三相鼓泡塔生物反应器培养云芝菌合成漆酶

为了提高云芝菌发酵生产漆酶的效率,提出了一种利用自絮凝菌丝球在三相鼓泡塔生物反应器中重复分批发酵产漆酶的新方法。在优化后的产酶条件下,考察维生素C的添加浓度对漆酶活力的影响,并通过在培养基中添加维生素C进行漆酶多批次培养。研究结果表明,维生素C的添加浓度为1.50mmol/L时,可使漆酶活力提高2.6倍。连续进行了10批培养,每批最大漆酶的活力均在1000 U/mL以上,最高酶活出现在第五批为1919.6 U/mL,总培养时间达25 d。此方法所得漆酶对染料靛蓝具有明显的脱色降解作用,在介体1-羟基苯并三唑（HBT）用量0.10%,漆酶用量100 U/L条件下作用40 min时,靛蓝脱色率达到96.7%。该方法采用的三相鼓泡塔生物反应器性能稳定、菌丝球可重复使用,该方法有利于漆酶的高效、规模化生产。     

疣孢漆斑菌Myrothecium verrucaria GH-01漆酶的纯化和酶学性质研究

疣孢漆斑菌具有生长周期短,分泌漆酶酶活高等特点。利用已分离得到的疣孢漆斑菌GH-01(Myrothecium verrucaria GH-01)发酵产生粗酶液。进而通过分级沉淀、透析和层析的方法对漆酶粗酶液进行纯化。SDS-PAGE和Native-PAGE结果表明纯化可获得具有漆酶活性的单体蛋白。酶学性质研究表明,该漆酶催化最适温度为40℃,在底物ABTS存在条件下的最适p H值为4.0,且在低温及碱性条件具有较好的稳定性。此外通过漆酶对4大类染料脱色能力的研究,发现该漆酶对偶氮类的橙黄Ⅰ和蒽醌类的茜素红脱色有较好的脱色效果,反应1 h脱色率达80%以上;对三苯甲烷类的碱性品红脱色能力较弱,脱色率只能达到20%左右;脱色率最差的是杂环类的亚甲基蓝。在含10 U漆酶的体系中,对50 mg/L的染料降解效果相对最佳。     

漆酶高产工程菌构建及漆酶对RBBR的脱色作用

研究提取产漆酶白腐菌 (Fomelignosus)的总RNA ,利用RT PCR克隆到漆酶的cDNA ,并将其克隆到表达载体pGAPZA ,重组质粒经线性化、电激转化PichiapastorisGS115、通过底物显色反应筛选漆酶生产工程菌株 ,在最适培养条件下该菌株产酶活力高达 9 0 3U·mL-1。纯化得到漆酶对RBBR(RemazolbrilliantblueR)有很好的脱色作用 ,该酶的最适脱色pH为 5 0 ,最适脱色温度为 30℃。当溶液中漆酶活力为 1 0U·mL-1,在最适脱色条件下作用12h ,10 0mg·L-1RBBR溶液脱色率可达 90 %以上。     

短小芽孢杆菌LC01漆酶基因在毕赤酵母中的胞外表达及重组漆酶酶学性质研究

为了获得表达量高、稳定性好及染料脱色效率高的细菌漆酶,通过PCR扩增出短小芽孢杆菌LC01的漆酶基因并构建重组表达载体pPICZαA-lac,转化毕赤酵母菌株SMD1168H后利用甲醇诱导培养重组菌获得重组漆酶,纯化并分析了重组漆酶的性质。重组菌株产漆酶活性在第7天达到最高,为1 390 U/L。纯化的重组漆酶分子量为65 kD,以丁香醛连氮为底物的最适反应温度和pH分别为70℃和6.8。在pH 9.0放置10 d活性没有下降,在70℃保温10 h后仍保留36%的酶活。Al~(3+)、Fe~(3+)和Mn~(2+)完全抑制漆酶活性。在介体乙酰丁香酮参与下该漆酶能够有效脱色RB亮蓝、活性黑5和靛红,在pH 9.0时6 h的脱色率达到了90%以上,表明该重组漆酶能有效应用于染料废水的脱色处理。     

