栓孔菌属漆酶高产菌株的初步筛选及其产酶条件的优化

利用显色反应对栓孔菌属(Trametes)进行了漆酶高产菌株的筛选,并对目标菌株的产酶条件进行了优化,在添加愈创木酚的固体培养基中,通过显色反应初步筛选出漆酶高产菌株东方栓孔菌Trametes orientalis Cui 6300;进一步通过单因子分析、正交试验和ABTS法确定了菌株Cui 6300的最适产酶条件:麦芽糖15 g/L,蛋白胨3 g/L,pH 4.8,Cu2+2.0 mmol/L,培养温度28°C,接种饼直径1.5 cm,此时酶活最高可达19.923 U/mL;同时探索了Cu2+浓度及添加时间对其菌丝生物量和漆酶活力的影响。研究表明,Cu2+最适添加浓度为2.0 mmol/L,添加时间为接种后第3天。     

白灵侧耳漆酶分离纯化及其酶学性质研究

为了探索白灵侧耳Pleurotus eryngii var.tuoliensis漆酶性质,以白灵侧耳菌株00485为试验材料,从发酵液中分离纯化得到胞外漆酶并对其酶学性质进行测定。纯化流程依次为DEAE-Cellulose阴离子交换层析,CM-Cellulose阳离子交换层析,SP-Sepharose强阳离子交换层析以及Superdex 75凝胶过滤层析,获得胞外白灵侧耳漆酶(Pn Lac)。SDS-PAGE检测结果表明Pn Lac为65k Da的单一蛋白。Pn Lac经过胰蛋白酶水解得到3种肽段,经过NBCI-BLAST后发现它们与糙皮侧耳、环柄韧伞、刺芹侧耳等的漆酶具有同源性。底物为2,2-联氮-二(3-乙基-苯并噻唑-6-磺酸)二铵盐(ABTS)时该种漆酶的最适反应温度和p H分别为50℃和3.0,Ca2+和Hg2+能够抑制它的活性,相反地Cu2+和Mn2+能够提高它的活性,米氏常数Km和Vmax分别是0.17mmol/L和1.76OD/min/U。     

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。     

黑木耳漆酶纯化及部分漆酶特性的研究

黑木耳漆酶研究可为漆酶的进一步分离纯化、基因克隆表达和大规模生产应用奠定基础。对黑木耳"黑29"菌株漆酶粗酶液进行硫酸铵分级沉淀后,通过Native SDS-PAGE电泳检测,存在3种漆酶LacA、LacB、LacC,分子量分别为60,34,19 kD。经硫酸铵分级沉淀和DEAE-Sephacel柱层析技术分离得一纯化成分LacC,纯化倍数7.60,酶活性回收4.28%。对LacC的pH、温度、金属离子和Km值等部分酶学性质进行研究发现,该酶氧化ABTS的Km值为1.18×10-6mol/L,催化氧化底物ABTS的最适pH为3.8,在pH 3.0~4.6表现出较强的稳定性;最适反应温度为55℃,低于50℃时有较好的热稳定性;金属离子Ag+对漆酶有激活作用,而Fe3+、Mn2+、Co2+则有抑制作用。     

胶质射脉革菌漆酶的复合诱导及其脱色性能

[目的]研究复合诱导对胶质射脉革菌BBEL0901产漆酶的影响及其粗酶液对染料的脱色性能。[方法]采用分光光度法测定漆酶活性及其染料脱色性能。[结果]甘草渣和Cu2+对BBEL0901产漆酶均有促进作用,于发酵的第6 d向含甘草渣的低氮培养基中添加Cu2+(0.5 mmol/L)对漆酶的协同诱导作用最显著,活性达325.1 U/m L,分别为Cu2+单独诱导、甘草渣单独诱导和未诱导的4倍、14.4倍和19.8倍。粗酶液对不同结构的染料均有较强的脱色能力,对三苯甲烷类染料的脱色效果最好,脱色率达80%以上。[结论]甘草渣与Cu2+对BBEL0901漆酶具有协同诱导作用,酶活最高可达325.1 U/m L,产业化潜力大,所得粗酶液在染料脱色方面具有良好的应用前景。     

