红曲多糖液态发酵工艺条件的优化

实验研究红曲多糖的液态发酵条件,得出优化后红曲菌ZKOA发酵工艺条件：蔗糖40g/L,酵母粉4．5g／L,KH2PO4·3H2O3．5∥L．MgSO40．4g／L,植物油2mL／L,接种量8％,种龄30h,发酵液起始pH5．0,发酵时间90h,在此条件下,摇瓶和中试发酵罐中的粗多糖质量浓度分别为7．6g／L和7．34g/L。     

植酸酶固体发酵条件的研究

黑曲霉Ｇ２.１．１．１．４菌株在产生植酸酶时受无机磷的反馈阻遏,并且植酸酶的产生与淀粉酶的产生存在相互抑制。对植酸酶固体发酵进行调控和通过响应面分析优化发酵条件,提高了植酸酶产量。最适发酵条件下,植酸酶（ＰｈｙｔＡ）的产量可达６２．１ｕ／ｇ．干基。     

植酸酶固体发酵条件的研究

黑曲霉Ｇ２．１．１．１．４菌株在产生植酸酶时受无机磷的反馈阻遏,并且植酸酶的产生与淀粉酶的产生存在相互抑制。对植酸菌固体发酵进行调控和通过响应面分析优化发酵条件,提高了植酸酶产量。最适发酵条件下,植酸酶（ＰｈｙｔＡ）的产量可达６２．１ｕ／ｇ．干基。     

粗糙脉孢菌(Neurospora crassa)木糖发酵的研究

研究了不同通氧条件和培养基初始pH等对粗糙脉孢菌(Neurospora crassa)AS3．1602木糖发酵的影响。结果表明,粗糙脉孢菌具有较强的发酵木糖产生乙醇及木糖醇的能力。通气量对木糖发酵有较大的影响。乙醇发酵适合在半好氧条件下进行,此时乙醇的转化率达到63．2％。木糖醇发酵适合在微好氧的条件下进行,转化率达到31．8％。木糖醇是在培养基中乙醇达到一定浓度后才开始积累。培养基的初始pH对木糖发酵产物有较大的影响,乙醇产生最适pH5．0,木糖醇产生最适pH4．0。在培养基pH为碱性条件时,木糖发酵受到很大的抑制。初始木糖浓度对产物乙醇及木糖醇的产率有很大的影响。葡萄糖的存在会抑制木糖的利用,对乙醇和木糖醇的产生也有很大的影响。     

糖蜜发酵生产丙酮丁醇的研究

分离选育出４株丙酮丁醇发酵菌种,分别编号为：ＣＬＳ．００１,００２,００３,００４,都属厌氧核状芽孢杆菌,它们可利用糖蜜发酵产生丙酮和丁醇。经正交试验,选出最佳发酵条件。分离株ＣＬＳ．００４在糖蜜浓度１０￣１５ＢＸ、３５￣３８℃、ｐＨ６．８￣７．２条件下,发酵总溶剂的生成率和糖利用率分别可达到３０％和８５％以上。     

木薯发酵产丁醇的研究

对丙酮丁醇梭菌发酵木薯产溶剂进行研究,分别考察了N源、木薯含量、酶处理条件和培养基pH对发酵产丁醇的影响。结果表明：最佳的产丁醇发酵培养基为木薯粉120g／L,乙酸铵6g／L;木薯粉先用高温淀粉酶按酶量20U／g、90℃水解60min,再糊化30min;发酵初始pH为6．0,发酵96h。在此条件下,5L发酵罐中丁醇产量达到13．5g／L,总溶剂达到22．8g／L。     

出芽短梗霉色素变异菌株R45的普鲁蓝糖发酵研究

用正交实验确定了出芽短梗霉（Aureobasidiumpullulans）色素变异菌株R45的发酵优化条件。在此条件下,摇瓶培养的普鲁蓝糖产量最高可达82．4g／L,转化率为54．9％。实验表明,CaCO3是多糖发酵的重要影响因素,多糖的合成与发酵pH值及细胞形态密切相关。     

丁酸梭杆菌发酵甘油制备1,3-丙二醇的研究

本研究采用丁酸梭芽孢杆菌(Clostridium butyricum)从甘油发酵制备1,3—丙二醇。该发酵需厌氧培养,发酵培养基为：甘油6％,葡萄糖1％,玉米浆2％,(NH4)2SO40．2％。发酵温度为34℃,pH为6．5～7。在最佳条件下,发酵50h可产1,3—丙二醇40．7g／L,甘油摩尔转化率达68％。     

