共查询到19条相似文献,搜索用时 109 毫秒
1.
微生物胞外多糖是一类由微生物产生的,有一定加工性能和/或人体健康增益效果的高分子聚合物。为了筛选胞外多糖高产的菌株并提高其多糖产量,以多糖含量为衡量指标,首先通过比较实验筛选目标菌株,然后采用生理生化和分子生物学的方法对该菌株进行菌种鉴定,最后运用单因素分析和响应面实验确定该菌株发酵脱脂乳产糖的最佳条件。结果表明,菌株B6的产糖能力显著高于其他常规乳酸菌,经鉴定为鼠李糖乳杆菌(CGMCC No.13310)。该菌株最优的产糖条件为发酵时间41 h,发酵温度39 ℃,脱脂乳浓度91 mg/mL,接种量5%(体积分数)。在此条件下获得的发酵乳中多糖含量可达354.5 mg/L,比优化前提高35.8%。 相似文献
2.
菌株SRF是1株从意大利树莓(Rubus corchorifolius)果实表面分离、可产胞外多糖的新菌株。在鉴定其分类归属的基础上,对其产生的胞外多糖进行了结构分析和发酵条件优化,为寻找微生物多糖提供新的菌株,为开发利用资源微生物提供借鉴。通过形态学和ITS序列对比分析进行菌株鉴定;通过薄层层析和红外光谱分析,确定胞外多糖结构;通过单因素检测试验,确定影响产糖量的主要因素;响应面Plackett-Burman和Box-Behnken设计筛选发酵产胞外多糖的最优条件。结果表明,出发菌株SRF隶属于出芽短梗霉属,命名为Aureobasidium sp. SRF;SRF所产胞外多糖为普鲁兰多糖;单因素检测表明,对多糖产量影响最大的因素为碳源浓度、氮源浓度、无机离子浓度,其次是碳源、氮源、无机离子、pH值;根据响应面结果确定最优发酵条件为麦芽糖8%(质量分数)、酵母提取物3%(质量分数)、钙离子0.3 g/L、pH 6,产糖量达5.93 g/L。SRF是1株来源于树莓浆果表面,可产胞外普鲁兰多糖的出芽短梗霉新菌株,是1株产微生物多糖的候选菌株。 相似文献
3.
【目的】以新疆古尔班通古特沙漠的生物结皮为样品,通过培养、筛选、分离得到一株高产胞外多糖(EPS)的菌株XJ-27,对XJ-27菌株所产的胞外多糖进行分离纯化,并对其絮凝性进行研究。【方法】利用DEAE sepharose CL-6B阴离子层析和Sephadex G100凝胶层析的方法对胞外多糖进行纯化,通过紫外分析方法和高效凝胶渗透色谱进行纯度的测定,利用高效凝胶渗透色谱法(HP-GPC)测定其分子量,以高岭土为体系对其絮凝性进行研究。【结果】利用层析分离的方法共得到2个胞外多糖的组分,对其中一个组分进一步纯化,得到组分EPS-I。结果表明,EPS-I纯度较高,分子量为575 kD。同时对胞外多糖的絮凝性进行了研究,结果表明该胞外多糖对高岭土为体系的絮凝率为80.4%。【结论】菌株XJ-27产胞外多糖,其胞外多糖具有絮凝性,对该胞外多糖进行分离纯化后,得到分子量为575 kD的多糖组分EPS-I。 相似文献
4.
筛选茯苓高产胞内多糖和胞内三萜的优良液体发酵出发菌株。采用PDA富集固体平板培养与液体发酵培养测定菌丝体生长速率;采用液体发酵策略分析16种茯苓菌株产胞内多糖与胞内三萜的潜能。实验结果表明菌株生长于固体培养基与种子培养基的生长速率之间没有关联性;降低一级种子培养基初始pH值到4.0时能有效缓解茯苓菌株培养物褐化现象;AS5.137胞内多糖含量最高,达377.60±0.10 mg/g,而DB菌株显示出最高的胞内多糖产量,达1.01±0.13 g/L;Y1菌株胞内三萜含量最高,达83.89±4.28 mg/g,而Jingzhou28菌株胞内三萜产量最高,达136.63±26.66 mg/L。就生产茯苓胞内多糖与胞内三萜而言,AS5.137与DB菌株适合作为液体发酵产胞内多糖的出发菌株;Y1,Jingzhou28,Z(z)与Xingpinzhong菌株均较适合作为液体发酵产胞内三萜的出发菌株。 相似文献
5.
