毛栓菌产漆酶条件优化及该酶对合成染料脱色的特性

【目的】提高菌株Trametes hirsuta SYBC-L19漆酶产量,并研究该酶对合成染料脱色的性质。【方法】通过单因素和响应面设计,对产漆酶培养基进行优化。【结果】最优培养基为:玉米粉20.0 g/L、马铃薯淀粉32.4 g/L、酒石酸铵2.9 g/L、吐温80 0.5 g/L、CuSO4.5H2O 2.0 mmol/L、香兰素0.54 mmol/L、NaH2PO4.2H2O 2.0 g/L、MgSO4.7H2O0.5 g/L、MnSO4.H2O 0.1 g/L;最佳培养条件为:培养温度30°C,初始pH 6.0,装液量40 mL/250 mL,接种量8%。【结论】培养8 d酶活达35 U/mL,是优化前的39倍。对漆酶催化合成染料脱色进行了考察,发现该酶在60°C下对偶氮类染料AR1和RB5能迅速脱色,5 min内即可完成。     

均匀设计法优化烟管菌产漆酶培养基

应用均匀设计、二次多项式逐步回归分析对烟管菌(Bjerkandera adusta)WZFF.W-Y11产漆酶液态发酵培养基进行优化。结果表明,培养基组成为麸皮水解液1%、淀粉24.0g/L、葡萄糖24.0g/L、豆饼粉4.8g/L、NH4Cl3.2g/L、KH2PO43.2g/L、MgSO4.7H2O0.2g/L、CuSO4.5H2O0.006g/L,起始pH6.5,在28℃、150r/min、250mL的摇瓶培养条件下可以稳定地获得9672U/L的漆酶活力。     

响应面法优化革耳Panus rudis FG-35菌株产漆酶培养基

采用Plackett-Burman设计和响应面分析相结合的方法,对革耳Panus rudis FG-35菌株产漆酶的液体培养基配方进行优化。单因素试验结果显示,发酵培养基中的最优碳源为可溶性淀粉,最优氮源为蛋白胨;Plackett-Burman设计筛选出影响漆酶产量的3个重要因素为可溶性淀粉、金属Ca2+离子和吐温-40,在此基础上运用最陡爬坡试验逼近最大响应值区域,最后利用Box-Behnken试验设计及响应面分析法进行回归分析,获得最佳培养基配方为:可溶性淀粉10.040 4 g/L、蛋白胨0.2 g/L、K2HPO41.00g/L、ZnSO4·7H2O 0.008 g/L、MgSO4·7H2O 0.5 g/L、CuSO4·7H2O 0.007 g/L、FeSO4·7H2O 0.005 g/L、MnSO40.035 g/L、CaCl20.0816 g/L、VB10.1 g/L、吐温-40 0.428%。在优化后的条件下摇瓶发酵产漆酶酶活力为263.31 U/mL,与模型预测值接近,发酵产酶量比优化前提高1.07倍,同时优化后的发酵液对木质素降解进行试验发现,优化后漆酶对木质素降解率提高了14.34%。     

假交替单胞菌Pseudoalteromonas sp. AJ5 产k-卡拉胶酶的培养条件优化

[目的]本研究的目的是优化Pseudoalteromonas sp. AJ5菌株的培养条件使之产生高活性的胞外κ-卡拉胶酶.[方法]通过富集培养技术从刺参肠道分离出一株卡拉胶降解菌AJ5,该菌株能利用卡拉胶作为惟一碳源和能源.依据形态学和生理学特征及16S rRNA基因序列分析,将该菌株鉴定为假交替单胞菌属(Pseudoalteromonas).通过单因素试验和正交试验对Pseudoalteromonas sp. AJ5菌株产胞外κ-卡拉胶酶的培养条件进行了优化.[结果]单因素试验结果表明,Pseudoalteromonas sp. AJ5菌株的最佳培养条件为250 mL三角瓶装入75 mL发酵培养基、摇床转速150 r/min、接种量7%、pH8.0.单因素试验和正交试验结果显示该菌株的最佳培养基组成为κ-卡拉胶 1 g/L、牛肉膏2 g/L、 NaCl 20 g/L、K2HPO4·3H2O 1 g/L、 MgSO4·7H2O 0.5 g/L、 MnCl2· 4H2O 0.2 g/L、 FePO4 · 4H2O 0.01 g/L; 培养温度为28℃,培养时间为28 h.[结论]Pseudoalteromonas sp. AJ5菌株分泌胞外κ-卡拉胶酶,在最佳培养条件下,该菌株的κ-卡拉胶酶活力比优化前提高了4倍.     

