分枝杆菌Mycobacterium ZLP生产雄烯二酮（4-AD）的优化工艺

利用正交实验对分枝杆菌降解植物甾醇生产雄烯二酮（4-AD）的发酵培养基进行优化,同时进行温度和pH的优化。结果表明：培养基的最佳组成为质量分数2．0％葡萄糖、2．0％蛋白胨、0．7％MgSO4、0．8％K2HPO4;最适温度28℃、最适pH7．0,在此基础上发酵96h,4-AD的产率可达到62．15％。     

海洋Cellulophagasp．QY201产生ι-卡拉胶酶的发酵条件优化

目的：通过发酵条件优化,提高海洋Cellulophagasp．QY201的l-卡拉胶酶产量。方法：采用正交试验分别对发酵条件、培养基配方进行优化。结果：该菌株最适培养基配方为（w／v）：3％NaCl、0．5％MgSO4·7H2O、0．02％CaCl2、0．01％KCl、0．002％FeSO4、0．25％CaSein、0．15％Na2HPO4、0．2％NaNO3、0．25％L-卡拉胶。最佳培养条件为：培养基体积为70ml／250ml三角瓶,接种量为1％,25℃,90r／min培养36h。优化后酶活最高可达2．64U／ml,较优化前提高了22倍。结论：QY201最佳发酵条件的建立,为ι-卡拉胶酶的大规模生产创造了条件。     

产胞外木聚糖酶链霉菌发酵条件的正交试验

通过正变试验,设计出适合链霉菌（Streptomycessp.Strz—6）产胞外木聚糖酶的发酵条件,培养基（g／L）含麦草半纤维素5,NaNO31.67,酵母膏2,乳糖2,Tween801.5K2HPO4·3H2O1,MgSO4·7H2O0.5,NaCl0．3,微量元素B、Mn、Fe、Zn、Mo。接种量为1．4×108个孢子／50ml培养基,振荡,（120r／min）培养5d.     

手性拆分环氧氯丙烷菌株的筛选、鉴定及产酶条件研究

从土壤中筛选到5株环氧化物水解酶生产菌,并通过ITS序列鉴定了其中的C375菌,结果为黑曲霉（Aspergillus nigerZJB-09103）。考察了培养基不同碳源、氮源、金属离子和pH等对产酶的影响,得到了较佳的培养基条件：淀粉16g／L,豆饼粉3g／L,蛋白胨3g／L,KH2PO4 0．4g／L,K2HPO4 0．8g／L,MgSO4 0．2g／L,ZnSO4 0．03g／L,pH6．5。采用优化后的培养基条件,酶活力达到156．1U／L,比优化前初始发酵培养条件下的酶活提高了252％,当环氧化物水解酶催化时间为10h时,（s）-环氧氯丙烷的对映体过量值（e．e．）可达99．0％。产率为18．6％。     

土壤放线菌FX05发酵培养基及发酵条件的优化

以高氏1号培养基为基础,通过单因素分析和正交试验,对土壤放线菌FX05最佳培养基扣最优培养条件进行了研究。结果表明：适宜FX05产抑绿脓杆菌活性物质的发酵培养基配方为玉米粉1％、NaNO30．3％、K2HPO40．075％、MgS040．075％,发酵条件为初始pH为7．0,培养温度为28℃,培养96h产抑菌物质迭最大值。     

响应面法优化波赛链霉菌JMC 06001发酵培养基

采用响应面法对产生抑菌活性物质的波赛链霉菌（Streptomyces peucetius）菌株JMC 06001的发酵培养基进行优化。首先采用Minnimum Run Equireplicated Res IV设计对初始发酵培养基的8个营养因素进行筛选,获得影响产生抑菌活性物质的3个主要影响因素：葡萄糖、大豆粉和NaCI;然后用最陡爬坡实验快速逼近最大响应区域;最后,结合Box-Behnken设计及响应面分析,确定主要影响因素的最佳浓度,得出该菌株产抑菌活性物质的最优发酵培养基配方为：葡萄糖1．2％,麦芽糖0．7％,蛋白胨0．9％,大豆粉1．4％,NaCl3．7％,CaCO3 0．1％,复合盐A液2．0％,复合盐B液0．1％,起始pH值7．0。用优化后的培养基发酵所得发酵液对敏感指示菌藤黄八叠球菌的抑菌圈直径达31．5mm,与预测值的相对偏差仅为1．59％,与用初始发酵培养基发酵所得发酵液的抑菌效果（抑菌圈直径26．5mm）相比提高了18．9％。     