利用平板涂布法从胡萝卜、芦荟、土豆、地瓜和紫薯样品中分离得到24株细菌,利用苯酚硫酸法测定菌株胞外多糖的产量,最终得到3株高产胞外多糖的细菌菌株25-Z-1、25-Z-3和12-L-6。经16S rDNA序列测定及系统发育分析,从紫薯样品中分离得到的25-Z-1与Bacillus pumilus strain ST277处于同一分支,相似性达到100%;25-Z-3与Bacillus cereus strain Se05处于同一分支,相似性达到99%;从芦荟中分离得到的12-L-6与Bacillus sp.GZT处于同一分支,相似性为99%。在LB液体培养基中,发酵温度30℃,摇床转数170 r/min条件下,发酵7 d后胞外多糖产量可分别达30.3 mg/L、29.1 mg/L及28.2 mg/L。 相似文献
6.
利用木糖-葡萄糖为原料产乙醇酵母的筛选、鉴定及发酵试验 总被引:1,自引:0,他引:1
建立筛选利用木糖为碳源产乙醇酵母模型,获得一株适合利用木质纤维素为原料产乙醇的酵母菌株。样品经麦芽汁培养基培养后,以木糖为唯一碳源的筛选培养基初筛,再以重铬酸钾显色法复筛。通过生理生化和26D1/D2区对筛选得到的菌株进行分析和鉴定,该菌初步鉴定为Pichia caribbica。经过筛选得到的菌株Y2-3以木糖(40g/L)为唯一碳源发酵时:生物量为23.5g/L,木糖利用率为94.7 %,乙醇终产量为4.57 g/L;以混合糖(葡萄糖40 g/L,木糖20 g/L)发酵时:生物量为28.6 g/L,木糖利用率为94.2 %,葡萄糖利用率为95.6%,乙醇终产量为20.6 g/L。Pichia caribbica是可以转化木糖及木糖-葡萄糖混合糖为乙醇的酵母菌株,为利用木质纤维素发酵乙醇的进一步研究奠定了基础。 相似文献
7.
抑制黑色素合成的乳酸菌胞外多糖的筛选和性质研究 总被引:1,自引:0,他引:1
【目的】筛选可抑制黑色素合成的乳酸菌胞外多糖。【方法】通过观察凝乳拉丝外观筛选产胞外多糖的乳酸菌菌株,测量胞外多糖对B16黑色素瘤细胞黑色素合成和细胞活力的影响。对胞外多糖进行纯化,并通过PMP衍生-HPLC、红外光谱、抑制酪氨酸酶活性、抗氧化能力对其单糖组成和结构、作用机制进行研究。【结果】筛选到一株乳酸菌Lactobacillus rhamnosus HLAB122,发酵产生的胞外多糖在5 g/L浓度下可使B16细胞黑色素产量下降至空白对照的32.7%,且在96 h内对细胞活力无影响。纯化后的多糖由鼠李糖、葡萄糖、半乳糖构成,各单糖摩尔比为1?5.44?5.37。该胞外多糖不抑制酪氨酸酶活力且抗氧化性微弱。【结论】L.rhamnosus HLAB122产生的胞外多糖在个人护理产品中有潜在应用价值。 相似文献
8.
