液态发酵条件下拟康宁木霉8985产纤维素酶能力初探

液态发酵条件下,以微晶纤维素为唯一碳源,比较了拟康宁木霉Trichoderma koningiopsis 8985和里氏木霉T.reesei QM9414产纤维素酶的能力。8985发酵12 h开始产生纤维素酶,36 h时酶活达到产酶峰值的50%,此时QM9414尚未诱导产酶。测定8985发酵84 h时上清液中滤纸纤维素酶、羧甲基纤维素酶、β-葡萄糖苷酶和木聚糖酶的酶活分别为1.06、3.62、1.80和6.67 IU/mL,分别是QM9414上述酶活的1.72、1.70、6.35和1.12倍。8985滤纸纤维素酶酶活的最适反应条件为pH 4.5,反应温度50℃,在Fe³⁺(≤4 mmol/L)和Cu²⁺(0–10 mmol/L)存在条件下酶活稳定。     

Acremonium纤维素酶在玉米芯糖化中的应用

玉米芯作为一种木质纤维素类农业废弃物,同时也是生产生物乙醇的潜在原料。在玉米芯糖化过程中,纤维素酶的作用是十分关键的。本研究比较了里氏木霉纤维素酶、绿色木霉纤维素酶和Acremonium纤维素酶各相关酶活。其中Acremonium纤维素酶的滤纸酶活约是里氏木霉纤维素酶的6倍,是绿色木霉纤维素酶的8倍。其羧甲基纤维素酶活和绿色木霉纤维素酶基本相等。Acremonium纤维素酶的β-葡萄糖苷酶酶活是里氏木霉纤维素酶的38倍,以及绿色木霉纤维素酶的41倍。而Acremonium纤维素酶的木聚糖酶活只相当于绿色木霉纤维素酶的70%。这说明Acremonium纤维素酶降解纤维素的能力可能强于另两种纤维素酶,而降解半纤维素类物质的能力要弱于绿色木霉纤维素酶。在玉米芯糖化实验中,使用Acremonium纤维素酶的糖化液中产生的最高葡萄糖浓度比里氏木霉纤维素酶的高14%,比绿色木霉纤维素酶的高58%。Acremonium纤维素酶用量在10 FPU/g时,反应16 h就基本可以达到最佳效果,而另两种酶用量则需达到30 FPU/g,反应48h才能达到最佳效果。使用Acremonium纤维素酶的糖化液中产生的最高木糖浓度与里氏木霉纤维素酶相等,比绿色木霉纤维素酶低42%。而同时使用Acremonium纤维素酶及绿色木霉纤维素酶时,其糖化液中最高木糖浓度有所提高,比绿色木霉纤维素酶的高31%。Acremonium纤维素酶可以有效地应用于玉米芯糖化,为玉米芯的资源化提供一种可能的方案。     

ARTP诱变选育鼠李糖脂高产菌及鼠李糖脂促进枯草芽孢杆菌产纤维素酶的研究

旨在选育鼠李糖脂高产菌株,以实验室筛选的产鼠李糖脂的Pseudomonas aeruginosa C3为出发菌株进行常压室温等离子体诱变(ARTP),选育出一株高产突变株Pseudomonas aeruginosa SC-11,产量比出发菌株提高了74.1%。进一步对产鼠李糖脂的摇瓶发酵培养基和发酵条件进行了优化,优化后的鼠李糖脂产量达42 g/L,底物转化率达到0.7 g/g底物。添加0.01%鼠李糖脂到Bacillus subtilis CL产羧甲基纤维素酶与木聚糖酶的培养基中,羧甲基纤维素酶活与木聚糖酶活分别提高12.9%和18.3%。研究表明,鼠李糖脂通过增加细胞通透性来提高胞外酶产量。     

里氏木霉与米根霉混合固态发酵产纤维素酶

以里氏木霉及米根霉单菌固态发酵为对象,考察不同混合发酵形式对里氏木霉与米根霉混合固态发酵产纤维素酶的影响。结果表明:同时接种里氏木霉与米根霉,试验考察的两菌种接种量比1∶1(以孢子个数计)及5∶1条件下,两菌未产生明显协同产酶作用。米根霉延时(24 h)接种且菌种量比5∶1以及米根霉延时(48 h)接种且菌种量比1∶1,2种发酵形式产酶情况类似,滤纸酶活(FPA)及羧甲基纤维素酶(CMCase)酶活相对米根霉单菌发酵有所提高,而β-葡萄糖苷酶(β-GA)酶活相对里氏木霉单菌固态发酵结束时分别增加4.66及4.40倍,可以发现两菌产生一定协同作用。在米根霉延时(48 h)接种且菌种量比5∶1的发酵形式下,FPA及CMCase在发酵第7天酶活分别达到44.04 IU/g、627.14 U/g(以1 g干曲计),分别是里氏木霉固态单菌发酵产酶达到稳定期时酶活的1.36和1.63倍,两菌产生了有效的协同作用。     

