共查询到19条相似文献,搜索用时 125 毫秒
1.
【目的】在毕赤酵母中表达特异腐质霉Humicola insolens的中性内切葡聚糖酶Ⅱ,并对其性质加以研究。【方法】利用RT-PCR的方法,以特异腐质霉(Humicola insolens)NC3总RNA为模板,克隆到中性内切葡聚糖酶Ⅱ基因(egⅡ)的cDNA。将其插入表达载体pPIC9K,重组质粒经线性化后电击转化毕赤酵母(Pichia pastoris)菌株GS115。【结果】SDS-PAGE和酶活的检测结果均表明:egⅡ基因在毕赤酵母中成功表达。重组酶的部分酶学性质研究表明,该酶的最适反应温度为70°C,且在65°C以下具有较好的热稳定性。最适反应pH为6.5,在pH 6.0?7.0之间有较好的稳定性。【结论】用重组毕赤酵母可高效表达外源中性内切葡聚糖酶,为其今后在工业应用奠定了基础。 相似文献
2.
3.
[目的]在毕赤酵母中表达特异腐质霉Humicola insolens的中性内切葡聚糖酶Ⅱ,并对其性质加以研究.[方法]利用RT-PCR的方法,以特异腐质霉(Humicola insolens)NC3总RNA为模板,克隆到中性内切葡聚糖酶Ⅱ基因(egⅡ的cDNA.将其插入表达载体pPIC9K,重组质粒经线性化后电击转化毕赤酵母(Pichia pastoris)菌株GS115.[结果]SDS-PAGE和酶活的检测结果均表明:egⅡ基因在毕赤酵母中成功表达.重组酶的部分酶学性质研究表明,该酶的最适反应温度为70℃,且在65℃以下具有较好的热稳定性.最适反应pH为6.5,在pH 6.0-7.0之间有较好的稳定性.[结论]用重组毕赤酵母可高效表达外源中性内切葡聚糖酶,为其今后在工业应用奠定了基础. 相似文献
4.
内切葡聚糖酶 (EG) 是纤维素酶的重要组分,在纤维素降解酶系中发辉重要作用。由于天然微生物来源的内切葡聚糖酶产量低,极大地制约了其生产和应用,所以对内切葡聚糖酶进行高效异源表达是解决这一问题的有效途径。为了获得高效内切葡聚糖酶酿酒酵母工程菌,本研究从纤维梭菌中克隆了内切葡聚糖酶 (EG) 基因,全长1 996 bp,编码440个氨基酸,并与来源于酿酒酵母的PGK启动子序列、来源于pPIC9K质粒的α-信号肽序列以及来源于pSH65质粒的CYC1终止子序列通过重叠延伸PCR法构建完整表达盒 (PαEGC),通过整合rDNA的方法构建内切葡聚糖酶酿酒酵母的表达载体,在酿酒酵母中进行内切葡聚糖酶的随机多拷贝表达。利用微滴数字PCR鉴定内切葡聚糖酶拷贝数,并探索拷贝数与蛋白表达量之间的关系。通过rDNA整合法获得了拷贝数为1、3、4、7、9、11、15、16、19、21、22、23的内切葡聚糖酶酿酒酵母工程菌,结果表明当拷贝数为15时,酶活性最高,为351 U/mL。本研究成功构建了内切葡聚糖酶酿酒酵母工程菌,为其他工业酶异源高效表达提供参考和借鉴。 相似文献
5.
中性内切型纤维素酶在毕赤酵母中高水平表达的研究 总被引:12,自引:0,他引:12
中性内切型纤维素酶在纺织及造纸工业具有重要的应用,为了进一步提高从我国草菇中克隆的一种新的中性内切型纤维素酶(EG1)在Pichiapastoris中的表达水平,我们进行了提高基因拷贝数及高密度发酵等多种手段实现其高水平表达的研究。在前期研究的基础上,利用对已整合eg1的重组子再转化的方法,从含有2000μgLZeocin的YPDSZ平板上筛选到高抗Zeocin转化子,在摇瓶培养条件下,该转化子表达量比原来提高了3.8倍,在pH4~8条件下均有稳定表达,接种量(OD600=5.0)表达水平最好,提高甲醇的诱导浓度对表达有显著的促进作用。用3.2L发酵罐进行了高密度发酵,甲醇诱导95.5h后达到最高值,比摇瓶培养再提高了6.4倍,因此利用高抗Zeocin转化子及高密度发酵的手段,使EG1的表达水平提高了34倍,蛋白表达量达8.80mgmL,EG1酶活达到543.36IUmL,实现了中性内切纤维素酶的高水平表达,本研究将大大促进建立我国纺织用纤维素酶大规模高效生产技术。 相似文献
6.