云南阳宗海酵母菌种群结构及产胞外酶测试北大核心CSCD 总被引:1,自引:0,他引:1
【目的】研究阳宗海酵母菌种群结构,分析生物因子及非生物因子对酵母菌种群分布的影响;测试阳宗海酵母菌产胞外酶活性。【方法】水样用醋酸纤维素滤膜过滤,原位培养分离酵母菌;梯度稀释法分离土样和底泥样品;对分离得到的菌株进行DNA提取和测序,分析26S rDNA的D1/D2区域,并结合形态及生理生化指标进行鉴定;用产酶筛选培养基对分离得到的酵母菌进行产胞外酶活性测试。【结果】共分离得到201株酵母菌,鉴定分属于15个属48个种,其中包括10个潜在的新种;普鲁兰类酵母(Aureobasidium pullulans),库德里阿兹威氏毕赤酵母(Pichia kudriavzevii),胶红酵母(Rhodotorula mucilaginosa),Cryptococcus podzolicus是优势种;15.9%的酵母菌具有产胞外酶活性,主要是脂肪酶和淀粉酶。【结论】阳宗海酵母菌有较为丰富的多样性,人为活动对阳宗海酵母菌分布影响较大,其次浊度、电导率也是影响酵母菌种群分布的重要因素;阳宗海产胞外酶酵母菌可能参与湖泊生态系统的自然循环。 相似文献
9.
【目的】研究有机溶剂胁迫处理对菌株分泌胞外多糖的影响并确定最佳条件。【方法】利用分泌抗氧化活性胞外多糖海洋细菌Bacillus subtilis OST23a及其突变菌株UD292为出发菌株,在考察菌株有机溶剂耐受性的基础上,测定不同浓度正己烷胁迫处理不同时间后该菌株抗氧化胞外多糖产量。【结果】结果表明最佳胁迫处理浓度和时间分别为3%和6 h,此时Bacillus subtilis OST23a和菌株UD292胞外多糖分泌量分别从9.02 mg/L和43.92 mg/L显著提高到52.97 mg/L和201.81 mg/L,且胞外多糖的抗氧化性能无显著变化。Bacillus subtilis OST23a和菌株UD292连续传代试验结果表明菌株遗传性状较稳定。【结论】有机溶剂胁迫可以提高细菌分泌胞外多糖的能力,在微生物育种方面有潜在的应用。 相似文献
10.
一株地衣芽胞杆菌产碱性蛋白酶条件优化 总被引:1,自引:1,他引:0
【背景】碱性蛋白酶是众多芽胞杆菌的发酵产物,是工业上极其重要的一类酶。【目的】利用酪素培养基从环境样品中筛选出一株产碱性蛋白酶的菌株,对传代次数、发酵的碳源、氮源、金属离子、磷酸盐、初始pH、接种量和温度进行优化,提高其产碱性蛋白酶的能力并降低发酵成本。【方法】采用革兰氏染色法、扫描电镜、生理生化试验、16S rRNA基因序列对分离的菌株进行鉴定;采用单因素、Plackett-Burman、最陡爬坡和响应面试验优化碱性蛋白酶的发酵条件,使用Minitab对试验数据进行分析。【结果】经鉴定分离菌株为地衣芽胞杆菌,命名为Bacillus licheniformis NWMCC0046。优化后的发酵培养基组成为(g/L):豆粕50.00,葡萄糖10.00,酵母浸膏13.46,CaCl2 0.50,Na2HPO4·12H2O 4.00,KH2PO4 0.30;优化后的培养条件为:pH 7.5,34.81℃,接种量4.13%。在此条件下,摇瓶发酵48 h时碱性蛋白酶... 相似文献
11.
