链霉菌Str s-2产木聚糖酶的条件及部分性质研究

通过碳氮源对链霉菌Str s-2产胞外木聚糖酶活性的影响,得出其适宜培养基为(g/L)：含半纤维素20,(NH4)2SO4 4．0,KH2PO4 1．0,MgSO4-7H2O 0．5,NaCl 0．3,CaCO3 1．0。用DNS法研究了该酶的性质结果表明其最适pH值为6．5,最适反应温度为55℃;Na^ 、K^ 、Ca^2 、Mg^2 等离子对酶有激活作用,而Zn^2 、Ag^ 、Fe^3 和Cu^2 离子则抑制酶的活性。     

一株产木聚糖酶链霉菌的鉴定及发酵产酶*

以木聚糖为唯一碳源,筛选出一株高产木聚糖酶生产菌株。该菌株经形态特征、 培养特征、生理生化和细胞壁组分分析等实验,鉴定为卷须链霉菌（Streptomyces cirratus).摇瓶发酵产酶实验表明：培养基最佳初始pH值为6．0;玉米芯水不溶木聚糖和蛋白胨分别是最佳的碳源和氮源;添加0．5％吐温80使得木聚糖酶活力提高到原来的2．5倍,发酵液最高酶活达到623u／mL。     

链霉菌发酵麦草产木聚糖酶的试验研究

通过正交设计试验 ,找出利用链霉菌和麦草基质发酵生产木聚糖酶的试验条件。培养基 (g/L) :麦草粉 ,4 5 ;(NH4 ) 2 SO4 ,7.5 ;酵母膏 ,8;K2 HPO4 ·3H2 O ,1;MgSO4 ·7H2 O ,0 .5 ;NaCl,0 .3。接种量为 5 .0× 10 8个孢子 / 5 0mL培养基 ,振荡培养 (12 0r/min) 5d     

一株高产木聚糖酶的枝链霉菌的分离鉴定及产酶

对1株高产木聚糖酶的链霉菌进行了鉴定并研究其木聚糖酶的生产过程及水解产物特点。分离得到1株产木聚糖酶的链霉菌Streptomyces sp.L2001,从形态学特征、培养特征和生理生化特征等方面对该菌株进行了鉴定。PCR扩增得到16S rDNA序列全长为1429bp,分析结果表明,菌株与Streptomyces rameus NBRC3782同源性达99.16%。结合传统生理生化实验结果鉴定为枝链霉菌。菌株液体发酵6d能产生842.0U/mL木聚糖酶活力。经HPLC分析酶解产物,结果显示木二糖、木三糖及木四糖含量之和高达93.5%,该酶适用于工业化生产低聚木糖。     

林肯链霉菌谷氨酰胺合成酶的酶学性质

在分离纯化的基础上,报道了pH、温度和金属离子对林肯链霉菌(Streptomyceslincolnensis)Z-512谷氨酸胺合成酶(GS)活力的影响及GS底物专一性的研究结果.在动力学性质的研究中,发现林肯链霉菌GS在生物合成反应系统中,对底物NH_4CI的饱和曲线不遵守米氏方程.Hill作图呈两相曲线.在NH_4CI浓度低的情况下,Hill系数大于1,具有正协同效应;当NH_4CI浓度增加到一定程度时,Hill系数小于1,具有负协同效应.这说明NH_4CI不仅作为林肯链霉菌GS的底物,而且作为一种效应物调节GS的活性.林肯链霉菌GS对底物Glu及ATP的饱和曲线遵守米氏方程.在不同的激活离子存在下,GS对Glu、ATP的Km值也不同.     

