产β-甘露聚糖酶菌株的筛选鉴定及产酶条件的优化

利用刚果红染色法从土壤中筛选到一株产β-甘露聚糖酶的菌株MY271,该菌株经形态学、生理生化及系统发育学方法鉴定为路德维希肠杆菌(Enterobacter ludwigii)。该菌株在初始条件下培养48 h,发酵上清液中β-甘露聚糖酶酶活可达2.87 U/m L。利用单因素试验对该菌产酶发酵条件进行优化以提高酶活,优化所得最佳发酵条件为:接种量9%,装液量50 m L/250 m L,初始p H7.0,发酵温度31℃,发酵周期48 h。最佳碳源为魔芋精粉(添加量0.8%),最佳氮源为蛋白胨(添加量1.9%)。在最佳条件下发酵48 h,发酵上清液中β-甘露聚糖酶活提升到38.42 U/m L,是优化前的13.4倍。     

洋葱伯克霍尔德氏菌Lu10-1产脂肪酶发酵条件优化及酶学性质研究

旨在对洋葱伯克霍尔德氏菌(Burkholderia cepacia)Lu10-1产脂肪酶的发酵条件及酶学性质进行研究。通过单因素和正交实验探讨了碳源、氮源、诱导物、初始p H值、温度等主要发酵参数的影响,并初步考察了温度、p H、金属离子和有机溶剂等对其催化反应的影响。结果表明,B.cepacia Lu10-1产脂肪酶最佳培养基组成和发酵参数为:可溶性淀粉1.5%,蛋白胨1.5%,橄榄油3 g/L,K2HPO4 2 g/L,发酵温度32℃,初始p H 9.0,培养48 h酶活达12.4 U/m L,比初始酶活提高了2.7倍。酶的最适温度和p H值分别为60℃和9,在60℃以下保持100 h酶活仍保持在80%以上,在p H5.0-10.0之间活性稳定,对甲醇、乙醇等有机溶剂耐受性好。     

MntH与含锰过氧化氢酶共表达基因工程菌的构建与发酵优化

构建Mn2+转运蛋白MntH与来源于Thermus thermophilus HB27的含锰过氧化氢酶的共表达基因工程菌,并进行了发酵培养基及培养环境条件的优化,确定培养基中最佳的碳氮源种类及其浓度分别为:甘油7.0 g/L,酵母粉3.75 g/L和蛋白胨11.25 g/L;当培养基中的Mn2+浓度为1 mmol/L时,最佳的IPTG诱导浓度为0.05 mmol/L。此外,最佳的培养基初始p H值及培养温度分别为:p H 8.0和37℃,在最优发酵条件下工程菌摇瓶发酵培养24 h,过氧化氢酶活最高可达476 U/m L是未优化前3倍。在5 L发酵罐的验证实验中,过氧化氢酶的酶活进一步提高至1 094 U/m L。     

产几丁质酶菌株S68-CM5产酶条件优化研究

为提高黏质沙雷氏菌株S68-CM5产几丁质酶能力,对产酶发酵条件进行优化研究。利用Plackett-Burman设计和响应面法对培养基和发酵条件进行摸索。结果显示,获得最佳发酵产酶培养基:胶体几丁质1.5%,牛肉膏7 g/L,酵母膏2 g/L,葡萄糖8 g/L,氯化钠3.5 g/L,蛋白胨2 g/L,磷酸氢二钾3.5 g/L;最佳产酶培养条件为:p H6.88,温度27.32℃,摇床转数155.82r/min,培养时间60 h,接种量1%,装液量50 m L/250 m L。优化后产酶量达到7.131 U/m L,比优化前产酶量提高了1.43倍。     