荷叶离褶伞高产漆酶菌株选育及其漆酶酶学特性

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。     

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。     

毛栓菌漆酶诱导及部分特性研究

研究了碳源、氮源、愈创木酚、香兰素及培养条件对漆酶分泌的影响 ;结果表明 ,麦草粉作碳源、(NH4 ) 2 SO4 作氮源有利于漆酶的分泌 ,适宜浓度的愈创木酚和香兰素等对漆酶的产生有一定的作用 ;pH在 3 0 - 8 0的范围内对漆酶的分泌影响差别不大 ,培养温度、接种量、通气量对漆酶的分泌有较大影响。漆酶最适pH值为 4 0 ,最适反应温度为 30℃ ,K+ 、Zn2 + 、Cu2 + 离子可激活漆酶 ;而Ag+ 、Fe3+ 、Cl- 离子可抑制漆酶活性。漆酶的Km值为 1 81× 10 - 3mol L。     

木霉LaTr 01菌株产漆酶发酵的条件

从华南地区采集土样,采用愈创木酚平板筛选产漆酶菌株,获得了一株短周期产漆酶的小型丝状真菌。通过观察菌落特征、生长情况以及显微镜下菌丝和孢子的形态,初步鉴定该菌株为木霉属的一个种（Trichodermaspp、）,命名为木霉LaTr01菌株。通过单因素方法研究该菌产漆酶的发酵条件,结果表明：LaTr01的产酶培养基以麦芽糖为最佳碳源;以酵母提取物为最适氮源;培养24h后加入Cu“比培养开始加入Cu ^2＋LaTr01产酶活高出约1倍。采用麦芽糖、酵母提取物、Cu^2＋浓度L9（3^3）的正交试验优化漆酶发酵条件,结果表明,氮源是影响该菌产漆酶的最重要因素,碳源次之,Cu^＋浓度影响较小;LaTr01菌株产生漆酶的最佳条件为：5g／L酵母提取物、20g/L麦芽糖、1．5mmol／LCu^2＋,Cu^2＋加入时间为培养24h后。在优化的培养条件下,该菌酶活可达480．556U／L。     

灵芝(Ganoderma lucidum)漆酶基因的克隆及其序列分析

漆酶(laccase EC1·10·3·2)是一种含Cu的多酚氧化酶,自从1883年日本学者吉田首次从漆树汁液中发现以来,漆酶特别是真菌漆酶一直是生物学、化学和环境科学等领域十分活跃的研究热点,在纸浆的生物漂白[1,2],有毒污染物的降解[3~5]等方面有较大的应用价值.根据其来源主要分为漆树漆酶和真菌漆酶两大类,由一个结构相似的基因家族所编码,目前,至少有40个以上的真菌漆酶基因被克隆和测序[6~9],最近也有从细菌中克隆到漆酶基因的报道[10~12].我国幅员辽阔,具有十分丰富的真菌资源,但是我国对漆酶的研究与发达国家相比还十分落后,对于漆酶基因资…     

Purification and characterization of extracellular laccase fromPleurotus ostreatus

Laccase (EC 1.10.3.2) from the culture filtrate of a strain of white rot basidiomycetePleurotus ostreatus was purified using DEAE-Toyopearl 650M and butyl-Toyopearl 650M column chromatographies and Superdex 75 HR 10/30 fast protein liquid chromatography. Molecular weight of the purified laccase was about 55,000, and the isoelectric point was 3.0. The optimum pH for enzyme activity was 6.5, and the optimum temperature was 50°C. This enzyme contained 7.4% sugar and two copper atoms per molecule. The substrate specificity was similar to those of other fungal laccases. Comparison of the N-terminal amino acid sequence of theP. ostreatus laccase with those fromPleurotus ostreatus Florida,Coriolus hirsutus, Phlebia radiata, basidiomycete PM1 (CECT 2971),Trametes villosa, Pycnoporus cinnabarinus, Ceriporiopsis subvermispora, andAgaricus bisporus showed 95, 65, 60, 55, 55, 55, 50, and 35% similarity, respectively, in the first 20 residues. No similarity in this region was detected with laccases fromNeurospora crassa, Aspergillus nidulans, andCryptococcus neoformans.     