真空微波诱变结合化学诱变选育酸性纤维素酶高产菌株

以酸性纤维素酶产生菌绿色木霉（Trichoderma viride）WL0512作为原始出发菌株,首先经自然分离筛选出一株产酶较稳定的菌株TVN-18,其羧甲基纤维素酶活（CMC酶活）达2765．8U／g,滤纸酶活（FPA酶活）达48．5U／g。再经真空微波和甲基磺酸乙酯（EMS）逐级诱变处理,获得了一株高产、稳产酸性纤维素酶的E6—1菌株,其CMC酶活达4396．6U／g,FPA酶活达126．0U／g,分别是菌株TVN-18的1．59倍和2．60倍。通过对固态发酵培养基麸皮和稻草比例、料水比以及初始pH值的优化,突变株的产酶能力进一步得到提高,其产的CIVIC酶活和FPA酶活分别提高了22．3％和22．4％。     

纤维基质对液体培养灵芝产纤维素酶的影响

本研究通过在培养基中添加滤纸、羧甲基纤维素(CMC)、蔗渣和玉米芯等纤维素类基质,观察纤维素基质对液体培养条件下灵芝产纤维素酶和半纤维素酶的影响.结果表明,这些纤维素基质能促进纤维素酶活力的增加,促进作用效果各异,当滤纸的添加量达到1 g/L时,滤纸酶活(FP酶活)达到空白对照的9.04倍,当蔗渣添加量为1 g/L时,灵芝β-1,4-葡聚糖酶酶活(Cx酶活)、FP酶活、半纤维素酶活分别比空白对照样增加了12%、534%、117.3%.     

绿色木霉原生质体诱变筛选纤维素酶高产菌株

以绿色木霉F264为出发菌株制备其原生质体,对其进行紫外线诱变处理,筛选出一株纤维素酶高产突变株绿色木霉F-UV264,其滤纸酶活由出发菌株的5.2IU/g干料提高到15.78IU/g干料,产酶能力提高了3倍。经过10代PDA斜面继代培养及发酵试验,表明该菌株是比原菌株更优秀的稳定高产株。     

康宁木霉QF-02纤维素酶酶学性质的研究

对康宁木霉QF-02生产的纤维素酶的一般酶学性质进行了研究。该纤维素酶系中滤纸酶、羧甲基纤维素酶、微晶纤维素酶、β-葡萄糖苷酶的最适作用温度分别为55℃、65℃、50℃和70℃,最适作用pH为4.0-5.0;在40-50℃范围内热稳定性较好,24 h保温后的残留酶活在48.5%以上;在pH3.0-8.0范围内比较稳定,4℃保存24h后的残留酶活在75.7%以上。与几种商品纤维素酶相比,该纤维素酶对未处理和碱预处理稻草都表现出较强的糖化能力。     

筛选最佳生物质材料诱导里氏木霉生产纤维素酶

本研究用小麦、芒草、水稻这三种低木质素突变株材料作为新型诱导物筛选的对象,对三种木质纤维素材料进行成分分析,然后利用它们分别作为诱导物诱导里氏木霉生产纤维素酶,对其诱导产生的酶活力,胞外蛋白含量,糖化能力进行比较。结果表明,对里氏木霉产纤维素酶诱导效果最好的是水稻H*14、芒草W56、小麦Q142。相比于玉米秸秆作为诱导物,水稻H*14单独诱导里氏木霉β-葡萄糖苷酶效果最好,β-葡萄糖苷酶酶活提高了75.2%,滤纸酶活提高了86.6%。相比玉米秸秆作为诱导物,芒草W56单独诱导里氏木霉木聚糖酶的效果最好,木聚糖酶酶活力提高了9.93%,内切葡聚糖酶酶活也提高了30.8%。相比玉米秸秆作为诱导物,小麦Q142诱导里氏木霉的外切葡聚糖酶酶活效果最好,里氏木霉的外切葡聚糖酶酶活提高了88.6%。本研究发现低木质素的木质纤维素材料作为诱导物对里氏木霉诱导产酶效果较好,并且促进真菌胞外蛋白的分泌,诱导纤维素酶酶系平衡分泌,使得纤维素酶糖化水解能力的提高。该研究为今后纤维素酶工业化生产提供参考和帮助。     