链霉菌壳聚糖酶的纯化及其酶学性质

分离纯化从烟台近海土壤筛选的链霉菌来源壳聚糖酶,并对其酶学性质进行研究。通过(NH4)2SO4分级沉淀分离得粗酶,透析后经Sephadex G-100柱纯化,得到2种壳聚糖酶(ChA和ChB)。SDS-聚丙烯酰胺凝胶电泳及Sephadex G-75凝胶过滤确定ChA的相对分子质量,研究ChA的最适底物水解条件、热稳定性、水解动力学及金属离子对酶活性影响。结果表明:ChA为单亚基蛋白,相对分子质量为4.16×104,在220和280 nm处呈现两个紫外吸收峰,催化水解壳聚糖的最适pH为5.0～5.5,最适温度为55℃。热稳定性实验表明:30℃温育1 h后酶活为初始酶活的33.3%,40℃温育1 h后酶活为初始酶活的22.2%。ChA的酶促反应初速率为6.2×10-3μmol/(mL.min),Vmax为0.318μmol/(mL.min),Km为1×10-2mg/mL,且对底物表现相对专一性。K+、Na+、Li+、Mg2+、Ca2+、Ba2+Zn2+、Cu2+和Co2+对ChA活力均表现为抑制作用,过渡金属离子Mn2+对酶有激活作用,重金属离子Hg2+、Ag+、Cd2+和Pb2+对酶均有较强的抑制作用。Mn2+和Zn2+的动力学研究表明,Mn2+对酶为混合型激活作用,Zn2+对酶为竞争性抑制作用。     

灰色链霉菌胰蛋白酶在变铅青链霉菌中的异源表达及酶学性质分析

胰蛋白酶作为一种重要的丝氨酸蛋白酶被广泛应用于食品、医药和皮革等工业领域.本文成功实现了灰色链霉菌来源的胰蛋白编码基因在变铅青链霉菌中的高效活性表达,并对其酶学性质进行分析比较.以灰色链霉菌ATCC10137基因组为模板,获得胰蛋白酶编码基因sprT并克隆至表达质粒pIJ86,成功构建了重组链霉菌工程菌TK24/pIJ86-sprT.以R2YE和SELF为发酵培养基,最高酶活分别达9.21 U/mL和8.61 U/mL.酶学性质分析表明,和牛胰蛋白酶(BT)相比,重组链霉菌胰蛋白酶(rSGT)的耐酸能力强,具有较广的pH;且rSGT对酰胺键具有更高的特异性;此外,Zn2+和有机溶剂分别对rSGT的酯酶活力和酰胺酶活力具有促进作用;本研究结果为rSGT的性质改造以及工业应用提供了依据.     

链霉菌Strz-6木聚糖酶的纯化和固定化研究

链霉菌胞外木聚糖酶经过盐析、离子交换和分子筛层析纯化,粗酶液被纯化了32.5倍,比活力达498u/mg,活力回收46.6%。纯化后的酶固定在戊二醛交联的壳聚糖上,酶活回收率为42.8%。固定化酶的最适pH为6.0,最适温度为60℃,且固定化酶在65~75℃活力都较高。该酶的耐热性比较强,固定化酶热稳定性优于原酶;以木聚糖为底物,固定化酶的表观米氏常数为0.93×10-2g/L。     

链霉菌产木聚糖酶条件和酶学性质以及重离子诱变对产酶的影响研究

以一株由青藏高原牦牛粪中分离出的链霉菌为出发菌株,对其培养特性、产酶条件和酶学性质进行初步研究.通过重离子诱变,筛选出遗传稳定的高产菌株.结果表明,该菌以玉米芯和麸皮(1∶1)为碳源能高效地诱导木聚糖酶的胞外分泌,其最适培养基和培养条件氮源为酵母膏、初始pH7、培养温度为25℃,在此条件下,第4天酶活力达到峰值3480.25 U/mL.说明该酶能够利用农业废弃物高效生产木聚糖酶.该菌株所产木聚糖酶的最适反应温度为15℃、pH4,属低温酸性木聚糖酶.经重离子诱变后,筛选出一株高产菌株SZ10-7,其酶活力可达5 338.42 U/mL.     