一色齿毛菌漆酶的酶学特性及染料脱色研究

染料由于具有复杂的化学结构通常难以降解。本文从白腐菌一色齿毛菌LS0547中纯化出胞外漆酶并用于染料脱色实验。SDS-PAGE结果显示纯化的漆酶分子量大小为63.7kDa。漆酶氧化底物ABTS的最适pH为2.2,最适温度为50℃。叠氮钠可强烈抑制漆酶活性,半胱氨酸和二硫苏糖醇可部分抑制漆酶活性。漆酶氧化ABTS,丁香醛连氮和2,6-二甲氧基苯酚的米氏常数分别为0.217,0.306和0.199mmol/L。粗酶和纯化的漆酶用于不同化学结构的染料的脱色研究,结果表明一色齿毛菌纯化漆酶可快速对RB亮蓝进行脱色,偶氮胭脂红和结晶紫的脱色效果低于RB亮蓝,测试的三种染料均可在没有介体存在的条件下被漆酶脱色,显示出一色齿毛菌漆酶在染料废水处理中的应用前景。     

端梗霉Z45产漆酶培养基的优化及其对染料的脱色

菌株Acrophialophora sp.Z45是一株产漆酶的端梗霉属真菌,本文依据不同培养基中菌株Z45对愈创木酚的氧化圈大小探究了影响该菌株产漆酶的因素并设计正交试验优化其产漆酶培养基,进而比较了菌株Z45在土豆葡萄糖培养基和优化后的产漆酶培养基中的漆酶活力差异,最后基于漆酶与染料脱色的相关性评价了菌株Z45对8种合成染料的脱色能力。结果表明,单因素及正交试验确定了菌株Z45优化后的产漆酶培养基为：基础产酶培养基中以蔗糖为碳源、硝酸钠为氮源、C/N比为45∶1、pH为5.0;在优化后的产漆酶培养基中菌株Z45的漆酶活性显著提高;菌株Z45对溴酚蓝、中性红、亚甲基蓝、甲基蓝和结晶紫等5种染料均有一定的脱色能力,其中对三苯甲烷染料甲基蓝的脱色能力最强,菌株Z45的粗酶液能使甲基蓝快速脱色。在较低甲基蓝浓度的固体培养基上,甲基蓝完全脱色的时间不受染料浓度的影响;而较高甲基蓝浓度下,甲基蓝完全脱色的时间随染料浓度升高逐渐延长。     

荷叶离褶伞高产漆酶菌株选育及其漆酶酶学特性北大核心CSCD

应用原生质体紫外诱变,对一株产漆酶荷叶离褶伞（Lyophyllum decastes）菌株紫外诱变,用愈创木酚马铃薯葡萄糖固体平板变色法初筛,然后用ABTS[2,2-联氮-二（3-乙基-苯并噻唑-6-磺酸）二铵盐]测定漆酶活性进行复筛,获得1株漆酶高产诱变菌株HY1022-01;对HY1022-01所产漆酶粗酶液酶学特性进行研究,结果表明,HY1022-01所产漆酶最大酶活力比出发菌株提高30.32%,最适条件下酶活达991.67 U/mL,且产酶稳定;HY1022-1所产漆酶最适作用温度为35℃,在30∽35℃较为稳定;最适反应pH值为3.0,pH在2.2∽3.8较为稳定,ABTS的漆酶动力学常数为72.622μM。     

