/mL). The study was carried out in a shaking flask environment at a shaking speed of 100 rpm for 96 h at 25 degrees C. Aliquot samples were taken periodically for the determination of phosphate, nitrate, COD and dissolved oxygen, using standard methods. The results revealed remarkable phosphate removal of 82-95% at biomass concentration of 10(3)cells/mL. A high nitrate removal of over 87% was observed at all initial biomass concentration in mixed liquor. There was an observed COD increase of over 50% in mixed liquor in at the end of 96-h incubation and this was irrespective of initial biomass concentration used for inoculation. The study shows the trend in nutrient and COD removal at different biomass concentrations of the test isolates in mixed liquor.     

Preparation of selenium yeasts I. Preparation of selenium-enriched Saccharomyces cerevisiae

Selenium (Se) is an essential micronutrient for human and animal organisms. Organic selenium complexes and selenium-containing amino acids are considered the most bioavailable.Under appropriate conditions yeasts are capable of accumulating large amounts of trace elements, such as selenium, and incorporating them into organic compounds. It has been found that introduction of water-soluble selenium salt as a component of the culture medium for yeasts produced by conventional batch processing results in a substantial amount of selenium being absorbed by the yeast.Using a culture medium supplemented with 30 μg/mL sodium-selenite added during the exponential growth phase results in selenium-accumulation in the range of 1200–1400 μg/g dried baker's yeast (Saccharomyces cerevisiae) measured by ICP-AES method. In our previous studies it was shown that higher amounts of sodium-selenite in the culture medium have a strong inhibitory effect on the growth of this yeast. As a consequence of variations in cultivation conditions we obtained selenium yeast with different inorganic selenium content. The most important parameters influencing incorporated forms of selenium are pH value and dissolved oxygen level in the culture medium, and depending on these the selenium consumption rate of the yeast. A 0.40–0.50 mg/g h-1 specific selenium consumption rate was found to be appropriate to obtain selenium-enriched bakers' yeast of a high quality. Under suitable conditions the undesirable inorganic selenium content of the yeast could be suppressed to as low as 5–6% at the expense, however, of approximately a 20% decrease in the final biomass.     

弧菌菌株发酵工艺初步研究

采用摇瓶培养和发酵罐培养并在不同培养时间测定菌液浊度和活菌数,为弧菌灭活疫苗生产工艺提供参数.研究结果表明,摇瓶培养装量以30%较为合适,培养基初始pH 7.5,发酵过程以不再控制为宜.初步确定了弧菌发酵培养工艺参数:弧菌菌株接种TSB,28 ℃摇瓶培养18～20 h,28 ℃种子罐通气搅拌培养12～14 h,28 ℃...     

土壤硒及其与植物硒营养的关系

综述了土壤中Se的形态分布、有效性及其与植物关系研究方面的进展。论述了不同形态的Se在土壤中分布情况、对植物的有效性与土壤pH值、化学及矿物学组成、吸附表面、氧化还原状态等物理化学性质的关系;Se在植物中的富集、转化及其对植物的抗氧化、促进生长、提高产量和质量等各种生物学效应;并在此基础上对Se的应用前景做了展望。     

云芝液体培养及富集硒研究

通过云芝 (Polystictusversicolor)液体培养及富集硒研究。在培养温度 2 5～ 2 8℃ ,pH5 5～ 6 0 ,振荡速度 16 0r/min ,培养基中硒含量为 2 0mg/kg的条件下 ,云芝生物转化量及硒回收率最高。     

Production of Selenium-Enriched Biomass by Enterococcus durans

Selenium (Se) is an essential micronutrient for several organisms, and there is an increased interest about adequate sources for dietary selenium supplementation. The aim of this study was to evaluate the selenium bioaccumulation capacity of an Enterococcus strain. The isolate LAB18s was identified as Enterococcus durans by the VITEK® 2 system and analysis of both 16S rDNA gene sequence (JX503528) and the 16S-23S rDNA intergenic spacer (ITS). After 24-h incubation, E. durans LAB18s bioaccumulated elevated Se(IV) concentrations, reaching 2.60 and 176.97 mg/g in media containing initial amounts of 15 and 240 mg/l sodium selenite, respectively. The isolate grew optimally and had high selenium bioaccumulation at initial pH of 7.0 and 30 °C. Time course studies showed that E. durans LAB18s displayed the highest bioaccumulation of Se(IV) after 6 h of incubation. Analyses from scanning electron microscopy (SEM) demonstrated the presence of filaments connecting the cells of E. durans LAB18s cultivated in the presence of sodium selenite. It was demonstrated that a considerable amount of Se(IV) was absorbed by E. durans LAB18s. Therefore, this strain may represent an alternative source of organic dietary selenium.