甘薯淀粉废水发酵生产微生物油脂的研究

研究了废水预处理方式及添加营养因子对产油菌株FR在甘薯淀粉废水中生长、产油及COD去除的影响。发现不经稀释的废水发酵效果优于稀释后的效果,采用淀粉酶液化处理、添加碳氮比、添加Mn2 均能够促进菌株FR生长、产油和COD去除,淀粉酶液化处理后的产油率可达45.3%,淀粉酶和糖化酶先后处理后的COD去除率可达66.3%。Mg2 的加入可以提高生物量。     

用连续发酵工艺由味精废液制取单细胞蛋白

用谷氨酸发酵液经一步冷冻等电法提取后的废液生产饲料酵母,经15m3气升式反应器连续发酵试验,其菌体干物质浓度平均为24．88g／L,稀释率0.187h-1,生产干酵母能力为4．65kg／m3·h,发酵单位电耗2．872kW·h／m3,生产成本在1700元,吨(饲料酵母)左右。饲料酵母粗蛋白含量在60％以上,18种氨基酸齐全,氨基酸总量达50％,达到部颁一级饲料酵母的标准。味精废液经酵母菌处理后,COD去除率74．7％。经试验统计,每开废液中获得1g菌体干物质需消耗COD 1625mg／L。     

产油真菌在甘薯淀粉废水中发酵的初步研究

目的:利用甘薯淀粉废水发酵低成本获取微生物油脂。方法:以甘薯淀粉废水为发酵基质,进行菌株筛选、发酵工艺优化及油脂成分的气相色谱分析。结果:筛选出一株刺孢小克银汉霉F7,生物量为19.375g/L,含油量为45.1%。菌株F7发酵第11天生物量达到18.140g/L,含油量达到51.2%,COD去除率87%。研究发现与对照相比,NaAc和KH2PO4对生长、产油以及出水COD去除有显著促进作用,NaAc2g/L时生物量提高了25.4%,含油量提高了4.4%,COD下降了52.0%,KH2PO4的作用稍次之。结论:资源化利用甘薯淀粉废水发酵生产微生物油脂同时降低废水COD是一条可行的途径,可以为生物柴油提供廉价油源。     

粘红酵母在味精废水中发酵生产油脂

对粘红酵母菌株进行驯化得到一株优良菌株Rh8,利用其在味精废水中发酵以去除废水中的化学需氧量(COD)并生产油脂;考察废水pH以及添加葡萄糖母液、营养因子等对菌株Rh8在味精废水中生长、产油和COD去除效果的影响,发现将废水稀释4倍、调节pH至5.5时,菌株可以较好地生长;而添加废葡萄糖母液、酵母粉、KH2PO4、MgSO4、MnSO4均能够促进菌体的生长、产油和废水中的COD去除,在250 mL摇瓶中,生物量最高可达15.6 g/L,干菌体中油脂质量分数达到29.61%,COD去除率达到45.1%。     

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。     

产胞外多糖酵母菌株的筛选鉴定及发酵产糖

【目的】微生物胞外多糖大多具有良好的功能和特性,但对酵母胞外多糖的研究甚少。本研究从自然界中筛选出产胞外多糖的酵母菌株,并对其发酵产糖条件进行初步研究。【方法】利用平板涂布法从自然界中分离得到酵母菌株,苯酚硫酸法测定菌株胞外多糖的产量,筛选出胞外多糖高产菌株,并对其进行5.8SrDNA分类鉴定,最后优化其产糖培养基组成。【结果】对从葡萄、蜜枣、土壤样品中分离得到的132株酵母进行筛选,最终得到3株高产胞外多糖的酵母菌株Z14、Z20和L25。经5.8S rDNA序列测定及系统发育分析,从左优红葡萄中分离得到的Z14和Z20与东方伊萨酵母(Issatchenkia orientalis)处于同一分支,相似性达到99%以上;从落叶松近表层土壤分离得到的L25与土生隐球酵母(Cryptococcus humicolus)处于同一分支,相似性为98.8%。经优化,利于Z20胞外多糖合成的最优发酵培养基配方为:葡萄糖8%,(NH4)SO40.2%,KH2PO40.1%,酵母浸粉0.1%,CaCl20.01%。在初始pH6.0,发酵温度28℃,摇床转数160 r/min条件下,在此培养基中发酵4 d后胞外多糖产量可达2.046 g/L,比复筛时的产量1.137 g/L提高了79.9%。【结论】文献已报道某些属的酵母可以生产胞外多糖,经本文研究发现Issatchenkia属的酵母也可以合成胞外多糖,并且改变基础产糖培养基的成分可以显着提高Z20胞外多糖的产量。     

