斜卧青霉L-06内切葡聚糖酶Ⅰ基因的克隆与表达

【目的】克隆斜卧青霉L-06的内切葡聚糖酶Ⅰ基因(egI),并实现其在大肠杆菌内的高效表达。【方法】利用RT-PCR技术克隆了斜卧青霉L-06的内切葡聚糖酶Ⅰ基因(egI),并将egI基因克隆到原核表达载体中,构建了重组质粒pET32a-egI。【结果】转化至大肠埃希菌Rosetta(DE3),经IPTG诱导重组蛋白表达,SDS-PAGE检测结果表明:重组表达产物的相对分子质量约为80 kD,与预期相符。重组表达的菌悬液,经破碎离心,取其上清液,进行纤维素酶活性染色,获得了活性条带。DNS法测得内切酶活力为2.56 IU/mL。【结论】构建了斜卧青霉L-06内切葡聚糖酶Ⅰ的原核表达系统。     

兔IFRG基因的克隆及表达分析

实验通过对兔子基因组DNA进行PCR获得兔IFRG基因,将其克隆到pGEM-T载体,双酶切鉴定和测序结果表明成功构建了重组克隆载体pGEM-T-IFRG。通过RT-PCR分析发现IFRG基因在兔不同组织中有不同程度的表达。将重组克隆载体pGEM-T-IFRG和表达载体pET-41（c）经过EcoR1和Xho1双酶切后连接构建重组表达载体pET-41（c）-IFRG,将双酶切鉴定正确的重组表达载体转化入E.coli BL21,IPTG诱导融合蛋白的表达,SDS-PAGE结果显示兔IFRG基因在大肠杆菌中得到了良好的表达。     

联合β-半乳糖苷酶和L-阿拉伯糖异构酶法合成D-塔格糖的研究

将大肠杆菌K-12中的B-半乳糖苷酶基因lacZ和L-阿拉伯糖异构酶基因araA以串联方式克隆到载体pET-28a（＋）上,并转入大肠杆菌BL21（DE3）中进行表达。通过SDS—PAGE分析发现,重组菌株能表达出大量可溶性B．半乳糖苷酶蛋白和L-阿拉伯糖异构酶蛋白。以重悬菌液为酶源,可将乳糖降解为D-半乳糖,并将D-半乳糖转化为D-塔格糖。在温度为50℃,pH7．0的缓冲液中,经一段时间反应后,D-塔格糖的转化率可达21％以上。加入Mn^2＋、Co^2＋和Fe^2＋均能够使D-塔格糖的转化率提高。     

α-葡萄糖苷酶基因序列分析及真核表达载体构建

目的：Aspergillus niger（CU-1）菌株α-葡萄糖苷酶基因（agdA）克隆并对其序列进行分析,构建该基因的真核表达载体。方法：设计合成的一对特异性引物,采用PCR以总DNA为模板,扩增得到DNA片段（D1）;采用RT-PCR方法扩增得到DNA片段（D2）。将DNA片段D1和D2转入大肠杆菌中并进行了序列测定,序列进行BLAST比对分析。将α-葡萄糖苷酶基因的cDNA片段与表达载体pGAPZαA连接,构建重组表达载体。结果：基因agdA大小为3 127bp,含有3个外显子和4个内含子。该基因的cDNA序列大小为2 958bp,包含完整的编码框,编码985个氨基酸。agdA基因序列与已发表的α-葡萄糖苷基因序列同源性达99%,其中有6个位置的碱基发生了变化。已成功构建重组表达载体pGAPZαA-agdA。结论：Aspergillus niger（CU-1）菌株α-葡萄糖苷酶基因序列分析及重组表达载体pGAPZαA-agdA的构建为在毕赤酵母中表达Aspergillus niger（CU-1）菌株的α-葡萄糖苷酶奠定基础。     

阴道毛滴虫蛋氨酸裂解酶的基因克隆及重组酶性质分析

为研究重组阴道毛滴虫蛋氨酸裂解酶的活性,从阴道毛滴虫提取RNA,经过RT-PCR克隆蛋氨酸γ-裂解酶基因,与pET-15b质粒连接构建原核表达载体pET-15b-mgl1,并测序。转化宿主菌BL21后进行诱导表达,分离纯化目的蛋白并研究其酶学性质。以L-蛋氨酸、DL-同型半胱氨酸、L-半胱氨酸为底物测定重组酶Km值为0.318、2.14、1.62mmol/L,比活性分别为20.17、318.69、56.96μmol/min/mg protein。MGL最适pH在5.0到6.0之间,在50℃可稳定30min无活性损失。实验结果显示重组酶具有较高的活性和较好的热稳定性,为临床应用研究奠定基础。     

辣根过氧化物酶同功酶C3基因在毕赤酵母中的表达

目的：克隆与表达辣根过氧化物酶同功酶C3（HRPC3）基因。方法：用PCR方法从辣根的总DNA中,扩增得到一种辣根过氧化物酶同功酶C3基因,将PCR产物连接到pMD18-T载体上,测序证明正确后,再将目的基因正确插入到巴斯德毕赤酶母表达载体pPIC9K中,含有目的基因的重组pPIC9K质粒在毕赤酶母中进行表达与分析。结果：应用毕赤酶母作为受体菌,成功表达了HRPC3基因,其活性为56IU/L。结论：毕赤酶母直接表达出了具有生物活性的辣根过氧化物酶同功酶C3。     