青霉菌聚半乳糖醛酸酶基因在毕赤酵母中的表达及酶学性质研究

筛选得到一株能分解果胶的青霉菌(Penicillium sp.),使用简并引物PCR和TAIL-PCR方法从该菌中克隆了一个聚半乳糖醛酸酶基因pgp1.pgp1基因全长1 225 bp,包含2个内含子,其cDNA全长1 104 bp,编码367个氨基酸和一个终止密码子,前18个氨基酸为信号肽序列.将pgp1基因连接pPIC9载体,在巴斯德毕赤酵母表达系统中进行了异源表达.在3L发酵罐水平,培养基中聚半乳糖醛酸酶活力达到700 U/mL.酶学性质测定表明,重组酶蛋白PGP1的最适pH为5.0,在pH4.0 -6.0下处理1h后,剩余酶活力超过90％;最适温度为38℃,以聚半乳糖醛酸为底物,PGP1的Km=(1.172±0.169)mg/mL,Vmax=(0.061±0.002) mg/min/mL.     

木聚糖酶异源表达的研究进展

木聚糖(xylan)在自然界中的含量极其丰富,在农作物和农林剩余物中大量存在。随着能源资源问题的日益凸显,对木聚糖的应用和研究越来越受到重视。木聚糖酶(xylanase)是可以将木聚糖降解为低聚木糖和木糖的一类水解酶,近年来,为了实现木聚糖酶的高产、高酶活表达,科研工作者做了大量的研究工作,就木聚糖酶异源表达(heterologous expression)的研究进展进行综述。     

链霉菌Strz-2胞外木聚糖酶的纯化和固定化研究

为探讨木聚糖酶被固定化后的酶活力变化 ,采用盐析、离子交换和分子筛层析方法对链霉菌胞外木聚糖酶进行了纯化 ,并采用DNS方法对固定化酶的性质进行了研究。结果如下 :粗酶液被纯化了 30 .5倍 ,比活力达 4 5 7.5 ,活力回收 4 2 .6 %。纯化后的酶固定在戊二醛交联的壳聚糖上 ,残活力为 4 1.8%。固定化酶的最适pH为 6 .0 ,最适温度为 5 5℃ ,且固定化酶在 6 5 -75℃活力都较高。该酶的耐热性比较强 ,固定化酶热稳定性优于原酶 ;以木聚糖为底物 ,固定化酶的表观米氏常数为 0 .83× 10 -2g/L。因此 ,固定化的木聚糖酶优于原酶     

A novel thermophilic xylanase from Achaetomium sp. Xz-8 with high catalytic efficiency and application potentials in the brewing and other industries

Thermophilic xylanases are of great interest for their wide industrial application prospects. Here we identified a thermophilic xylanase (XynC01) of glycoside hydrolase (GH) family 10 in a thermophilic fungal strain Achaetomium sp. Xz-8. The deduced amino acids of XynC01 showed the highest identity of ≤52% to experimentally verified xylanases. XynC01 was functionally expressed in Pichia pastoris, showed optimal activity at pH 5.5 and 75 °C with stability over a broad pH range (pH 4.0–10.0) and at temperatures of 55 °C and below. XynC01 had the highest catalytic efficiency (k_cat/K_m, 3710 mL/s/mg) ever reported for all GH 10 xylanases, and was resistant to all tested metal ions and chemical reagents. Its hydrolysis products of various xylans were simple, mainly consisting of xylobiose and xylose. Under simulated mashing conditions, XynC01 alone had a comparable effect on filtration improvement with Ultraflo from Novozymes (20.24% vs. 20.71%), and showed better performance when combined with a commercial β-glucanase (38.50%). Combining all excellent properties described above, XynC01 may find diverse applications in industrial fields, especially in the brewing industry.     

耐碱性木聚糖酶基因在短小芽孢杆菌中高效分泌表达的研究

从木聚糖酶高产短小芽孢杆菌 (Bacilluspumilus)BP5 1中克隆得到木聚糖酶基因xynA ,将其构建在芽孢杆菌表达载体pWH1 5 2 0中得到重组质粒pWSX1 1。xynA由木糖诱导xylA启动子调控xynA表达。采用同源高效表达策略 ,以原生质体转化方法将pWSX1 1转回原始菌株BP5 1中 ,获得重组菌株BPX1 1。通过木糖诱导重组菌株中的xy nA基因高效分泌表达 ,使木聚糖酶产酶活力比原菌株BP5 1提高了 87% ,同时对重组表达的木聚糖酶的酶学性质进行了初步研究     