酵母产γ-氨基丁酸发酵条件的研究

目的：研究酵母产γ-氨基丁酸的发酵条件,提高其产γ-氨基丁酸的能力。方法：以高产γ-氨基丁酸的酵母突变株为材料,通过单因素实验研究培养温度、摇床转速、接种量、种龄和培养时间等条件对菌株发酵生产γ-氨基丁酸的影响。结果：最适发酵条件为：培养温度30℃,摇床转速220 rpm,接种量4%,种龄为2d的种子菌,培养时间4d。在此发酵条件下,变异菌发酵液中γ-氨基丁酸含量高达2.588 g.L-1,较优化前提高了53%。结论：发酵条件的优化,提高了菌株产γ-氨基丁酸的能力。     

酵母产γ- 氨基丁酸发酵条件的研究

目的:研究酵母产γ-氨基丁酸的发酵条件,提高其产γ-氨基丁酸的能力。方法:以高产γ-氨基丁酸的酵母突变株为材料,通过单因素实验研究培养温度、摇床转速、接种量、种龄和培养时间等条件对菌株发酵生产γ-氨基丁酸的影响。结果:最适发酵条件为:培养温度30℃,摇床转速220 rpm,接种量4%,种龄为2d的种子菌,培养时间4d。在此发酵条件下,变异菌发酵液中γ-氨基丁酸含量高达2.588 g.L-1,较优化前提高了53%。结论:发酵条件的优化,提高了菌株产γ-氨基丁酸的能力。     

利用亚硝酸钠选育法夫酵母虾青素高产菌株

以亚硝酸钠作为筛选剂选择性分离法夫酵母虾青素高产菌株。实验研究表明,在亚硝酸钠存在的情况下,法夫酵母的生长和虾青素合成量均会减少;当亚硝酸钠浓度为5000μmol/L时,法夫酵母的致死率为100%。挑取200株经过甲基磺酸乙酯（EMS）诱变后的法夫酵母,以5000μmol/L的亚硝酸钠为筛选剂摇瓶发酵后测得虾青素体积产率为正突变的菌株有87株,正突变率为43.5%。挑取其中8株进行复筛,编号为N030的菌株比出发菌株的虾青素体积产率和细胞产率分别提高了39.3%和89.3%。结果说明,亚硝酸钠可作为法夫酵母虾青素高产菌株的筛选剂,用于提高菌种的筛选效率。     

中条山野生葡萄产香酵母的筛选及其混菌发酵对葡萄酒香气成分的影响

【背景】产香酵母可赋予葡萄酒独特的香气,因此,分离筛选优良产香酵母对酿造具有地域风味的特色葡萄酒具有重要意义。【目的】从中条山野生葡萄中筛选产香酵母,进行种群鉴定和生理生化特性研究,并将其应用于葡萄酒发酵过程,研究其对葡萄酒香气成分的影响。【方法】采用稀释涂布平板法从中条山野葡萄中分离筛选酵母菌,对其进行分子生物学鉴定。优选其中具有显著香气的产香酵母,与酿酒酵母F15进行混合发酵,采用气相色谱质谱联用(gas chromatograph-mass spectrometer,GC-MS)对香气成分进行分析,采用半定量法测定香气成分含量。【结果】共分离获得各种菌株13株,26S rRNA基因D1/D2区序列分析表明它们分布于Issatchenkia、Torulaspora、Pichia、Saccharomyces和Rhodotorula等5个不同属内。优选其中一株香气较为浓郁的酵母菌株Issatchenkia orientalis strain XS-6开展研究,结果发现该菌株最高耐受乙醇浓度为8%,最高耐受NaCl浓度为6%,最适生长温度为38℃。与酿酒酵母F15混菌发酵的葡萄酒中共检测出31种香气成分。香气物质总含量较单菌发酵增加19.8%,其中11种香气成分含量增加明显,尤其是具有玫瑰香气的苯乙醇。醇类与酯类物质含量较单菌发酵增加19.6%,并发现了香草酸乙酯(ethyl vanillate)、邻苯二甲酸二丁酯(dibutyl phthalate)等7种新的酯类物质。【结论】产香酵母XS-6对乙醇、NaCl、温度等具有良好的耐受性,而且与酿酒酵母F15混菌发酵对西拉葡萄酒香气成分具有明显的影响,可能在改善葡萄酒风味方面具有潜在的应用价值。     