【目的】马奶酒样乳杆菌ZW3含有一段长度为14.4 kb的胞外多糖合成基因簇,包含17个与胞外多糖合成相关的基因(WANG_1283?WANG_1299),主要分析17个基因在马奶酒样乳杆菌ZW3生长过程中不同时间段的表达量,探究其中一个表达量发生变化的基因对乳酸菌产胞外多糖的影响。【方法】通过半定量RT-PCR实验,对基因簇上各基因的表达量进行分析;通过构建含有表达量变化基因的重组乳酸乳球菌,比较重组菌与野生菌的产胞外多糖差异。【结果】经分析,WANG_1284、WANG_1286、WANG_1287、WANG_1288、WANG_1290、WANG_1291、WANG_1292、WANG_1294、WANG_1296、WANG_1297、WANG_1298、WANG_1299这12个基因在菌体生长的50 h和60 h (产糖量上升阶段)表达量最高,推测这些基因在多糖聚合过程中起作用。从这12个基因中选出一个表达量发生明显变化的基因WANG_1291做进一步研究。将WANG_1291插入乳酸菌表达载体pMG36e中,构建了重组表达载体pMG36e-1291。将构建的重组表达载体转化到乳酸乳球菌WH-C1中,得到重组菌株。测定重组菌与野生菌生长特性,发现重组菌与野生菌之间的生长速度存在一定差异。然后利用苯酚-硫酸法测得重组乳酸乳球菌的胞外多糖产量是野生菌的2.1倍,胞外多糖产量有了明显的提高。【结论】确定WANG_1291基因是调控马奶酒样乳杆菌ZW3产胞外多糖的关键基因之一。 相似文献
12.
Tuftsin and some analogs: synthesis and interaction with human polymorphonuclear leukocytes 总被引:5,自引:0,他引:5
The phagocytosis-stimulating tetrapeptide tuftsin, L-threonyl-L-lysyl-L-prolyl-L-arginine, was synthesized by both conventional and polymeric-reagent approaches. Using a combination of the two methods several analogs were prepared, including: [Ala1]tuftsin, [Lys1]tuftsin, [Ser1]tuftsin, [Val1]tuftsin, acetyl-tuftsin, p-aminophenylacetyl-tuftsin and tyrosyl-tuftsin. [Des-Thr1]tuftsin and [omega-NO2(4)]tuftsin were synthesized using a conventional procedure. The effects of synthetic peptides on the phagocytosis of heat-killed yeasts and on the reduction of the dye nitroblue tetrazolium by normal human polymorphonuclear leukocytes were investigated. Tuftsin and to a lesser extent [Lys1]tuftsin and [Ser1]tuftsin were found to stimulate phagocytosis, whereas the other analogs synthesized as well as [Ser1]tuftsin exhibited inhibitory effects to tuftsin's action. Tuftsin alone has stimulated nitroblue tetrazolium reduction; [Des-Thr1]tuftsin and [Ala1]tuftsin repressed this stimulation, while the other peptides showed no effect. 相似文献
13.
Ibarburu I Soria-Díaz ME Rodríguez-Carvajal MA Velasco SE Tejero-Mateo P Gil-Serrano AM Irastorza A Dueñas MT 《Journal of applied microbiology》2007,103(2):477-486
AIMS: To study the influence of medium constituents on growth, and exopolysaccharide (EPS) production by a strain of Oenococcus oeni. The structure of one of the EPSs has also been characterized. METHODS AND RESULTS: EPS concentration was estimated by the phenol/sulfuric acid method. After purification and fractionation of crude EPSs, the sugar composition was determined by GLC-MS of the TMS methyl glycosides. The major polysaccharide is 2-substituted-(1-3)-beta-D-glucan. This structure was determined by methylation analysis and conventional (1)H- and (13)C-nuclear magnetic resonance spectroscopy. In addition, O. oeni synthesized two heteropolysaccharides, although a lesser proportion, constituted by galactose and glucose, and one of them also showed rhamnose. The sugar source has a clear influence on growth and EPS synthesis, and EPS production was not enhanced by adding ethanol or increasing the nitrogen source. EPS biosynthesis starts in the exponential growth phase, and continued during the stationary growth phase. CONCLUSIONS: Higher EPS yields were obtained on cultures grown on glucose + fructose. O. oeni produces a beta-glucan, as the predominant EPS, and it is also able to produce two heteropolysaccharides. Significance and Impact of the Study: This work provides a better understanding of EPS synthesis by O. oeni and shows the first EPS structure described for this species. 相似文献
14.