1株抑制土传病原菌且产纤维素酶芽胞杆菌筛选及产酶条件的研究

通过刚果红染色法和DNS分光光度法对6种芽胞杆菌分泌胞外纤维素酶进行筛选,再通过管碟法测试对5种病原菌的抑菌作用,得到1株芽胞杆菌（菌株编号为X-02）酶活达182.5 U/mL,而且对几种土传病害有抑制作用。并对其产酶发酵培养基碳源、氮源及初始pH、发酵温度、接种量、摇瓶转速和时间进行优化,结果显示该菌株最佳碳源是2%CMC-Na,其次是葡萄糖,二者产酶之差只为21 U/mL。考虑大量生产的成本和方便性（CMC-Na溶解慢）,选择葡萄糖为碳源,氮源为2.0%蛋白胨与酵母膏复合氮源,在pH值为8.0、温度37℃、接种量为2%、转速为180 r/m in、时间48 h条件下酶活达到391.0 U/mL酶液,比优化前提高了2.1倍。     

茶树内生真菌CSN-4产漆酶培养基及培养条件研究

从茶树内生真菌筛选产漆酶的菌株,分析不同营养因素和培养条件对菌株漆酶酶活力的影响。采用6种显色底物的平板初筛和酶活测定的复筛方法,从15株茶树内生真菌菌株中筛选获得1株产漆酶酶活较高的菌株CSN 4。单因素分析结果显示,液态发酵条件下菌株CSN-4适宜的主要培养基成分是麸皮和蛋白胨;菌株CSN-4分别在麸皮30 g/L、蛋白胨2.5 g/L、CuSO₄·5H₂O 0.015 g/L和茶水6 g/L时发酵产漆酶酶活最高。发酵条件试验结果表明,菌株CSN-4分别在接种量为6个菌饼（直径6 mm）、装液量60 mL/250 mL、pH 4.8、摇床转速120 r/min,培养温度为28 ℃时产漆酶酶活较高。在培养基中添加麸皮和茶水对菌株CSN-4产漆酶有明显的促进作用。经过培养基成分及培养条件优化后,菌株CSN 4产漆酶酶活显著升高,达到2 417 U/L。     

红树林微生物DH-2胞外蛋白酶的性质及产酶条件优化

从大亚湾红树林土壤样品中分离得到产蛋白酶菌株,鉴定所产胞外蛋白酶的酶学性质以及菌株的最佳发酵培养条件。采用平板透明圈法筛选菌株,福林酚显色法测定蛋白酶的酶活,通过单因素和正交试验确定其最佳发酵培养基以及发酵条件。从壤样品中分离得到一株产蛋白酶的枯草芽孢杆菌DH-2,该菌株分泌的蛋白酶最适反应pH和温度分别为8.0和65℃,50℃保温处理60 min后,剩余酶活仍保留80%以上。该蛋白酶对多种金属离子、有机溶剂及表面活性剂均有较好的耐受性。确定该菌株产蛋白酶的最适条件:1%(m/V,下同)可溶性淀粉,1%胰蛋白胨、1%NaCl,初始pH 5.5及7%的接种量,40℃培养36 h。在最适条件下测得其发酵液的酶活为236.30 U/mL,约为初筛时的酶活的8倍。该蛋白酶具有较为广阔的作用温度和pH范围,金属离子、有机溶剂及表面活性剂耐受性好,酶的性质比较稳定。     

哈茨木霉产β-1,3-葡聚糖内切酶的发酵工艺条件研究

对哈茨木霉(Trichoderma harzianum GIM 3.442)产β-1,3-葡聚糖内切酶的液体发酵条件进行了单因素优化实验,确定了最佳培养基成分和培养条件,在此基础上通过正交试验设计对复合碳源(葡萄糖、茯苓多糖)、胰蛋白胨、Na NO3和磷酸盐进行了L9(34)试验,研究了4种因素对哈茨木霉产酶的影响,确定了最佳培养条件:葡萄糖42.0 g/L,茯苓多糖18.0 g/L,胰蛋白胨15.0 g/L,Na NO35.0 g/L,初始p H 6.0,接种量8%,28℃,110 r/min培养6 d。优化后总酶活Etotal和β-1,3-葡聚糖内切酶Eendo活力达到了471.6 U/m L和327.4 U/m L,比优化前分别提高了7.3倍和23倍,且内切酶占总酶活的比例Eendo/Etotal由0.24增加到0.71,效果显著。     