壳聚糖载体的改性及其用于固定化漆酶的研究

利用有机酸改性壳聚糖,并用交联法制备酸化的壳聚糖载体,然后用改性壳聚糖载体固定漆酶。甲酸、乙酸改性壳聚糖的最适条件:壳聚糖与甲酸、乙酸的质量摩尔比(g/mol)分别为100∶1、100∶1.5,戊二醛的质量分数为1%,缓冲溶液的pH分别是4.4、5.0,反应时间为3h;壳聚糖与酒石酸、草酸的质量摩尔比(g/mol)分别为100∶0.5、100∶2,戊二醛的质量分数为2%,缓冲溶液的pH分别是3.6、4.2,反应时间为4.5h。不同有机酸改性的壳聚糖用于漆酶的固定,其酶活都有不同程度的提高,尤其用酒石酸改性的壳聚糖载体效果最好,其酶活提高了57%。     

野桑蚕GST-Omega1基因在草地贪夜蛾Sf9细胞中的表达

谷胱甘肽 S-转移酶（glutathione S-transferases,GSTs）是昆虫的重要解毒酶之一。为了研究野桑蚕Bombyx mandarina中谷胱甘肽S-转移酶在真核表达系统中的表达情况。本研究通过RT-PCR从野桑蚕中肠中获得GST-Omega1基因的cDNA序列,该基因的开放读码框为771 bp,编码256 个氨基酸。对推导的氨基酸序列用NCBI的蛋白质Conserved Domains工具进行在线分析,结果显示GST-Omega1的氨基酸序列中具有Cys38和8个GSH结合位点的Omega类基因保守序列。对所获得的基因克隆进表达载体pFastBacHT b中获得pFast-GST-Omega1,将其转化DH10Bac感受态细胞,获得Bac-GST-Omega1重组病毒DNA,用脂质体法转染草地贪夜蛾Sf9细胞,获得重组病毒。对表达产物经SDS-PAGE和Western blotting分析,能检测到一条分子量约为33 kD的特异性条带,与推导的融合蛋白大小相符,该目的蛋白的表达量占总蛋白的14.4%。目的蛋白经His·Bind树脂纯化,用Lineweaver Burk作图法测定其K_m和V_max,结果显示其K_m为2.81 µmol/L,V_max为2.70 µmol/(mg·min）。     

Biochemical and mutational analysis of a plant virus polyprotein cleavage site.

The RNA genome of tobacco etch virus (TEV) is organized as a single translational unit coding for a 346,000 (346 kd) mol. wt (Mr) polyprotein. The 346 kd Mr polyprotein is cleaved by a 49 kd Mr virus-encoded proteinase at five different sites between the dipeptides Gln-Ser or Gln-Gly. These cleavage sites or gene product boundaries are defined by the heptapeptide sequence...Glu-Xaa-Xaa-Tyr-Xaa-Gln-Ser or Gly.... We have used the 54 kd Mr nuclear inclusion protein/30 kd Mr capsid protein junction as a model to examine the role of these conserved amino acids in defining a cleavage site. The 54 kd/30 kd Mr protein cleavage site sequence of 10 TEV isolates from geographically distinct locations has been deduced. The conserved amino acids are present in all isolates. To determine if these four amino acids are an absolute requirement for polyprotein substrate activity, a site-directed mutational analysis has been performed. A recombinant cDNA molecule encoding the TEV 54 kd/30 kd Mr gene product cleavage site was mutated and polyprotein substrates were synthesized and processed in a cell-free system. Single amino acid substitutions made at the different positions reveal a strong preference for the naturally conserved amino acids.     

Purification of branched-chain amino acid aminotransferase from <Emphasis Type="Italic">Helicobacter pylori</Emphasis> NCTC 11637

Summary. Branched-chain amino acid aminotransferase was purified by several column chromatographies from Helicobacter pylori NCTC 11637, and the N-terminal amino acid sequence was analyzed. The enzyme gene was sequenced based on a putative branched-chain amino acid aminotransferase gene, ilvE of H. pylori 26695, and the whole amino acid sequence was deduced from the nucleotide sequence. The enzyme existed in a homodimer with a calculated subunit molecular weight (MW) of 37,539 and an isoelectric point (pI) of 6.47. The enzyme showed high affinity to 2-oxoglutarate (K _m = 0.085 mM) and L-isoleucine (K _m = 0.34 mM), and V _max was 27.3 μmol/min/mg. The best substrate was found to be L-isoleucine followed by L-leucine and L-valine. No activity was shown toward the D-enantiomers of these amino acids. The optimal pH and temperature were pH 8.0 and 37 °C, respectively.     