粗毛栓菌漆酶的诱导及其对中性染料和有机磷农药的降解

研究了不同初始培养pH和培养时间下,不同诱导剂对粗毛栓菌产漆酶诱导特性的影响及漆酶对中性染料、有机磷农药的降解.结果表明： RB-亮蓝、ABTS和邻联甲苯胺对粗毛栓菌产漆酶均有不同程度的诱导作用,其中ABTS的诱导作用最好,其诱导的最适初始pH为4.0,最佳时间为13 d;所产漆酶的适宜反应温度为38 ℃,酶在40 ℃保温20 min仍可保留786%的酶活力,稳定性较好;在ABTS介导下,漆酶降解6种中性染料的最佳温度分别为30 ℃(中性黑、中性枣红、中性桃红、甲基橙)和60 ℃(中性深黄、甲酚红),最适pH分别为6.0(中性黑)、2.0(中性枣红、中性桃红)和4.0(甲基橙、中性深黄、甲酚红),最佳降解时间分别为6 h(甲基橙、中性深黄和甲酚红)、12 h(中性桃红)和24 h(中性枣红).而漆酶降解乐果、毒死蜱、敌百虫、哒嗪硫磷4种有机磷农药的最佳温度均为25 ℃,最佳降解时间为9 h,最佳pH分别为10.0(乐果、毒死蜱、哒嗪硫磷)和8.0(敌百虫).     

红平菇产漆酶条件优化及对孔雀绿染料脱色的研究

采用LNAS(低氮天冬酰胺-琥珀酸)培养基添加方式,对红平菇Pleurotus djamor HP1进行培养,检测不同时间培养液对不同底物的氧化作用,进而得到光密度值的变化情况,作为漆酶的产生及活性测定的主要依据。结果表明:在含Cu2+的培养液中漆酶最大酶活为235.4 U/L。含Cu2+的培养液添加底物木屑后漆酶最大酶活为458.8 U/L。提取经优化筛选后的培养基培养出的漆酶粗酶液,对4种具有不同化学结构的染料进行了脱色试验。结果表明:三苯基甲烷类的孔雀绿在6 h时脱色率为87.5%,蒽醌类的SN4R在24 h时脱色率为49.4%,偶氮类的甲基橙在24 h时脱色率为45%,杂环类的中性红在24 h时脱色率为23.6%。因此,显示出红平菇漆酶对孔雀绿染料脱色具有较大的应用潜力,进而对废水处理具有更好的应用前景。     

东方栓孔菌在染料脱色中的应用及其脱色条件的优化

本研究利用东方栓孔菌(Trametes orientalis)菌株Cui 6300发酵所得的粗酶液,对刚果红、结晶紫、铬天青、亚甲基蓝和中性红5种染料进行了催化脱色试验,并对其中脱色效果较好的染料进行了脱色条件优化.结果表明:东方栓孔菌漆酶粗酶液对结晶紫有相对较好的脱色效果.添加2,2'-连氮-双(3-乙基苯并噻唑-6-磺酸) (ABTS)的粗酶液对结晶紫的降解效果没有明显促进作用,因此后续试验中直接采用粗酶液.脱色条件优化结果为:最佳初始pH值6.0,最佳培养温度55℃,最佳接种量2.0%,最佳转速160 r/min,最佳底物浓度160 mg/L.在此条件下反应96 h,脱色率可达98.45%.本试验说明东方栓孔菌在印染废水治理方面具有较好的应用前景,可以作为一种新型菌株应用于染料脱色.     

Induction of a white laccase from the deuteromycete Myrothecium verrucaria NF-05 and its potential in decolorization of dyes

Myrothecium verrucaria NF-05 is a deuteromycete fungus capable of producing a white laccase. The optimal concentration of Cu²⁺ for laccase production by this strain is 0.2 mM (43.23 ± 1.16 U mL^{? 1}). A comprehensive investigation of the induction demonstrated that NF-05 laccase production could be synergistically enhanced by various inducers, including aromatic phenols, amines and recalcitrant dyes, in the presence of 0.2 mM Cu²⁺. Sixteen phenols, fourteen amines and four dyes exhibited significant inductive effects on laccase production. The best inducer was 3, 3’-dimethylbenzidine, which increased laccase production to 258.1 ± 11.1 U mL^{? 1}. These results suggest that M. verrucaria NF-05 is a promising industrial laccase producer. Based on the increased production, purified NF-05 laccase was used to decolorize dyes of various structural types in the presence of six redox mediators. Among the 26 tested dyes, the decolorization rate of six azo dyes, chromotrope 2R, orange G6, Congo red, Ponceau S, amaranth and reactive yellow 135 and two arylmethane dyes, fast green 3 and neutral red, were significantly increased by each of the six mediators. These results demonstrate the potential use of the NF-05 laccase for the decolorization of recalcitrant dyes in dye bleaching and effluent detoxification.     

