木质素过氧化物酶LiPH2合成基因在毕赤酵母中的表达

应用化学合成方法获得了碱基序列优化后的木质素过氧化物酶LiPH2合成基因.分别将去除和含有自身信号肽的合成基因与几种选定的表达载体连接,并转化进入相应的Pichiapastoris宿主菌中,共构建了8个不同的毕赤酵母表达系统.对酵母转化子基因及对其发酵液中重组蛋白的分析结果表明,其中1个表达系统的酵母转化子能够成功分泌LiPH2重组蛋白.同时,对影响目的基因表达的各种因素的分析结果表明:就不同宿主菌而言,SMD1168与表达成功的X-33受体菌在其余因素相同的情况下无分泌蛋白表达,pep4基因的缺失对LiPH2蛋白的表达有不利影响;;就不同分泌信号肽而言,与α因子信号肽相比,LiPH2自身信号肽更有利于引导LiPH2的分泌表达;;就不同表达载体而言,其对外源蛋白的表达存在较大差别.本研究中得到的重组蛋白分子量有所增加,说明很可能存在过度糖基化的影响,过度糖基化和C-端氨基酸的增加可能是造成表达蛋白没有活性的原因.     

工程菌及其固定化细胞对有机磷农药的降解

将抗性库蚊解毒酶酯酶B1基因片段引入融合表达载体pThioHisA中,转化入大肠杆菌DH5α,在IPTG诱导下,经过8h,酯酶B1在大肠杆菌中获得融合高效表达。重组质粒pThioHisA-B1表达的酯酶融合蛋白具有较高的酯酶B1活性,能高效降解酯酶的特异性底物α-乙酸萘酯(α-NA)和β-乙酸萘酯(β-NA),将工程菌固定化后,固定化细胞在3h内对1000mg/L的甲基对硫磷降解率>65%。     

木质素过氧化物酶降解四环素机理的研究

为探究过氧化物酶对四环素类抗生素的降解机理,以白腐真菌Phanerochaete chrysosporium表达的木质素过氧化物酶(LiP)粗酶为研究对象,研究其产酶条件及其降解四环素(TC)的机理。结果表明:低浓度Mn2+可促进产酶,碳源、氮源限制是产酶的重要条件;降解反应进行10min后,H2O2消耗至阈值0.045mmol/L,LiP对TC的降解停止,其降解率达到82%;TC降解反应趋于平衡时,补加TC和H2O2后,LiP依然可以高效发挥作用,其二次降解率达到65%;LiP作用于不同初始浓度(10mg/L、25mg/L、50mg/L、100mg/L)TC,显示LiP对不同浓度TC均可有效降解,TC降解率分别为62%、80%、82%和90%;降解产物的抑菌性试验反映出降解产物较TC母体的抑菌性明显降低;LC/MS捕获到6种可能的降解产物E-TC、TP 461、E-TP 461、TP 477、TP 475和TP 445,并推测出LiP降解TC可能的降解途径。     

城市污水中病原性大肠埃希氏菌毒力基因eaeA和rfbE的实时荧光定量PCR检测

针对病原性大肠埃希氏菌EHEC和EPEC的毒力基因eaeA和rfbE,选用特异性引物,建立了实时荧光定量PCR检测方法. 利用从污水中分离出的目的核酸片段构建重组质粒,通过测序和BLAST比对分析,确定了PCR扩增的特异性. 将重组质粒作为模板,分别测定标准曲线,在eaeA基因模板量8.77～8.77×105 copy,rfbE基因模板量4.98～4.98×105copy的范围内,Ct(循环阈值)与模板量的对数值具有良好的线性关系〔R2为0.997(eaeA)和1.000(rfbE)〕. 结合膜吸附洗脱浓缩方法,对于实际水样,eaeA和rfbE基因的检测限分别为1.75×102和9.96×101copy/100 mL. 利用该方法对城市污水处理厂进、出水进行检测的结果显示,污水二级处理工艺对这2种毒力基因的去除效果明显.      