内切葡聚糖酶基因在大肠杆菌与毕赤酵母中的表达 总被引:4,自引:1,他引:4
根据绿色木霉(Trichoderma viride)WL 0422菌株内切葡聚糖酶基因egⅡ的cDNA序列,设计特异引物,以重组质粒pTG19-T-egⅡ为模板,扩增得到全长1 194bp的egⅡ成熟肽cDNA片段.将该片段分别克隆到大肠杆菌(Escherichia coil)表达载体pET-28a( )和毕赤酵母(Pichia pastoris)表达载体pPIC9K中,并在大肠杆菌Rosset(DE3)和毕赤酵母GS115中进行了表达.重组大肠杆菌表达蛋白占菌体总蛋白的15%,表达产物无内切葡聚糖酶活性.重组毕赤酵母经甲醇诱导实现了分泌表达,在摇床水平上酶活性达到2 788U/ml.酶学性质分析表明,该酶作用的最适pH为4.5,pH 3.5~6.0范围内酶活性保留在80%以上;最适温度为50℃,55℃以下酶的稳定性在90%以上. 相似文献
7.
纤维素酶基因在毕赤酵母中的拷贝数对其表达的影响 总被引:1,自引:0,他引:1
将PCR扩增得到的瑞氏木霉纤维素内切酶Ⅲ(Endo--β1,4-glucanaseⅢ,EGⅢ)基因片段插入巴斯德毕赤酵母(Pichia pastoris)质粒pPIC9K中,构建了EGⅢ的分泌表达质粒pPIC9K-eg3,然后经线性化后电转化导入P.pastorisGS115受体菌中。获得的阳性克隆经SDS-PAGE和酶活检测,证明工程菌株发酵上清液中含有表达的EGⅢ蛋白并具有纤维素内切酶酶活。通过荧光定量PCR确定了各菌株的拷贝数并对不同拷贝数范围的菌体生长和EGⅢ的表达做了比较。实验结果表明,低拷贝重组菌有着相对较好的EGⅢ表达量。 相似文献
8.
9.
从拟康氏木霉3.3002基因组中克隆了内切葡聚糖酶EGI基因,该基因全长1566 bp,由3个外显子2个内含子组成,编码461个氨基酸.编码蛋白EGI的N端为22aa组成的信号肽,其后依次为催化结构域、连接肽和结合结构域.采用重叠PCR法获得无内含子的内切葡聚糖酶基因eg1,并将其成熟肽编码序列插入酿酒酵母分泌型表达载体pYEα中,构建成pYEα-Peg1重组质粒,转化酿酒酵母.重组转化子经β-半乳糖诱导,检测表达产物的分子大小以及酶活,结果表明,转化子在刚果红平板上可产生明显的水解圈;酶活检测显示该基因能在酿酒酵母中表达有生物活性的EG I并分泌到胞外;SDS-PAGE电泳显示EGI蛋白分子量比预期目的蛋白稍偏大. 相似文献
10.
里氏木霉内切-β-葡聚糖酶Ⅱ基因在毕赤酵母中的表达及酶学性质研究 总被引:12,自引:0,他引:12
采用外显子拼接的方法,以里氏木霉Trichoderma reesei基因组 DNA 为模板,克隆出内切-1,4-β-D-葡聚糖酶II基因egl2的全编码序列,将其插入巴斯德毕赤酵母Pichia pastoris表达载体pPIC9K中,并位于α-因子信号肽序列的下游,获得重组质粒pQY2025。重组质粒线性化后用电穿孔法导入毕赤酵母Pichia pastoris菌株GS115中,经大量筛选,获得高效分泌表达内切葡聚糖酶II的毕赤酵母工程菌株Gp2025。用甲醇诱导培养基进行摇瓶发酵,培养基中内切葡聚糖酶II的活力可达1573.0U/mL,同时对重组内切葡聚糖酶II的性质进行了初步研究。 相似文献
11.
