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1.
先对不同产地采集的竹黄菌进行筛选,得到优产竹红菌素的菌株,然后采用单因子和3因素3水平正交试验法对竹红菌素液体发酵条件进行优化,在优化培养基的基础上,选用不同浓度的Cr3+、Fe3+、Cu2+和Ca2+对竹红菌素进行离子调控研究.结果表明:从休宁所采集的菌株不仅生长速度最快,发酵所产的竹红菌素含量也最高;竹红菌素最佳发酵碳源是葡萄糖,最佳发酵氮源是硝酸钠,最佳培养基组合为2%葡萄糖,0.2%硝酸钠,pH7.5;Cr3+和Fe3+浓度为0.005%时竹红菌素含量均最高;0.05%的Ca2+最有利于竹红菌素的分泌;Cu2+为0.03%时竹红菌素含量达到最大值. 相似文献
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目的:筛选并优化竹黄菌液体发酵培养基。方法:采用单因子和3因素3水平正交试验法,从生物量和竹红菌素两方面筛选碳源、氮源和pH,探讨该菌生长的最佳培养条件。结果:最佳发酵碳源是葡萄糖,最佳发酵氮源是硝酸钠。竹红菌素生长的最佳配方为2%葡萄糖,0.2%硝酸钠,pH7.5;菌丝体生长的最佳组合为2%葡萄糖,0.3%硝酸钠,pH7.5。 相似文献
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目的:对产淀粉酶嗜热菌Anoxybacillu sp.菌株进行培养基优化及产酶条件研究,以便提高菌株的产酶能力,并为下一步菌
株的诱变育种研究提供基础。方法:常规方法液体培养菌株,用平板初筛和DNS法复筛选择产淀粉酶能力较高的菌株;单因素筛
选培养基最适的碳源、氮源、Ca2+浓度和Mg2+浓度,对单因素筛选的最佳碳源、氮源、Ca2+和Mg2+的三个较佳浓度进行四因素三
水平正交试验优化培养基;对培养基不同pH值及不同培养温度进行培养条件研究。结果:产淀粉酶菌株筛选结果显示:六株菌中
淀粉酶酶活力值最大的是菌株Anoxybacillu sp.DL4,差异有统计学意义(P<0.05)。培养基单因素筛选结果显示:最适碳源为麦芽糖、最适氮源为
硝酸铵、最适Ca2+、Mg2+浓度均为0.02%,差异有统计学意义(P<0.05)。培养基优化结果显示:C 源0.1 %,N源0.2 %,Mg2+ 0.04%,
Ca2+ 0.04 %为最佳的培养基成分组合。产酶条件筛选结果显示:培养基pH 值为6、培养温度为55 ℃时菌株产酶水平最高,差异有
统计学意义(P<0.05)。结论:培养基的优化及最适的产酶条件能提高嗜热菌Anoxybacillu sp.DL4 产淀粉酶能力,Ca2+、Mg2+离子
对菌株产淀粉酶有促进作用。 相似文献
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对产竹红菌素的菌株SUPER-H168的ITS-5.8S rDNA进行了序列测定和进化树聚类分析,表明其属于竹黄属;对该菌株固态发酵产竹红菌素的条件进行了初步优化,得到的初步优化条件为玉米渣25g,麸皮5g,葡萄糖1.5g,NaNO3 0.15g,ZnSO4·7H2O 0.03g,起始含水量为50%,起始pH为7.0,培养温度为30℃。在该条件下发酵18d,竹红菌素的产量为9.37mg/g干基。 相似文献
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桔青霉生产核酸酶的发酵条件研究 总被引:1,自引:0,他引:1
对通过紫外线和60Co两次育种得到的桔青霉W48高产菌株培养基的单组分和发酵条件进行了优化,最后又用正交实验对培养基的各组分的浓度进行了优化。得到了产酶量最高的培养基组分(质量分数)是:KH2PO40.05%,K2HPO40.03%,酵母膏+蛋白胨0.7%,CaCl20.02%,MgSO40.04%,ZnSO40.03%,葡萄糖5%,pH5.5。最佳发酵条件是:接种量10%,装液量50 mL,摇床转速180 r/min,温度30℃,发酵时间66 h。用最佳培养基和最佳发酵条件发酵生产核酸酶的酶活力为758.10 U/mL,原始菌种产核酸酶的酶活力为272.26 U/mL,提高了2.78倍。 相似文献
6.