多粮浓香型白酒中特征酵母菌与耐酸乳杆菌的关系

【背景】多菌种协同代谢是浓香型白酒发酵的根本特征之一。【目的】探究多粮浓香型白酒发酵过程中功能微生物菌株间的相互协作关系,为实现发酵过程优化提供理论基础。【方法】采用传统分离培养法获得了多粮浓香型白酒发酵过程中的特征酵母菌和耐酸乳杆菌,并探讨了共培养过程中菌株的相互关系以及主要挥发性代谢产物的变化。【结果】共分离到3株优势特征性酵母菌(KazachstaniahumilisZ1、PichiakudriavzeviiZ2、CandidaethanolicaZ3)和1株耐酸乳杆菌(Lactobacillus acetotolerans W)。K. humilis Z1和L. acetotolerans W共培养体系中耐酸乳杆菌数量明显少于纯培养L. acetotolerans W的菌体数量;3株酵母菌均一定程度抑制L. acetotolerans W产乳酸,K. humilis Z1能抑制L. acetotolerans W不产乳酸;K. humilis Z1纯培养与Z1W共培养体系的挥发性代谢产物的构成相似;纯培养P. kudriavzevii Z2与Z2W共培养体系的挥发性代谢产物差异明显,主要表现为共培养时乙酸乙酯和乳酸乙酯含量显著增加。【结论】在共培养体系条件下,产乙醇酵母菌对耐酸乳杆菌的乳酸代谢有抑制作用,而耐酸乳杆菌又对酵母菌的乙醇代谢有一定影响,这对多粮浓香型白酒品质调控和菌群间相互关系具有重要意义。     

代谢工程与全基因组重组构建酿酒酵母抗逆高产乙醇菌株

将酿酒酵母海藻糖代谢工程与全基因组重组技术相结合,改良工业酿酒酵母菌株的抗逆性和乙醇发酵性能。对来源于二倍体出发菌株Zd4的两株优良单倍体Z1和Z2菌株进行杂交获得基因组重组菌株Z12,并对Z1和Z2先进行(1)过表达海藻糖-6-磷酸合成酶基因 (TPS1) ,(2)敲除海藻糖水解酶基因 (ATH1), (3)同时过表达 TPS1和敲除ATH1, 经此三种基因工程操作后再进行杂交获得代谢工程菌株的全基因组重组菌株Z12ptps1、Z12 Δath1和Z12pTΔA。与亲株Zd4相比,Z12及结合代谢工程获得的菌株在高糖、高乙醇浓度与高温条件下生长与乙醇发酵性能都有不同程度的改进。对比研究结果表明:在高糖发酵条件下,同时过表达 TPS1和敲除ATH1 的双基因操作工程菌株胞内海藻糖积累、乙醇主发酵速率和乙醇产量相对于亲株的提高幅度要大于只过表达 TPS1,或敲除ATH1 的工程菌。结合了全基因组重组后获得的二倍体工程菌株Z12pTΔA,与原始出发菌株Zd4及重组子Z12相比,主发酵速率分别提高11.4%和6.3%,乙醇产量提高7.0%和4.1%,与其胞内海藻糖含量高于其它菌株、在胁迫条件下具有更强耐逆境能力相一致。结果证明,海藻糖代谢工程与杂交介导的全基因组重组相结合,是提高酿酒酵母抗逆生长与乙醇发酵性能的有效策略与技术途径。     