AIMS: The objective of this study was to design an economically feasible process for endoglucanase (EG) production. METHODS AND RESULTS: Trichoderma pseudokoingii S-38 EG synthesis was studied. Initially, either glucose at 2.5, 5 or 10 g l-1, or cellulose powder (CF11) at 5 g l-1 was used as the sole carbon source. The results showed that enzyme synthesis and biomass formation were closely correlated, and both were affected by the carbon source. To improve EG volumetric product efficiency, a new technique was developed. Glucose and CF11 (2.5 and 5 g l-1, respectively) were used as initial carbon source, and glucose was added at 2.5 g l-1 day-1. EG activity, volumetric and specific EG productivities were 6.17 IU l-1, 53 IU l-1 h-1 and 114.3 IU (g cell protein)-1 h-1, respectively. Batch production in a 2-l laboratory fermenter confirmed the advantage of the technique. The product contained 10.86 IU ml-1 EG activity in 88 h. The volumetric and specific EG productivities were 123.4 IU l-1 h-1 and 177.8 IU (g cell protein)-1 h-1, respectively. CONCLUSIONS: These results suggest that optimization of the ratio of glucose to CF11 for balancing the induction and growth rate in the production of EG may lead to technical and economical benefits. SIGNIFICANCE AND IMPACT OF THE STUDY: A new technique was developed for the production of EG which improves both the volumetric product efficiency and the specific activity. 相似文献
12.
13.
从匍枝根霉cDNA文库中筛选得到组成型内切葡聚糖酶基因( zeg1和zeg2),经比对zeg1和zeg2相似度为86%,有相似的催化活性区域,经CDD(保守序列数据库)分析,该蛋白归属于糖苷水解酶第5家族,对比PDB(蛋白结构数据库)中第五家族的关键催化残基,预测该两个蛋白的第147位的谷氨酸( E)及199位的色氨酸( W)为该蛋白的关键催化残基。重组zeg1发酵至20 h时达到最高酶活为0.422 IU/mL;重组zeg2发酵至24 h达到最高酶活为0.509 IU/mL。酶学性质研究表明重组zeg1和zeg2的最适温度均为50℃,最适pH值均为5.0。通过CMC-SDS-PAGE电泳,复性后染色,测得重组zeg1和zeg2的分子量分别约为55 kD和58 kD。 相似文献
14.
Three endoglucanase cDNAs, eg65a, eg65b, and eg65c, were cloned from the mollusk Ampullaria crossean in previous work. To characterize the full-length enzymes as well as their individual functional modules via heterologous expression analysis, the three full-length putative endoglucanases (rEG65a, rEG65b, and rEG65c) and the corresponding catalytic modules (EG65a-CM, EG65b-CM, and EG65c-CM) were expressed in Pichia pastoris GS115, and the three corresponding carbohydrate-binding modules (EG65a-CBM, EG65b-CBM, and EG65c-CBM) were expressed in Escherichia coli BL21 (DE3). The properties of recombinant rEG65b, EG65a-CM, EG65b-CM, and EG65c-CM were characterized. Binding assays of CBMs with insoluble polysaccharides indicated that both EG65b-CBM and EG65c-CBM bound to phosphoric-acid swollen cellulose (PASC), Avicel, and oat-spelt xylan, while EG65a-CBM did not. The relative equilibrium constants (K(r)) of EG65b-CBM and EG65c-CBM were determined by absorption isotherm measurements. In this study, the CBMs of animal cellulases were expressed and characterized for the first time. 相似文献
15.
Bin Tang Yingying Zhang Yaping Yang Zhewei Song Xianglin Li 《World journal of microbiology & biotechnology》2014,30(11):2943-2952
A novel endoglucanase gene was cloned from Rhizopus stolonifer and expressed in Escherichia coli, the gene product EG II (45 kDa) was assigned to Glycoside Hydrolase Family 45 (GH45), and its specific activity on phosphoric acid-swollen cellulose (PASC) was 48 IU/mg. To solve the problem of substrate accumulation in the cellulose hydrolysis and enhance the catalytic efficiency of endoglucanase, the eg2 gene was modified by site directed mutagenesis. Mutations generated by overlapping PCR have been proven to increase its catalytic activity on carboxymenthyl cellulose, microcrystalline cellulose (Avicel) and PASC, among which the mutant EG II-E containing all 6 mutations (N39S, V136D, T251G, D255G, P256S and E260D) peaked 121 IU/mg on PASC. The bioinformatic analysis showed that 2 key catalytic residues (D136 and D260) moved closer with the opening of a loop after mutagenesis, and a tunnel was formed by structural transformation. This structure was conducive for the substrate to access the active centre, and D136 played an indispensable role in the substrate recognition. 相似文献
16.