不同化学物质对银耳孢子细胞膜通透性影响

为了提高外源基因表达胞外分泌水平,本研究通过测定不同化学物质对银耳孢子转化子细胞生物量、培养液电导率及胞外漆酶酶活的影响,探索不同化学物质对银耳孢子细胞膜通透性的影响。结果表明,浓度分别为1%、0.3%、0.2%和0.1%的二甲基亚砜、triton X‐100、氯化钾、两性霉素B均可显著提高电导率;同时银耳孢子胞外漆酶酶活分别提高至7.00U/L、6.67U/L、5.00U/L和5.00U/L,与对照达到显著差异。而表面活性剂(SDS)及有机溶剂(甲苯、戊二醛)则不利于银耳孢子的生长及漆酶的分泌。该研究结果显示,添加一定的化学物质对促进目标产物的外泌有较为明显的作用,这将为银耳孢子作为生物反应器高效表达外源基因提供科学依据。     

产γ-谷氨基甲酰胺合成酶菌株的筛选及产酶条件研究

以假单胞菌(Pseudomonas sp.)为出发菌株,通过紫外诱变筛选得到一株γ-谷氨基甲酰胺合成酶高产菌株UV-19,其酶活提高32.54%。以突变株UV-19为供试菌株,对γ-谷氨基甲酰胺合成酶的发酵条件进行优化。首先利用Plackett-Burman设计筛选出影响较大的4个因素:葡萄糖、蛋白胨、起始pH值、装液量。在此基础上再利用CCD响应面分析法进行优化,得到最佳产酶培养条件为(g/L):葡萄糖15、蛋白胨12、NaCl 5.0、MgSO4.7H2O 0.2、K2HPO4.3H2O 0.5、甲胺盐酸盐1.0g/L、起始pH值6.5、装液量72mL/250mL。该优化条件下进行产酶培养,假单胞菌发酵产γ-谷氨基甲酰胺合成酶酶活力可达32.68U/mL。     

响应面法优化类芽胞杆菌HB172198产褐藻胶裂解酶发酵培养基

为了提高类芽胞杆菌新种HB172198产褐藻胶裂解酶活力,本研究采用响应面法对该菌株液体发酵培养基进行了优化实验。在单因素实验和Plackett-Burman试验筛选出海藻酸钠、胰蛋白胨、NaCl、MgSO4·7H2O等4个显著影响产酶因素的基础上,通过Box-Behnken设计及响应面法进行回归分析,得出产褐藻胶裂解酶最佳发酵培养基,其成分为:海藻酸钠7.50 g/L、胰蛋白胨13.57 g/L、NaCl 29.75 g/L、MgSO4·7H2O 0.08 g/L。优化条件下该菌株最大酶活性达14.60 U/mL,是优化前的1.87倍。本研究为菌株HB172198产褐藻胶裂解酶的大规模生产和工业应用提供了重要的理论依据。     

煤附生真菌产漆酶菌株的分离鉴定及产酶特性研究

从煤炭样品中筛选到一株产漆酶活性菌株,经菌体形态观察和ITS序列分析,鉴定为Trichoderma asperellum W03。菌株所产漆酶的最适反应pH为3.5-4.5,最适反应温度45℃,类似于白腐真菌漆酶。液态发酵条件的均匀设计实验表明,适宜的发酵培养基组成为:土豆200.00g/L、葡萄糖9.36g/L、米糠粉37.44g/L、硝酸钾4.00g/L、KH2PO43.20g/L、MgSO4·7H2O2.00g/L、CuSO4·5H2O0.005g/L、初始pH8.0;在33℃、180r/min、50mL/250mL的摇瓶培养条件下,棘孢木霉W03在孢子接种培养后48h、84h产酶量较高,分别处在菌体的快速生长期和衰亡期;菌体产酶受Cu2+、联苯胺诱导,而受1-萘酚、愈创木酚和2,4-D抑制。     

