耐碱性木聚糖酶基因在巨大芽孢杆菌中的表达及其酶学性质

摘要：【目的】从耐碱性木聚糖酶高产短小芽孢杆菌中克隆得到带有自身启动子的木聚糖酶基因,将其在巨大芽孢杆菌中进行表达,并对表达产物进行性质分析。【方法】将克隆得到的木聚糖酶基因xynA以及带有自身启动子序列的结构基因, 构建在芽孢杆菌表达载体pWH1520和改造后的载体pWG03中,得到重组质粒pWTEJX和pWGXYN,分别转化到巨大芽孢杆菌BM70中,获得重组巨大芽孢杆菌BMJXH9和BMGpp12;经过诱导产酶培养,均得到分泌表达。【结论】重组巨大芽孢杆菌BMGpp12比BMJXH9产酶活力提高了三倍     

细菌麦芽糖淀粉酶在枯草芽孢杆菌中的诱导型异源表达

【目的】实现地衣芽孢杆菌麦芽糖淀粉酶在枯草芽孢杆菌中的高效异源表达,并研究该重组酶的酶学性质。【方法】克隆巨大芽孢杆菌木糖异构酶基因的启动子区域及其调控蛋白,构建一个大肠杆菌/芽孢杆菌穿梭型诱导表达质粒,使用该诱导型启动子介导麦芽糖淀粉酶编码基因,实现其在枯草芽孢杆菌中的功能表达。对重组枯草芽孢杆菌的诱导条件进行优化,提高麦芽糖淀粉酶的产量。【结果】获得了诱导表达麦芽糖淀粉酶基因的重组枯草芽孢杆菌菌株。最适诱导温度为45°C,最适诱导剂添加浓度为1%,最适添加诱导剂时间为接种培养9 h后。重组酶蛋白分子量大小为67 k D,对该酶的酶学性质研究发现,以可溶性淀粉为底物,反应生成麦芽糖和葡萄糖,其中麦芽糖含量为60.42%。重组酶最适作用温度为45°C,最适作用p H为6.5,Ca2+、Co2+、EDTA对该重组麦芽糖淀粉酶具有激活作用。【结论】通过木糖诱导表达系统可以实现麦芽糖淀粉酶在枯草芽孢杆菌中的高效诱导型表达,酶活最高可达296.64 U/m L发酵液,在工业上有着较好的应用前景。     

强化底物利用酶系表达,提升地衣芽孢杆菌生产碱性蛋白酶性能

地衣芽孢杆菌2709由于易于培养、GRAS状态和完善的蛋白质分泌能力,是已经投入工业生产碱性蛋白酶的菌株。为改善该菌株的发酵生产性能,提高菌体对培养基成分的利用和碱性蛋白酶产量,对菌株的胞外分泌酶系进行完善。利用同源重组机制,在基因组复制起始位点附近引入了来源于短小芽孢杆菌的木聚糖酶基因xynA和在复制起始位点中心对称的位置引入耶氏解脂酵母来源的脂肪酶基因lipY2。整合菌株在摇瓶发酵44h时,木聚糖酶、脂肪酶酶活力分别达(58±2.07)U/mL和(207±10.62)U/mL,其分泌表达促进了地衣芽孢杆菌对发酵培养基的分解与利用,提高了培养基中还原糖、上清总氮的含量和沉淀中含氮化合物的分解;细菌生物量较地衣芽孢杆菌原始菌株提高了11.76%,同时碱性蛋白酶的发酵周期较原始菌提前了4h,碱性蛋白酶产量提高了14.41%。地衣芽孢杆菌2709分泌酶系的丰富和发酵性能的改善为在饲料行业中作为微生物制剂的地衣芽孢杆菌提供了改造的方法。     

