Determination of an economical medium for growth of Clostridium butyricum fermentum

本文重点在于提高酪酸梭状芽孢杆菌活菌数量,降低发酵培养基成本.通过对发酵培养基中不同碳源、氮源、生长因子等进行单因素研究,得到最佳培养基组成:可溶性淀粉10 g/L,豆粕(中性蛋白酶水解3 h)20 g/L,玉米浆3g/L.用此培养基在37℃培养24h,采用高层半固体琼脂试管法对酪酸梭状芽孢杆菌进行活菌计数,活菌数可达8.2×108 cfu/mL.培养基中添加K2HPO4 5g/L、MgSO4·7H2O 0.2 g/L、MnSO4·H2O 0.2 g/L培养32 h时,酪酸梭状芽孢杆菌芽孢转化率可达95％.     

水产动物益生菌乳酸杆菌LH发酵工艺的研究

目的从生产实际出发,对1株高效乳酸杆菌（Lactobacillus spp）LH进行液体发酵培养基优化及发酵条件研究。方法通过碳源、氮源、无机盐、促生长素等单因子筛选及正交试验设计获得以下最佳培养基：糖蜜12 g/L,酵母膏5 g/L,蛋白胨1 g/L,葡萄糖4 g/L,玉米浆3 g/L,乙酸钠5 g/L,NaC l 5 g/L,K2HPO42.5 g/L,KH2PO42.5 g/L,MgSO40.5g/L,MnSO40.25 g/L。在此培养基上研究了该菌株最佳发酵条件。结果培养基初始pH 6.0,接种量2%（v/v,相对装液量）,500 m l三角瓶中装液量为500 m l,发酵温度为30～35℃,静置培养。在最佳培养条件下,LH活菌量达到1.74×10^9CFU/m l。结论通过活菌平板计数法测定了乳酸杆菌LH生长曲线,24 h为最佳种龄,生产收获时间是36 h。     

裸脚菇0612-9液体菌种优化及其对后续发酵产活性物质的影响

裸脚菇0612-9次级代谢产物具有强烈抗青绿霉活性,可作为微生物源防腐剂用于柑橘保藏,但是其发酵周期长,产出能耗大效率低。用摇瓶对裸脚菇0612-9的液体菌种培养基、培养条件进行优化并对优化后液体菌种接种种龄、接种量进行探索,最后用5L发酵罐进行放大发酵验证。取样计数测定菌丝球数量、过滤称重测定菌丝干重、HPLC监测活性物质Ⅱ的积累、牛津杯法评价抗青绿霉活性。经研究最佳碳源为玉米粉和麦芽糖,最佳氮源为蛋白胨,最佳液体菌种培养基组成为：玉米粉30g/L、麦芽糖10g/L、蛋白胨15g/L、KH₂PO₄ 2g/L、MgSO₄·7H₂O 1g/L;最佳培养条件：起始pH 5、接种3×Ф7mm菌块、装液量100mL/250mL三角瓶、温度28℃、转速160r/min;优化前菌丝球数46个/10mL,菌丝干重0.28g/100mL,优化后菌球数达985个/10mL,菌丝干重达0.69g/100mL,分别为优化前的21.4倍、2.43倍;后续发酵使用种龄9d的液体菌种、接种量7.5%。优化后液体菌种在发酵罐中后续发酵周期从10d缩短至5d,缩短50%,产量比优化前提高8.28%。     

