一个推测的拟南芥漆酶基因在巴斯德毕赤酵母中的表达

At5g01040基因是一个推测的拟南芥漆酶基因。根据其编码序列设计引物,利用RT—PCR方法扩增出1755bp的片段。测序结果表明,该片段存在3个突变位点,其中一个突变位点改变了所编码的氨基酸。将该片段克隆到表达载体pPICZaB上,电击转化毕赤酵母。经筛选获得80个候选重组菌株,其中18个菌株的培养液中存在漆酶活性,说明所克隆的基因在毕赤酵母中实现了分泌表达,证实了At5g01040编码的蛋白具有漆酶活性。     

信号肽序列对毕赤酵母表达外源蛋白质的影响

乙醇氧化酶启动子被分离、克隆 ,并建立了转化方法后 ,毕赤酵母已被发展成为一种高效的外源蛋白表达宿主。为了进一步提高外源蛋白质的分泌表达 ,对信号肽序列进行了研究。首先按毕赤酵母的偏爱密码合成了酿酒酵母的α因子信号肽序列MF4I,随后在MF4I信号肽序列的N端分别引入 1～ 10个毕赤酵母Aox1蛋白质的N端氨基酸 ,构成 10种不同的分泌信号肽序列 ,10种不同的分泌信号肽序列被用于植酸酶基因的毕赤酵母分泌表达。以上新的信号肽序列都可使植酸酶的分泌表达量增加 ,而以N端增加A、I、P三个氨基酸的信号肽序列引起的提高最大 ;和野生型的酿酒酵母α因子信号肽序列相比 ,使植酸酶分泌表达量增加 5倍 ,摇瓶中植酸酶的分泌表达量为 90mg/L。此外在MF4I信号肽的引导序列和内切蛋白酶间增加了EEAEAEAEP和K共 10个氨基酸 ,进一步提高信号肽的分泌效率 ,使表达又提高约 35 % ,使得摇瓶中酸性植酸酶的表达量达到 12 0mg/L ,是pPCI9K表达量的 8倍。     

平菇漆酶基因在毕赤酵母中的分泌表达及酶学性质研究

采用RTPCR技术克隆到一个平菇(Pleurotusostreatus)漆酶基因的全长cDNA,命名为lccPo1,其序列提交GenBank,登录号为AY450404。将其ORF克隆到毕赤酵母表达载体pHBM906,转化3株毕赤酵母GS115、KM71和SMD1168,该漆酶基因在3种毕赤酵母菌株中均实现了分泌表达。3种摇瓶培养条件①25℃,1.0%(VV)甲醇;②20℃,1.0%(VV)甲醇;③20℃,0.5%(VV)甲醇,进行比较研究后发现适当提高甲醇浓度有利于漆酶在低温条件下表达,而降低培养温度到20℃则可以提高漆酶的产量2～6倍。3株重组毕赤酵母在其最适反应条件下测得三者粗酶液最高漆酶酶活分别为3.19UmL[GS115(pHBM565)]、2.56UmL[KM71(pHBM565)]和2.49UmL[SMD1168(pHBM565)]。对重组酶进行相关的酶学性质分析表明,三者的最适反应pH值约为4.2,最适反应温度约为60℃。重组毕赤酵母GS115(pHBM565)所产酶的热稳定性稍好,在pH稳定性方面三者没有太大差异。     