酪酸梭状芽孢杆菌低成本培养基的优化

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/L,豆粕（中性蛋白酶水解3h）20g／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8．2×10^8cfu／mL.培养基中添加K2HPO45g／L、MgSO4·7H2O0．2g／L、MnSO3·H2O0．2g/L培养32h时,酪酸梭状芽孢杆菌芽孢转化率可达95％。     

鱼腥藻SP.595液泡化原生质球诱导条件的研究

用浓度为0．15mol／L的KNO3、KCl、K2SO4、KH2PO4、K2HPO4、NaNO3、NaCl、Na2SO4、NaH2PO4、Na2HPO4、(NH4)2SO4、MgSO4、CaC12等单盐分别配合0．1％的溶菌酶处理鱼腥藻sp．595(Anabaenasp．595)。经4h,KH2PO4、K2SO4、Na2SO4、NaH2PO4、(NH4)2SO4、MgSO4、CaC12能诱导形成原生质球,但液泡化原生质球极少,而KNO3、NaNO3、NaC1诱导形成少量液泡化原生质球。用相近浓度的双盐,即KNO3和NaC1、KNO3和(NH4)2SO4、NaC1和(NH4)2SO4分别配合0．1％的溶菌酶处理,诱导效果亦不佳。用相近浓度的三盐NaC1、KNO3和(NH4)2SO4及五种盐NaC1、KNO3、(NH4)2SO4、Na2HPO4和KH2PO4分别配合0．1％的溶菌酶处理,诱导原生质球和液泡化原生质球的效果明显提高,液泡化原生质球比例达到66．90％—79．97％。     

酵母菌产麦角固醇发酵条件的研究

为了提高酵母菌麦角固醇的产量,采用摇瓶培养法,对筛选出的一株酵母菌YN2产麦角固醇发酵条件进行了研究。结果表明,酵母菌YN2产麦角固醇适宜的培养基配方为：酵母粉1％,牛肉膏2．5％,葡萄糖8％,K2HPO4 0．3％,MgSO4 0．15％,该菌株产麦角固醇最适培养条件为：培养温度28℃,起始pH6．5,发酵时间72h。在优化的实验条件下,麦角固醇含量可达2．2％,100ml发酵液中麦角固醇产量达25．30mg。     

响应面法优化毛霉菌发酵培养基

采用响应面分析方法优化毛霉菌B的发酵培养基,首先通过单因素试验筛选出葡萄糖为最适碳源,酵母膏和玉米浆为最适氮源,用Plackett—Burman试验对葡萄糖、酵母膏、玉米浆、MgSO4、FeSO4、NILCl/、HPO4进行评估并筛选出具有显著效应的3个因素：葡萄糖、酵母膏、玉米浆,再通过最陡爬坡试验逼近其最大响应区域,最后采用Box—Behnken试验对其用量进行优化,得到毛霉菌最佳发酵培养基（g/L）：葡萄糖51．54,酵母膏5．22,玉米浆14．31,MgSO40．5,FeSO40．1,NH4Cl3,k2HPO43,pH6．0～6．5。培养基优化后,毛霉生物量由23．51g／L提高至31．13g/L,比对照组提高32．41％,腺嘌呤转化率由53．59％提高至59．97％,ATP产率由6．56g／L提高至7．34g／L,比对照组提高11．89％。     

Screening strains for directed biosynthesis of β-d-mono-glucuronide-glycyrrhizin and kinetics of enzyme production

One fungus, tentatively named Penicillium sp. Li-3, was screened to biosynthesize β-d-mono-glucuronide-glycyrrhizin (GAMG), directly. Using glycyrrhizin as elicitor and the sole carbon source, this strain was capable of expressing β-d-glucuronidase, one intracellular enzyme with high substrate specificity. And glycyrrhizin was hydrolyzed directly into GAMG by enzyme from Penicillium sp. Li-3 with high production. It was found that the mol conversion ratio of this reaction was up to 88.45%. Research about kinetics of β-d-glucuronidase production showed that the cell growth and enzyme production of this strain was partial coupled. During the expressing of target enzyme, carbon catabolite repression existed, so only glycyrrhizin was the best carbon source as well as the elicitor. It was found that the surfactant (Tween 80 0.12%) could improve the ability of enzyme production markedly. Under the condition of initial pH 4.8 of the medium and 32 °C of the culture temperature, the maximum enzyme activity of 181.53 U ml⁻¹ was obtained.     