木耳浸提物与复合乳酸菌相互作用的研究

摘要：目的 研究木耳浸提物的制备及其与候选乳酸菌的相互作用,为开发具有木耳免疫多糖和复合产乳酸菌共存的新型微生态制剂新工艺提供理论依据。方法 （1）通过不同浸提时间,浸提次数,料液比以及温度的搭配,制定出一种含木耳多糖较高的木耳浸提液的制备方案。（2）筛选出生存能力强的双歧杆菌（Bf）和凝结芽胞杆菌（Bc）并绘制出其生长曲线以及菌落特征。（3）优化复合菌所用的培养基,探究Bf︰Bc（v/v）的最佳比例及添加量,及其达生长稳定期所需时间。结果 （1）浸提时间4 h,浸提1次,料液比1︰60,温度80℃;（2）得到了生存能力强的双歧杆菌和凝结芽胞杆菌各1株,并绘制出了其生长曲线及菌落特征;（3）优化复合菌所用的培养基：木耳汁200 g/L,蛋白胨10 g/L,酵母粉5 g/L,葡萄糖6 g/L,磷酸氢二钾2.0 g/L,硫酸锰50 mg/L,硫酸锌0.25 g/L,硫酸镁0.1 g/L;（4）复合菌Bf︰Bc（v/v）=1︰1;复合菌达生长稳定期需13h。结论：木耳浸提物对复合乳酸菌的生长有促进作用,并且选用的两种乳酸菌之间有相互促进作用。     

解淀粉芽孢杆菌M1摇瓶发酵条件优化及脱氮性能评价

旨在提高解淀粉芽孢杆菌M1液体发酵产芽孢量,并考察其对实际废水的反硝化脱氮效果。首先采用单因子实验研究了碳源、氮源、初始pH值、温度、转速和装液量等因子对M1液体发酵产芽孢量的影响。然后对其中显著性因子:氮源浓度、接种量、装液量、温度4个因素进行正交试验,进一步优化发酵条件。结果显示,优化后的培养基成分为:5 g/L碳源(可溶性淀粉)、10 g/L氮源(酵母粉∶蛋白胨=2∶1)、1 g/L NaCl;最佳培养条件为:初始pH6.5、发酵温度34℃、摇床转速180 r/min、培养瓶装液量30%、接种量7%。在此条件下,芽孢杆菌M1芽孢数可达到6.8×108 CFU/mL,高于优化前的2.08×108 CFU/mL。将芽孢杆菌M1投加于反应器中,与不加菌种相比,反硝化脱氮效果提升15%-34%。     

圆红冬孢酵母菌发酵产油脂培养基及发酵条件的优化研究

采用均匀设计和单因子试验法,系统考察了圆红冬孢酵母菌(Rhodosporidiumtoruloides)在不同碳氮比条件下产油发酵情况以及添加无机盐对产油发酵的影响,通过均匀设计软件对二次多项回归方程求解及单因素分析得知在培养基组成分别为葡萄糖70g/L,硫酸铵0.1g/L,酵母粉0.75g/L,磷酸二氢钾0.4g/L,七水硫酸镁1.5g/L,初始pH6.0,在灭菌(121℃15min)后添加ZnSO41.91×10-6mmol/L、CaCl21.50mmol/L、MnCl21.22×10-4mmol/L、CuSO41.00×10-4mmol/L。发酵摇瓶装液量为250mL三角瓶装培养基50mL,接种量为10%(种龄28h)。在上述条件下,30℃振荡(200r/min)培养120h,所得菌体油脂含量高达76.1%,脂肪得率系数可达22.7。     

冠突散囊菌发酵黑毛茶提取液的研究

以冠突散囊菌菌丝干质量为考察指标,以黑毛茶提取液为原料,对冠突散囊菌液态发酵培养基成分、发酵条件进行优化,并分析发酵过程中理化成分和功能成分的动态变化,比较发酵前后芳香性成分组成。得到的最佳培养基为9 g/L的黑毛茶提取液中添加90 g/L葡萄糖、7.5 g/L NH_4Cl和5 g/L CaCl_2;最佳发酵条件为250 mL摇瓶中装液量100 mL、接种冠突散囊菌孢子数2.4×10~6个(V(装液量)∶V(孢子悬液)=20∶1)、初始pH 4.0、28℃发酵8 d。在最优条件下发酵,发酵结束后菌丝干质量增加约10倍,发酵过程中发酵液中各成分呈现动态变化,茶多酚、总蛋白和水浸出物质量浓度分别减少了36.36%、53.80%和21.95%,总黄酮类、游离氨基酸和茶褐素质量浓度分别增加了14.40%、76.75%和5.08%,茶黄素、茶红素发酵前后含量都较低,芳香性成分增加了12种,多为酯类和醇类。     