Biochemical characterization of laccase from hairy root culture of <Emphasis Type="Italic">Brassica juncea</Emphasis> L. and role of redox mediators to enhance its potential for the decolorization of textile dyes

In vitro transgenic hairy root cultures provide a rapid system for physiological, biochemical studies and screening of plants for their phytoremediation potential. The hairy root cultures of Brassica juncea L. showed 92% decolorization of Methyl orange within 4 days. Out of the different redox mediators that were used to achieve enhanced decolorization, 2, 2′-Azinobis, 3-ethylbenzothiazoline-6-sulfonic acid (ABTS) was found to be the most efficient. Laccase activity of 4.5 U mg⁻¹ of protein was observed in hairy root cultures of Brassica juncea L., after the decolorization of Methyl orange. Intracellular laccase produced by B. juncea root cultures grown in MS basal medium was purified up to 2.0 fold with 6.62 U mg⁻¹ specific activity using anion-exchange chromatography. Molecular weight of the purified laccase was estimated to be 148 kDa by sodium dodecyl sulfate polyacrylamide gel electrophoresis. The purified enzyme efficiently oxidized ABTS which was also required for oxidation of the other tested substrates. The pH and temperature optimum for laccase activity were 4.0 and 40°C, respectively. The purified enzyme was stable up to 50°C and was stable in the pH range of 4.0–6.0. Laccase activity was strongly inhibited by sodium azide, EDTA, dithiothreitol and l-cysteine. The purified enzyme decolorized various textile dyes in the presence of ABTS as an efficient redox mediator. These findings contribute to a better understanding of the enzymatic process involved in phytoremediation of textile dyes by using hairy roots.     

Continuous multiplication of rabbit tracheal epithelial cells in a defined,hormone-supplemented medium

Summary An improved Ham’s F12 nutrient medium supplemented with epidermal growth factor (EGF), insulin (INS), and transferrin (TF) was developed for continuous proliferation and clonal growth of primary rabbit tracheal epithelial (TE) cells in culture. The addition of small quantities of fetal bovine serum (FBS) (0.01 to 0.1%) to cultures had little measurable stimulation on TE cell growth and plating efficiency. However, serum levels higher than 0.1% inhibited cell growth and also masked the growth stimulating activities of EGF and INS despite an increase in cell attachment. Under this defined, hormone-supplemented medium, and in the presence of a trace amount of serum (0.01%), 10 to 20% of the protease-dissociated TE cells attached to the culture dish followed by at least four population doublings during 7 to 10 d of culture. Clonal growth occurred at a seeding density of 17 cells/cm² with a plating efficiency of 6 to 8%. Confluent primary cultures could be passaged two to four times by treatment with a 0.1% trypsin-1 mM EDTA solution and a total of 10 to 30 population doublings of in vitro life span were obtained. The epithelial nature of cultured cells was confirmed by indirect immunofluorescent staining with antikeratin antibody as well as by transmission electron microscopy. This study shows that using this improved hormone-supplemented medium, rabbit TE cells can be maintained in culture for extended periods of time without the aid of a fibroblast feeder layer or explant tissue. This system could be useful for the study of cell differentiation of tracheal epithelium.     