Effects of physico-chemical factors influencing tyramine production by Carnobacterium divergens

Tyramine production by a strain of Carnobacterium divergens was tested in relation to different conditions of pH, temperature, glucose, oxygen availability, potassium nitrate and sodium chloride content, using a combination of a Doehlert and Plackett-Burman experimental design. A second degree polynomial model was chosen to describe tyramine production which was quantified by high performance liquid chromatography. Maximal tyramine production occurred during the stationary phase in acidic conditions obtained by low initial pH (<5) or addition of glucose (0·6%) to the medium. Production was slower at 5°C than at 23°C and 10% sodium chloride inhibited this production. However, the formation of tyramine was not affected by the presence of potassium nitrate or oxygen availability.     

Screening strains for directed biosynthesis of β-d-mono-glucuronide-glycyrrhizin and kinetics of enzyme production

One fungus, tentatively named Penicillium sp. Li-3, was screened to biosynthesize β-d-mono-glucuronide-glycyrrhizin (GAMG), directly. Using glycyrrhizin as elicitor and the sole carbon source, this strain was capable of expressing β-d-glucuronidase, one intracellular enzyme with high substrate specificity. And glycyrrhizin was hydrolyzed directly into GAMG by enzyme from Penicillium sp. Li-3 with high production. It was found that the mol conversion ratio of this reaction was up to 88.45%. Research about kinetics of β-d-glucuronidase production showed that the cell growth and enzyme production of this strain was partial coupled. During the expressing of target enzyme, carbon catabolite repression existed, so only glycyrrhizin was the best carbon source as well as the elicitor. It was found that the surfactant (Tween 80 0.12%) could improve the ability of enzyme production markedly. Under the condition of initial pH 4.8 of the medium and 32 °C of the culture temperature, the maximum enzyme activity of 181.53 U ml⁻¹ was obtained.     

Isolation of a starch utilizing, phosphate solubilizing fungus on buffered medium and its characterization

A phosphate solubilizing fungus, Paecilomyces marquandii AA1 was isolated from phosphate deficient soil on Pikovskaya's medium buffered with Tris-HCl pH 8. The organism was identified on the basis of morphological characterization and by sequencing of 18S rRNA gene. The organism could release phosphate from both buffered and unbuffered medium and solubilized rock phosphates from various places. The effect of concentration of ore, temperature, carbon and nitrogen sources on solubilization of rock phosphate was studied. Ammonium salts were the best nitrogen source, followed by asparagine, sodium nitrate, potassium nitrate, urea and calcium nitrate in that order.     

含离子液体体系中固定化细胞转化甘草酸生成单葡萄糖醛酸基甘草次酸

研究疏水性离子液体1-丁基-3-甲基咪唑六氟磷酸盐([BMIM]PF6)与醋酸-醋酸钠缓冲液两相体系中,固定化产紫青霉Penicillium purpurogenum Li-3细胞转化甘草酸(GL)生成单葡萄糖醛酸基甘草次酸(GAMG)的反应,并与缓冲液单相体系作为对照.确定了在[BMIM]PF6/缓冲液两相体系中,最适离子液体加入比例、缓冲液pH、反应温度、底物浓度分别为10%、5.8、35℃和6.0mmol/L,在此条件下反应58h,甘草酸转化率为87.03%,比缓冲液单相体系提高了15.02%.离子液体循环使用8次后,回收利用率维持在85.28%.主产物GAMG和副产物甘草次酸(GA)在两相体系中得到有效分离,为后续产物分离带来便利.     

