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1.
苏云金杆菌33菌株最佳培养基和发酵条件研究 总被引:1,自引:1,他引:0
应用正交试验L27(313)对鳞翅目昆虫高毒效的苏云金杆菌33菌株的发酵培养基进行研究,得到了适合其发酵培养的优化复合培养基配方—0.5%玉米粉 2.00%黄豆粉 0.15%酵母粉 0.25%鱼粉 0.075%蛋白胨 0.25%磷酸二氢钾 0.05%碳酸钙 0.035%硫酸镁。另外实验还证实适当增加通气量、发酵初始酸碱度控制在pH7.5、发酵温度30℃、转速180r/min、培养40h更适合该菌株液体深层发酵。 相似文献
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目的:对一株从广西山口红树林保护区筛选得到的具有广谱抗菌活性的红树林细菌G1进行发酵条件的研究.方法:采用单因素实验法对G1产抗菌活性物质的发酵培养基及培养条件进行研究.结果:确定了红树林细菌G1的最佳发酵培养基为:蔗糖2.0%、酵母粉1.5%、NaCl1%.最佳发酵培养条件为:装液量40%、接种量5%、发酵时间84h、初始pH值8.0,优化后G1发酵液的抗菌活性提高了2倍.结论:初步确定了G1发酵的条件,为工业化生产抗菌活性物质提供了理论依据. 相似文献
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对1株产抑菌物质的海洋真菌Caldariomyces fumago S-5的培养条件的优化进行研究,探讨该菌株的发酵产抑菌物质的性能。通过抗菌谱实验、单因素及正交实验设计研究了该菌株所产抗菌物质的押菌特征和最适发酵条件。结果表明,S-5菌株发酵液对几种G^+和G^-致病细菌具有快速的生长抑制作用,而对真菌没有明显抗菌性。发酵条件优化结果表明:菌株在葡萄糖4%、(NH4)2SO4 0.2%、KCl 0.2%、K2HPO40.2%、Fe2SO4·7H2O 0.002%、MgSO4-2H2O 0.1%、20%马铃薯浸出液的培养基中,控制发酵温度25℃,pH值5.0,接种量1-2cm。菌苔/100mL培养液,摇瓶转速240r/min条件下培养120h,发酵液中抑菌效价最高。实验结果可为该海洋微生物资源的开发利用提供依据。 相似文献
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蜡状芽孢杆菌S1发酵条件的研究 总被引:4,自引:0,他引:4
对一种新近分离的蜡状芽孢杆菌(Bacillus Cereus)菌株S1发酵产新型抗真菌多肽APS的发酵培养基组成(碳,氮源)和工艺条件(发酵温度,初始,PH,通气方式和通气量)进行了摸索,通过单因互实验和正交优化实验,确定了S1发酵培养基的组成。麸皮5%,玉米粉5%,尿素0.2%,或NH4NO31.5%,酵母浸亮1.5%,葡萄糖6%,NaCl0.1%;最适发酵培养温度为28度;最适发酵培养初始Ph为7.4或6.8,。在优化条件下,效价最高为8-10mg/ml,S1生长的最适温度和初始PH为30度和7.0,通气对S1发酵具有显著的影响。 相似文献
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本文研究了少孢根霉RT-3固态发酵生产SOD的条件。结果表明该菌发酵培养基的优化组成为:大豆,麸皮5%,硫酸氢0.3%,磷酸二氢钠0.03%,硫酸铜0,04%。培养基经代化后,每克培养物SOD酶活提高53%。适宜的乳酸加入量为1%。吐温-80、醋酸钠和抗坏血酸对菌体产酶没有作用。 相似文献
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对生防链霉菌Ⅲ-61产生抗真菌活性物质的摇瓶发酵工艺进行了研究。利用正交试验设计优化了发酵培养基组分,其最适配方为黄豆粉1.5%,蛋白胨0.3%,蔗糖1.0%,淀粉1.3%,磷酸二氢钾0.02%,硫酸镁0.025%,氯化钠0.5%,配咸水溶液,调pH至7~7.4,加碳酸钙1%。通过单因素试验,筛选获得了最优培养条件组合:液体种龄24h,接种量5%~10%,500mL摇瓶培养基装量为80mL,摇床转速240r/min,培养温度31℃,发酵周期96~120h。此优化的发酵培养基与发酵条件的组合昕得菌株Ⅲ-61发酵液对主要靶标黄瓜灰霉病菌的抑菌圈直径达49.5mm,较优化前提高了45.59%。 相似文献
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采用响应面法对产生抑菌活性物质的波赛链霉菌(Streptomyces peucetius)菌株JMC 06001的发酵培养基进行优化。首先采用Minnimum Run Equireplicated Res IV设计对初始发酵培养基的8个营养因素进行筛选,获得影响产生抑菌活性物质的3个主要影响因素:葡萄糖、大豆粉和NaCI;然后用最陡爬坡实验快速逼近最大响应区域;最后,结合Box-Behnken设计及响应面分析,确定主要影响因素的最佳浓度,得出该菌株产抑菌活性物质的最优发酵培养基配方为:葡萄糖1.2%,麦芽糖0.7%,蛋白胨0.9%,大豆粉1.4%,NaCl3.7%,CaCO3 0.1%,复合盐A液2.0%,复合盐B液0.1%,起始pH值7.0。用优化后的培养基发酵所得发酵液对敏感指示菌藤黄八叠球菌的抑菌圈直径达31.5mm,与预测值的相对偏差仅为1.59%,与用初始发酵培养基发酵所得发酵液的抑菌效果(抑菌圈直径26.5mm)相比提高了18.9%。 相似文献
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通过对怀山药(Dioscorea opposita)种质资源的包埋玻璃化超低温保存与植株再生进行研究,结果表明:将低温下锻炼7天的怀山药试管苗带芽茎段放入预培养基中,低温下培养3天,然后在室温下用3%的海藻酸钠和0.5mol·L-1CaCl2包埋,包埋珠用MS+0.2mol·L-1蔗糖+2mol·L-1甘油+50g·L-1二甲基亚砜在0°C下装载60分钟,用30%甘油+15%乙二醇+10%二甲基亚砜+15%聚乙二醇+0.4mol·L-1蔗糖在0°C下脱水60分钟,迅速投入液氮,24小时后立即用40°C水浴快速化冻,再用MS+0.5mol·L-1蔗糖溶液洗涤2次,转入再生培养基中培养,可获得再生植株。再生植株成活率因基因型而异,铁棍山药、太谷山药、怀庆1号山药和B号山药的成活率分别为64.29%、49.21%、13.11%和39.81%。 相似文献
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Plant regeneration from immature embryos of 48 elite CIMMYT bread wheats 总被引:13,自引:0,他引:13
S. Fennell N. Bohorova M. van Ginkel J. Crossa D. Hoisington 《TAG. Theoretical and applied genetics. Theoretische und angewandte Genetik》1996,92(2):163-169
Forty-eight bread wheat (Triticum aestivum L.) released cultivars and elite advanced lines were evaluated for their ability to produce embryogenic callus using three different media. Basal N6 medium supplemented with dicamba (E1), MS medium containing 2,4-D (E3) or MS medium containing 2,4-D plus different amino acids (E5) were used for callus initiation and maintenance. Plant regeneration was achieved on basal MS medium with indole-3-acetic acid (IAA) and 6-benzylamino purine (BAP) and rooting on MS with 1-naphthaleneacetic acid (NAA). Percentage regeneration varied widely with both genotype and initiation