一株产漆酶真菌新月弯孢霉JQH-100在染料脱色中的应用

从感染叶斑病的玉米叶片中分离、纯化得到一株高产漆酶的新月弯孢霉Curvularia lunata JQH-100菌株。液体培养Curvularia lunata JQH-100可产漆酶且活性较高,产酶高峰出现在第3天;以ABTS为底物粗酶液的最适反应温度是30℃,最适反应pH是2.8;染料脱色的研究表明,共培养体系对茜素红的脱色率达到了92.6%,对中性红和刚果红的脱色率也都在80%以上;Curvularia lunata JQH-100所产漆酶经纯化后对染料茜素红和刚果红有较高的脱色率,分别为82.1%和81.2%。研究结果显示Curvularia lunata JQH-100在染料废水处理中有较大应用潜力。     

Effects of trace element supplementation on the inflammatory response in a rabbit model of major trauma

Patients with a severe trauma exhibit a strong oxidative stress, an intense inflammatory response, and long-lasting hypermetabolism, all of which are proportional to the severity of injury. In this study, we investigated the impact of trace element (TE) supplementation on the inflammatory response in an animal model of major trauma. New Zealand White rabbits were randomly assigned as a control group (n=5) and an experimental group (n=70) that, after receiving a major trauma, was subdivided into Trauma-Control (n=35) and Trauma-TE (n=35) groups. Systemic inflammatory response syndrome (SIRS) was observed in 40 out of 70 rabbits with a trauma, with a higher incidence in the Trauma-Control group (88.6%; 31/35) than the Trauma-TE group (28.6%; 10/35) (p<0.01). The mortality rate was significantly different between the Trauma-Control and the Trauma-TE groups; (34% vs. 8%; p<0.01).There were significant post-trauma alterations in the levels of (1) serum and spleen zinc (Zn), copper (Cu), selenium (Se), and manganese (Mn), (2) serum AST and ALT, (3) serum interleukin-6/10, and (4) nuclear factor kappa binding (NF-κB) activity and the expression. TE supplementation: (1) improved blood urea nitrogen (BUN), and creatinine (Cr) levels, (2) stabilized IL-6/10 production, (3) decreased NF-κB p⁶⁵ production. Appropriate TE supplementation can improve the TE status, mitigate SIRS, and reduce the mortality due to multiple organ dysfunction syndromes (MODS)/multiple organ failure (MOF) after major trauma.     

Decolourisation of mushroom farm wastewater by <Emphasis Type="Italic">Pleurotus ostreatus</Emphasis>

Mushroom production on coffee pulp as substrate generates an intense black residual liquid, which requires suitable treatment. In the present study, Pleurotus ostreatus growth in wastewater from mushroom farm was evaluated as a potential biological treatment process for decolourisation as well as to obtain biomass (liquid inoculum). Culture medium components affecting mycelial growth were determined, evaluating colour removal. Laccase activity was monitored during the process. P. ostreatus was able to grow in non diluted WCP. Highest biomass yield was obtained when glucose (10 g/l) was added. The addition of this carbon source was necessary for efficient decolourisation. Agitation of the culture improved biodegradation of WCP as well as fungal biomass production. Laccase and manganese-independent peroxidase activities were detected during fungal treatment of the WCP by P. ostreatus CCEBI 3024. The laccase enzyme showed good correlation with colour loss. Both wastewater colour and pollution load (as chemical oxygen demand) decreased more than 50% after 10 days of culture. Phenols were reduced by 92%.     

An arabinogalactan protein(s) is a key component of a fraction that mediates local intercellular communication involved in tracheary element differentiation of zinnia mesophyll cells

Local intercellular communication is involved in tracheary element (TE) differentiation of zinnia (Zinnia elegans L.) mesophyll cells and mediated by a proteinous macromolecule, which was designated xylogen. To characterize and isolate xylogen, a bioassay system to monitor the activity of xylogen was developed, in which mesophyll cells were embedded in microbeads of agarose gel at a low (2.0-4.3x10(4) cells ml(-1)) or high density (8.0-9.0x10(4) cells ml(-1)) and microbeads of different cell densities were cultured together in a liquid medium to give a total density of 2.1-2.5x10(4) cells ml(-1). Without any additives, the frequency of TE differentiation was much smaller in the low-density microbeads than in the high-density microbeads. This low level of TE differentiation in the low-density microbeads was attributable to the shortage of xylogen. When cultures were supplemented with conditioned medium (CM) prepared from zinnia cell suspensions undergoing TE differentiation, the frequency of TE differentiation in the low-density microbeads increased remarkably, indicating the activity of xylogen in the CM. The xylogen activity in CM was sensitive to proteinase treatments. Xylogen was bound to galactose-specific lectins such as Ricinus communis agglutinin and peanut agglutinin, and precipitated by beta-glucosyl Yariv reagent. These results indicate that xylogen is a kind of arabinogalactan protein.     