植物乳杆菌发酵、冻干工艺及其益生特性的研究

目的以Lactobacillus plantarum SQ-2506为目标,研究该菌株的发酵、冻干工艺及其益生特性。方法通过对培养基中C源、N源和刺激因子的浓度改变考察对活菌数的影响,从而确定培养基的最佳配方;在确定最佳培养基后做出该菌的生长曲线以确定最佳发酵时间点;同时考察冻干保护剂的配方和预冷时间对菌粉活菌数的影响;此外,对植物乳杆菌进行产酸、产H_2O_2、生物膜形成能力、抑菌特性以及抗氧化能力的检测。结果最佳MRS培养基中葡萄糖浓度为0.8%、酪蛋白胨为0.4%、牛肉粉为0.6%、吐温为0.06%;植物乳杆菌的生长曲线在5h时达到稳定期,此时发酵液活菌数为3.16×10~9 CFU/mL,发酵液的pH为4.45。最佳冻干保护剂的配方:脱脂乳100g/L,蔗糖120g/L,抗坏血酸20g/L,谷氨酸钠30g/L;冻干前对上机液预冻时间为2h,此时菌粉冻干存活率为70.21%。该菌株具有产酸、产H_2O_2能力,并对大肠埃希菌、金黄色葡萄球菌和白色假丝酵母均有一定的抑制作用,形成膜能力较强,且具有一定的抗氧化能力。结论通过培养基成分、发酵条件和冻干工艺的优化以及对其益生特性的研究,为下一步新药开发和规模化生产奠定基础。     

重组大肠杆菌Bgl2238的发酵优化

本研究对前期实验室从黑龙江玉米土壤中筛选并构建的β-葡萄糖苷酶Bgl2238的重组大肠杆菌(E.coliBL21(DE3)-pET32a-bgl2238)采用响应面(Box-Behnken)优化的方法进行摇瓶发酵,优化培养基组分,而培养条件即温度、pH值、接种量及装液量则采用单因素法优化。结果显示最佳培养基配比为:甘油9.32g/L、酵母提取粉12g/L、胰蛋白胨19.13g/L、NaCl8g/L、K_2HPO_4·3H_2O 19.13g/L、KH_2PO_42g/L、柠檬酸高铁胺0.2g/L和微量元素母液6mL/L。重组大肠杆菌Bgl2238最佳的发酵条件为:发酵温度37℃、起始pH8.0、3%接种量、25mL装液量、IPTG终浓度为0.25mmol/L。在250mL锥形瓶对重组子Bgl2238进行发酵,在最优化的发酵培养基成分和培养条件下,Bgl2238的酶活力可以达到2910U/L,比起始培养基中的酶活提高了61.77%。     

益生菌Lactobacillus casei Zhang增殖培养基的优化

Lactobacillus casei Zhang 是一株分离自传统酸马奶中的益生菌.本文研究了不同碳源、氮源、碳氮比例、微量元素及缓冲盐对 Lactobacillus casei Zhang 增殖培养的效果,并采用响应面法对优选的碳源、氮源和缓冲盐类的组成含量进行优化,得到 Lactobacillus casei Zhang 的增殖培养基为:葡萄糖20.9 g/L、大豆蛋白胨10.45 g/L、酵母粉10.45 g/L、K2HPO4 3.5 g/L、醋酸钠14.6 g/L、柠檬酸钠2.3 g/L、MgSO4·7H2O 1 g/L,MnSO4·5H2O 54 mg/L、CuSO4·5H2O 10 mg/L、吐温80为1 g/L.Lactobacillus casei Zhang 在此增殖培养基中经37℃ 18 h培养活茵数可达到4.78×109 CFU/mL,比在MRS中(4.8×108 CFU/mL)提高近10倍.     

Anaerobic digestion of spent mushroom substrate under thermophilic conditions: performance and microbial community analysis

Applied Microbiology and Biotechnology - Spent mushroom substrate (SMS) is the residue of edible mushroom production occurring in huge amounts. The SMS residue can be digested for biogas production...     