血红密孔菌(Pycnoporussanguineus)漆酶基因的克隆与序列分析

为克隆血红密孔菌 (Pycnoporussanguineus)漆酶基因 ,根据真菌漆酶氨基酸序列保守区设计了 1对简并引物 .以血红密孔菌基因组DNA为模板 ,PCR扩增出长 12 2 7bp的漆酶基因片段 .以此序列为基础 ,通过 5′及 3′RACE技术克隆出漆酶全长cDNA序列 ,序列长为 190 2bp ,其 5′端和 3′端非编码区长分别为 5 1bp和 2 97bp ,开放阅读框长 15 5 4bp ,编码 5 18个氨基酸的蛋白 .该蛋白具有 4个铜离子结合区域 ,预测其相对分子量为 5 6 313 2 ,等电点为 5 5 9,其氨基酸序列与Pycnoporuscinnabarinus漆酶 (lcc3 2 )的同源性最高 ,为 96 % .以该cDNA编码区的两端序列为引物 ,PCR扩增得到漆酶的长度为 2 15 4bp的全长DNA序列 ,序列中包括 10个内含子序列 ,长为 5 2～ 70bp     

Diversity of laccase among Cryptococcus neoformans serotypes

The pathogenic yeast C. neoformans is classified into three varieties with five serotypes; var. grubii (serotype A), var. neoformans (serotype D), var. gattii (serotypes B and C), and serotype AD. Melanin is a virulence factor in the species, and its biosynthesis is catalyzed by laccase, encoded by the LAC1 gene. In order to estimate the natural variability of the LAC1 gene among Cryptococcus serotypes, the laccase protein sequence from 55 strains was determined and the phylogenetic relationships between cryptococcal and related fungal laccases revealed. The deduced laccase proteins consisted of 624 amino acid residues in serotypes A, D and AD, and 613 to 615 residues in serotypes B and C. Intra-serotype amino acid variation was marginal within serotypes A and D, and none was found within serotypes AD and C. Maximum amino acid replacement occurred in two serotype B strains. The similarity in the deduced sequence ranged from 80 to 96% between serotypes. The sequence in the copper-binding regions was strongly conserved in the five serotypes. The laccases of the five serotypes were grouped together in the same clade of the phylogenetic tree reconstructed from different fungal laccases, suggesting a monophyletic clade.     

Effects of Homocysteine on ERK Signaling and Cell Proliferation in Fetal Neural Stem Cells In Vitro

The aim of the present study was to determine if the excitatory amino acid homocysteine (Hcy) alters ERK signaling and cell proliferation in fetal neural stem cells (NSCs) in vitro. NSCs were isolated from fetal rats and grown in serum-free suspension medium. The cells were identified as NSCs by their expression of immunoreactive Sox2. NSCs were assigned to one of four treatment groups: vehicle control, low-dose Hcy group (Hcy-L, medium contained 30 μmol/L Hcy), middle-dose Hcy group (Hcy-M, 100 μmol/L Hcy) and high-dose Hcy group (Hcy-H, 300 μmol/L Hcy). Cell proliferation was evaluated by 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide assay. Protein expression levels of ERK1/2 and phosphorylated ERK1/2 were detected by Western blot. The effects of Hcy on NSC death, including apoptosis, were assessed by using flow cytometry and trypan blue exclusion. The results showed that NSCs grew as neurospheres in the serum-free medium. Hcy decreased ERK1/2 protein phosphorylation and NSC proliferation, but it did not induce cell death or apoptosis within the concentration from 30 to 300 μmol/L. The above results are consistent with the hypothesis that Hcy decreases fetal NSC proliferation by inhibiting ERK signaling.