Some physicochemical properties of the microbial exopolysaccharide (EPS) ethapolan synthesized by Acinetobacter sp. 12S depended on whether the producer was grown on a mixture of ethanol and glucose or on single substrates. Irrespective of the carbon source in the nutrient medium, the contents of carbohydrates, pyruvic acid, uronic acids, and mineral components in the EPS remained unchanged. The EPS were also identical in their monosaccharide composition: the molar ratio of glucose, mannose, galactose, and rhamnose was 3:2:1:1. EPS with a higher proportion of fatty acids was synthesized during growth on the mixture of ethanol and glucose. Average molecular weight and the proportion of high-molecular (over two million) fractions were greater in ethapolan produced on the substrate mixture. In the presence of 0.1 M KCl, after transformation into the H+ form, and in the Cu(2+)-glycine system, solutions of these EPS showed higher viscosity than solutions of EPS synthesized on single substrates. The reasons for the improved rheological properties of the EPS produced on the substrate mixture are discussed. 相似文献
15.
Some physicochemical properties of the microbial exopolysaccharide (EPS) ethapolan synthesized by Acinetobacter sp. 12S depended on whether the producer was grown on a mixture of ethanol and glucose or on a single substrate. Irrespective of the carbon source in the nutrient medium, the contents of carbohydrates, pyruvic acid, uronic acids, and mineral components in the EPS remained unchanged. The EPS were also identical in their monosaccharide composition: the molar ratio of glucose, mannose, galactose, and rhamnose was 3 : 2 : 1 : 1. EPS with a higher content of fatty acids was synthesized during growth on the mixture of ethanol and glucose. The average molecular mass and the content of high-molecular (M > 2 MDa) fractions were greater in ethapolan produced on the substrate mixture. In the presence of 0.1 M KCl, after transformation into the H+ form, and in the Cu2+–glycine system, solutions of these EPS showed higher viscosity than solutions of EPS synthesized on single substrates. The reasons for the improved rheological properties of the EPS produced on the substrate mixture are discussed. 相似文献
16.
【背景】胞外多糖(exopolysaccharide,EPS)是乳酸菌生长代谢过程中所产生的一种次级代谢产物,除了可以改善产品质构和品质外,其生理功能也是近年来研究人员追捧的热点。【目的】探究乳酸菌EPS的表征特性和分子结构,揭示其与EPS益生特性之间的联系。【方法】以产EPS的嗜热链球菌(Streptococcus thermophilus,S. thermophilus) MGB80-7为研究对象,利用苯酚-硫酸法测定菌株EPS产量。采用离子交换柱层析和凝胶分子筛层析对该菌株所产EPS进行分离纯化,结合凝胶色谱、红外光谱及高效液相色谱对EPS表型结构进行剖析。此外,为确定EPS表型特征对其抗氧化活性的影响,测定了EPS对超氧阴离子、羟自由基及DPPH自由基等的清除能力。【结果】S. thermophilus MGB80-7在M17培养基中EPS产量较高,为(268.25±5.36) mg/mL,分离纯化后共得到2种多糖组分,其中中性多糖(WPS-807)分子量为1.028×105 Da,主要由葡萄糖、半乳糖和甘露糖组成,并含有少量的鼠李糖和阿拉伯糖,酸性多糖(... 相似文献
17.