medium, with values ranging from 2% to 94%. The number of plantlets produced per embryo ranged from 6 to 42. Thirteen genotypes showed at least 50% regeneration after culture on E5 medium; 3 genotypes after culture on E3 initiation medium and 1 after initiation on E1. After four subcultures, over a 16-week period, 41 genotypes (85%) lost their ability to regenerate plants while the remaining 7 lines (15%) retained plant regeneration potential but at reduced levels. E3 medium was found to be the best for maintaining regeneration potential after four subcultures. 相似文献
13.
Simon N. Gray Peter Robinson Neil Wilding Paul Markham 《FEMS microbiology letters》1990,68(1-2):131-136
Abstract The aphid-pathogenic fungus Erynia neophidis grew on a semi-defined medium containing 16 g·1−1 glucose, 3 g·1−1 yeast extract and 5 g·1− mycological peptone only when the medium was supplemented with low concentrations of certain fatty acids. Of these, oleic acid fulfilled the growth requirement at a concentration of 0.02% (v/v), but higher concentrations were toxic, causing complete loss of viability of cultures at a concentration of 0.2% (v/v) in liquid medium and at 4% (v/v) on solid medium. The reduced viability of the fungus in liquid culture compared to that on equivalent solid medium, and at low inoculum density compared to high inoculum density in liquid medium, is explicable in terms of this toxicity. 相似文献
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A rapid regeneration protocol for proembryos of Phaseolus angustissimus as young as 1 day after pollination (DAP) involving pod culture for 1 week followed by embryo culture for 2 weeks and embryo germination for 1 or 2 weeks is provided. Optimization of the media was conducted with pods collected 3 DAP. The best pod culture medium was composed of basal medium [(Phillips and Collins 1979) salts with (Geerts et al. 2001) vitamins], 1000 mg l−1 glutamine, 1000 mg l−1 casein hydrolysate, 3% sucrose and 0.5% agar. Embryo culture medium consisted of basal medium with 500 mg l−1 glutamine, 250 mg l−1 casein hydrolysate, 1.9 μM ABA, 3% sucrose and 0.5% bacto-agar. Embryos developed into plantlets on germination medium containing basal medium with 0.25 μM BA, 3% sucrose and 0.7% bacto-agar. Fertile, normal plants were recovered from direct embryogenesis and from micrografted embryo-derived shoots. Embryos obtained from pods collected 3 DAP regenerated plantlets at a rate of 29.3%, while embryos from pods collected 2 DAP and 1 DAP regenerated at rates of 20.2 and 4%, respectively. A second accession of P. angustissimusregenerated at a rate of 26.2%. Using this 5-week protocol for P. vulgaris resulted in a plantlet regeneration rate of 12.5%. 相似文献
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An attempt is made to determine the optimum concentration of bile and brilliant green in brilliant green lactose peptone bile medium, for use in the presumptive test in the bacteriological examination of water. Comparisons, showing the effect of bile and brilliant green upon the development of the colon organism, were made by making actual bacterial counts after a definite short incubation period. The results indicate that the original medium described by Muer and Harris, (5% dried bile, 1% peptone, 1% lactose, and 1:10,000 billiant green) when adjusted to pH = 7.1, did not show an appreciable inhibition of the colon organism. It is further shown that a medium containing 2% bile, 1% peptone, 1% lactose and 1:75,000 brilliant green supports a more rapid development of the colon organism at pH = 6.9 than does the original brilliant green bile medium at its optimum pH. 相似文献
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《Biotechnic & histochemistry》2013,88(4):129-134