一种pH稳定的黄色漆酶的快速纯化和性质特征

通过丙酮沉淀和 DEAE- cellulose DE52 柱层析, 快速、有效地从一株白腐菌 Trametes sp. SQ01 的发酵液中纯化了漆酶。纯化的漆酶并非传统漆酶那样呈现蓝色, 而是一种黄色蛋白。以 ABTS 为底物时, 该酶的最适 pH 和温度分别是 pH 4.5 和 70°C, Km 为 0.029 mmol/L。T. SQ01 漆酶在 pH 3.0~11.0时, 酶活相对稳定, 在 pH 5.0 时最为稳定, 是目前报道的 pH 稳定性最好的漆酶。低浓度的金属离子(1 mmol/L) Cu2+、Mg2+ 、Ca2+ 和Co2+ 对漆酶有促进作用, 而高浓度(5 mmol/L)的Co2+、Zn2+、 Mn2+、Mg2+ 却抑制漆酶酶活。SDS 对该酶有激活作用, 当其浓度为1 mmol/L时, 漆酶相对酶活达到128%。DTT对漆酶强烈抑制, 即使是浓度为1 mmol/L, 亦可完全抑制漆酶酶活。纯化后的漆酶对亮蓝(RBBR) (100 mg/L)的脱色能力显著, 0.5 U/mL 的漆酶在 10 min内即可达到 80%的脱色率。T. sp. SQ01 漆酶的快速纯化以及高效脱色的能力表明该酶在染料脱色降解方面有着广阔的应用前景。     

假单胞菌属No.2120生产D-甘露糖异构酶发酵培养基的优化

通过单因子实验、Plackett-Burman实验设计、响应面分析法对假单胞菌属No.2120产D-甘露糖异构酶的培养基进行优化,确定发酵优化条件:果糖15.26 g/L,牛肉膏20 g/L,酵母膏2 g/L,K2HPO42 g/L,MgSO4.7H2O0.5 g/L,NaCl 0.5 g/L,Tween-80 1.54 g/L。采用优化配方异构酶比酶活可以达到68.28 U/mL。     

Copper induction of lignin-modifying enzymes in the white-rot fungus Trametes trogii

Trametes trogii, a white rot basidiomycete involved in wood decay worldwide, produces several ligninolytic enzymes, laccase being the dominant one, with higher titers than those reported for most other white rot fungi studied up to date. The effect of copper on in vitro production of extracellular ligninolytic activities was studied. CuSO(4)·5H(2)O concentrations from 1.6 μM to 1.5 mM were tested in a synthetic medium with glucose 20 g/L and asparagine 3 g/L. The addition of copper (up to 1 mM) did not affect growth but strongly stimulated ligninolytic enzyme production; faster decolorization of the polymeric dye Poly R-478 was observed as well. Maximal production of manganese peroxidase, laccase, and glyoxal oxidase [1.28 U/mL, 93.8 U/mL (with a specific activity of 720 U/mg protein), and 0.46 U/mL respectively] was attained with 1 mM CuSO(4)·5H(2)O. However, higher copper concentrations inhibited growth and notably decreased manganese peroxidase production, although they did not affect laccase secretion. Laccase activity in the culture filtrate was maximal at 50 C and pH 3.4, and the enzyme was completely stable at pH 4.4 and above, and at 30 C for up to 5 d. Denaturing polyacrylamide gel electrophoresis of extracellular culture fluids showed two laccase activity bands (mol wt 38 and 60 kDa respectively). The pattern of isoenzyme production was not affected by medium composition but differed with culture age.     

黄孢原毛平革菌产漆酶优化培养及其对刚果红的脱色降解

以白腐真菌模式菌株黄孢原毛平革菌Phanerochaete chrysosporium为研究对象,探讨培养条件、重金属和芳香族化合物对产漆酶的影响,并进一步研究漆酶对刚果红的降解效果。结果表明,P. chrysosporium产漆酶最适培养条件：葡萄糖为碳源,蛋白胨为氮源,碳氮比为90。培养8d后,漆酶酶活为911.1U/L;Mn²⁺严格地控制着P.chrysosporium产漆酶,而Cu²⁺对其影响不大,在添加4.0mmol/L Mn²⁺时,漆酶酶活为2 001.7U/L;芳香族化合物中藜芦醇（veratryl alcohol,VA）、4-香豆酸、香草醛和香草酸对菌体产漆酶能力均有促进作用,最高可提升至1 459.1U/L,而咖啡酸对菌体产漆酶稍有抑制。100U/L漆酶粗酶液可降解40mg/L刚果红,降解率为24.0%;而当介体物质VA存在时,该降解效率可提升至87.7%。     

Effect of inducers and process parameters on laccase production by Streptomyces psammoticus and its application in dye decolourization

The process parameters influencing the production of extracellular laccases by Streptomyces psammoticus MTCC 7334 were optimized in submerged fermentation. Coffee pulp and yeast extract were the best substrate and nitrogen source respectively for laccase production by this strain. The optimization studies revealed that the laccase yield was maximum at pH 7.5 and temperature 32 degrees C. Salinity of the medium was also observed to be influencing the enzyme production. An agitation rate of 175 rpm and 15% inoculum were the other optimized conditions for maximum laccase yield (5.9 U/mL). Pyrogallol and para-anisidine proved to be the best inducers for laccase production by this strain and the enzyme yield was enhanced by 50% with these inducers. S. psammoticus was able to decolourize various industrial dyes at different rates and 80% decolourization of Remazol Brilliant Blue R (RBBR) was observed after 10 days of incubation in dye based medium.     