漆酶高产菌株的诱变选育及其产酶条件

以粗毛栓菌Trametesgallica为出发菌,通过紫外诱变处理其担孢子、PDA-RBBR平板变色法初筛、ABTS法测定培养液漆酶酶活力复筛,获得1株漆酶高产诱变菌株SAH-12。用高氮低碳无机盐培养液(LM3)培养时,其峰值酶活力比出发菌株高出4倍,达到5002.6U/L,且产酶稳定。对SAH-12液体培养产酶条件的研究表明:以纤维二糖和蔗糖为碳源明显优于麦麸、淀粉和葡萄糖,其最高酶活分别达18526U/L和13436U/L;有机氮源较无机氮源更有利于SAH-12漆酶的分泌,以蛋白胨、大豆粕和胰化蛋白胨为氮源时其峰值酶活分别达到20544U/L、19671U/L和16180U/L;适宜初始培养pH为4.0;ABTS、单宁酸、没食子酸对产酶均有明显的诱导作用,其中ABTS和单宁酸的诱导效果相对更好,愈创木酚和吐温80对产酶有一定的抑制作用。     

粘质沙雷氏菌产几丁质酶发酵条件的研究

目的：通过对粘质沙雷氏菌发酵条件的优化,提高其产几丁质酶的能力。方法：以实验室保存菌种粘质沙雷氏菌S418为对象,通过单因素试验和三因素三水平正交试验筛选出了菌株S418产几丁质酶的最佳培养基配方及培养条件。结果：该菌种产酶的最佳发酵条件：0.2%（w/v）胶体几丁质,1%蛋白胨,0.05%KH2PO4,在28℃、pH7.0、接种量6%,培养72h,酶活达到5.49U/mL。结论：优化后菌株S418产几丁质酶的条件。     

桑黄液体发酵工艺的研究

通过对桑黄液体发酵培养基、培养条件优化实验研究,以获得具有与桑黄子实体相似功效成分的桑黄菌丝体液体发酵工艺。以菌丝体收率为主要考察指标,采用单因子及L9(34)正交实验的方法,对桑黄液体发酵培养基及培养条件进行优化,确定桑黄液体发酵工艺条件。桑黄液体发酵最佳培养基及培养条件:玉米粉2%,葡萄糖3%,酵母膏0.5%,蛋白胨0.5%,KH2PO40.3%,Mg SO4·7H2O 0.15%,VB120μg/100 m L,p H5.5,接种量8%,培养温度28℃,摇床转数180 r/min,培养周期82 h。优化条件下所获得桑黄菌丝体粉为土黄色,菌丝体平均得率为1.67%,菌丝体黄酮含量(0.84%)与桑黄子实体(0.88%)相当,菌丝体多糖含量(5.15%)是子实体(1.71%)的3倍。可见,该桑黄液体发酵工艺具有较大的推广应用价值。     

一株虫草头孢菌深层培养条件的研究

采用摇瓶培养的方法,以菌丝体收率为指标,通过单因子实验和正交实验确定了虫草头孢菌最佳培养条件和最佳发酵培养基配方。在相同条件下,优化培养基比原培养基的菌丝体收率提高了31.75%。     

紫色红曲霉Mp-24高产Monacolin K发酵工艺响应面优化

将单因素实验结果与响应面法相结合,对高产Monacolin K的紫色红曲霉Mp-24菌株进行发酵工艺条件优化。通过摇瓶发酵对碳源、氮源、碳源含量、氮源含量、培养时间等进行单因素优化,确定Mp-24菌株摇瓶发酵适宜条件：乳糖为碳源、酵母膏为氮源、碳源含量7%、氮源含量2%、培养时间12 d,Monacolin K产量为167 mg/L。应用Box-Behnken中心组合试验设计建立数学模型,进行响应面分析优化发酵条件,结果显示最佳发酵工艺条件为：碳源(乳糖)8%,氮源(酵母膏)3%,培养时间11 d,在此条件下Monacolin K的含量达到247.8 mg/L,比优化前提高1.5倍。     