分子伴侣及信号肽对毕赤酵母中分泌蛋白表达水平的影响

目的：探索定位于细胞质、内质网膜及内质网腔中的分子伴侣及其组合对于带有不同信号肽的胞外β-1,3-葡聚糖酶（EXGl）在巴斯德毕赤酵母GS200中表达水平的影响。方法：通过融合PCR技术分别构建带有酵母a交配因子引导肽序列（仅MF）、酵母仅交配因子信号肽序列（ccPre）和重链结合蛋白（Bip）信号肽序列的报告蛋白EXGl的表达质粒pPIC9-EXG1,同时构建分子伴侣基因及其组合的表达质粒pBLArg-IV,然后将2种重组质粒共转化至毕赤酵母宿主菌GS200,转化子经筛选获得共表达菌株,通过测定EXG1酶活来评价分子伴侣与信号肽对其表达水平的影响。结果：细胞质及内质网膜上的分子伴侣Sec61a、Sec61B及胞质中的分子伴侣Ydjl、Ssal、Hsp104及其组合对各种信号肽引导的报告蛋白EXG1的表达水平没有显著影响。然而,内质网腔中的分子伴侣Bip、EroI、PDI与HacI组合能显著提高报告蛋白EXG1的表达水平,其中,以aMF或ctPre作为信号肽引导的报告蛋白EXG1的表达水平分别提高了2．6倍和3．8倍,以Bip信号肽引导的报告蛋白EXGl的表达水平提高了20％～45％,而对于以EXG1自身信号肽引导的报告蛋白EXG1的表达水平没有显著影响。结论：在酵母表达体系中,内质网腔中的分子伴侣是报告蛋白EXG1表达水平的重要影响因素．但分子伴侣对于信号肽的选择性还须进一步证明。     

不同信号肽对胞外β-(1,3)-葡聚糖酶在巴斯德毕赤酵母中表达的影响

目的:在胞外β-(1,3)-葡聚糖酶成熟肽的N端添加不同类型的信号肽,研究不同信号肽对其在巴斯德毕赤酵母中表达水平的影响。方法:通过融合PCR方法将α成熟交配因子(MFα)、成熟交配因子Pre肽(αPre)和共翻译转运信号肽(Bip信号肽)等3种信号肽的DNA片段连接至胞外β-(1,3)-葡聚糖酶成熟肽基因的5′端,利用PCR扩增包含其自身信号肽的胞外β-(1,3)-葡聚糖酶基因,将上述4种基因片段分别插入pPIC9质粒,再转化巴斯德毕赤酵母GS115宿主菌并诱导表达;测定胞外β-(1,3)-葡聚糖酶的活性,检测其表达水平。结果:目前在毕赤酵母中已广泛使用的MFα信号肽介导的胞外β-(1,3)-葡聚糖酶表达水平最高,其次是αPre,Bip信号肽介导的该酶表达水平是酶自身信号肽介导的表达水平的2倍。结论:共转运信号肽能够提高胞外β-(1,3)-葡聚糖酶的表达水平。     

栓菌漆酶在毕赤酵母中高效表达及重组酶的性质

栓菌420（Trametes sp. 420）漆酶基因lacD以两种方式在巴斯德毕赤酵母（Pichia pastoris）进行异源表达,产生两种重组漆酶：rLacDx（具有天然N-末端）和rLacDe（N-末端带有8个额外的氨基酸残基）。摇瓶发酵18d,rLacDx和rLacDe的产量分别为1.21×10⁵u/L、7.38×10⁴u/L ［以2,2′-连氮-3-乙苯-二噻唑-6磺酸（ABTS）为底物］。在高密度发酵条件下,rLacDx的产量增加到2.39×10⁵u/L,同时其生产周期降至7.5 d。两种重组酶对愈创木酚底物的氧化特性相似,且在50℃和pH3～10的范围内均稳定。然而,rLacDx对底物ABTS的比活力（1761u/mg）高于rLacDe （1122u/mg）,其表观K_m值(427μmol/L)低于rLacDe (604μmol/L)。     

栓菌漆酶在毕赤酵母中高效表达及重组酶的性质

栓菌420(Trametes sp.420)漆酶基因lacD以两种方式在巴斯德毕赤酵母(Pichia pastoris)进行异源表达,产生两种重组漆酶:rLacDx(具有天然N-末端)和rLacDe(N-末端带有8个额外的氨基酸残基)。摇瓶发酵18d,rLacDx和rLacDe的产量分别为1.21×105u/L、7.38×104u/L[以2,2′-连氮-3-乙苯-二噻唑-6磺酸(ABTS)为底物]。在高密度发酵条件下,rLacDx的产量增加到2.39×105u/L,同时其生产周期降至7.5d。两种重组酶对愈创木酚底物的氧化特性相似,且在50℃和pH3~10的范围内均稳定。然而,rLacDx对底物ABTS的比活力(1761u/mg)高于rLacDe(1122u/mg),其表观Km值(427μmol/L)低于rLacDe(604μmol/L)。     