Characterization of the steam-exploded spent Shiitake mushroom medium and its efficient conversion to ethanol

Spent Shiitake mushroom medium was subjected to steam explosion followed by simultaneous saccharification and fermentation (SSF) using Meicelase and Saccahromyces cerevisiae AM12. Water extraction of the medium exposed to steam at 20 atm for 5 min enhanced the saccharification rate by about 20% compared to steam-exploded medium before water extraction and resulted in the production of 23.8 g/l ethanol from a substrate concentration of 100 g/l. This corresponded to 87.6% of the theoretical ethanol yield, i.e., 15.9 g ethanol was obtained from 100 g of spent Shiitake mushroom medium. Spent Shiitake mushroom medium subjected to steam explosion and then water extraction appears to be a candidate for efficient bioconversion to ethanol.     

Novel fermentation media for production of Bacillus thuringiensis subsp. israelensis

The production of Bacillus thuringiensis subsp. israelensis (deBarjac) (Bti) as a biopesticide is not cost-effective using existing fermentation technology. In this study, we explored the use of several less expensive alternative culture media (potato, common sugar, and Bengal gram) for the growth and production of Bti. Growth was obtained in all tested media and was comparable to that obtained in conventional medium (Luria-Bertani). Toxicity assays showed that the toxin produced from the novel growth media were effective in killing larvae of Culex quinquefasciatus, Anopheles stephensi, and Aedes aegypti and toxicity was comparable to that produced from Luria-Bertani medium. These observations suggest that potato can be used as a cheap source of culture medium for the production of Bti toxin in mosquito control programs.     

Production of spent mushroom substrate hydrolysates useful for cultivation of Lactococcus lactis by dilute sulfuric acid, cellulase and xylanase treatment

Spent mushroom substrate (SMS) was treated with dilute sulfuric acid followed by cellulase and xylanase treatment to produce hydrolysates that could be used as the basis for media for the production of value added products. A L9 (3⁴) orthogonal experiment was performed to optimize the acid treatment process. Pretreatment with 6% (w/w) dilute sulfuric acid at 120 °C for 120 min provided the highest reducing sugar yield of 267.57 g/kg SMS. No furfural was detected in the hydrolysates. Exposure to 20 PFU of cellulase and 200 XU of xylanase per gram of pretreated SMS at 40 °C resulted in the release of 79.85 g/kg or reducing sugars per kg acid pretreated SMS. The dilute sulfuric acid could be recycled to process fresh SMS four times. SMS hydrolysates neutralized with ammonium hydroxide, sodium hydroxide, or calcium hydroxide could be used as the carbon source for cultivation of Lactococcus lactis subsp. lactis W28 and a cell density of 2.9 × 10¹¹ CFU/mL could be obtained. The results provide a foundation for the development of value-added products based on SMS.     

Improvement of Bacillus thuringiensis bioinsecticide production by sporeless and sporulating strains using response surface methodology

Statistical experimental designs, involving a Plackett-Burman design followed by a rotatable central composite design were used to optimize the culture medium constituents for Bacillus thuringiensis bioinsecticide production. This was carried out by using firstly an asporogenic strain and extrapolated to some sporeless and sporulating strains. Initial screening of production parameters was performed and the variables with statistically significant effects on delta-endotoxin production were identified: glucose, glycerol, yeast extract and MnSO(4). These variables were selected for further optimization by response surface methodology. The obtained results revealed that the optimum culture medium for delta-endotoxin production consists of 22.5 g/l of glucose, 4.8g/l of glycerol, 5.8 g/l of yeast extract and 0.008 g/l of MnSO(4). Under these conditions, delta-endotoxin production was 2,130 and 2,260 mg/l into 250 and 1,000 ml flask respectively, which represent more than 38% improvement in toxin production over the basal medium (1,636 mg/l). Such medium composition was shown to be suitable for overproducing delta-endotoxins by sporeless and sporulating strains.     

