营养物质对桑黄菌丝生物量及胞外多糖产量的影响

研究了不同碳源、氮源和无机盐对桑黄深层培养菌丝生物量和胞外多糖产量的影响,结果表明：在培养温度为26℃、摇床转速为160r／min、发酵时间为10d的条件下,以桑黄菌丝生物量为指标,最适碳源、氮源和无机盐分别是果糖或葡萄糖、酵母粉或酵母膏、KH2P04或MgSO4·7H2O;菌丝生物量分别达到1．51、1．31、1．69、1．52、1．52、1．36g／100mL;以胞外多糖为指标,最适碳源、氮源和无机盐分别是葡萄糖、酵母膏、ZnSO4·7H2O,胞外多糖产量分别达到0．49、0．45、0．22g／100mL。     

高产大豆异黄酮糖苷水解酶菌株的发酵工艺研究*

Absidia sp．R是从酒曲中分离出的一株产大豆异黄酮糖苷水解酶活性较高的菌株。该菌最佳产酶条件为：2．5％的麦麸为碳源,1％的硝酸钠为氮源,培养基起始pH为7．0,瓶装量为40mL/250mL,接种量8％,培养温度为30℃,转数为160r／min,培养时间为84h,其酶活力可达到82U／mL。除Cu^2 对该菌产酶有较强的抑制作用外,金属离子对产酶影响不大。     

曲霉M—2降解有机磷农药(甲胺磷)的研究

分离了一株能降解甲胺磷的曲霉Ｍ－２。Ｍ－２能以甲胺磷为唯一碳源、氮源及磷源生长。在０．２％甲胺磷无机盐发酵液中,培养５ｄ后,降解率达８１．５％。添加少量有机氮能促进Ｍ－２对甲胺磷的利用。     

几丁质酶产生菌的筛选及产酶条件的研究*

从301株几丁质降解菌包括细菌、放线菌和真菌中,筛选出一株产几丁质酶活力较高的链霉菌A048(Streptomycessp．A048)。其产酶的适宜条件是,培养温度30℃,培养基pH7．0～7．5,碳源几丁质,氮源NH4NO3,体积溶氧系数kd值为1．56×10-6mol／(mL·min·atm),振荡培养120h,产酶可达15．1U／mL。     

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％。     

利用海洋微生物降解有机磷农药MAP的研究

目的分离及筛选降解海水养殖区甲胺磷的降解菌,并确定最适的降解条件。方法从被有机磷污染的海水样中分离,以有机磷为唯一碳源反复驯化,分离筛选出1株高效降解甲胺磷的菌株M-1,并对其降解能力和所需条件进行测试。通过离子交换层析、凝胶过滤层析等方法从发酵液中分离纯化了有机磷农药降解酶。结果初步鉴定菌株M-1属于腊样芽胞杆菌。菌株M-1最适生长温度和pH分别为25℃和8．0。Zn^2＋（200mg／L）、Cd^2＋（50mg／L）与Pb^2＋（200mg／L）不影响菌株M-1对甲胺磷的降解作用,但Cu^2＋（50mg／L）、Cr^2＋（50mg／L）对菌株M-1有毒性作用。SDS-PAGE测得降解菌的有机磷农药降解酶的分子质量约为45kD。结论海洋微生物在甲胺磷污染的海水养殖区自净中起着重要作用。     

绿色糖单孢菌降解木质纤维胞外酶的分泌条件及其生物漂白研究

以一株耐热耐碱放线菌-绿色糖单孢菌（Saccharomonospora viridis）为研究对象,探讨其产胞外木素过氧化物酶、木聚糖酶、纤维素酶的优化发酵条件。结果表明,其最佳碳氮源分别为葡萄糖和蛋白胨,最佳接种量为1％,不同的诱导底物对三种木质纤维降解酶有不同的诱导效果,其中麦草浆的诱导效果最好。在培养基中添加0．01mol／L的Mn^2＋和0．1％的土温80能够显著促进木质纤维降解酶的产生。在pH8．0,45℃条件下,培养120h后木素过氧化物酶的酶活达到最大0．36U／mL,培养156h后木聚糖酶和纤维素酶的酶活达到最大,最高酶活分别为18．46U／mL,10．42u／mL。用含有这三种酶的粗酶液对麦草烧碱蒽醌浆进行生物漂白表明,绿色糖单孢菌所产的木质纤维降解酶具有较好的漂白效果。     