金针菇漆酶基因的克隆及其在毕赤酵母中的表达研究

综合运用cDNA末端快速扩增 (RapidAmplificationofcDNAEnds ,RACE )和基因组步行等技术克隆到一个金针菇 (Flammulinavelutipes)的漆酶结构基因和其对应的全长cDNA ,经测序和BLAST比对分析表明该基因属于多铜氧化酶基因家族 ,与已发表的漆酶基因 (AF176 2 30 )的同源性最高 ,在氨基酸水平为 72 %。该结构基因命名为gl ccFv,cDNA命名为lccFv ,其序列提交GenBank ,登录号分别为AY4 85 82 6和AY4 5 0 4 0 6。将lccFv的开放阅读框克隆到毕赤酵母表达载体pHBM90 6 ,转化毕赤酵母GS115且实现了分泌表达。将重组毕赤酵母GS115 (pHBM5 6 5 )诱导产酶 ,在培养温度 2 0℃、甲醇流加量为 1 0 % (V V)的情况下 ,其分泌表达的LCCFv的最高酶活为 0 10 70U mL ,最适反应温度为 4 5℃ ,最适反应pH值为 3 9,在最适反应条件下其热稳定性和pH值稳定性均较好     

重组人肝素酶在毕赤酵母中的表达

目的:建立肝素酶表达系统,大量制备人肝素酶,用于肝素酶的深入研究,及其抑制剂筛选模型的建立。方法:采用RT-PCR方法从肝癌细胞HepG2中克隆肝素酶全长cDNA,转入毕赤酵母表达体系,经甲醇诱导表达。结果:四唑蓝活性检测结果表明,表达产物具有肝素酶活性;Western印迹证实表达产物可被肝素酶抗体识别。结论:表达产物中含具有肝素酶活性的重组人肝素酶。     

大豆过氧化物酶在毕赤酵母中功能表达

【目的】大豆过氧化物酶(SBP)作用底物广泛、比活高、热稳定性好,使其在免疫检测、工业污染废水处理领域有着广泛的应用潜力。现有的生产方法主要是从大豆壳中提取,这种方法产量低,成本高,远不能满足于工业应用要求,本研究希望实现在毕赤酵母中高效表达有功能活性的大豆过氧化物酶。【方法】将大豆过氧化物酶基因以及C末端截短20个氨基酸的基因克隆pPIC-9K载体中,并在毕赤酵母X-33中诱导表达。同时还将糖基化位点的天冬酰胺突变成为谷氨酰胺,研究糖基化位点对表达的影响。【结果】全长SBP在毕赤酵母中表达是无活性的,只有截短的SBP△20在试管发酵的表达活力达23.5 U/mL,经过糖基化位点的突变表明130、144、185、197对酶活非常重要,不能突变;211和216位点去糖基化突变对酶活有所提高。【结论】经过发酵条件的优化,在5 L的发酵罐中发酵液上清最高酶活力达510 U/mL,是目前报道的最高水平。     

Fermentation strategies for improved heterologous expression of laccase in Pichia pastoris

Improved expression of recombinant laccase by Pichia pastoris carrying the lcc1 cDNA isolated from Trametes versicolor was achieved by optimization of the cultivation conditions in a fermentor equipped with a methanol sensor system. The results indicated that the activity obtained in fermentor cultivations was at least 7 times higher than in shake-flask cultures. Three different strategies for fermentor cultivations were compared: A (30 degrees C, 1.0% methanol), B (20 degrees C, 1.0% methanol), and C (20 degrees C, 0.5% methanol). The laccase activity, particularly the specific activity, could be improved by decreasing the cultivation temperature. The mechanisms behind the temperature effect on the laccase activity may be ascribed to poor stability, release of more proteases from dead cells, and folding problems at higher temperature. The results showed that the methanol concentration had a marked effect on the production of active heterologous laccase. A fivefold higher volumetric laccase activity was obtained when the methanol concentration was kept at 0.5% instead of 1.0%. The detrimental effect of methanol on the production of recombinant laccase may be attributed to lower laccase stability, a higher proteolytic activity, and folding problems due to higher growth rate at 1.0% methanol.     