An attempt is made to determine the optimum concentration of bile and brilliant green in brilliant green lactose peptone bile medium, for use in the presumptive test in the bacteriological examination of water. Comparisons, showing the effect of bile and brilliant green upon the development of the colon organism, were made by making actual bacterial counts after a definite short incubation period. The results indicate that the original medium described by Muer and Harris, (5% dried bile, 1% peptone, 1% lactose, and 1:10,000 billiant green) when adjusted to pH = 7.1, did not show an appreciable inhibition of the colon organism. It is further shown that a medium containing 2% bile, 1% peptone, 1% lactose and 1:75,000 brilliant green supports a more rapid development of the colon organism at pH = 6.9 than does the original brilliant green bile medium at its optimum pH. 相似文献
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A simple method for mouse embryo cryopreservation in a low toxicity vitrification solution, without appreciable loss of viability 总被引:33,自引:0,他引:33
M Kasai J H Komi A Takakamo H Tsudera T Sakurai T Machida 《Journal of reproduction and fertility》1990,89(1):91-97
Mouse morulae were exposed to solutions containing 30-50% of permeable agents (ethylene glycol, glycerol, propylene glycol) in modified phosphate-buffered saline (PB1 medium) at 20 degrees C for 20 min. A high percentage of them developed to expanded blastocysts in culture, after exposure to 30% and 40% ethylene glycol (98 and 84%, respectively), or 30% glycerol (88%). Ethylene glycol and glycerol were diluted to 30 and 40% with PB1 medium or with PB1 containing 30% Ficoll or 30% Ficoll + 0.5 M-sucrose, immersed in liquid nitrogen in straws and warmed in 20 degrees C water. Solutions containing 40% of a permeable agent with Ficoll did not crystallize during cooling or warming. Mouse morulae were exposed to 40% ethylene glycol in PB1 medium containing 30% Ficoll (EF) or PB1 medium + 30% Ficoll + 0.5 M-sucrose (EFS) for 5-20 min at 20 degrees C. EFS solution was non-toxic to the embryos during 5 min of exposure. When embryos, equilibrated in EFS solution for 2 or 5 min at 20 degrees C, were vitrified at -196 degrees C and were warmed rapidly, nearly all embryos developed in culture (97-98%), and 51% developed to live young at term after transfer. This method, which results in virtually no decrease in embryonic viability, may be of practical use for embryo preservation. 相似文献
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Rabbit retinas were maintained in vitro in medium that resembled CSF but with leucine varied from 2 to 1000 microM. Both leucine and threonine were isotopically labelled. When leucine in the medium was 100-1000 microM, leucine was incorporated into protein at 2.03 +/- 0.04 (S.E.M.) mumol/g dry wt./h, a turnover per h of 0.55% of the leucine in retinal protein. Incorporation was constant for at least 7 h. It was reduced 34% when the other amino acids were omitted from the medium and 24% when they were increased 15 fold above physiological levels. When medium leucine was reduced to 2 microM with other amino acids constant, 14C-leucine incorporation fell 70% without significant change in 3H-threonine incorporation, indicating a fall in intracellular specific activity of leucine. The intracellular/extracellular concentration ratio of labelled leucine was 4:1 with medium leucine 23 microM. It fell markedly when medium leucine was reduced to 2 microM or increased to 1000 microM. The concentration ratio of labelled threonine was 15:1 with medium leucine at physiological levels but fell to 6:1 when medium leucine was increased to 1000 microM. Decarboxylation removed 1.5% of free intracellular leucine per min and, at physiological concentrations, was 7.7% the rate of protein incorporation. The ratio of protein synthesis/breakdown, estimated from changes in leucine and 7 other essential amino acids in the medium, was nearly unity. The potential of this preparation for study of CNS protein metabolism is discussed. 相似文献