巨大芽孢杆菌β-淀粉酶在枯草芽孢杆菌中诱导表达及碳代谢去阻遏

【背景】β-淀粉酶在食品和医疗领域应用广泛。目前工业上使用的β-淀粉酶主要从植物中提取,生产成本高,限制了β-淀粉酶的应用。微生物生产的β-淀粉酶尽管早有报道,但由于产酶水平低下,因而一直未能实现工业化。【目的】实现巨大芽孢杆菌β-淀粉酶在枯草芽孢杆菌中的高效诱导表达,缓解碳分解代谢物阻遏(Carbon catabolite repression,CCR)对该重组酶表达的影响,并研究其酶学性质。【方法】克隆枯草芽孢杆菌木糖诱导启动子,构建木糖诱导表达载体以介导巨大芽孢杆菌1514的β-淀粉酶编码基因amyM在枯草芽孢杆菌中的异源表达。定点突变位于amyM信号肽编码区的分解代谢物响应元件(Catabolite responsive element,CRE),降低碳源代谢对重组β-淀粉酶施加的阻遏。【结果】构建了诱导表达β-淀粉酶基因的重组枯草芽孢杆菌菌株。同义替换amyM-CRE保守碱基在不同程度上缓解了碳源所施加的CCR效应,重组酶的表达水平得到显著提高。重组酶的分子量为57 kD,水解可溶性淀粉主要生成麦芽糖和少量葡萄糖,其中麦芽糖含量为72%。该酶最适作用温度为50°C,最适反应pH为6.0。Co2+、Ca2+对重组β-淀粉酶具有激活作用。【结论】通过木糖诱导表达系统和碳代谢去阻遏实现了β-淀粉酶在枯草芽孢杆菌中的高效表达,酶活最高可达97.16 U/mL发酵液,比amyM基因来源菌巨大芽孢杆菌1514的β-淀粉酶产量提高了440倍,为β-淀粉酶发酵生产的工业化提供了支撑。     

解淀粉芽孢杆菌β-1,3-1,4-葡聚糖酶的高效表达

目的:克隆解淀粉芽孢杆菌β-1,3-1,4-葡聚糖酶基因(bglA)使其在解淀粉芽孢杆菌CICIM B4081中高效表达,并对重组酶进行酶学性质研究.方法:以解淀粉芽孢杆菌(CICIM B4801)染色体DNA为模板,经过PCR扩增得到了大小约为0.8kb的β-1,3-1,4-葡聚糖酶基因(bglA),构建了重组表达质粒pQ-bglA,通过电转化的方法将其转化人解淀粉芽孢杆菌(CICIM B4801)中.结果:得到了能高效表达β-1,3-1,4-葡聚糖酶的重组解淀粉芽孢杆菌.在250mL摇瓶条件下,重组菌分解地衣多糖的胞外最高酶活达到了1515.7U/mL,重组酶的最适作用温度为55℃,最适反应pH值为6.5.结论:重组菌的β-1,3-1,4-葡聚糖酶的酶活为原始菌株的11.84倍,实现了bglA基因在解淀粉芽孢杆菌中的高效表达.     

Cry1Ac基因载体构建及其在枯草芽孢杆菌中的杀虫活性表达

根据苏云金芽孢杆菌Bacillus thuringiensis HD-73基因Cry1Ac和枯草芽孢杆菌Bacillus subtilis木糖诱导型启动子PxylR序列, 分别设计2对特异引物Cry1Ac F/R和Pxy F/R,扩增获得了完整的启动子PxylR和Cry1Ac基因序列,进一步以上述产物混合物为模板,以Pxy F/Cry1Ac R作引物进行重迭PCR,获得了载体PxylR-Cry1Ac,经SphⅠ和BamHⅠ完全酶切后,将PxylR-Cry1Ac插入大肠杆菌-苏云金芽孢杆菌穿梭载体pHT315,重组表达质粒pCry1Ac315转化枯草芽孢杆菌感受态细胞。工程菌株质粒酶切电泳分析、SDS-PAGE电泳分析和杀虫生物活性测定结果证实了Cry1Ac基因的导入及其在枯草芽孢杆菌JAAS01D中的有效表达。     

枯草芽孢杆菌β-甘露聚糖酶在毕赤酵母中的分泌表达

目的:研制高效分泌表达枯草芽孢杆菌β-甘露聚糖酶的毕赤酵母基因工程菌株。方法与结果:将优化设计的枯草芽孢杆菌MA139β-甘露聚糖酶基因用EcoRⅠ/XbaⅠ双酶切,克隆到诱导型表达载体pPICzαA中α因子信号肽编码序列的下游,转化大肠杆菌筛选重组质粒,转化毕赤酵母X-33感受态细胞,经Zeocin筛选,获得重组表达菌株X-33/mann。将重组菌株在10L全自动发酵罐中进行高密度发酵培养,甲醇诱导72h发酵活力达到2100U/mL。重组甘露聚糖酶的最适催化温度为40℃,最适催化pH值为6.0。结论:枯草芽孢杆菌β-甘露聚糖酶在毕赤酵母中获得了高效分泌表达,具有开发作为饲料添加剂的潜能。     