Optimisation of the expression of a Trametes versicolor laccase gene in Pichia pastoris

A cDNA encoding a laccase enzyme was isolated from a Trametes versicolor cDNA library. The gene was subcloned into the Pichia pastoris expression vector pPIC3.5 and transformed into the P. pastoris strains KM71 and GS115. Laccase-secreting transformants were selected by their ability to oxidise the substrate ABTS. No difference in laccase activity was observed between culture supernatants from GS115 (proteolytic) and KM71 (nonproteolytic) strains. The presence of at least 200 μM copper was necessary for optimal laccase activity in the culture supernatants. During growth of P. pastoris on minimal medium the pH of the medium was reduced to <3.0. If alanine was added to the medium the pH reduction was not as pronounced and at alanine concentrations >0.6% w/v the pH was kept constant for >7 days. Cultures in which the pH was maintained by alanine metabolism produced higher levels of laccase activity than those grown in the absence of alanine. This study describes the development of a medium that allows convenient pH control of P. pastoris without the need for continuous neutralisation. Journal of Industrial Microbiology & Biotechnology (2002) 29, 55–59 doi:10.1038/sj.jim.7000268 Received 08 August 2001/ Accepted in revised form 18 April 2002     

Endogenous signal peptides efficiently mediate the secretion of recombinant proteins in Pichia pastoris

By predicting the potential signal peptides from proteins that are naturally secreted by Pichia pastoris, we identified three possible endogenous signal peptides: Scw, Dse and Exg. We compared their capability to mediate the secretion of enhanced green fluorescent protein (EGFP) and Candida antarctica lipase B (CALB) with that of the Saccharomyces cerevisiae α-factor prepro-signal. EGFP entered the secretory pathway of P. pastoris and was efficiently secreted into the culture medium by all three endogenous peptides. Further, these three putative endogenous signal peptides were also effective in secreting CALB. These endogenous signal peptides thus have the potential to mediate the efficient secretion of heterologous proteins in P. pastoris.     

Electrochemical studies of a truncated laccase produced in Pichia pastoris

The cDNA that encodes an isoform of laccase from Trametes versicolor (LCCI), as well as a truncated version (LCCIa), was subcloned and expressed by using the yeast Pichia pastoris as the heterologous host. The amino acid sequence of LCCIa is identical to that of LCCI except that the final 11 amino acids at the C terminus of LCCI are replaced with a single cysteine residue. This modification was introduced for the purpose of improving the kinetics of electron transfer between an electrode and the copper-containing active site of laccase. The two laccases (LCCI and LCCIa) are compared in terms of their relative activity with two substrates that have different redox potentials. Results from electrochemical studies on solutions containing LCCI and LCCIa indicate that the redox potential of the active site of LCCIa is shifted to more negative values (411 mV versus normal hydrogen electrode voltage) than that found in other fungal laccases. In addition, replacing the 11 codons at the C terminus of the laccase gene with a single cysteine codon (i.e., LCCI-->LCCIa) influences the rate of heterogeneous electron transfer between an electrode and the copper-containing active site (k(het) for LCCIa = 1.3 x 10(-4) cm s(-1)). These results demonstrate for the first time that the rate of electron transfer between an oxidoreductase and an electrode can be enhanced by changes to the primary structure of a protein via site-directed mutagenesis.     

