纳豆激酶豆乳液体发酵条件优化

心脑血管疾病已经严重威胁人类健康,其发病率和死亡率均居各种疾病之首。纳豆激酶作为一种理想的预防和治疗血栓的天然功能食品被广泛关注,因此研究纳豆激酶的规模化生产对于推进溶栓类功能食品的开发具有重要意义。在前期发酵豆乳工艺优化的基础上,对因素顺序及因素水平稍作调整,以全豆豆乳为发酵基质,以纳豆激酶为功能评价指标,发酵后出渣率及终点p H为参考指标,通过单因素及正交试验确定最佳发酵工艺。结果表明,发酵豆乳的最佳工艺条件为:发酵时间30 h,装液量5%,初始p H5.5,接菌量1.5%。在此发酵条件下,酶活可高达660 184.14 IU/mL,是优化前(79 434.68 IU/mL)的8.31倍,是前期最佳工艺下纳豆激酶表达量(429 869.34 IU/mL)的1.54倍。与前期全豆豆乳最佳工艺条件相比,通过调整初始pH和接菌量的先后顺序,可以在更低接菌量(前期研究,最佳接菌量为1.75%)的基础上,显著增加纳豆激酶表达量。通过本实验研究既节约了成本也提升了纳豆激酶的表达量,对纳豆激酶的规模化生产具有重要意义。     

纳豆芽孢杆菌菌种纯化及不同氮源对其产纳豆激酶的影响

纳豆激酶(nattokinase, NK)是一种由纳豆芽孢杆菌发酵产生的丝氨酸蛋白酶,具有良好的纤溶活性。本研究从wako Nattokinase中分离纯化出高品质的纳豆芽孢杆菌,旨在探究最适宜该菌产纳豆激酶的发酵培养基氮源。研究人员选择了6种氮源对其进行发酵实验,通过连续测定发酵液的菌量、pH和纤溶活性以观察不同氮源对纳豆芽孢杆菌产纳豆激酶的影响。研究结果表明:最优氮源为乳清蛋白,在以此为氮源的培养基中发酵培养120 h后,纳豆激酶的纤溶活性高达1 757.79 U/mL。以乳清蛋白发酵培养基对纳豆芽孢杆菌进行发酵,不仅可以得到高活性的纳豆激酶,还可为纳豆激酶应用于食品、保健品领域提供思路。     

纳豆激酶固态发酵的参数优化

方法:在对实验室分离的纳豆激酶产生菌进行菌株鉴定及其酶学性质研究的基础上,对影响菌株固态发酵产酶的工艺参数进行了优化研究.结果:发酵温度、发酵时间及培养基碳氮比、料水比、pH对纳豆激酶的产生都有较大影响,而接种量对纳豆激酶影响较小;在优化条件下,纳豆激酶固态发酵酶活可达到8 300U/g,为已知最高纳豆激酶单位酶活.     

纳豆激酶的液体发酵条件优化

以纳豆素中分离的纳豆芽孢杆菌进行纳豆激酶发酵试验,考察装液量、接种量、摇床转速等因素对生物量和纳豆激酶纤溶活性的影响,揭示产酶规律并确定最优产酶条件。发酵培养基配方为2%葡萄糖、2%蛋白胨、0.05%Mg SO4、0.01%Ca Cl2、0.6%Na2HPO4、0.4%Na H2PO4。最终确定的发酵条件为:p H 6.9,2%接种量,45 m L/250 m L的装液量,33.5℃,摇床转速为165 r/min,在此条件下发酵33~34 h为产酶高峰期,纳豆激酶的纤溶活性达到1 004 U/m L,结果也表明纳豆激酶是一种生长关联型代谢产物,纤溶活性与生物量变化趋势高度一致。     

高产纳豆激酶液态发酵工艺的优化

通过用纳豆杆菌进行液态发酵生产纳豆激酶的培养基的优化实验,确定最佳产酶培养基组成为麦芽糖2%,酵母膏4%,CaCl20.03%,pH 7.0。在此基础上,设计发酵条件的优化实验,实验结果表明,在接种量为1%,装液量为100mL/500mL挡板瓶,200 r/min的条件下,34℃培养48 h达到产酶高峰,产酶活力可达4300U/mL发酵液。在此基础上,通过Luedking-Piret模型来描述纳豆激酶的生成,确定纳豆激酶的液态发酵属于部分生长偶联型。     