Inorganic phosphate has a crucial effect on Cry3Aa delta-endotoxin production

AIMS: The study aimed at increasing Cry3Aa delta-endotoxin production by a local isolate of Bacillus thuringiensis (B.t. strain Mm2). To this end, different nutritional conditions were tested for their effects on Cry3Aa yields. METHODS AND RESULTS: Bacillus thuringiensis Mm2 was grown by shaking at 30 degrees C in different media. Samples were taken from the cultures at intervals and used for protein extraction. SDS-PAGE was performed for toxin analysis. Inclusion of inorganic phosphate (Pi) into the Difco's sporulation medium at an increased level of 200 mmol l-1 caused a fivefold increase (from 3 to 15.6 microg ml-1) in toxin production. Omission of FeSO4 from the medium decreased this yield by half. Resuspension experiments suggested catabolite repression of toxin biosynthesis by glucose. The inclusion of high Pi invariably increased toxin synthesis, even in the absence of sugars. CONCLUSIONS: Inorganic phosphate had the most striking effect on toxin biosynthesis. Iron effect was found to be unique to our isolate whereas Pi effect seemed to be common to the biosynthesis of Cry3Aa-type toxins. Stimulation of toxin synthesis by Pi did not seem to represent a relief from glucose repression. SIGNIFICANCE AND IMPACT OF THE STUDY: Bacillus thuringiensis is the most versatile biopesticide for use in pest management. Regarding cost-effectiveness of related fermentations, high Pi supplement drastically increases Coleoptera-specific toxin synthesis.     

产几丁质酶的苏云金杆菌菌株筛选及酶合成条件研究

从本室保存的 64株苏云金芽孢杆菌中 ,筛选出一株几丁质酶活力较高的菌株WB 50。产酶条件研究表明 :在pH 7.0的基础培养基中添加 2 .0 %的细粉几丁质 ,1.0 %的酵母膏 ,2 2 0rpm 30℃下培养 72小时 ,几丁质酶的产出最大。     

富铬蚁巢伞（鸡菌）液体培养(英文)

A species of mushroom, Termitomyces albuminosus, was cultured in liquid medium for production of chromium-enriched mycelium. The influence of chromium (Ⅲ ) on mycelial growth of T. albuminosus was investigated. An optimum medium composed of 5.6g/L yeast extract, 51.6g/L hydrolyzed rice, 2g/L KH2PO4, and 20mg/L chromium(Ⅲ ) with initial pH of 4.5 was obtained by using method of central composite design (CCD). After incubation of 84h, the maximal biomass of chromium-enriched mycelia reached 24.23g DMW(dried mycelial weight)/L with 272μg/g DMW chromium content in 500mL flasks containing 100mL medium with an inoculum of 8% on a shaker of 100r/min under an optimized cultivation condition at 28℃.     

Fermentation broth of Bacillus thuringiensis as a source of precursors for production of nikkomycins

Production of nikkomycins (nucleoside antibiotics inhibiting chitin synthesis) by Streptomyces tendae (ATCC 31160) was considerably enhanced by addition of fermentation wastes of Bacillus thuringiensis var. kurstaki (HD 263) to the basal soymannitol medium. Analysis of this fermentation broth for nucleic acid derivatives showed that they contained about 0·8 g/l of various nucleosides and bases (uracil 0·43 g/l; hypoxanthine 0·21 g/l; as well as uridine, cytosine and adenine).     

Medium optimization of antifungal activity production by Bacillus amyloliquefaciens using statistical experimental design

In order to overproduce biofungicides agents by Bacillus amyloliquefaciens BLB371, a suitable culture medium was optimized using response surface methodology. Plackett-Burman design and central composite design were employed for experimental design and analysis of the results. Peptone, sucrose, and yeast extract were found to significantly influence antifungal activity production and their optimal concentrations were, respectively, 20 g/L, 25 g/L, and 4.5 g/L. The corresponding biofungicide production was 250 AU/mL, corresponding to 56% improvement in antifungal components production over a previously used medium (160 AU/mL). Moreover, our results indicated that a deficiency of the minerals CuSO(4), FeCl(3) · 6H(2)O, Na(2)MoO(4), KI, ZnSO(4) · 7H(2)O, H(3)BO(3), and C(6)H(8)O(7) in the optimized culture medium was not crucial for biofungicides production by Bacillus amyloliquefaciens BLB371, which is interesting from a practical point of view, particularly for low-cost production and use of the biofungicide for the control of agricultural fungal pests.