链霉菌酪氨酸酶基因的克隆与表达

本文综述了近年来对链霉菌酪氨酸酶基因的研究。由酪氨酸酶合成黑色素是链霉菌属各个种的共同特性,并受到酪氨酸酶基因的控制。链霉菌几个种的酪氨酸酶基因已克隆到,其产黑色素的特性使之作为重要的标记基因得以广泛应用,同时,该基因在链霉菌的不同种及不同属的微生物中得到了高水平的表达。链霉菌酪氨酸酶基因表达调控的分子机制也得到较深入的研究。     

Antimicrobial potential of phylogenetically unique actinomycete,Streptomyces sp. JRG-04 from marine origin

Due to the emergence of severe infectious diseases and thriving antibiotic resistance, there is a need to explore microbial-derived bioactive secondary metabolites from unexplored regions. Present study deals with a mangrove estuary derived strain of Streptomyces sp. with potent antimicrobial activity against various pathogens, including methicillin resistant Staphylococcus aureus. Bioactive compound was effective even at low MIC level, damages the membrane of methicillin resistant S. aureus and causes cell death, however it has no cytotoxic effect on H9C2 cells. 16S rRNA shared 99.5% sequence similarity to Streptomyces longispororuber. Optimum biomass and antimicrobial compound production were observed in production medium supplemented with 1.0% maltose and 0.5% yeast extract. The active compound purified from the chloroform extract of the cell-free supernatant was studied by FT-IR, 1H NMR, 13C NMR and LC ESI-MS and identified as aromatic polyketide. β-ketosynthase (KS) domain of the Streptomyces strain revealed 93.2% sequence similarity to the benzoisochromanequinone, an actinorhodin biosynthetic gene cluster of Streptomyces coelicolor A3(2). However, the region synthesizing the secondary metabolite produced by the S. longispororuber was not related to the KS domain of the strain, due to the phenomenon of horizontal gene transfer over the period of evolutionary process, thus generating metabolic compound diversity.     

木霉T6木聚糖酶制剂研究

本文研究了木霉Ｔ６（Ｔｒｉｃｈｏｄｅｒｍａ ｓｐ．）产木聚糖酶固态发酵过程和木聚糖酶制剂制备,结果显示,固体曲培养４ｄ时酶活力最高,固体曲最适液固浸提比为７：１。木聚糖酶在６０～６５％硫酸铵饱和度下盐析效果最好。冷冻干燥和４０℃烘干酶粉得率分别为６８．３％和４５．７％。酶最适反应ＰＨ为４．５,最适反应温度５０℃,在不同温度下１小时后的半失活温度为４７．７℃。     

Streptomyces sp. TEM 33 possesses high lipolytic activity in solid-state fermentation in comparison with submerged fermentation

Solid-state fermentation (SSF) is a bioprocess that doesn’t need an excess of free water, and it offers potential benefits for microbial cultivation for bioprocesses and product development. In comparing the antibiotic production, few detailed reports could be found with lipolytic enzyme production by Streptomycetes in SSF. Taking this knowledge into consideration, we prefer to purify Actinomycetes species as a new source for lipase production. The lipase-producing strain Streptomyces sp. TEM 33 was isolated from soil and lipase production was managed by solid-state fermentation (SSF) in comparison with submerged fermentation (SmF). Bioprocess-affecting factors like initial moisture content, incubation time, and various carbon and nitrogen additives and the other enzymes secreted into the media were optimized. Lipase activity was measured as 1.74 ± 0.0005 U/g dry substrate (gds) by the p-nitrophenylpalmitate (pNPP) method on day 6 of fermentation with 71.43% final substrate moisture content. In order to understand the metabolic priority in SSF, cellulase and xylanase activity of Streptomyces sp. TEM33 was also measured. The microorganism degrades the wheat bran to its usable form by excreting cellulases and xylanases; then it secretes the lipase that is necessary for degrading the oil in the medium.