培养基种类和培养条件对白腐真菌生长和产酶特性的影响

以白腐真菌(Phanerochaete chrysosporium)为研究对象,比较了该菌种在人工合成培养基和天然培养基中的生长和产酶特性,考察了竹子浸出液,pH,载体和抗生素等对白腐真菌在天然培养基中生长和产酶特性的影响.结果表明,天然培养基中白腐真菌的生物量、菌丝小球直径和木质素过氧化物酶(LiP)活性均大于人工培养基.以天然培养基为基础培养基,加入竹子浸出液可以促进白腐真菌的生长和提高木质素过氧化物酶活性;较低pH(4.5)条件下菌丝小球直径较小;载体的加入使得菌体以附着形式生长;抗生素两性霉素B对白腐真菌的生长和产酶的影响存在阈值,当ρ(两性霉素B)超过50　mg/L时,白腐真菌的生长和产酶受到明显的抑制.      

白腐真菌F2的生长及产木质素降解酶特性的研究

考察了从我国生物资源中筛分出的白腐真菌F2的生长特性,采用多因素试验法研究了F2菌产木质素降解酶的特性;用统计学方法对试验数据进行了误差分析,并分析了多种影响因素对F2菌产木质素降解酶的影响.实验结果表明:F2菌在PDA培养基平板上和Tien＆Kirk培养基中都生长良好且生长速率较高;在自由悬浮振荡培养(不通氧气)条件下,F2菌产LiP的最高酶活可达60 5U·L-1,MnP的最高酶活可达263 4U·L-1,其产酶能力超过了黄孢原毛平革菌在自由悬浮振荡培养(不另外通入氧气)条件下的产酶能力.本研究还发现向培养基中添加的Cu2+浓度超过1μmol·L-1时会抑制F2菌产LiP,以往的文献未报道过Cu2+的这种抑制作用.     

Polycyclic aromatic hydrocarbon biodegradation and extracellular enzyme secretion in agitated and stationary cultures of Phanerochaete chrysosporium

The extracellular enzyme secretion and biodegradation of polycyclic aromatic hydrocarbons (PAHs) were studied in agitated and shallow stationary liquid cultures of Phanerochaete chrysosporium. Veratryl alcohol and Tween80 were added to cultures as lignin peroxidase (LIP) and manganese peroxidase (MnP) inducer, respectively. Shallow stationary cultures were suitable for the production of enzyme, whereas agitated cultures enhanced overall biodegradation by facilitating interphase mass transfer of PAHs into aqueous phases. The use of a LIP stimulator, veratryl alcohol, did not increase PAH degradation but significantly enhanced LiP activity. In contrast, Tween80 increased both MnP secretion and PAH degradation in shallow stationary cultures. On the other hand, high PAH degradation was observed in agitated cultures in the absence of detectable LIP and MnP activities. The results suggested that extracellular peroxidase activities are not directly related to the PAH degradation, and the increased solubility rather than enzyme activity may be more important in the promotion of PAH degradation.     

黄孢原毛平革菌在多种氨氮浓度下木质素降解酶的产生

在氨氮浓度0．0308-0．924g／L，下对黄孢原毛平革菌(Phanerochaete chrysosporium)在空气环境中进行自由悬浮振荡培养，在氨氮浓度0．0308-0．308g／L下可检测到木质素过氧化物酶活性，最高酶活为42．8U/L；在氨氮浓度0．0308g／L和0．154g/L下可检测到漆酶活性，最高酶活为35．0U／L，在氨氮浓度不低于0．154g/L时，葡萄糖消耗速率大致相当，明显高于在氨氮浓度0．0308g／L下的葡萄糖消耗速率；氨氮在葡萄糖耗尽时达到最低值，然后开始增大；木质素过氧化物酶和漆酶的活性峰与葡萄糖和氨氮的最大消耗基本对应。实验结果对木质素降解酶发酵和白腐真菌在环境工程中的直接应用具有启发意义。     