一株可乳化降解原油的Compostibacillus的分离及特性

【背景】通过实施多轮次微生物采油,华北油藏产出液菌浓达到了106个/mL以上,油藏内部已经形成了较稳定的微生物发酵场,从其中筛选出能够乳化降解原油的微生物,并在地面对其进行扩大培养,然后再应用到微驱油藏,以进一步提高微生物采油实施效果。【目的】筛选乳化降解原油性能良好的菌株,对其进行多相分类学鉴定和性能评价。【方法】利用原油为底物筛选乳化降解性能良好的菌株,通过形态特征观察、生理生化测定、16S rRNA基因序列分析等确定菌株的分类地位。通过乳化能力、降解率等方法确定菌株的原油乳化降解特性。【结果】从华北油田采集的地层水样品中分离得到一株乳化原油的菌株BLG74,经多相分类鉴定表明其是土壤堆肥芽孢杆菌(Compostibacillus humi)的新菌株,亲源性99.6%。该菌株的生长温度为30-60℃ (最适温度45℃),pH6.5-9.5(最适pH7.0),NaCl浓度0%-7%(质量体积比)。菌株BLG74在玉米浆培养基中培养,其发酵液的表面张力为56.3 mN/m,乳化力约95%,在初始原油质量浓度0.5%、温度45℃的条件下培养20d,对原油的降解率可达40.8%。【结论】菌...     

利用人工锌指文库选育高乙醇耐受性工业酵母菌株

选育高乙醇耐性的酿酒酵母菌株对提高燃料乙醇的发酵效率具有重要意义.锌指蛋白广泛存在于多种生物中,对基因的转录和翻译起重要的调节作用.利用人工设计的锌指蛋白可定向设计锌指序列及其排列顺序,实现对细胞内多个基因的全局调控.由于与环境胁迫反应相关的基因很多,因此可利用人工锌指蛋白技术获得耐受性提高的微生物重组菌.文中将人工锌指文库转入到酿酒酵母模式菌株S288c,选育了具有高乙醇耐受性的重组菌株M01,并分离了与乙醇耐受性提高相关的人工锌指蛋白表达载体pRS316ZFP-M01,转入工业酿酒酵母Sc4126,在含有不同浓度乙醇的平板上,工业酵母Sc4126的重组菌株表现出显著的耐受性提高.在高糖培养基(250 g/L)条件下进行乙醇发酵,发现重组菌的乙醇发酵效率明显快于野生型,发酵时间提前24 h,且发酵终点乙醇浓度提高6.3％.结果表明人工锌指文库能够提高酵母的乙醇耐受性,为构建发酵性能优良的酵母菌种奠定了基础.     

A novel strategy to construct yeast Saccharomyces cerevisiae strains for very high gravity fermentation

Very high gravity (VHG) fermentation is aimed to considerably increase both the fermentation rate and the ethanol concentration, thereby reducing capital costs and the risk of bacterial contamination. This process results in critical issues, such as adverse stress factors (ie., osmotic pressure and ethanol inhibition) and high concentrations of metabolic byproducts which are difficult to overcome by a single breeding method. In the present paper, a novel strategy that combines metabolic engineering and genome shuffling to circumvent these limitations and improve the bioethanol production performance of Saccharomyces cerevisiae strains under VHG conditions was developed. First, in strain Z5, which performed better than other widely used industrial strains, the gene GPD2 encoding glycerol 3-phosphate dehydrogenase was deleted, resulting in a mutant (Z5ΔGPD2) with a lower glycerol yield and poor ethanol productivity. Second, strain Z5ΔGPD2 was subjected to three rounds of genome shuffling to improve its VHG fermentation performance, and the best performing strain SZ3-1 was obtained. Results showed that strain SZ3-1 not only produced less glycerol, but also increased the ethanol yield by up to 8% compared with the parent strain Z5. Further analysis suggested that the improved ethanol yield in strain SZ3-1 was mainly contributed by the enhanced ethanol tolerance of the strain. The differences in ethanol tolerance between strains Z5 and SZ3-1 were closely associated with the cell membrane fatty acid compositions and intracellular trehalose concentrations. Finally, genome rearrangements in the optimized strain were confirmed by karyotype analysis. Hence, a combination of genome shuffling and metabolic engineering is an efficient approach for the rapid improvement of yeast strains for desirable industrial phenotypes.     

Mixed culture of killer and sensitive Saccharomyces cerevisiae strains in batch and continuous fermentations

This paper presents a kinetic study of the dynamics of the population of two Saccharomyces cerevisiae strains (designated K1 and 522D) in mixed culture. These two strains are commonly used in wine making. The K1 strain (killer yeast) secretes a glycoprotein (killer toxin) which causes the death of the 522D strain (sensitive yeast). Initially, the mixed cultures were realized in batch fermentations. Initial concentrations of killer yeast were 5 and 10% of the total population. The influence of the killer strain on the sensitive cultures was measured in comparison with a reference fermentation. The reference fermentation was inoculated only with the sensitive strain. Results show that an initial concentration of 10% of killer strain affects the microbial population balance and the rate of ethanol production. However the fermentation was only slightly disturbed when the proportion of killer to sensitive yeast at the beginning of mixed culture was 5%. To achieve total displacement by the killer yeast at low concentrations, the mixed cultures were carried out in a continuous system. The results obtained in continuous fermentations with the same strains have shown that a level of contamination as low as 0.8% of killer strain was sufficient to completely displace the original sensitive population after 150 h incubation.     