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。     

碱性蛋白酶提取变性脱脂豆粕中蛋白质

以高温变性脱脂大豆粕为原料,用正交实验法对变性豆粕在蛋白酶作用下的水解特性进行了深入研究。选用国产胰蛋白酶为水解酶对变性豆粕进行水解,研究了变性豆粕中蛋白质溶出率随温度,pH值,时间,低物浓度及用酶量的变化规律,找到了水解变性豆粕的最佳实验条件,结果表明,胰蛋白酶水解高温变性豆粕的最佳条件为,温度50℃,时间60h,底物浓度11%,用酶量10000u/g,pH值8.0,在此条件下,变性豆粕中蛋白质可有69.34%水解溶出。     

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。     

华根霉产纤溶酶液体发酵条件的研究

研究了华根霉TCCC 41014产纤溶酶液态发酵的工艺条件,采用单因素实验对液态发酵培养基的碳源、氮源、初始pH值、温度和装液量进行了优化.结果表明,实验范围内华根霉TCCC41014液态发酵产纤溶酶的适宜培养基组成(g桙L):糊精80,蛋白胨60,豆粕60,初始pH为4.5.适宜培养条件:培养温度为29℃,装液量为5...     

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,MnSO4-H2O 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10^7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。     

Response surface methodology for lovastatin production by Aspergillus terreus GD13 strain

A wild type Aspergillus terreus GD13 strain, chosen after extensive screening, was optimized for lovastatin production using statistical Box-Behnken design of experiments. The interactive effect of four process parameters, i.e. lactose and soybean meal, inoculum size (spore concentration) and age of the spore culture, on the production of lovastatin was evaluated employing response surface methodology (RSM). The model highlighted the positive effect of soybean meal concentration and inoculum level for achieving maximal level of lovastatin (1342 mg/l). The optimal fermentation conditions improved the lovastatin titre by 7.0-folds when compared to the titres obtained under unoptimized conditions.     

链霉菌FIM-0916产安福霉素的发酵条件优化

本文采用单因素和正交试验设计,对链霉菌 Streptomyces canus sp. FIM-0916产安福霉素的发酵培养基配方及发酵条件进行了优化。优化后的最佳培养基配方为：蔗糖1.5%,黄豆粉1.0%,组氨酸0.1%,KNO3 0.1%, CaCO3 0.1%。最佳发酵条件为：种子菌龄54 h,装液量120 mL/500 mL,接种量2%,发酵温度28℃,摇床转速250 r/min;最佳发酵时间为5 d。在该优化条件下,安福霉素的发酵效价比对照提高248%,为安福霉素的后续开发奠定了基础。     

高产纤维素酶枯草芽胞杆菌S-16的筛选及其发酵工艺优化

利用刚果红鉴别培养基及基础液体筛选培养基进行菌种筛选,从新疆盐碱地分离得到的16株菌株中筛选获得一株产纤维素酶活力较高的菌株S-16,对该菌株进行16SrDNA鉴定,确定该菌为枯草芽胞杆菌(Bacillus subtilis)。对S-16发酵产纤维素酶的主要影响因素进行研究,分别考察了碳源、氮源、培养基初始pH和接种量等因素对发酵产纤维素酶的影响。结合单因素影响实验得到优化后的培养基配方为:羧甲基纤维素钠1.5%,酵母粉1%,NaCl 1%,MgSO_4·7H_2O 2‰,KH_2PO_4·3H_2_O 1‰。优化后的发酵条件为:初始pH为8,接种量1%,种龄8h,培养时间48h。经过发酵工艺优化,S-16产生的羧甲基纤维素酶活(CMCase)和滤纸酶活(FPase)分别达到4.64IU/mL和0.46IU/mL,与初始培养条件下的酶活相比分别提高了3.14倍和1.30倍。本研究得到的枯草芽胞杆菌S-16及其优化发酵工艺为秸秆的快速腐熟和高产纤维素酶的应用奠定了基础。     

洋葱假单胞菌(Pseudomonas cepacia)PCL-3产脂肪酶发酵条件研究

研究了洋葱假单胞菌(Pseudomonas cepacia) PCL-3发酵产碱性脂肪酶培养条件的优化。采用单因子试验筛选出糊精为最适碳源,蛋白胨和尿素为复合氮源。通过Plackett-Burman设计试验,对影响产酶条件的8个相关因子进行评估并筛选出具有显著效应的三个因子：尿素、接种量以及初始pH值。用最陡爬坡实验逼近显著因子的最大响应区域后,采用响应面分析法,确定尿素、接种量以及初始pH值最优值分别为0.15％,3.05%和8.59。优化后液体发酵培养基中脂肪酶活力提高到48.88 U/mL,比初始酶活25.37U/ml提高了1.93倍。10 L 的发酵罐中,脂肪酶活力在52h达到最大,为47.69U/mL。     

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%。     

Influence of cultivating conditions on the alpha-galactosidase biosynthesis from a novel strain of Penicillium sp. in solid-state fermentation