褐煤降解真菌—青霉菌P6的胞外酶研究

具有强降解褐煤能力的青霉菌株P6在液体培养条件下,可产生较强的过氧化物酶(包括木素过氧化物酶和锰过氧化物酶)活性,并具有酯酶活性,不产生内葡聚糖酶和木聚糖酶.粗酶液依次经80%饱和度的硫酸铵盐析、DEAE-纤维素离子交换树脂层析、Sephadex G-100凝胶过滤,得到一个具有藜芦醇氧化活性的的木素过氧化物酶洗脱峰,藜芦醇氧化活性达5760U/L,比活力达7.52U/mg,纯化倍数150.4倍.     

工程菌及其固定化细胞对有机磷农药的降解

用抗性库蚊酯酶基因,引入原核表达载体pRL439,转化大肠杆菌HB101细胞,获得表达.通过酶切、Southern杂交鉴定重组质粒.研究了重组菌酯酶的活性,重组质粒pRL-B1表达的酯酶具有高酶活并能高效降解酯酶的特异性底物a-乙酸萘酯(a-NA)和β-乙酸萘酯(β-NA);经对重组菌进行细胞固定化后降解有机磷农药对硫磷(1605),反应时间短,降解效率高.     

遗传工程菌Fhhh降解精对苯二甲酸与mnp基因表达

跨界融合构建的遗传工程菌Fhhh及其亲株黄孢显毛平革菌 (PC) ,降解精对苯二甲酸的比降解率受到Mn2 + 、酒石酸铵、H2 O2 、pH共 4因素的影响 .除pH值外 ,其余 3个因素影响 2菌株比降解率大小的排序完全一致 .pH值对PC菌的影响排序处于第 3位 ,对Fhhh则处于第 1位 .Fhhh比降解率比PC高出 11 11% ;mnp基因表达的锰过氧化物酶 (MnP)比活力水平比PC高出 15 2 2 % .降解精对苯二甲酸 4因素优化水平 ,也是mnp基因表达的优化条件 .比降解率与MnP的比活力水平之间有显著或极显著正相关性 (r>r0 .0 5( 4) ,r >r0 .0 1( 4) ) .研究结果为高效处理精对苯二甲酸废水提供了重要的分子生物学依据     

Variation of peroxidase isoenzyme and biofilm of Phanerochaete chrysosporium in continuous membrane bioreactor for Reactive Brilliant Red X3-B treatment

The influence of a Reactive Brilliant Red X-3B (RBR X-3B) dye on the peroxidase isoenzyme of Phanerochaete chrysosporium was determined, and the biofilm structure in a white rot fungal continuous membrane bioreactor (MBR) was also investigated by scanning electron microscope (SEM). The variation of peroxidase isoenzyme and the decolorization rate in the continuous MBR were evaluated. The results showed that the 100 mg/L RBR X-3B could stimulate the production of the peroxidase isoenzyme in the shaking-flask culture. In addition, two new peroxidase isoenzyme bands with relative mobility (Rf) value of 0.27 and 0.28 appeared, but the activity was lower than the blank control of 11 d. In the continuous MBR, the system worked stably during the first 60 d, the main peroxidase isoenzyme bands existed and three new bands with Rf value of 0.10, 0.27, and 0.28 appeared. Meanwhile, the biofilm grew well and the average decolorization rate could reach 90.6%. But the bands of peroxidase isoenzyme decreased rapidly at day 65, only two bands with Rf value 0.24 and 0.26 existed, and the decolorization rate decreased to 78.3%. Therefore, 5 bottles of P. chrysosporium mycelial pellet were added into the MBR, and then the activity of the peroxidase isoenzyme and the decolorization rate had a slight recovery. Finally, the decolorization rate finally decreased to 75.2%. These results contribute to a comprehensive understanding of the variation of peroxidase isoenzyme and biofilm in continuous MBR by white rot fungi.     