Evaluation of Argentinean white rot fungi for their ability to produce lignin-modifying enzymes and decolorize industrial dyes

The decolorizing capacity of 26 white rot fungi from Argentina was investigated. Extracellular production of ligninolytic enzymes by mycelium growing on solid malt extract/glucose medium supplemented with different dyes (Malachite Green, Azure B, Poly R-478, Anthraquinone Blue, Congo Red and Xylidine), dye decolorization and the relationship between these two processes were studied. Only ten strains decolorized all the dyes, all ten strains produced laccase, lignin peroxidase and manganese peroxidase on solid medium. However, six of the strains could not decolorize any of the dyes; all six strains tested negative for lignin peroxidase, and produced less than 0.05 U/g agar of manganese peroxidase. Comparing the isolates with the well-known dye-degrader Phanerochaete chrysosporium, a new fungus was identified: Coriolus versicolor f. antarcticus, potentially a candidate for use in biodecoloration processes. Eighteen day-old cultures of this fungus were able to decolorize in an hour 28%, 30%, 43%, 88% and 98% of Xylidine (24 mg/l), Poly R-478 (75 mg/l), Remazol Brilliant Blue R (9 mg/l), Malachite Green (6 mg/l) and Indigo Carmine (23 mg/l), respectively. Laccase activity was 0.13 U/ml, but neither lignin peroxidase nor manganese peroxidase were detected in the extracellular fluids for that day of incubation.     

响应面法优化荷叶离褶伞菌丝体产漆酶条件

为了对荷叶离褶伞产漆酶条件进行优化,在单因素实验基础上,通过最陡爬坡实验(PB)对培养基8因素进行筛选,获得影响产漆酶的3个显著性因素:葡萄糖,pH和KH₂PO₄;通过中心组合(CCD)设计及响应面分析确定了最优发酵条件:葡萄糖20.09g/L,酪蛋白1.5g/L,酵母提取物1.5g/L,MgSO₄ 3g/L,CuSO₄ 3.75mg/L,KH₂PO₄ 3.97g/L,pH 4.98,VB₁ 0.1g/L,愈创木酚12mg/L,该条件下,漆酶酶活为829.83U/mL,较未优化对照提高46.6%.     

Medium optimization of antifungal activity production by Bacillus amyloliquefaciens using statistical experimental design

In order to overproduce biofungicides agents by Bacillus amyloliquefaciens BLB371, a suitable culture medium was optimized using response surface methodology. Plackett-Burman design and central composite design were employed for experimental design and analysis of the results. Peptone, sucrose, and yeast extract were found to significantly influence antifungal activity production and their optimal concentrations were, respectively, 20 g/L, 25 g/L, and 4.5 g/L. The corresponding biofungicide production was 250 AU/mL, corresponding to 56% improvement in antifungal components production over a previously used medium (160 AU/mL). Moreover, our results indicated that a deficiency of the minerals CuSO(4), FeCl(3) · 6H(2)O, Na(2)MoO(4), KI, ZnSO(4) · 7H(2)O, H(3)BO(3), and C(6)H(8)O(7) in the optimized culture medium was not crucial for biofungicides production by Bacillus amyloliquefaciens BLB371, which is interesting from a practical point of view, particularly for low-cost production and use of the biofungicide for the control of agricultural fungal pests.     

Production of Laccase by Trametes hirsuta Grown in an Immersion Bioreactor and its Application in the Docolorization of Dyes from a Leather Factory

An alternative system for producing laccase on a bioreactor scale by the white‐rot fungus Trametes hirsuta is proposed. The experiments were performed in an immersion bioreactor (employing cuttings of stainless steel sponges as a support) and the culture medium was supplemented with copper sulfate (1 mM). Operating under these conditions, it was possible to obtain a maximum laccase activity of nearly 5,000 U/L within 9 days. In addition, the ability of the crude laccase produced to decolorize two synthetic acid dyes utilized in the leather industry (Luganil Green and Sella Solid Red) was investigated. The effect of the pH and the enzyme activity on decolorization was analyzed. It was found that a pH of 4.0 and a laccase activity of 300 U/L were optimal for Luganil dye decolorization (16.2 % in 2 hours). Sella Solid Red showed its highest decolorization (around 40 % in 2 hours) when used at pH 5.0 and at a laccase activity of 1,000 U/L.