米曲霉(Aspergillus oryzae)FSO179产α-淀粉酶固体发酵优化结果表明:最佳有机碳源为玉米粉,最佳有机氮源为花生饼粉;培养基正交试验表明最佳培养基配方为:花生饼粉20%,玉米粉5%,无机盐为c组配方;初始发酵pH为7.4;最适的发酵温度为33℃;在以上最适条件下固体培养6d,发酵产酶水平可达1300.6u/g,优化结果比初始设计提高了42.9%。该酶酶学特性研究表明:该酶作用的最适温度为55℃;最适作用pH为4.0;Fe2 、Ba2 、Cu2 、Mn2 、Fe3 金属离子对酶具较强抑制作用,而Ca2 对酶具有一定激活作用。 相似文献
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目的:提高酵母产γ-氨基丁酸的能力。方法:采用单因素及正交设计实验对酵母产γ-氨基丁酸(GABA)的培养基进行优化。结果:确定最适碳源为葡萄糖,最佳氮源为蛋白胨和硫酸铵复合氮源,合适的无机盐为KH2PO4;最佳发酵培养基为3%葡萄糖,3%蛋白胨,0.3%(NH4)2SO4和0.1%KH2PO4。在此培养条件下,摇瓶发酵可以获得1.690g.L-1的GABA产量。结论:发酵培养基的优化,提高了菌株产γ-氨基丁酸的能力。 相似文献
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对极地适冷菌Pseudoalteromonas sp. QI-1产适冷蛋白酶的发酵条件进行优化。结果表明:菌株QI-1的最适生长和产酶温度均为5℃;最佳接种量为1%;发酵培养基的最适初始pH和最佳装样量分别为5和10%;盐度为2%时对菌株的生长和产酶最为有利;麸皮和醋酸钠分别为最佳N源和C源;添加0.75%酪蛋白时菌株QI-1胞外蛋白酶的活性最高;10 mmol/L Mg2+和0.5%Tween-80有利于产酶。正交试验结果表明:菌株Pseudoalteromonassp. QI-1产蛋白酶较佳培养基配方(g/L)为麸皮5,酵母粉2.5,酪蛋白3,MgCl2.6H2O 3,KCl 1.5;发酵液比酶活为166.20 U/mL,较优化前提高了约56%。 相似文献
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以紫外(UV)与亚硝基胍诱变的竹黄菌(Shiraia bambusicola)菌株NU12和UV4为出发菌株,60℃处理5 min、紫外(距离30 cm,30 W)照射90s进行双亲原生质体灭活,通过30%聚乙二醇PEG6000介导原生质体融合20 min.结合平板初筛和高效液相色谱( HPLC)分析进行复筛,通过3轮重组融合操作,筛选出6株高产竹红菌甲素的融合株.其中融合菌株FIII - 21的竹红菌甲素产量达到80.4 mg/L,比原始出发菌株提高了58.9%~167.1%,且遗传稳定,具有较高的医药及工业应用价值. 相似文献
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还原六价铬细菌及其还原酶的研究 总被引:1,自引:0,他引:1
从活性污泥中筛选出的C-2苏云金芽孢杆菌,能耐受250mg/L的六价铬,并具有较好的还原能力。研究表明木糖、果糖、玉米饼粉、苹果酸、琥珀酸、柠檬酸及Cu2+、Fe2+、Ca2+离子对C-2菌的还原有积极作用,菌体的接种量影响还原的速率。C-2菌还原的最适温度为37℃,最适pH为9.0;六价铬还原酶的最适pH为7.0、温度为37℃,Co2+、Cu2+、Fe2+、DTT、NADH对酶的还原有积极影响。 相似文献
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1,5-Dihydroxy-3-methoxy-7-methylanthracene-9,10- dione (shiraiarin) is a kind of antitumor and antibacterial anthraquinone, and was produced for the first time from the submerged fermentation of Shiraia bambusicola, as confirmed by ESI-MS and NMR. The production of shiraiarin was significantly influenced when varying the carbon source, and a high amount of shiraiarin was only achieved when using lactose. The production of shiraiarin was also stimulated when using NaNO3 as the nitrogen source, whereas other nitrogen sources inhibited its production. Shiraiarin was formed during the stationary phase with a pH value higher than 8. The production of shiraiarin was inhibited by sporulation. 相似文献
15.
