Gene Cloning of Cellobiohydrolase II from the White Rot Fungus Irpex lacteus MC-2 and Its Expression in Pichia pastoris

A gene (cel4) coding for a cellobiohydrolase II (Ex-4) was isolated from the white rot basidiomycete, Irpex lacteus strain MC-2. The cel4 ORF was composed of 452 amino acid residues and was interrupted by eight introns. Its deduced amino acid sequence revealed a multi domain structure composed of a cellulose-binding domain, a linker, and a catalytic domain belonging to family 6 of glycosyl hydrolases, from the N-terminus. cel4 cDNA was successfully expressed in the yeast Pichia pastoris. Recombinant Ex-4 showed endo-processive degrading activity towards cellulosic substrates, and a synergistic effect in the degradation of Avicel was observed when the enzyme acted together with either cellobiohydrolase I (Ex-1) or endoglucanase (En-1) produced by I. lacteus MC-2.     

Purification of Oat Debranching Enzyme and Occurrence of Inactive Debranching Enzyme in Cereals

The interaction of some anthracycline antibiotics (adriamycin, daunomycin, aclacinomycin-A) with bacteriophage ?X174 was investigated. Adriamycin and daunomycin inactivated the infectivity of both free ?X174 phage and naked single-stranded ?X174 DNA without DNA strand scission, but aclacinomycin-A did not show this action. The phage inactivation reaction was reversibly inhibited by Superoxide dismutase, catalase or other oxygen radical scavengers. The inactivation of ?X174 by adriamycin and aclacinomycin-A was stimulated by the addition of Cu²⁺, while the ?X174 inactivation by daunomycin was inhibited by the addition of Cu²⁺. The ?X174 inactivation by adriamycin and aclacinomycin-A in the presence of Cu²⁺ was caused by degradation of DNA, and this inactivation reaction was inhibited irreversibly by oxygen radical scavengers. These results indicate that anthracycline antibiotics bind to ?X174 DNA in the form of free radicals and that during the auto-oxidation of these antibiotics in the presence of Cu²⁺, oxygen radicals were generated to cause the degradation of ?X174 DNA.     

Preparation and properties of an immobilized cellulase on the reversibly soluble matrix Eudragit L-100

Abstract

To prepare a smart biocatalyst, cellulase was immobilized on the reversibly soluble matrix Eudragit L-100 by non-covalent and covalent methods. Covalent immobilization using carbodiimide coupling exhibited superior enzyme loading and reusability compared with non-covalent immobilization, and the covalent loading was increased by almost 20% through the addition of N-hydroxysuccinimide. The temperature optimum of the cellulase was not improved apparently by immobilization but the pH optimum increased from 4.75 to 5.25. Immobilized cellulase was more active than free cellulase above pH 5.0. Immobilized cellulase was more stable than free cellulase during storage at 4°C, room temperature and 50°C. K_m values of immobilized and free cellulase were 85.55 and 73.84 g L^?1, respectively. About 50% productivity was retained after five cycles for hydrolysis of steam-exploded straw.     

OPTIMIZATION OF AFFINITY DIGESTION FOR THE ISOLATION OF CELLULOSOMES FROM Clostridium thermocellum

The affinity digestion process for cellulase purification consisting of binding to amorphous cellulose, and amorphous cellulose hydrolysis in the presence of dialysis (Morag et al., 1991), was optimized to obtain high activity recoveries and consistent protein recoveries in the isolation of Clostridium thermocellum cellulase. Experiments were conducted using crude supernatant prepared from C. thermocellum grown on either Avicel or cellobiose. While no difference was observed between Avicel-grown or cellobiose-grown cellulase in the adsorption step, differences were observed during the hydrolysis step. The optimal amorphous cellulose loading was found to be 3 mg amorphous cellulose per milligram supernatant protein. At this loading, 90–100% of activity in the crude supernatant was adsorbed. Twenty-four-hour incubation with the amorphous cellulose during the adsorption stage was found to result in maximal and stable adsorption of activity to the substrate. By fitting the adsorption data to the Langmuir model, an adsorption constant of 410 L/g and a binding capacity of 0.249 g cellulase/g cellulose were obtained. The optimal length of time for hydrolysis was found to be 3 hr for cellulase purified from Avicel cultures and 4 hr for cellulase purified from cellobiose cultures. These loadings and incubation times allowed for more than 85% activity recovery.     

近暗散白蚁β-葡糖苷酶基因RpBg7的克隆及其在毕赤酵母中的表达

【目的】白蚁是自然界中利用木质纤维素能力很强的生物,是纤维素酶的天然资源库。本研究旨在挖掘新来源的纤维素酶基因,为生物质能源的高效利用提供新的天然酶。【方法】根据前期蛋白质组测序的结果,利用PCR结合RACE克隆了近暗散白蚁Reticulitermes perilucifugus β-葡糖苷酶7(β-glucosidase 7)基因RpBg7 cDNA全长序列;通过生物信息学软件分析了RpBg7的序列;用表达载体pPICZαA在毕赤酵母Pichia pastoris X-33中表达RpBg7蛋白,并用4-硝基苯基-β-d-吡喃葡萄糖苷(4-nitrophenyl β-d-glucopyranoside, 4pNPG)为底物检测了表达的RpBg7蛋白的酶活性。【结果】获得了近暗散白蚁的一个内源性β-葡糖苷酶7基因RpBg7(GenBank登录号: MN944395),其开放阅读框长1 485 bp,编码495个氨基酸残基。RpBg7蛋白预测分子量为57 kD,属于糖苷水解酶1(glycosidehydrolase 1, GH1)家族,具有保守的碱性氨基酸残基Glu187和Glu394。通过毕赤酵母表达系统成功表达RpBg7蛋白。酶活性分析结果表明,毕赤酵母胞外分泌蛋白粗酶液和胞内蛋白粗酶液中RpBg7酶活性分别为4.43和7.47 U/mL。【结论】克隆并利用毕赤酵母表达了近暗散白蚁的GH1家族的一个β-葡糖苷酶7基因RpBg7,为后期纤维素酶的改造和应用提供了条件。     

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。     

兼性厌氧纤维素降解菌的筛选和产酶研究

从我国天津地区堆肥中分离筛选出一株兼性厌氧的纤维素分解细菌D1,初步鉴定为纤维单孢菌(Cellulomonas sp.)。产酶最适碳源为葡萄糖,氮源为复合蛋白胨,酶的最适作用温度和pH值是50℃和6．4,在70℃以下和pH在5．2～8．4里稳定。     

微生物纤维素酶的应用研究

我国纤维素酶的应用研究近年来取得了很大进展。阐述了纤维素分解菌的选育 ,酶学性质以及在发酵、纺织和洗涤剂工业中的应用。     

酶法降解植物纤维素技术研究

用正交试验法探讨了以麦秸为原料进行纤维素酶降解的工艺条件。正交试验的结果表明,影响麦秸纤维素降解的因素的主次顺序为A（酶添加量）＞B（底物浓度）＞E（时间）＞C（温度）＞D（pH值）,纤维素酶解麦秸纤维素的最佳组合为A3B1E3C3D2,即纤维素酶的添加量为0．2％,底物浓度为5％,反应时间为2h,反应温度50℃,pH5.0时为最佳条件。在比常规酶解法时间缩短12－30倍的条件下,能使纤维素降解葡萄糖的转化率达22．3％。