米曲霉M-4降解己烯雌酚的条件优化

【目的】以米曲霉(Aspergillus oryzae)M-4对己烯雌酚(Diethylstilbestrol,DES)的降解率为响应值,对其降解条件进行优化。【方法】采用Plackett-Burman法对培养基组分和降解条件筛选显著性影响因素,并通过Box-Bohnken设计试验优化降解条件。【结果】最优培养基配方为:蛋白胨1.3%,CaCl_2 0.045%,葡萄糖0.5%,K_2HPO_4 0.15%,KH_2PO_4 0.05%,NaCl 0.05%,Tween 80 0.2%,DES质量浓度44 mg/L;最优培养条件为:初始p H 7.5,种龄72 h,转速140 r/min,培养温度28°C,培养时间72 h。【结论】在最优条件下菌株M-4对DES降解率为83.89%,比优化前(60.98%)提高1.38倍,差异极显著(P0.01)。     

球形红杆菌积累聚β-羟基链烷酸(PHA)的研究

通过对球形红杆菌(Rhodobacter sphaeroides)生长和积累聚卢-羟基链烷酸(PHA)条件的研究,确定采用两段培养法提高PHA的产量。第一阶段提供适合菌体生长的条件:以葡萄糖作碳源,尿素为氮源,光照微好氧培养。第二阶段则提供使菌体积累PHA的条件:补加乙酸钠厌氧光照培养。经两段培养后菌体PHA含量可占细胞干重的45％,PHA产量每升发酵液可达1.7g。     

Study of the Conditions for the Biosynthesis of Bacterial Cellulose by the Producer <Emphasis Type="Italic">Medusomyces gisevii</Emphasis> Sa-12

The effect of culture conditions on the bacterial cellulose (BC) yield synthesized by symbiotic culture Medusomyces gisevii Sa-12 grown in synthetic nutrient medium was studied for the first time. The conditions providing the maximum yield of bacterial cellulose were evaluated: the initial glucose concentration in the culture medium was 20–25 g/L, the temperature was 24–27°C, the ratio of the nutrient medium to the air volume was 1: 10, and the content of the black tea extracts comprised 1.6–4.8 g/L. A sample of chemically pure BC with the following characteristics was obtained under the selected culture conditions: moisture— 99.0%, degree of polymerization—4800, average width of microfibrillar ribbons—30.6 nm, degree of crystallinity— 86%, and the content of triclinic modification Iα—98%.     

Optimization of submerged culture conditions for mycelial polysaccharide production in Cordyceps pruinosa

Cordyceps pruinosa is an entomogenous fungus noteworthy for its various bioactivities. The influence of synthetic medium and cultural conditions on polysaccharides production was investigated in shake flask culture. In the present study, optimal medium and submerged culture conditions were investigated using an orthogonal layout. Media and cultural conditions including potato starch 2% (w/v), sucrose 2.5%, soybean 0.5%, beef extract 0.5%, yeast extract 0.1%, KCl 0.02%, K₂HPO₄ 0.1%, MgSO₄·7H₂O 0.05%, pH 7.0, inoculum size 5%, medium capacity 50 ml/250 ml flask, dispersant 15 beads, culture time 7 days were employed. In fermentation medium, sucrose, beef extract and yeast extract were replaced with molasses of sucrose, groundnut and Vitamin B complex, respectively. Under optimal culture conditions, the yield of polysaccharides production was 9.51 g l⁻¹ after 54 h of fermentation in a 25 l fermenter, which was approximately twice as high as that in shake flask cultures. In addition the entire period of fermentation was shorted to around 1/4 of flask culture time (9 days). Thus, it will meet closely the requirements of industrial fermentation scale of polysaccharides production in C. pruinosa.     