甘蔗渣固态发酵产纤维素酶

以甘蔗渣和麸皮混合作为固态发酵产酶培养基,采用单因素优化实验对里氏木霉固态发酵产纤维素酶进行优化。结果表明,在50 m L体系培养基中,在底物绝干原料5.2 g、甘蔗渣与麸皮质量比7∶3、氮源((NH4)2SO4)7.5 g/L、产酶诱导物1.6 g/L、表面活性剂(聚乙二醇PEG6000)0.1 g、发酵起始p H 4.4、培养基中里氏木霉孢子接入量5×105个的条件下,温度30℃时发酵120 h,里氏木霉固态发酵产纤维素酶的酶活达76.39 IU/g,是起始优化前20.29 IU/g的3.76倍。     

The stimulatory effects of surfactants on composting of waste rich in cellulose

The chemical surfactant Tween 80 and biosurfactant rhamnolipid were respectively added to the composting substrate, a mixture of rice straw and bran, and their effects on the composting process were investigated. Samples were analysed for microbial communities of bacteria, actinomycetes and fungi, carboxymethylcellulose hydrolysis (CMCase) and xylanase activities, cellulose and hemicellulose fractions, water-soluble carbon (WSC) contents in the substrates, organic matter contents and pH values during the composting process. The results showed that both Tween 80 and rhamnolipid had slight stimulatory effects on the microbial populations of bacteria, actinomycetes and fungi. In addition, rhamnolipid increased the peak xylanase activity 15% higher than that of the control, while Tween 80 increased the maximum CMCase activity 35% higher than that of the control. As a result of the increased enzyme activities, treatments with Tween 80 and rhamnolipid were of higher WSC contents than the control during the whole composting process. Accordingly, the composting process was accelerated by the surfactants, since the organic matter was decomposed more quickly and the breakdown of cellulose and hemicellulose was better in the treatments with Tween 80 and rhamnolipid.     

Effects of Tween 80 and rhamnolipid on the extracellular enzymes of Penicillium simplicissimum isolated from compost

Extracellular enzymes of microorganisms play an important role in the decomposition of macromolecules in the composting process. In this study, the effects of Tween 80 and rhamnolipid on the extracellular amylase, carboxymethyl cellulose enzyme (CMCase), xylanase and protease of Penicillium simplicissimum isolated from compost were investigated during solid-state fermentation. The results showed that the enzyme activities of amylase, CMCase and xylanase were increased by Tween 80 and rhamnolipid, which, however, had a negative effect on the protease production. The stimulative effects on the three enzymes were quite different during the whole fermentation process. Tween 80 and rhamnolipid also increased the fungal biomass slightly. As a result of the enhanced enzyme activities, the organic matter were also improved to different extents by both surfactants, and the decomposition rates of hemicellulose and cellulose were increased about 8.0% and 11.6% by Tween 80 at best, respectively, as well as 5% and 5.5% by rhamnolipid.     

Characterization of the interaction between surfactants and enzymes by fluorescence probe

In order to investigate the mechanism of the different stimulatory effects of the biosurfactant rhamnolipid and the chemical surfactant Tween 80 on enzymatic hydrolysis of lignocellulose, the interaction between surfactants and enzymes was analyzed by the fluorescence probe method using pyrene as probe. Based on the evolution law of pyrene fluorescence spectroscopy in the “surfactants-enzymes” systems, the interaction relationship between surfactants and enzymes was analyzed and discussed in this paper. The results show that enzyme molecules bind with rhamnolipid molecules, participate in the formation of rhamnolipid micelles, and increase the inner hydrophobic polarity of micelles, but do not change the properties of rhamnolipid micelles above the CMC (Critical Micelle Concentration). Nevertheless, for Tween 80, enzyme molecules also participate in the forming of micelles, however, they exhibit a stronger interaction with enzymes above the CMC. Both rhamnolipid and Tween 80 bind more strongly with xylanase than cellulase. Considering also previous experimental results, it can be concluded that the interaction between surfactants and enzymes improve enzyme stability and activity, and, therefore, the efficiency of enzymatic hydrolysis of lignocellulose is enhanced. The findings further provide theoretical knowledge about the mechanism of the stimulative effects of surfactants on enzymatic hydrolysis of lignocellulose.     

Secretion of cellulase and beta-glucosidase by Trichoderma viride ITCC-1433 in submerged culture on different substrates.