Recombinant protein expression in Pichia pastoris

The methylotrophic yeast Pichia pastoris is now one of the standard tools used in molecular biology for the generation of recombinant protein. P. pastoris has demonstrated its most powerful success as a large-scale (fermentation) recombinant protein production tool. What began more than 20 years ago as a program to convert abundant methanol to a protein source for animal feed has been developed into what is today two important biological tools: a model eukaryote used in cell biology research and a recombinant protein production system. To date well over 200 heterologous proteins have been expressed in P. pastoris. Significant advances in the development of new strains and vectors, improved techniques, and the commercial availability of these tools coupled with a better understanding of the biology of Pichia species have led to this microbe's value and power in commercial and research labs alike.     

巴斯德毕赤酵母表达系统研究进展

巴斯德毕赤酵母表达系统现在已经发展成为一种高效的外源蛋白基因优秀表达系统,该系统具有高表达、高稳定、高分泌、容易放大和成本低等优点,目前已有多种外源蛋白基因在该系统中实现高效表达,对巴斯德毕赤酵母表达系统的进一步研究将会促进其大规模的工业化应用。     

Improving the expression of mini-proinsulin in Pichia pastoris

Increased expression of recombinant mini-proinsulin in Pichia pastoris in 2.5 l bioreactors was achieved by increasing the cultivation pH from 5.1 to 6.3, by decreasing the temperature from 28 to 22 degrees C, and by periodical addition of ammonium sulfate and EDTA to the culture broth. Using this procedure, mini-proinsulin reached nearly 0.3 g l(-1) in the culture supernatant after 160 h of growth.     

Molecular cloning of the cDNA encoding laccase from Pycnoporus cinnabarinus I-937 and expression in Pichia pastoris.

Laccases are multicopper-containing enzymes which catalyse the oxidation of phenolic and nonphenolic compounds with the concomitant reduction of molecular oxygen. In this study, a full-length cDNA coding for laccase (lac1) from Pycnoporus cinnabarinus I-937 was isolated and characterized. The corresponding open reading frame is 1557 nucleotides long and encodes a protein of 518 amino acids. The cDNA encodes a precursor protein containing a 21 amino-acid signal sequence corresponding to a putative signal peptide. The deduced amino-acid sequence of the encoded protein was similar to that of other laccase proteins, with the residues involved in copper coordination sharing the greatest extent of similarity. The cDNA encoding for laccase was placed under the control of the alcohol oxidase (Aox 1) promoter and expressed in the methylotropic yeast Pichia pastoris. The laccase leader peptide, as well as the Saccharomyces cerevisiae alpha-factor signal peptide, efficiently directed the secretion into the culture medium of laccase in an active form. Moreover, the laccase activity was directly detected in plates. The identity of the recombinant product was further confirmed by protein immunoblotting. The expected molecular mass of the mature protein is 81 kDa. However, the apparent molecular mass of the recombinant protein is 110 k Da, thus suggesting that the protein expressed in P. pastoris may be hyperglycosylated.     

Purification and characterization of a laccase from Coprinopsis cinerea in Pichia pastoris

A modified laccase gene, CcLCC6, from Coprinopsis cinerea was chemically synthesized according to the yeast codon bias and expressed in Pichia pastoris. The main properties of laccase, effects of ions and inhibitors, and optimal condition for decolouring malachite green (MG) were investigated in this study. The optimal pH level and temperature of laccase are 3.0 and 40 °C, respectively. The metal ions Mn²⁺, Zn²⁺, Fe³⁺ and Al³⁺ could inhibit laccase activity, as well as 1 mM of sodium dodecyl sulphate and sodium thiosulphate. 2,2′-Azino-bis(3-ethylbenzothiazoline-6-sulfonic acid), as a mediator, was necessary in decolorizing MG. The optimal pH and temperature for MG decolorization were 3.0 and 50 °C, respectively. Approximately 0.02 μM recombinant laccase could effectively decolour 0.05 mM of MG in 1 h. CcLCC6I could inhibit the toxicity of MG to P. pastoris. This is the first report on the successful expression in P. pastoris of CcLCC6I and its enzymatic property. Laccase can also be considered as a candidate for treating industrial effluent containing MG.