千层塔内生真菌SHB发酵产石杉碱甲条件的研究

为提高千层塔产黄青霉属内生真菌SHB液体发酵产石杉碱甲的产量,通过单因子和正交试验研究了真菌SHB液体发酵的条件。结果表明,千层塔内生真菌SHB液体发酵产石杉碱甲的适宜条件：温度为28℃,起始pH为6．4,接种量为12％,种龄为48h,转速为160r／min,发酵时间为8d。在此条件下,石杉碱甲的产量可达4．761μg／mL。     

少根根霉菌株发酵生产纤溶酶条件的研究

发酵条件优化可提高少根根霉菌株8B所产纤溶酶的活性。使用单因素试验和正交试验确定该茵发酵产酶的最佳条件。试验确定最优化发酵条件,培养基：麸皮水5g／L,尿素5g／L,胰蛋白胨0．5g／L,K2HPO4·3H2O 0．3g／L,MgSO4·7H2O 0.15g／L,pH5.5,摇床转速160r／min,30℃发酵56h。在此优化条件下培养,8B产纤溶酶活力达到345．41U／mL,是初始培养基发酵产酶活力的7．52倍。     

牲畜粪便与麦秆混合厌氧发酵的产气量、发酵时间及最优温度

探索牲畜粪便与作物秸秆混合发酵的产气量和发酵时间与发酵温度之间的关系,是解决农村户用沼气原料选择、确定最优发酵温度和提高农作物秸秆资源化利用效率的关键.采用可控型恒温发酵装置,以猪粪、牛粪和麦秆作为发酵原料,以常温厌氧发酵池的底物为接种物,在总固体（total solid,TS）质量分数为8%的条件下进行批量试验,研究了混合发酵的产气量、发酵时间及最优温度.结果表明：粪便与麦秆混合发酵明显提高了原料的产气效率,其中猪粪与麦秆混合发酵的累积产气量比猪粪作为单一发酵原料高24倍,而牛粪与麦杆混合发酵的累积产气量与单一牛粪无显著差异.猪粪、牛粪与麦秆混合发酵的最优温度均在30 ℃以上,发酵时间在60 d左右.厌氧发酵的发酵时间不总是随着温度的升高而缩短,单一以温度来断定厌氧发酵时间的长短是不可行的.     

Novel Method of Lactic Acid Production by Electrodialysis Fermentation

In lactic acid fermentation by Lactobacillus delbrueckii, the produced lactic acid affected the lactic acid productivity. Therefore, for the purpose of alleviating this inhibitory effect, an electrodialysis fermentation method which can continuously remove produced lactic acid from the fermentation broth was applied to this fermentation process. As a result, the continuation of fermentation activity was obtained, and the productivity was three times higher than in non-pH-controlled fermentation. In electrodialysis fermentation, the amount of produced lactic acid was 82.2 g/liter, which was about 5.5 times greater than that produced in non-pH-controlled fermentation. It was concluded that these good results were obtained on account of alleviating the lactic acid inhibitory effect by electrodialysis fermentation. However, the fouling of anion-exchange membranes by cells was observed in electrodialysis fermentation.     

固态发酵降低上部低次烟叶中淀粉及蛋白质的含量

利用固态发酵的方法降低上部低次烟叶中淀粉和蛋白质的含量,并对发酵过程中的厌氧细菌和酵母的数量进行检测。采用单因素和正交试验对固态发酵的条件进行优化,结果表明:各因素对发酵上部低次烟叶影响显著性主次次序依次为发酵时间(C)、发酵温度(A)和发酵水分质量分数(B),固态发酵的最佳条件为A2B2C3,即温度45℃、水分质量分数50%、发酵时间9 d。在该发酵条件下,上部低次烟叶的淀粉降解率为20.41%,蛋白质降解率为12.35%。通过固态厌氧发酵的方法可取得较好的、短期内快速降解上部低次烟叶中淀粉和蛋白质含量的效果。     

农抗120发酵高产培养基优选

采用正交试验浓度加倍的方法 ,进行了农抗 12 0发酵培养基筛选 ,获得两种培养基配方Q1和Q2 。经摇瓶发酵试验 ,发酵水平分别比原始配方提高了 197 3%和 130 9%。摩式自动控制发酵罐试验 ,发酵水平是原始配方的 32 7%和 181%。 2 0M3发酵罐中试 ,发酵水平比原始配方提高了 30 0 0～ 50 0 0单位。     

Production of Botrytis cinerea for potential introduction into a vineyard

Botrytis cinerea was produced in solid-phase fermentation, liquid fermentation and on potato dextrose agar. Stored products were evaluated for grape colonization in grape bioassays and in field trials, and for B. cinerea density using colony forming unit analyses and a nucleic-acid-based method. B. cinerea colony forming unit density was significantly correlated to the probability of successful grape colonization in grape bioassays (p-value=0.0002). Solid fermentation products could be stored longer than liquid fermentation and potato dextrose agar products. There was little difference in the rate of grape colonization in laboratory bioassays among solid-phase fermentation, liquid fermentation and plate culture products. Although the initial B. cinerea colonization rate of field grapes was slightly greater on vines treated with solid-phase fermentation and plate culture products compared to vines treated with product from liquid fermentation, there was no significant difference in final colonization between vines treated with solid-phase fermentation, liquid fermentation and plate culture products and untreated vines.     