Isolation and propagation of keratinocytes derived from Cashmere goat fetus

The study was conducted to isolate epidermal keratinocytes from Cashmere goat fetus with the aim to develop suitable conditions for keratinocyte cultivation and propagation. The methods developed for keratinocyte culture include (i) use of a feeder-layer of mitotically inactivated fibroblasts obtained from goat and mouse fetal skin, (ii) use of a substrate such as collagen IV, or (iii) without use of any substrate. Epidermal cell removal was established by enzymatically separating keratinocytes from 12 to 16 weeks aged fetal skin tissues treated with 0.125% trypsin solution overnight at 4 degrees C. The cells were maintained in all culture conditions with serum containing medium. Keratinocyte multiplication and proliferation were comparable in different culture conditions and the improved cellular attachment and growth have been obtained in cultures on feeder layers. Colony forming keratinocytes on feeder layer were heterogeneous in their growth potential. In feeder free conditions, high cellular density was required at plating for sub-cultivation as their poor attachment in culture dishes. This study reports the comparative efficacy of different culture conditions for keratinocyte isolation and in vitro propagation originating from Cashmere goat fetus.     

甲烷利用菌培养条件的优化及其初步应用

利用统计学实验设计（RSM）对能够利用甲烷的假单胞菌菌株ME16主要培养条件进行了优化。以液体无机盐和甲烷气体作为培养基分别进行了温度、接种量、甲烷含量和培养pH对细菌生长影响的研究,并在此基础上,利用响应面法分析优化了ME16菌株的主要培养条件,得到最佳培养条件为：温度29.4℃,接种量1.8%,甲烷含量25%。采用优化培养条件进行培养,细菌生物量增大0.8倍,达到稳定期的培养时间缩短了50h。该菌株初步应用于甲烷气体的脱除,脱除率达65.7 %,表明该菌株能良好的脱除空气中甲烷。     

Optimum Culture Conditions for Production of Exfoliative Toxin by Staphylococcus hyicus

Optimum culture conditions for the production of exfoliative toxin by Staphylococcus hyicus (shET) were examined. High shET activity was obtained from the culture filtrate of HI and TY broth inoculated with S. hyicus. The pH in these two media ranged from 7 to 8.5 during bacterial culture, while the lowest pH in TS and BHI broth was less than 6. shET activity in the culture filtrate from TY broth inoculated with 10⁷ CFU of S. hyicus per ml was higher than that in TY broth inoculated with 10⁶ and 10⁸ CFU of bacteria per ml. When shET activity in the culture filtrate was measured under various shaking conditions, the culture filtrate shaken at 75 oscillations per min had the highest shET activity of the five shaking conditions. shET activity of the culture filtrate of TY broth to which protease inhibitor had been added was the same as that of TY broth without inhibitor. shET activity in a shaking culture in an Erlenmeyer flask was also the same as that in sac culture and that in shaking culture using a shaking (Sakaguchi) flask. shET activity in TY broth supplemented with 100 mM glucose was significantly lower than that in TY broth without glucose. Based on the above results, the optimum culture conditions for the production of shET were as follows: inoculation of 3 × 10⁹ CFU of S. hyicus strain P-1 into 300 ml of TY broth in a 2,000-ml Erlenmeyer flask, and incubation at 37 C with shaking at 75 oscillations per min. Then shET activity of the culture filtrate under appropriate culture conditions was measured after various incubation periods. shET activity was detected 6 hr after inoculation, reached the maximum (2⁵³ exfoliative unit/0.1 ml) at 16 hr and decreased between 20 and 48 hr. Thus, the optimum incubation period was determined to be 16 hr. Then the optimum concentration of ammonium sulfate for isolation of shET from the culture filtrate under appropriate culture conditions was examined. The greatest shET activity was obtained from the fraction salted out with 90% saturated ammonium sulfate. Thus, the optimum concentration of ammonium sulfate for the isolation of shET was determined to be 90% saturation.