甲胺磷降解细菌的分离鉴定及其降解效能的研究

从土壤中分离筛选获得两株对甲胺磷农药有较强降解效能的细菌,经鉴定分别为头状葡萄球菌(Staphylococcus capitis)(称为D菌)和粪产碱菌(Alcaligenes faecalis)(称为J菌)。D菌和J菌在甲胺磷浓度为500mg.L-1,30℃,180r.min-1摇床上用基础培养基中培养72h,对甲胺磷的降解率分别达到58.49%和65.80%。D菌和J菌混合培养可提高对甲胺磷的降解效能,对甲胺磷72h的降解率达到72.93%。     

层孔菌产漆酶的摇瓶最适培养条件研究

筛选到一株高产漆酶的层孔菌W－1,对其兴体产漆酶的培养条件进行了优化,确定了最适的碳源、氮源,并用正交试验确定了培养基中碳源和氮源的浓度。在最优化的培养条件下,培养7d后,W－1产生的漆酶活力可以达到7．1U／mL。采用补料的方法,可以得到大量的漆酶粗酶液。     

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％。     

根霉12号固体发酵产生纤溶酶工艺条件的研究*

研究了根霉12号固体发酵产生纤溶酶的工艺条件。采用单因素试验、均匀设计方法对固体发酵培养基的碳源、氮源、碳氮比、初始pH、加水量、无机盐加量进行了优化;采用正交试验对发酵时间、接种量进行了研究。结果表明,实验范围内根霉12固体发酵产纤溶酶的适宜培养基组成为:麸皮∶豆粕=1∶2,初始pH5.0,加水量0.75ml/g物料, MnSO4H2O和 (NH4)2SO4加量分别为0.25%和 1.42%(对物料)。适宜培养条件为接种量107个孢子/g物料,培养时间72h。优化条件下的纤溶酶产量平均达791.81u/g物料。     

非水溶性甲胺磷降解酶的检测

甲胺磷农药是一种水溶性广谱、剧毒杀虫剂,化学名称：Ｏ,Ｓ－二甲基胺基硫代磷酸酯．目前,它在我国的生产和使用量已相当可观,并由此造成了严重的生态破坏和环境污染［１］．近几年,作者针对上述问题,结合国内外对甲胺磷代谢和有关酶知识缺乏了解的实际［２］,开展...     

碳源和氮源对彩绒革盖菌液体发酵合成漆酶的影响

研究了碳源、氮源对彩绒革盖菌液体发酵合成漆酶的影响。结果表明,在所选的几种碳、氮源中,麸皮为试验菌株合成漆酶的较好碳源;酵母浸膏、酒石酸铵、蛋白胨均是比较理想的氮源。不同的碳氮比对彩绒革盖菌漆酶的产量有着显著的影响,高碳高氮是其生产漆酶的最佳条件。在适宜的培养条件下该菌株能合成高活力的漆酶,其酶活力可达298 U/mL以上,产酶周期为6~7 d。     

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。     

Utilization of carbon and nitrogen sources and acid/alkali production by cowpea rhizobia

Summary Sixteen slow-growing strains of rhizobia (15 cowpea rhizobia and oneR. japonicum) were examined to determine the effects of carbon and nitrogen sources on acid/alkali production in culture media. We found that the pH changes of the medium were more influenced by nitrogen sources than carbon sources (with the exception of ribose). When ammonium sulphate was used as a nitrogen source, all the cowpea rhizobia strains produced acid. When yeast-extract was used as a nitrogen source, however, a heterogenous pattern for acid/alkali production was found. The majority of the strains produced alkali from nitrate, glutamate and urea irrespective of carbon sources and acid from ribose irrespective of nitrogen sources.     

Production of scleroglucan from Sclerotium rolfsii MTCC 2156

Scleroglucan, a neutral homopolysaccaride consisting of a linear chain of beta-D-(1-3)-glucopyranosyl and beta-D-(1-6)-glucopyranosyl groups, was produced by pure culture fermentation from Sclerotium rolfsii MTCC 2156 by submerged culture. Fermentation process was optimized in two steps. In the first step, one-factor-at-a-time method was used to investigate the effects of medium constituents such as carbon and nitrogen sources. In the second step, concentration of medium components was optimized using an L16-orthogonal array method. In all, 10 different carbon sources and eight different nitrogen sources were evaluated. Maximum yield of 16.58 g/l was obtained in a medium containing sucrose as a carbon source and sodium nitrate and yeast extract as nitrogen source.     