Ethanol fermentation of crude acid hydrolyzate of cellulose using high-level yeast inocula

High-level yeast inocula was investigated as a means of overcoming the toxicity problem in ethanol fermentation of acid hydrolyzate of wood cellulose. When the inoculum level exceeded 10(8) initial cells/mL, 50% of the yeast cells survived the initial cell death period during which furfural and HMF were depleted. The fermentation thus proceeded to completion by virtue of cell regrowth. The specific ethanol productivity in batch fermentation on the basis of viable cells was comparable to that of pure glucose fermentation. Continuous fermentation with cell recycle was superior to batch fermentation in that there was no overall cell decline and the ethanol yield was substantially higher. The maximum ethanol productivity in continuous fermentation was 4.9 g/L h and it occurred at a dilution rate of 0.24 hr(-1).     

链霉菌A048产几丁质酶最佳发酵工艺研究

将链霉菌A048在完全培养基中培养至对数生长末期,离心洗涤收集菌丝体,然后接种入发酵产酶培养基中,进行二步发酵工艺牛产几丁质酶,几丁质酶活力比一步发酵工艺提高1．1倍,发酵周期共54h,比一步发酵工艺缩短66h;把菌丝体与几丁质粉共固定化,接入发酵产酶培养基中培养36h,几丁质酶活力比一步发酵工艺提高1．8倍,发酵周期缩短54h;在二步发酵工岂中另添加0．4％纤维素,几丁质酶活力可提高4倍,比一步发酵工艺提高10倍,酶活力达18．52U／mL。采用几丁质和纤维索双因子诱导二步发酵工艺可能是链霉菌A048生产几丁质酶的最佳工艺。     

Multi-energy metabolic mechanisms of the fungus Fusarium oxysporum in low oxygen environments

The fungus Fusarium oxysporum produces energy under hypoxic and anoxic conditions by denitrification (nitrate respiration) and ammonia fermentation respectively. Here we found that glucose repressed both of these metabolisms, whereas it supported another anoxic metabolism, hetero-lactic acid fermentation. Ammonia fermentation occurred only after the glucose present in the medium was metabolized to ethanol via alcohol fermentation. During this transition, clear diauxic growth was observed. Glucose regulated the activity of the enzymes involved in ammonia fermentation, hetero-lactic acid fermentation, and denitrification. Highest cell growth was supported by hetero-lactic acid fermentation, followed by denitrification and ammonia fermentation. These results indicate that the energy metabolisms of F. oxysporum are dependent not only on environmental O(2) tension but also on the carbon source, and that ammonia fermentation is an adaptative mechanism acting physiologically as a secondary fermentative mechanism replacing the primary hetero-lactic acid fermentation.     

Potential of solid state fermentation for production of ergot alkaloids

Production of total ergot alkaloids by Claviceps fusiformis in solid state fermentation was 3.9 times higher compared to that in submerged fermentation. Production was equal in the case of Claviceps purpurea but the spectra of alkaloids were advantageous with the use of solid state fermentation. The data establish potential of solid state fermentation which was not explored earlier for production of ergot alkaloids.     

多元混菌发酵对纤维素酶活性的影响

研究了两种曲霉(UF2和UA8)二元混菌体系和两种曲霉与1种酵母菌组成的三元混菌体系混合发酵对纤维素酶系三种酶组分活性的影响。结果表明：两种霉菌按一定比例接种进行混合发酵时三种纤维素酶组分的活性较单菌发酵大幅度提高,滤纸酶(FPA)、微晶纤维素酶(AVI)和羧甲基纤维素酶(CMC)活性分别较UA8单菌发酵提高2.2％～51.1％、20．7％～332．6％和29．4％～299．6％;向由两种霉菌组成的二元混菌发酵体系中接入酵母菌可显著降低3种纤维素酶组分的活性;三菌混合发酵能使纤维素酶3组分的产酶高峰出现时间较双菌混合发酵滞后约24h,但三菌与双菌混合发酵3种纤维素酶组分的酶活峰值无明显差异;双菌混合发酵有利于缩短纤维素酶生产发酵周期。