几株啤酒酵母的筛选及发酵性能比较*

啤酒酵母是啤酒酿造的灵魂,可以直接影响啤酒品质。在啤酒酿造过程中,由于啤酒酵母被多次传代和保藏,造成优良菌种发酵性能衰退等问题,导致发酵不彻底,影响最后啤酒的风味质量。为此以8株Lager型啤酒酵母为出发菌株,通过平板分离纯化获得80株分离菌株,再经过三角瓶发酵初筛和复筛、发酵罐中试发酵实验最终获得了8株发酵性能优良的啤酒酵母。其中,6株酵母可应用于酿造双乙酰含量低于0.1 mg/L的啤酒;3株酵母发酵度高于70%,适合酿造干啤酒;1株酵母发酵度低于50%,适合酿造低醇啤酒。在风味方面:1株酵母酿造的啤酒醇酯比为3.3,啤酒酯香味较突出;另1株酵母酿造的啤酒醇酯比为4.5,啤酒高级醇含量较高。8株经过选育的啤酒酵母发酵特征明显,便于精酿啤酒厂实际应用。     

Mixed culture of killer and sensitive Saccharomyces cerevisiae strains in batch and continuous fermentations

This paper presents a kinetic study of the dynamics of the population of two Saccharomyces cerevisiae strains (designated K1 and 522D) in mixed culture. These two strains are commonly used in wine making. The K1 strain (killer yeast) secretes a glycoprotein (killer toxin) which causes the death of the 522D strain (sensitive yeast). Initially, the mixed cultures were realized in batch fermentations. Initial concentrations of killer yeast were 5 and 10% of the total population. The influence of the killer strain on the sensitive cultures was measured in comparison with a reference fermentation. The reference fermentation was inoculated only with the sensitive strain. Results show that an initial concentration of 10% of killer strain affects the microbial population balance and the rate of ethanol production. However the fermentation was only slightly disturbed when the proportion of killer to sensitive yeast at the beginning of mixed culture was 5%. To achieve total displacement by the killer yeast at low concentrations, the mixed cultures were carried out in a continuous system. The results obtained in continuous fermentations with the same strains have shown that a level of contamination as low as 0.8% of killer strain was sufficient to completely displace the original sensitive population after 150 h incubation.     

Copper Tolerance and Biosorption of Saccharomyces cerevisiae during Alcoholic Fermentation

At high levels, copper in grape mash can inhibit yeast activity and cause stuck fermentations. Wine yeast has limited tolerance of copper and can reduce copper levels in wine during fermentation. This study aimed to understand copper tolerance of wine yeast and establish the mechanism by which yeast decreases copper in the must during fermentation. Three strains of Saccharomyces cerevisiae (lab selected strain BH8 and industrial strains AWRI R2 and Freddo) and a simple model fermentation system containing 0 to 1.50 mM Cu²⁺ were used. ICP-AES determined Cu ion concentration in the must decreasing differently by strains and initial copper levels during fermentation. Fermentation performance was heavily inhibited under copper stress, paralleled a decrease in viable cell numbers. Strain BH8 showed higher copper-tolerance than strain AWRI R2 and higher adsorption than Freddo. Yeast cell surface depression and intracellular structure deformation after copper treatment were observed by scanning electron microscopy and transmission electron microscopy; electronic differential system detected higher surface Cu and no intracellular Cu on 1.50 mM copper treated yeast cells. It is most probably that surface adsorption dominated the biosorption process of Cu²⁺ for strain BH8, with saturation being accomplished in 24 h. This study demonstrated that Saccharomyces cerevisiae strain BH8 has good tolerance and adsorption of Cu, and reduces Cu²⁺ concentrations during fermentation in simple model system mainly through surface adsorption. The results indicate that the strain selected from China’s stress-tolerant wine grape is copper tolerant and can reduce copper in must when fermenting in a copper rich simple model system, and provided information for studies on mechanisms of heavy metal stress.