Trichoderma viride ITCC-1433 produces high yields of cellulase and especially beta-glucosidase when grown in submerged culture on different carbon sources. Cellulase synthesis was strongly repressed in the presence of glucose and only a low constitutive activity of beta-glucosidase and carboxymethylcellulase, but no Avicelase, could be demonstrated when culturing T. viride on glucose. With carboxymethylcellulose (CMC) as a substrate the secretion of enzyme as well as growth depended on the degree of substitution, but in general CMC cannot be regarded either as a powerful inducer or as a carbon source. With insoluble cellulose, maximum enzyme production and activities were obtained using an alkali-treated cellulose powder. On this substrate the excretion of soluble protein into the culture broth increased and the protein concentration corresponded to cellulolytic activities.     

Adsorption of surfactants on a <Emphasis Type="Italic">Pseudomonas aeruginosa</Emphasis> strain and the effect on cell surface lypohydrophilic property

The adsorption behavior of five surfactants, cetyltrimethylammonium bromide (CTAB), Triton X-100, Tween 80, sodium dodecyl sulfate (SDS), and rhamnolipid, on a Pseudomonas aeruginosa strain and the effect of temperature and ionic strength (IS) on the adsorption were studied. The change of cell surface lypohydrophilic property caused by surfactant adsorption was also investigated. The results showed that the adsorption kinetics of the surfactants on the cell followed the second-order law. CTAB adsorption was the fastest one under the experimental conditions, and it took longest for SDS adsorption to equilibrate because of electric repulsion. The adsorption of Triton X-100 and Tween 80 was characterized by short equilibration time, and rhamnolipid adsorption reached equilibrium in about 90 min. The adsorption isotherms of all the surfactants on the bacterium fitted Freundlich equation well, but the adsorption capacity and mode were variations for the surfactants as indicated by k and n parameters in the equations. The adsorption mode for all the surfactants except SDS is probably hydrophilic interaction because the adsorption totally turned the cell surface to be more hydrophobic. Neither the temperature nor the IS had significant effect on CTAB adsorption, but higher IS significantly enhanced SDS adsorption and modestly strengthened adsorption of Triton X-100, Tween 80, and rhamnolipid. Higher temperature strengthened adsorption of SDS but weakened the adsorption of Triton X-100, Tween 80, and rhamnolipid.     

Adsorption of cellulase from Trichoderma viride on cellulose

The adsorption of cellulase from Trichoderma viride (Meicelase CEP) on the surface of pure cellulose was studied. The adsorption was found to obey apparently the Langmuir isotherm. From the data concering the effects of temperature and the crystallinity of cellulose on the Langmuir adsorption parameters, the characteristics of the adsorption of the individual cellulase components, namely CMCase (endoglucanase) and Avicelase (exoglucanase), were discussed. While beta-glucosidase also adsorbed on the surface of cellulose at 5 degrees C, it did not at 50 degrees C.     

Properties of cellulase immobilized on agarose gel with spacer

Cellulase produced by fungus Trichoderma viride was immobilized on agarose beads (Sepharose 4B) activated by cyanogen bromide and also on activated agarose beads that contained spacer arm (activated CH-Sepharose 4B and Affi-Gel 15). The CMCase activity retained by immobilized cellulase on activated Sepharose containing the spacer tended to be higher than that immobilized without spacer, although the extent of protein immobilization was lower. Also, the higher substrate specificity for cellulase immobilized on beads with spacer was obtained for cellobiose, acid-swollen cellulose, or cellulose powder. The hydrolysis product from their substrates was mainly glucose.     

Mutarotation of hydrolysis products by different types of exo-cellulases from Trichoderma viride.

Mutarotation of products from p-nitrophenyl beta-D-cellobioside and cellopentaitol by two different types of exo-cellulases from Trichoderma viride was investigated. It was found that an exo-cellulase of glucosidase type produced from the former substrate D-glucose which was mutarotated in a downward direction, while another exo-cellulase of Avicelase type produced from the latter substrate cellobiose which was mutarotated in an upward direction.     

Isolation and mutation of cellulolytic fungi

Nineteen fungi were isolated from different soil samples on the basis of clear zones formed on Rose Bengal Cellulose agar medium. In shake flasks th isolate K1 gave 12.1 units/ml of CMCase activity. A mutant of the isolate K1, KM7, was selected after N-methyl-N'-nitro-N-nitrosoguanidine treatment of the wild-type. This mutant differed morphologically from the parent strain on RBCA medium and gave 36.2 units/ml of CMCase activity which represented about 50% of the enzyme yield from the standard organism, Trichoderma viride QM 9414 (80 units/ml of CMCase activity). The isolate K1, which was identified as a Phoma species, produced 48 units of beta-glucosidase. The yield of beta-glucosidase was increased about 8-fold in the mutant KM7 and was about 68% higher than the level found in T. viride QM 9414.