A re-appraisal of multiplicity of endoglucanase I from Trichoderma reesei using monoclonal antibodies and plasma desorption mass spectrometry 总被引:1,自引:0,他引:1
M E Luderer F Hofer K Hagspiel G Allmaier D Blaas C P Kubicek 《Biochimica et biophysica acta》1991,1076(3):427-434
An endo beta-1,4-glucanase (EC 3.2.1.4, 1.4-(1,3;1,4)-beta-D-glucan 4 glucanhydrolase) was purified to apparent homogeneity from culture filtrates of Trichoderma reesei QM 9414. Identity of the protein with endoglucanase I (EG I) was examined by subjecting CNBr fragments of the protein to analysis by plasma desorption mass spectrometry. Seven non-glycosylated fragments, mapped on the eg1 gene sequence, could be identified, hence proving at least 39.4% identity of the amino acid sequence. No sign for microheterogeneity was observed. Purified EG I was used to prepare monoclonal antibodies. 17 stable clones were obtained, of which one--Mab EG 3--was used to analyze several commercial T. reesei cellulase preparations as well as culture filtrates from T. pseudokoningii and T. longibrachiatum for the presence of EG I. Most of them contained immunoreactive material migrating as a prominent 50-55 kDa band on SDS-PAGE, resembling EG I, but in some instances additional lower molecular weight bands were also observed. Cultivation of T. reesei at low pH led to an increase of these lower molecular weight bands. EG I was rather stable against proteolysis by papain in vitro, but after prolonged treatment, immunopositive products of 50 and 45 kDa were produced at the expense of the 55 kDa band. Our monoclonal antibodies failed to react with a low-molecular-weight endoglucanase, which was previously shown to be detectable with polyclonal antiserum against EG I. However, all monoclonals reacted with a 118 kDa protein which is most probably a dimer of EG I. These results are discussed with respect to the occurrence of multiple forms of EG I in T. reesei cellulase preparations. 相似文献
17.
18.
Harinder Singh Oberoi Rekha Rawat Bhupinder Singh Chadha 《Antonie van Leeuwenhoek》2014,105(1):119-134
Fungi isolated from partially decayed wood log samples showing characteristic diversity for spore colour, colony morphology and arrangement of spores were assessed for cellulolytic enzyme production. Isolates showing a cellulolytic index of ≥2.0 were assayed for filter paper (FP) cellulase and β-glucosidase (BGL) production. Molecular characterization confirmed the identity of the selected cellulolytic isolate as a strain of Aspergillus niger (A. niger HN-2). Addition of 2 % (w/v) urea enhanced FP and BGL activity by about 20 and 60 %, respectively. Validation studies conducted at parameters (29 °C, pH 5.4, moisture content 72 % and 66 h) optimized through response surface methodology in a solid-state static tray fermentation resulted in FP, BGL, cellobiohydrolase I (CBHI), endoglucanase (EG), xylanase activity and protein content of 25.3 FPU/g ds, 750 IU/g ds, 13.2 IU/g ds, 190 IU/g ds, 2890 IU/g ds and 0.9 mg/ml, respectively. In comparison, A. niger N402 which is a model organism for growth and development studies, produced significantly lower FP, BGL, CBHI, EG, xylanase activity and protein content of 10.0 FPU/g ds, 100 IU/g ds, 2.3 IU/g ds, 50 IU/g ds, 500 IU/g ds and 0.75 mg/ml, respectively under the same process conditions as were used for A. niger HN-2. Process optimization led to nearly 1.8- and 2.2-fold increase in FP and BGL activity, respectively showing promise for cellulase production by A. niger HN-2 at a higher scale of operation. Zymogram analysis revealed two isoforms each for EG and cellobiohydrolase and three isoforms for BGL. Crude cellulase complex produced by A. niger HN-2 exhibited thermostability under acidic conditions showing potential for use in biofuel industry. 相似文献
19.
Abstract Three clostridial cellulases viz. a hydrophilic cellobiohydrolase (CBH3), a hydrophobic endoglucanase (EG1), and an aggregate-forming hydrophilic endoglucanase (EG5), all purified from recombinant strains of Escherichia coli , were used in different combinations to reconstitute the synergistic effect during cellulose hydrolysis. EG1 and EG5 were weakly active on crystalline cellulose, if added separately or together in the reaction mixture. However, when CBH3 was added to the reaction mixture, its hydrolytic activity was increased to 1.8-fold in the presence of EG1 and EG5. A further increase in the activity from 1.8 to 2.2-fold was observed when calcium and dithiothreitol were added to the reaction mixture containing all three enzymes and filter paper as substrate. The synergistic effect remained unaffected even when EG1 was replaced by its 33-amino acid C-terminal deleted variant BL35. BL35 was less active compared to EG1, but was equally hydrophobic as EG1. These results suggest that the hydrophobic interaction between cellulolytic components and/or with the crystalline substrate is important for positive synergistic effect. 相似文献