Statistical optimization of culture media for growth and lipid production of <Emphasis Type="Italic">Botryococcus braunii</Emphasis> LB572

Botryococcus braunii has an outstanding ability to produce lipid; however, it is a slow-growing green microalgae. Statistical optimization of growth media was performed to faster growth and to increase lipid concentration. The effect of media composition on the growth of B. braunii LB572 was examined using fractional factorial design and central composite design. The media components examined include sodium carbonate, potassium phosphate, calcium chloride, magnesium sulfate, ferric citrate, and sodium nitrate. The results indicated that potassium phosphate and magnesium sulfate were major impact factors. The optimum concentrations of potassium phosphate and magnesium sulphate were found to be 0.058 and 0.09 g/L, respectively, for growth and 0.083 and 0.1 g/L, respectively, for lipid production. These values were validated using bubble column photobioreactors. Lipid productivity increased to 0.19 g/L/day in lipid-optimized media, with an average biomass productivity of 0.296 g/L/day and 64.96% w/w. In growth-optimized media, lipid productivity was 0.18 g/L/day, with an average biomass productivity of 0.304 g/L/day and 59.56% w/w.     

Statistical optimization of medium composition for growth of<Emphasis Type="Italic">Leuconostoc citreum</Emphasis>

Leuconostoc citreum is one of the representative strains ofLeuconostoc spp. that show fast growth rates in fermented vegetables. Sequential experimental designs including the Plackett-Burman design, fractional factorial design, steepest ascent analysis, central composite design and response surface methodology were introduced to optimize and improve the medium forL. citreum. Fifteen medium ingredients were examined and glucose (20 g/L), yeast extract (12.5 g/L), sodium acetate trihydrate (6.12 g/L), potassium phosphate (42.55 g/L) and dibasic ammonium citrate (4.12 g/L) were chosen as the best components to give a critical and positive effect for cell-growth. The biomass was increased to 2.79 g/L (169%), compared to the 1.65 g/L in MRS medium.     

Optimization of culture medium for enhanced production of exopolysaccharide from Aureobasidium pullulans

Polysaccharides produced by microorganisms are utilized for a variety of purposes, including the use in cosmetics and as food additives. More recently, polysaccharides have been exploited by the medical and pharmaceutical industries, and those originated from many species of mushrooms have been especially useful in industrial applications; however, the production and synthesis of these compounds is costly and time consuming. In this study, we developed a method for low-cost production of exopolysaccharide (EPS) that effectively screens components and optimizes medium composition using statistical methods (Plackett-Burman and Box-Behnken design). As a result, we obtained the following optimized medium: sucrose 165.73 g/L, sodium nitrate 3.08 g/L, dipotassium phosphate 1.00 g/L, potassium chloride 0.50 g/L, magnesium sulfate 0.50 g/L, ferrous sulfate 0.01 g/L, and 0.71 g/L of Ashbya gossypii extract. The maximum production of about 29 g/L EPS was achieved in the optimized medium during 84 h batch fermentation.     

细菌素发酵培养基的优化及动力学初步分析

用响应面方法对Lactococcus lactis生产细菌素乳链菌肽的培养基进行了优化。首先用部分重复因子实验对培养基组份蔗糖,大豆蛋白胨,酵母粉,KH₂PO₄,NaCl,MgSO₄·7H2O对乳链菌肽的影响进行评价,并找出主要影响因子为大豆蛋白胨和磷酸二氢钾,前者为负影响,后者为正效应,其它组份对乳链菌肽产量的影响不显著。第二步用最陡爬坡路径逼近最大响应区域。最后用中心组合设计及响应面分析确定主要影响因子的最佳浓度。菌株在优化培养基中的乳链菌肽产量增加1倍为2150(IU/mL)。动力学分析表明,菌株生长与细菌素的产生为部分耦联型,进入对数中期菌体比生长速率和细菌素比产率在优化培养基中均大于优化前培养基。     

Bacteria of the genus Acinetobacter. Methods for their isolation and primary identification

A liquid accumulation medium and a solid isolation medium for primary identification of bacteria of the genus Acinetobacter have been proposed. Both media have identical composition and contain ethanol as the only source of carbon and energy and sodium ammonium phosphate as the source of nitrogen. Besides, the modification of Baumann's medium with sodium acetate as the source of carbon and potassium nitrate as the source of nitrogen has been developed. This modified medium has simplified composition and is not inferior to the above-mentioned media in selectivity, though its use gives less satisfactory results. The two proposed media, both liquid and solid, are recommended for wide use.