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Lim KT Jang G Ko KH Lee WW Park HJ Kim JJ Kang SK Lee BC 《Animal reproduction science》2008,103(3-4):239-248
The aim of this study was to examine the effects of modifications to a standard slow freezing protocol on the viability of in vitro produced bovine embryos. Bovine oocytes were matured, fertilized with frozen-thawed semen, and presumptive zygotes cultured in defined two-step culture media. The standard freezing medium was 1.5M ethylene glycol (EG), 0.1M sucrose, 10% fetal bovine serum (FBS) in Dulbecco's phosphate buffered saline (D-PBS). A preliminary trial showed that in vitro produced embryos cryopreserved in this medium had a survival rate of 74.6% at 24h and 53.5% at 48 h post-thaw. Experiment 1 studied the effects of omitting the sucrose supplement or replacing it with 0.1M xylose. In Experiment 2, the effects of partial (0%, 25% or 50%) or total (100%) replacement of sodium chloride with choline chloride in the cryopreservation medium were examined (the medium with 100% replacement was designated CJ1). The effects of replacing the 10% FBS with 0.4% BSA or 0.4% lipid-rich BSA (Albumax I) in CJ1 was studied in Experiment 3. In Experiment 4, pregnancy/calving rates following the post-thaw transfer of in vitro produced embryos cryopreserved in the standard freezing medium were compared with those of in vitro and in vivo produced embryos cryopreserved in the improved medium (Albumax I in CJ1). Supplementation of the cryopreservation medium with 0.1M sucrose resulted in higher post-thaw survival rates at 24 h (71.3% versus 53.5 and 51.7%; P<0.05), 48 h (51.1% versus 45.3 and 40.2%), and 72 h (34.0% versus 24.4 and 23.0%) than 0.1M xylose or no supplement, respectively, in Experiment 1. Experiment 2 showed that embryos cryopreserved in the standard medium had poorer survival rates at 24 h (72.8% versus 86.5%; P<0.05), 48 h (53.1% versus 66.3%) or 72 h (28.4% versus 44.9%) than those frozen in CJ1. The post-thaw survival rate of embryos frozen in medium supplemented with Albumax I was better than that for the FBS or BSA supplements at 24h (92.0% versus 90.7 and 87.3%), 48 h (87.3% versus 76.9 and 70.9%; P<0.05), and 72 h (70.4% versus 49.1 and 46 4%; P<0.05; Experiment 3). In Experiment 4, in vitro produced embryos cryopreserved in CJ1 medium supplemented with Albumax I resulted in higher pregnancy rates at Day 35 (31.9% versus 22.9%) and Day 60 (24.1% versus 14.3%) of gestation, and calving rates (22.6% versus 10.0%; P<0.05) than similar embryos frozen in the standard medium. However, in vivo produced embryos cryopreserved in Albumax I in CJ1 resulted in higher pregnancy rates at Day 35 (50.7%; P<0.05) and Day 60 (45.1%; P<0.05) of gestation, and calving rate (43.7%; P<0.05). It was concluded that modification of the freezing medium by addition of lipid-rich BSA and replacing sodium chloride with choline chloride improves the post-thaw survival of in vitro produced embryos, and their viability post-transfer. 相似文献
20.
怀山药种质资源的包埋玻璃化超低温保存与植株再生 总被引:3,自引:0,他引:3
通过对怀山药(Dioscorea opposita)种质资源的包埋玻璃化超低温保存与植株再生进行研究,结果表明:将低温下锻炼7天的怀山药试管苗带芽茎段放入预培养基中,低温下培养3天,然后在室温下用3%的海藻酸钠和0.5mol·L-1CaCl2包埋,包埋珠用MS+0.2mol·L-1蔗糖+2mol·L-1甘油+50g·L-1二甲基亚砜在0°C下装载60分钟,用30%甘油+15%乙二醇+10%二甲基亚砜+15%聚乙二醇+0.4mol·L-1蔗糖在0°C下脱水60分钟,迅速投入液氮,24小时后立即用40°C水浴快速化冻,再用MS+0.5mol·L-1蔗糖溶液洗涤2次,转入再生培养基中培养,可获得再生植株。再生植株成活率因基因型而异,铁棍山药、太谷山药、怀庆1号山药和B号山药的成活率分别为64.29%、49.21%、13.11%和39.81%。 相似文献