葡萄糖醛酸木聚糖酶在枯草芽孢杆菌中的表达及发酵条件优化

为了研究葡萄糖醛酸木聚糖酶在枯草芽孢杆菌中异源表达,笔者从枯草芽孢杆菌中克隆得到带有自身信号肽的葡萄糖醛酸木聚糖酶基因,将其构建到大肠杆菌-枯草芽孢杆菌穿梭质粒中,转化入枯草芽孢杆菌WB800,得到重组菌。通过发酵条件以及培养基成分优化,重组菌中葡萄糖醛酸木聚糖酶酶活达到76.0 U/mL,约为优化前产酶量的5.4倍。葡萄糖醛酸木聚糖酶在枯草芽孢杆菌中实现高效异源表达,为其进一步的实际应用奠定了基础。     

巨大芽孢杆菌青霉素G酰化酶基因在枯草杆菌中的高表达

用ＰＣＲ方法从巨大芽孢杆菌的基因组ＤＮＡ中扩增到青霉素Ｇ酰化酶基因,并装载到枯草杆菌质粒ｐＰＺＷ１０３中,将其转化到枯草杆菌ＤＢ１０４中进行了分泌表达,重组菌株产酶无需苯乙酸诱导。在３７℃培养２４ｈ,菌液酶活力可达６ｕ／ｍｌ。１０天的连续传代实验表明重组菌株的稳定性很高。     

链霉菌Streptomyces olivaceoviridis A1 木聚糖酶基因xynA在大肠杆菌及毕赤酵母中的高效表达

从橄榄绿链霉菌StreptomycesolivaceoviridisA1中克隆出木聚糖酶基因xynA ,将带与不带原基因信号肽编码序列的xynA分别以正确的阅读框架克隆到大肠杆菌表达载体pET 2 2b( )上的pellB信号肽编码序列之后 ,得到 2种构建的重组载体 ,在重组大肠杆菌中木聚糖酶得到了表达 ,表达产物具有生物活性。进一步将不带原基因信号肽编码序列的xynA插入到毕赤酵母转移载体pPIC9中 ,转化毕赤酵母得到重组子 ,在重组子中木聚糖酶基因得到了高效分泌表达 ,在摇床培养水平上的表达量达到 2 0 0mg L ,且表达产物具有生物学活性。     

外源木聚糖酶在枯草芽胞杆菌中信号肽筛选

[目的]本试验旨在筛选引导表达外源木聚糖酶基因高效分泌的信号肽,为枯草芽胞杆菌木聚糖酶高效分泌表达系统提供元件.[方法]构建信号肽筛选载体,载体是以含壮观霉素抗性基因的大肠-枯草穿梭载体为基本骨架,目标蛋白为耐碱性木聚糖酶,可在麦芽糖启动子Pglv诱导下表达.从枯草芽胞杆菌A1747基因组中扩增获得24个Sec途径信号肽,并将其全部链接到至筛选载体上,并在枯草芽胞杆菌WB700中实现表达分泌.重组菌在3%麦芽糖诱导下培养24h后用DNS法测定上清酶活.[结果]成功构建信号肽筛选载体pGPSX及24个表达载体,实现木聚糖酶表达分泌.且不同信号肽对于引导外源木聚糖酶分泌能力不同,其中YnfF信号肽引导分泌目标蛋白效率最高,上清酶活为37.2IU/mL.[结论]试验证明在枯草杆菌中对外源蛋白进行信号肽筛选是提高其分泌的有效途径,并获得了针对木聚糖酶高效分泌信号肽YnfF.     

Heterologous expression of the Bacillus pumilus endo-beta-xylanase (xynA) gene in the yeast Saccharomyces cerevisiae

The endo-beta-xylanase-encoding gene (xynA) of Bacillus pumilus PLS was isolated from a genomic DNA library and the open reading frame (ORF) was inserted in expression vectors for the yeast Saccharomyces cerevisiae. Plasmid pFN3 harboured the xynA ORF fused to the yeast mating pheromone alpha-factor signal sequence (MFalpha1s) under the control of the alcohol dehydrogenase II gene promotor (ADH2P) and terminator (ADH2T) sequences. In plasmid pFN4, the MFalpha1S-xynA ORF was brought under the control of the phosphoglycerate kinase I gene promotor (PGK1p) and terminator (PGK1T) sequences. Autoselective, recombinant S. cerevisiae [fur1::LEU2] strains bearing pFN3 or pFN4 secreted functional endo-beta-xylanase when grown in complex medium. Enzymatic activities in the culture supernatants reached maximum levels of 8.5 nkat/ml and 4.5 nkat/ml, respectively. The temperature and pH optimum for both the bacterial and the recombinant xylanase were 58 degrees C and pH 6.2.     