AIMS: The work is intended to achieve optimum culture conditions of alpha-galactosidase production by a mutant strain Penicillium sp. in solid-state fermentation (SSF). METHODS AND RESULTS: Certain fermentation parameters involving incubation temperature, moisture content, initial pH value, inoculum and load size of medium, and incubation time were investigated separately. The optimal temperature and moisture level for alpha-galactosidase biosynthesis was found to be 30 degrees C and 50%, respectively. The range of pH 5.5-6.5 was favourable. About 40-50 g of medium in 250-ml flask and inoculum over 1.0 x 10(6) spores were suitable for enzyme production. Seventy-five hours of incubation was enough for maximum alpha-galactosidase production. Substrate as wheat bran supplemented with soyabean meal and beet pulp markedly improved the enzyme yield in trays. CONCLUSIONS: Under optimum culture conditions, the alpha-galactosidase activity from Penicillium sp. MAFIC-6 indicated 185.2 U g(-1) in tray of SSF. SIGNIFICANT AND IMPACT OF THE STUDY: The process on alpha-galactosidase production in laboratory scale may have a potentiality of scaling-up.     

Streptomyces sp.FIM-16-06产他克莫司摇瓶发酵条件的优化

采用单因素试验和正交试验研究发酵培养基组成,优化Streptomyces sp. FIM-16-06产他克莫司的发酵条件,探讨摇瓶发酵的主要影响因子初始p H、装液量、转速等发酵参数的影响。确定了适宜的发酵培养基和发酵参数:6. 0%玉米淀粉、2. 0%黄豆粉、2. 0%葡萄糖和0. 5%玉米浆,初始pH 7. 5,装液量50 m L/500 m L三角瓶,种子菌龄48 h,接种量10%,摇床转速250 r/min,发酵温度27℃,发酵周期7 d。优化后的发酵水平较原生产工艺提高60%以上。他克莫司的优化发酵工艺为其工业化生产奠定了基础。     

胶质芽孢杆菌突变株021120的培养条件及发酵工艺优化

对离子束诱变所获得的突变菌株021120进行了培养条件和发酵工艺研究。单因子及正交试验结果表明,碳源对生物量和芽孢形成的影响最大,其次是氮源,磷和钾的影响较小;添加CaCO3和增加氧通量显著促进芽孢的形成。发酵培养基的理想配方为：2%淀粉、0.4% 酵母、0.1% K2HPO4、0.1％ MgSO4·7H20、0.5 ％CaCO3,pH 7.5。种子菌经二级扩大培养后,按6％的接种量接入70 L发酵罐,在32℃进行发酵,氧通量2.0-2.5 vvm,培养周期38-42 h,芽孢量达到9.80×108 cfu ml-1。通过以上培养基和发酵条件的优化,有效控制了多糖荚膜的产生,并促进了芽孢的形成,获得合格产品。     

Screening of lactic starter from Tunisian fermented vegetables and application for the improvement of caper (Capparis spinosa) fermentation through an experimental factorial design

This study aims at designing a lactic starter for caper fermentation isolated from Tunisian fermented vegetables to improve the process and produce consistent and high-quality product. In this study, the lactic starter was isolated by exploring the lactic acid bacteria (LAB) of Tunisian artisanal fermented vegetables. Identification was carried out by partial 16S rRNA gene sequencing. Screening was based on salt tolerance and antagonistic activities against Escherichia coli ATCC 10536 and Enterococcus faecalis ATCC 10541. Caper fermentation was optimized through a full factorial experimental design (23), by exploring three factors: starter inoculum size, NaCl concentration, and acetate content. Differences in pH values, Total aerobic mesophilic bacteria and LAB counts between the beginning and end of fermentation are selected as responses and corresponding regression coefficients were calculated. The lactic microbiota is mainly represented by Lactobacillus plantarum group. Based on salt tolerance and antimicrobial activity, the strain Lactobacillus plantarum F3 was selected as starter for caper fermentation. The effect of NaCl concentration, acetate content, and inoculum size on acidity, total aerobic mesophilic bacteria count, and LAB count after 1 week and 1 month of caper fermentation was studied. Depending on the fermentation time, either 1 week or 1 month, the initial conditions should comprise 0% acetate, 108 CFU/mL inoculum, and 5% NaCl for 1 week against 5% acetate, 107 CFU/mL inoculum, and 10% NaCl for 1 month lasting caper fermentation. A protocol for caper fermentation was set up ensuring hygienic quality and LAB viability. Lb. plantarum F3 was selected as lactic starter for caper fermentation, and initial fermentation conditions were optimized through a full factorial design. This work has shown loss in LAB viability after 1 week of fermentation. Based on results obtained, an optimized fermentation protocol was set up. This protocol ensures LAB survival and high hygienic quality of the product.