The Effect of Different Plant Growth Regulators on Adventitious Shoot Formation from Virginia Pine (Pinus virginiana) Zygotic Embryo Explants

The effects of different plant growth regulators on in vitro adventitious shoot formation in Virginia pine (Pinus virginiana Mill.) zygotic embryo explants were quantitatively evaluated. Using Tang and Ouyang (1999) (TE) basal medium supplemented with 11.4 μM indole-3-acetic acid (IAA) and 2.2 μM N⁶-benzyladenine (BA), callus was observed after 3–6 weeks of culture. Calluses were transferred to TE basal medium supplemented with 0.49 μM indole-3-butyric acid (IBA) and 8.8 μM BA for 6–9 weeks, where they produced numerous small shoot primordia. They were then transferred to TE basal medium supplemented with 0.49 μM IBA and 4.4 μM BA to promote growth and elongation of adventitious shoots. After elongated shoots were transferred to TE medium containing 0.05 μM α-naphthaleneacetic acid (NAA) for 6 weeks, adventitious roots were formed. Regenerated plantlets were established in soil in greenhouse.     

异丙酚对大鼠心肌缺血/再灌注损伤时NF-κB活化和细胞凋亡的影响

目的:观察异丙酚对大鼠心肌缺血/再灌注时核因子-κB(NF-κB)的活化和细胞凋亡的影响,以探讨异丙酚的心肌保护作用机制。方法:采用阻断大鼠左冠状动脉前降支30min,再灌注2h心肌缺血/再灌注损伤模型。60只SD大鼠随机分为假手术组(Sham)、缺血/再灌注组(I/R)和异丙酚3、6、12mg/(kg.h)组。光、电镜观察心肌组织的形态学变化。免疫组化染色分析心肌组织中NF-κB的核移位,Western blot检测心肌组织NF-κB和caspase-3的表达。原位末端标记(TUNEL)检测心肌细胞凋亡。结果:I/R组心肌纤维排列紊乱,心肌细胞水肿;线粒体膜肿胀,嵴排列紊乱甚至溶解消失。与I/R组相比,6,12mg/(kg·h)组异丙酚组心肌损伤明显减轻。与Sham组相比,I/R组NF-κB活化,明显从细胞浆移位于细胞核,表达量也显著增加(P0.05);心肌caspase-3表达增强(P0.01),心肌细胞凋亡指数升高(P0.05)。而异丙酚6mg/(kg·h)、12mg/(kg·h)组,NF-κB从细胞浆向细胞核的移位被明显限制,NF-κB的表达量也明显低于I/R组(P均0.05);心肌caspase-3表达减弱,心肌细胞凋亡指数减少(与I/R组相比,P0.05)。结论:异丙酚的心肌保护作用可能与其抑制NF-κB的活化,下调caspase-3的表达,从而抑制心肌细胞凋亡有关。     

火炬松成熟合子胚培养直接器官发生和植株再生

基因型Ｈｂ,Ｍａ和Ｍｃ的火炬松成熟合子胚在附加１．０ｍｇ／ＬＮＡＡ,４．０ｍｇ／ＬＢＡ,５００ｍｇ／ＬＬＨ和５００ｍｇ／Ｌ谷氨酰胺的ＴＥ培养基上培养１２周后,在子叶和胚轴部位形成不定芽原基。然后将合子胚转移到附加０．５ｍｇ／／ＬＮＡＡ,０．０５ｍｇ／ＬＩＢＡ,２ｍｇ／ＬＢＡ,５００ｍｇ／ＬＬＨ和５００ｍｇ／Ｌ谷氨酰胺的ＴＥ不定芽分化培养基上,６周后分化产生大量不定芽,３种基因型中,Ｈｂ的直接不定芽