[目的]研究云南5个地区(晋宁、祥云、程海、泸沽湖、洱海)的戟叶酸模(Rumex hastatus)花中的酵母菌和类酵母.[方法]采用涂布平板法对5个地区的戟叶酸模花中酵母菌和类酵母进行分离,通过26S rDNA Dl/D2区域序列分析并结合形态观察对分离获得的酵母菌和类酵母进行鉴定;采用胞外酶定性筛选培养基进行产酶筛选;用苏丹黑B染色法筛选产油脂菌株.[结果]从戟叶酸模花中分离得到82株酵母菌和99株类酵母;82株酵母菌鉴定为6个属16个种和1个潜在新种,99株类酵母鉴定为短梗霉属(Aureobasidium)的普鲁兰类酵母(A.pullulans)及3个变种;戟叶酸模花中的优势属是类酵母短梗霉属,其次为红酵母属(Rhodotorula)和隐球酵母属(Cryptococcus);筛选到134株具有产胞外酶活性和83株产油脂的酵母菌和类酵母.[结论]研究结果显示5个地区的戟叶酸模花中酵母菌和类酵母种类多样性较为丰富,并具有产淀粉酶、蛋白酶、纤维素酶、脂肪酶和油脂的特点,有潜在的应用前景. 相似文献
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【目的】嗜热链球菌IMAU20246是一株具有良好发酵特性且高产胞外多糖(exopolysaccharides,EPS)的菌株,但其EPS基因簇及合成途径尚不清晰。因此可通过全基因组测序及生物信息学分析菌株基因组序列,探究EPS合成及调控机制。【方法】本实验对嗜热链球菌IMAU20246进行全基因组测序并进行生物信息学分析,解析EPS生物合成相关基因簇及EPS合成途径,同时采用实时荧光定量PCR技术(quantitative real-time PCR,qRT-PCR)对其不同时间点EPS基因簇的表达进行定量分析。【结果】嗜热链球菌IMAU20246基因组中有一个18.1 kb的EPS生物合成基因簇,编码15个与EPS生物合成相关的基因。嗜热链球菌IMAU20246通过转运葡萄糖、甘露糖、果糖、半乳糖、乳糖、海藻糖、纤维二糖及蔗糖合成UDP-葡萄糖、dTDP-葡萄糖、dTDP-鼠李糖、UDP-半乳糖、UDP-呋喃半乳糖、UDP-N-乙酰葡萄糖胺和UDP-N-乙酰半乳糖胺等7种糖核苷酸。qRT-PCR的结果表明,EPS基因簇中的基因在细胞生长阶段均能表达,特别是糖基转移酶基因epsE、epsF、epsH和epsJ在培养6 h时表达量最高,此时EPS产量达到最高。【结论】本研究从基因组解析了嗜热链球菌IMAU20246 EPS基因簇及其合成途径,为菌株的进一步开发提供了理论依据。 相似文献
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Qi-Long Qin Yi Li Mei-Ling Sun Jin-Cheng Rong Sheng-Bo Liu Xiu-Lan Chen Hai-Nan Su Bai-Cheng Zhou Bin-Bin Xie Yu-Zhong Zhang Xi-Ying Zhang 《PloS one》2015,10(2)
Many marine bacteria secrete exopolysaccharides (EPSs) that have important ecological and physiological functions. Numerous nutritional and environmental factors influence bacterial EPS production. However, the regulatory mechanisms of EPS production are poorly understood. The deep-sea Bacteroidetes bacterium Zunongwangia profunda SM-A87 can produce high quantities of EPS, and its EPS production is enhanced significantly by lactose. Here, we studied the reasons behind the significant advantage that lactose has over other carbon sources in EPS production in SM-A87. RNA-seq technologies were used to study lactose-regulated genes in SM-A87. The expression level of genes within the EPS gene cluster was up-regulated when lactose was added. Supplement of lactose also influenced the expression of genes located outside the EPS gene cluster that are also involved in EPS biosynthesis. The major glycosyl components of SM-A87 EPS are mannose, glucose and galactose. Genomic metabolic pathway analyses showed that the EPS precursor GDP-mannose can be synthesized from glucose, while the precursor UDP-glucose must be synthesized from galactose. Lactose can provide glucose and galactose simultaneously and prevent glucose inhibition. Lactose can also greatly stimulate the growth of SM-A87. Taken together, lactose acts not only as an inducer but also as a carbohydrate source for EPS production. This research broadens our knowledge of the regulation of EPS production in marine bacteria. 相似文献