米根霉糖化酶、类芽孢杆菌木聚糖酶融合蛋白的真核分泌表达

以米根霉(Rhizopus oryzae)3.866基因组DNA为模板,克隆得到糖化酶基因(glucoamylase gene, amyA),基因全长2 049 bp,编码604个氨基酸;以类芽孢杆菌(Paenibacillus sp.)H10-3基因组DNA为模板,克隆出基因木聚糖酶基因(xylanase A gene, xynA)的成熟肽编码序列,长636 bp,编码211个氨基酸。通过重叠延伸PCR(SOE-PCR)得到拼接片段amyA-l-xynA,并将其克隆到毕赤酵母表达载体pPIC9中,得到重组质粒pPIC9-amyA-l-xynA,重组质粒线性化后经电击转化到毕赤酵母(Pichia pastoris)GS115中,得到了表达成功的工程菌AX11。在AX11发酵上清液中同时检测到糖化酶活性(5.8 U/mL)和木聚糖酶活性(32.3 U/mL)。     

Cloning, sequencing, and expression of a xylanase gene from the anaerobic ruminal bacterium Butyrivibrio fibrisolvens.

A gene coding for xylanase activity, xynA, from the anaerobic ruminal bacterium Butyrivibrio fibrisolvens 49 was cloned into Escherichia coli JM83 by using plasmid pUC19. The gene was located on a 2.3-kilobase (kb) DNA insert composed of two adjacent EcoRI fragments of 1.65 and 0.65 kb. Expression of xylanase activity required parts of both EcoRI segments. In E. coli, the cloned xylanase enzyme was not secreted and remained cell associated. The enzyme exhibited no arabinosidase, cellulase, alpha-glucosidase, or xylosidase activity. The isoelectric point of the cloned protein was approximately 9.8, and optimal xylanase activity was obtained at pH 5.4. The nucleotide sequence of the 1,535-base-pair EcoRV-EcoRI segment from the B. fibrisolvens chromosome that included the xynA gene was determined. An open reading frame was found that encoded a 411-amino-acid-residue polypeptide of 46,664 daltons. A putative ribosome-binding site, promoter, and leader sequence were identified. Comparison of the XynA protein sequence with that of the XynA protein from alkalophilic Bacillus sp. strain C-125 revealed considerable homology, with 37% identical residues or conservative changes. The presence of the cloned xylanase gene in other strains of Butyrivibrio was examined by Southern hybridization. The cloned xylanase gene hybridized strongly to chromosomal sequences in only two of five closely related strains.     

Cloning, sequence analysis, and expression of genes encoding xylan-degrading enzymes from the thermophile "Caldocellum saccharolyticum"

A lambda recombinant bacteriophage coding for xylanase and beta-xylosidase activity has been isolated from a genomic library of the extremely thermophilic anaerobe "Caldocellum saccharolyticum." Partial Sau3AI fragments of the lambda recombinant DNA were ligated into pBR322. A recombinant plasmid with an insertion of ca. 7 kilobases of thermophilic DNA expressing both enzymatic activities was isolated. The location of the genes has been established by analyzing deletion derivatives, and the DNA sequence of 6.067 kilobases of the insert has been determined. Five open reading frames (ORFs) were found, one of which (ORF1; Mr 40,455) appears to code for a xylanase (XynA) which also acts on o-nitrophenyl-beta-D-xylopyranoside. Another, ORF5 (Mr 56,365), codes for a beta-xylosidase (XynB). The xynA gene product shows significant homology with the xylanases from the alkalophilic Bacillus sp. strain C125 and Clostridium thermocellum.     

The xynC gene from Fibrobacter succinogenes S85 codes for a xylanase with two similar catalytic domains.

The xynC gene of Fibrobacter succinogenes S85 codes for a 66.4-kDa xylanase which consists of three distinct domains separated by two flexible regions rich in serine residues. Domains A and B of XynC code for catalytic domains with 56.5% identity and 9.6% similarity with each other, and both domains share homology with xylanases of Ruminococcus flavefaciens, Neocallimastix patriciarum, Clostridium acetobutylicum, Bacillus pumilus, Bacillus subtilis, and Bacillus circulans. More than 88% of the xylanase activity of Escherichia coli cells carrying the original 13-kb recombinant plasmid was released from intact cells by cold water washes. The major products of hydrolysis of xylan by both domains were xylose and xylobiose, indicating that the xynC gene product exhibits catalytic properties similar to those of the XynA xylanases from R. flavefaciens and N. patriciarum. So far, these features are not shared broadly with bacteria from other environments and may indicate specific selection for this domain structure in the highly competitive environment of the rumen.