为研究竹黄菌与竹红菌化学成分及细胞毒活性的差异,本研究通过高效液相色谱(HPLC)分析结合常规色谱方法,分离鉴定了两种真菌的6个相同成分,分别为3个主要成分竹红菌甲素(1)、竹红菌乙素(2)和竹红菌丙素(3),以及3,6,8-三羟基-1-甲基口山酮(7)、3,8-二羟基-6-甲氧基-1-甲基口山酮(8)和过氧麦角甾醇(9)。另外,从竹黄菌中还分离得到11,11′-二去氧沃替西林(5)、麦角甾-7,22E-二烯-3β,5α,6β-三醇(10)和麦角甾-7,22E-二烯-2β,3α,9α-三醇(11),并首次从竹红菌中分离得到竹红菌丁素(4)、灰黄霉素(6)、化合物7和8。活性筛选发现,化合物5对三株肿瘤细胞NCI-H1975、HepG2和MCF-7有很强细胞毒活性,化合物1有较强细胞毒活性,而化合物6活性较弱。 相似文献
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研究了里氏木霉GXC产木聚糖酶的条件和酶学性质。结果表明,适宜产酶碳源为乳糖、甘露糖、棉子糖、木聚糖和麸皮,氮源为牛肉膏和酵母膏;产酶的最适初始pH为4.0,30℃培养60h。对以麸皮为碳源的培养液进行纯化的酶特性研究表明,木聚糖酶的最适反应温度为50℃,pH为5.5,该酶在pH5.0(7.0和40℃以下相对稳定。Fe3+和Mn2+对木聚糖酶有较大的促进作用,Cu~2+、Fe~2+和Ca~2+ 具有抑制作用。 相似文献
18.
R S Green 《Journal of general microbiology》1985,131(11):2871-2876
Three proteinase isoenzymes from one benign strain of Bacteroides nodosus and five proteinase isoenzymes from each of two virulent strains of B. nodosus were purified by horizontal slab polyacrylamide gel electrophoresis. The purified isoenzymes hydrolysed casein, collagen I, collagen III, elastin, alpha-elastin, fibrinogen, gelatin, haemoglobin and alpha-keratin. The pH optima of all the isoenzymes lay between 7.25 and 9.5, the range of 8.75-9.25 being common to all. The isoenzymes were inhibited by phenylmethylsulphonyl fluoride, diphenylcarbamyl chloride, L-(1-tosylamide-2-phenyl)ethyl chloromethyl ketone, EGTA and EDTA, indicating that they were chymotrypsin-like serine proteinases that require a metal ion for stability or activity. EDTA inhibition was not reversed by addition of Ca2+ or Mg2+. Some isoenzymes were activated by Mg2+, Ca2+, Cr3+ and Se4+ and all were inhibited by Fe2+, Co2+, Cu2+, Zn2+, Cd2+ and Hg2+. Isoenzymes from benign strains had a lower temperature stability, losing all activity at 55 degrees C, whereas those from virulent strains lost all activity at 60 degrees C. 相似文献
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报道了弹性蛋白亲和层析分离纯化芳香黄杆菌产胞外弹性蛋白酶。经一步柱层析可获聚丙烯酰胺凝胶电泳均一的酶制品,收率可达50%,并制备了酶的结晶。该酶在SDS-PAGE上测得分子量为21380,IEF-PAGE测得等电点8.9,最适作用温度为50℃,最适作用pH为7.4,在40℃以下热稳定性良好,pH4.5-9.5范围内稳定,重金属离子Fe3+、Zn2+、Cr3+、Co2+、Hg2+、Ni2+、Ag+、Cu2+等严重抑制酶活性,黄杆菌弹性蛋白酶除了特异水解弹性蛋白外,对干酪素、血纤维蛋白、白蛋白、明胶、血红蛋白等多种蛋白质均能水解。 相似文献
20.
B. F. Cooper V. Sideraki D. K. Wilson D. Y. Dominguez S. W. Clark F. A. Quiocho F. B. Rudolph 《Protein science : a publication of the Protein Society》1997,6(5):1031-1037
For murine adenosine deaminase, we have determined that a single zinc or cobalt cofactor bound in a high affinity site is required for catalytic function while metal ions bound at an additional site(s) inhibit the enzyme. A catalytically inactive apoenzyme of murine adenosine deaminase was produced by dialysis in the presence of specific zinc chelators in an acidic buffer. This represents the first production of the apoenzyme and demonstrates a rigorous method for removing the occult cofactor. Restoration to the holoenzyme is achieved with stoichiometric amounts of either Zn2+ or Co2+ yielding at least 95% of initial activity. Far UV CD and fluorescence spectra are the same for both the apo- and holoenzyme, providing evidence that removal of the cofactor does not alter secondary or tertiary structure. The substrate binding site remains functional as determined by similar quenching measured by tryptophan fluorescence of apo- or holoenzyme upon mixing with the transition state analog, deoxycoformycin. Excess levels of adenosine or N6- methyladenosine incubated with the apoenzyme prior to the addition of metal prevent restoration, suggesting that the cofactor adds through the substrate binding cleft. The cations Ca2+, Cd2+, Cr2+, Cu+, Cu2+, Mn2+, Fe2+, Fe3+, Pb2+, or Mg2+ did not restore adenosine deaminase activity to the apoenzyme. Mn2+, Cu2+, and Zn2+ were found to be competitive inhibitors of the holoenzyme with respect to substrate and Cd2+ and Co2+ were noncompetitive inhibitors. Weak inhibition (Ki > or = 1000 microM) was noted for Ca2+, Fe2+, and Fe3+. 相似文献