Exopolysaccharide production and mycelial growth in an air-lift bioreactor using Fomitopsis pinicola

For effective exopolysaccharide production and mycelial growth by a liquid culture of Fomitopsis pinicola in an air-lift bioreactor, the culture temperature, pH, carbon source, nitrogen source, and mineral source were initially investigated in a flask. The optimal temperature and pH for mycelial growth and exopolysaccharide production were 25degrees C and 6.0, respectively. Among the various carbon sources tested, glucose was found to be the most suitable carbon source. In particular, the maximum mycelial growth and exopolysaccharide production were achieved in 4% glucose. The best nitrogen sources were yeast extract and malt extract. The optimal concentrations of yeast extract and malt extract were 0.5 and 0.1%, respectively. K2HPO4 and MgSO4 x 7H2O were found to be the best mineral sources for mycelial growth and exopolysaccharide production. In order to investigate the effect of aeration on mycelial growth and exopolysaccharide production in an air-lift bioreactor, various aerations were tested for 8 days. The maximum mycelial growth and exopolysaccharide production were 7.9 g/l and 2.6 g/l, respectively, at 1.5 vvm of aeration. In addition, a batch culture in an air-lift bioreactor was carried out for 11 days under the optimal conditions. The maximum mycelial growth was 10.4 g/l, which was approximately 1.7-fold higher than that of basal medium. The exopolysaccharide production was increased with increased culture time. The maximum concentration of exopolysaccharide was 4.4 g/l, which was about 3.3-fold higher than that of basal medium. These results indicate that exopolysaccharide production increased in parallel with the growth of mycelium, and also show that product formation is associated with mycelial growth. The developed model in an air-lift bioreactor showed good agreement with experimental data and simulated results on mycelial growth and exopolysaccharide production in the culture of F pinicola.     

蛹虫草菌丝产虫草素液体培养条件的研究

通过对蛹虫草菌丝产虫草素液体培养条件的研究,明确蛹虫草菌丝产虫草素的适宜碳源及浓度,适宜氮源及浓度,最适pH值,最适培养温度,最适转速以及最适培养时间,以便应用于虫草素的工厂化生产。结果表明,蛹虫草菌丝产虫草素的条件：适宜碳源为D-果糖,最适浓度为10g/L;适宜氮源为蛋白胨,最适浓度为15g/L;最适初始pH为7,最适培养温度为24℃,最适转速为180r/min,最适培养时间为9d,其培养液虫草素含量可达到0.537g/L。     

Tropane alkaloid production in Datura stramonium suspension cultures: elicitor and precursor effects

The effects of elicitation, carbon, and nitrogen sources, and precursors on cell growth and tropane alkaloid production in Datura stramonium cell cultures were studied. D. Stramonium cell cultures responded very well to elicitors in the late exponential phase. Addition of cell wall fragments of Phytophotora megasperma (Pmg) enhanced the final tropane alkaloid yield by fivefold compared with control culture. Supply of carbon culture. Supply of carbon and nitrogen sources, at a ratio (C/N) of up to 70, to cell cultures in the early stationary phase, suppressed tropane alkaloid production; whereas C/N rations beyond about 100 increased the final product yield by more than 100% compared to that of the control experiment. Total alkaloid production in the cell culture supplemented with phenylalanine and ornithine was five times higher that that in the control culture. Higher rations of tropine to tropic acid also stimulated alkaloid production. At a ratio of 20, the productivity was seven times higher that that in the control culture. Adding precursors at high concentrations (e.g., 3 to 10 mM) to the cell culture reduced the final cell yield by less than 40%, while elicitation did not affect the cell yield. On the other hand, cell yield in the cultures supplemented with carbon and nitrogen sources was influenced by the C/N ratio. The highest cell yield was obtained at C/N = 70. (c) 1993 Wiley & Sons, Inc.     

Effects of carbon and nitrogen sources on fatty acid contents and composition in the green microalga, Chlorella sp. 227

In order to investigate and generalize the effects of carbon and nitrogen sources on the growth of and lipid production in Chlorella sp. 227, several nutritional combinations consisting of different carbon and nitrogen sources and concentrations were given to the media for cultivation of Chlorella sp. 227, respectively. The growth rate and lipid content were affected largely by concentration rather than by sources. The maximum specific growth was negatively affected by low concentrations of carbon and nitrogen. There is a maximum allowable inorganic carbon concentration (less than 500~1,000 mM bicarbonate) in autotrophic culture, but the maximum lipid content per gram dry cell weight (g DCW) was little affected by the concentration of inorganic carbon within the concentration. The lipid content per g DCW was increased when the microalga was cultured with the addition of glucose and bicarbonate (mixotrophic) at a fixed nitrogen concentration and with the lowest nitrogen concentration (0.2 mM), relatively. Considering that lipid contents per g DCW increased in those conditions, it suggests that a high ratio of carbon to nitrogen in culture media promotes lipid accumulation in the cells. Interestingly, a significant increase of the oleic acid amount to total fatty acids was observed in those conditions. These results showed the possibility to induce lipid production of high quality and content per g DCW by modifying the cultivation conditions.