与黄孢原毛平革菌协同降解稻草的混合菌筛选

在纤维素筛选培养基中加入黄孢原毛平革菌稻草固态发酵的浸提液,用这种培养基从自然环境中筛选出与黄孢原毛平革菌相容的菌株,在PDA和MEA平板上进行相容性测试,选择出生长稳定,可以与黄孢原毛平革菌较好共存的6株真菌.考察了6株真菌分别与黄孢原毛平革菌混合培养降解稻草时的酶活和对木质纤维素类组分的降解,筛选出3组更优的组合,其混合培养时,对于纤维素酶能产生较好的协同效果,纤维素降解效果较好.对于木质素降解效率的显著提高,可能是由于发酵体系内的胞外酶和一些活性因子的作用.     

Effects of culture conditions on ligninolytic enzymes and protease production by Phanerochaete chrysosporium in air

The production of ligninolytic enzymes and protease by Phanerochaete chrysosporium was investigated under different culture conditions. Different amounts of medium were employed in free and immobilized culture, together with two kinds of medium with different C/N ratios. Little lignin peroxidase （LIP） （〈 2 U/L） was detected in free culture with nitrogen-limited medium （C/N ratio： 56/2.2, in mmol/L）, while manganese peroxidase （MnP） maximum activity was 231 and 240 U/L in 50 and 100 ml medium culture, respectively. Immobilized culture with 50 ml nitrogen-limited medium gave the highest MnP and LiP production with the maximum values of 410 and 721 U/L separately on the day 5; however, flasks containing 100 ml nitrogen-limited medium only produced less MnP with a peak value of 290 U/L. Comparatively, carbon-limited medium （C/N ratio： 28/44, in mmol/L） was adopted in culture but produced little MnP and LiE Medium type had the greatest impact on protease production. Large amount of protease was produced due to glucose limitation. Culture type and medium volume influence protease activity corporately by affecting oxygen supply. The results implied shallow immobilized culture was a possible way to gain high production of ligninolytic enzymes.     

电气石和微生物对水溶液中铅吸附研究

论文探讨了电气石、不同微生物、以及电气石与枯草芽孢杆菌(Baccillus subtilis,简写B.subtilis)联合对Pb2+的吸附效果。研究表明,溶液pH=5时,电气石吸附效率比B.subtilis高7.9％,当溶液pH值升到55时,B.subtilis和电气石对Pb2+的吸附效率均升高,但B.subtili...     

黄孢原毛平革菌降解磷酸三苯酯的性能和机理

以白腐真菌的中的黄孢原毛平革菌（Phanerochaete chrysosporium）为实验菌种，考察不同环境条件因素对P.chrysosporium降解磷酸三苯酯（TPhP）的影响以及TPhP降解过程中菌体细胞特性的变化.结果表明，当孢子液的接种量为4%（V/V），葡萄糖浓度为5g/L，pH值为5~6时，经过6d的处理P.chrysosporium对5mg/L TPhP的降解率可达到60%以上.菌体的细胞色素P450酶在TPhP的降解转化过程中发挥了重要的作用，抑制P450酶的活性会导致TPhP降解率下降.在降解反应的前期，为加快TPhP的代谢转化，菌体胞内蛋白含量以及ATP酶活性出现明显升高.在TPhP胁迫下，菌体SOD和CAT的活性随降解反应的进行呈现先升高后降低的趋势，2种抗氧化酶协同作用维持TPhP降解过程中菌体胞内的氧化还原平衡.     

黄孢原毛平革菌降解磷酸三苯酯的性能和机理

以白腐真菌的中的黄孢原毛平革菌（Phanerochaete chrysosporium）为实验菌种,考察不同环境条件因素对P.chrysosporium降解磷酸三苯酯（TPhP）的影响以及TPhP降解过程中菌体细胞特性的变化.结果表明,当孢子液的接种量为4%（V/V）,葡萄糖浓度为5g/L,pH值为5~6时,经过6d的处理P.chrysosporium对5mg/L TPhP的降解率可达到60%以上.菌体的细胞色素P450酶在TPhP的降解转化过程中发挥了重要的作用,抑制P450酶的活性会导致TPhP降解率下降.在降解反应的前期,为加快TPhP的代谢转化,菌体胞内蛋白含量以及ATP酶活性出现明显升高.在TPhP胁迫下,菌体SOD和CAT的活性随降解反应的进行呈现先升高后降低的趋势,2种抗氧化酶协同作用维持TPhP降解过程中菌体胞内的氧化还原平衡.     

Effect of nitrogen concentration in culture mediums on growth and enzyme production of Phanerochaete chrysosporium

Effect of different nitrogen concentration in the mediums on growth and enzyme production of Phanerochaete chrysosporium was studied when glucose concentration was l0 g/L. The results showed that the medium contained 0.8 g/L ammonium tartrate is the best. It not only supply abundant nutrients for the growth of Phanerochaete chrysospodum, which make mycelia the best grow compared with the other medium, but also produce higher manganese-dependent peroxidase(Mnp) and laccase(Lac) activity. In addition, it is observed that the variation of mycelia surface is related to ligninolytic enzyme secreted by Phanerochaete chrysosporium. When the surface of mycelium pellets appeared burs, it predicts secondary metabolism begin. This experimentation demonstrated that when the ratio of carbon and nitrogen in nitrogen limited medium is equal to 100:8, growth and enzyme production of Phanerochaete chrysosporium is the best, it could achieve the maximum Mnp and Lac activity.     

角蛋白酶产生菌的分离鉴定及其kerC的克隆表达

以四川农业大学养鸡场堆砌废弃羽毛处土壤为样品,筛选出一株具有较强降解羽毛能力的细菌B-3菌株.经形态学、生理生化特性和16S rRNA基因序列分析,鉴定其为枯草芽孢杆菌(Bacillus subtilis),命名为枯草芽孢杆菌B-3.并成功克隆到该菌株的角蛋白酶基因kerC(GenBank No.:JN021789),在大肠杆菌BL21(Escherichia coli BL21)中获得了高效表达.该基因全长1146bp,GC含量46.5%,编码381个氨基酸,与已报道的枯草芽孢杆菌YYW-1的kerC基因(GenBank No.: EU362730)同源性达到100%.重组菌株经IPTG诱导后角蛋白酶酶活力达14.8U/mL,经His-Tag纯化和SDS-PAGE分析表明,重组角蛋白酶分子量约为60kDa(融合了硫氧还蛋白,Trx).重组角蛋白酶最适反应温度和pH值分别为65℃与7.0.     

Cloning and expression of the first gene for biodegrading microcystin LR by Sphingopyxis sp. USTB-05

Harmful cyanobacterial blooms are a growing environmental problem worldwide in natural waters, the biodegradation is found to be the most efficient method for removing microcystins (MCs) produced by harmful cyanobacteria. Based on the isolation of a promising bacterial strain of Sphingopyxis sp. USTB-05 for biodegrading MCs, we for the first time cloned and expressed a gene USTB-05-A (HM245411) that is responsible for the first step in the biodegradation of microcystin LR (MC-LR) in E. coli DH5αup, with a cloning vector of pGEM-T easy and an expression vector of pGEX-4T-1, respectively. The cell-free extracts (CE) of recombinant E. coli DH5αup containing USTB-05-A had high activity for biodegrading MC-LR. The initial MC-LR concentration of 40 mg/L was completely biodegraded within 1 hr in the presence of CE with a protein concentration of 0.35 mg/mL. Based on an analysis of the liquid chromatogram-mass spectrum (LC-MS), the enzyme encoded by gene USTB-05-A was found to be active in cleaving the target peptide bond between 3-amino-9-methoxy-2,6, 8-trimethyl-10-phenyl-deca-4,6-dienoic acid (Adda) and arginine of MC-LR, and converting cyclic MC-LR to linear MC-LR as a first product that is much less toxic than parent MC-LR, which offered direct evidence for the first step on the pathway of MC-LR biodegradation by Sphingopyxis sp. USTB-05.