酶法转化DL-ATC合成L-半胱氨酸的酶促反应条件研究

目的:考察酶源保存方式、酶促反应时间、底物pH值、底物浓度、酶浓度、金属离子等因素对酶活力的影响。方法:以假单胞菌(Pseudomonassp.)TS1138为供试菌株,采用酸式茚三酮法测定L-半胱氨酸含量,研究了酶法转化DL-ATC合成L-半胱氨酸的酶促反应条件。结果:TS1138菌株中L-半胱氨酸脱巯基酶具有较高的活性,而且Mg2 、Mn2 、Fe2 、Zn2 、Cu2 等5种金属离子对DL-ATC水解酶酶系有不同程度的抑制,其中Cu2 对该酶系的抑制作用很大。结论:确定了TS1138菌株酶法转化DL-ATC合成L-半胱氨酸的最适酶促反应条件,为酶促反应动力学的研究奠定了基础。     

烟草β—1,3—葡聚糖酶cDNA克隆,大肠杆菌表达及植物表达载体的 …

用０．１５％乙烯利诱导烟草幼苗后,提取叶片总ＲＮＡ,并通过反转录及多聚酶链式反应（ＲＴ－ＰＣＲ）扩增出β－１,３－葡聚糖酶基因的ｃＤＮＡ。将其克隆至载体ｐＢｌｕｅｓｃｒｉｐｔ ＳＫ后,完成了此基因的全序列分析。测序结果表明：所克隆的ｃＤＮＡ除第１００８位碱基与所报道的不同外,其它序列完全一致。为制备抗血清,构建了此基因的大肠杆菌表达载体,并在表达宿主菌ＢＬ２１（ＤＥ３）ｐｌｙＳ中得到表达,进行了Ｗ     

人核糖核酸酶抑制因子基因重组腺病毒载体的构建及鉴定

目的构建含有人核糖核酸酶抑制因子（hRI）基因的重组腺病毒载体。方法以含有全长cDNA的pT7-RI为模板,PCR扩增hRI,经T载体克隆后,酶切亚克隆到穿梭质粒pAdTrack—CMV上,在BJ5183细菌内和pAdEasy-1同源重组。筛选阳性克隆,酶切、PCR及测序鉴定,线性化后脂质体法转染293细胞进行包装、扩增。通过观察绿色荧光蛋白（GFP）的表达及PCR扩增目的基因等方法鉴定重组的腺病毒。结果酶切鉴定及PCR结果证明hRI基因重组腺病毒载体构建成功,病毒滴度为1．5×10^10 pfu/ml。结论应用细菌内同源重组法成功构建了含hRI基因的重组腺病毒载体。     

Effect of drug transporter genes on cysteine export and overproduction in Escherichia coli

L-cysteine is an important amino acid in terms of its industrial applications. We previously found a marked production of L-cysteine from glucose in recombinant Escherichia coli cells expressing an altered cysE gene encoding feedback inhibition-insensitive serine acetyltransferase. Also, a lower level of cysteine desulfhydrase (CD) activity, which is involved in L-cysteine degradation, increased L-cysteine productivity in E. coli. The use of an L-cysteine efflux system could be promising for breeding L-cysteine overproducers. In addition to YdeD and YfiK, which have been reported previously as L-cysteine exporter proteins in E. coli, we analyzed the effects of 33 putative drug transporter genes in E. coli on L-cysteine export and overproduction. Overexpression of the acrD, acrEF, bcr, cusA, emrAB, emrKY, ybjYZ, and yojIH genes reversed the growth inhibition of tnaA (the major CD gene)-disrupted E. coli cells by L-cysteine. We also found that overexpression of these eight genes reduces intracellular L-cysteine levels after cultivation in the presence of L-cysteine. Amino acid transport assays showed that Bcr overexpression conferring bicyclomycin and tetracycline resistance specifically promotes L-cysteine export driven by energy derived from the proton gradient. When a tnaA-disrupted E. coli strain expressing the altered cysE gene was transformed with a plasmid carrying the bcr gene, the transformant exhibited more L-cysteine production than cells carrying the vector only. A reporter gene assay suggested that the bcr gene is constitutively expressed at a substantial level. These results indicate that the multidrug transporter Bcr in the major facilitator family is involved in L-cysteine export and overproduction in genetically engineered E. coli cells.     

One-step elimination of L-cysteine desulfhydrase from crude enzyme extracts of Pseudomonas sp. TS1138 using an immunomagnetic affinity matrix improves the enzymatic production of L-cysteine

In this study, a high efficiency immunomagnetic affinity matrix was developed to eliminate L-cysteine desulfhydrase (CD), which decomposes L-cysteine, in crude enzyme extracts from Pseudomonas sp. TS1138. After cloning and expression in Escherichia coli, recombinant CD was purified to raise polyclonal antibodies from mice. The anti-CD antibody was cross-linked to staphylococcal protein A-magnetic cellulose microspheres (MCMS) with dimethyl pimelimidate (DMP). The natural CD was eliminated from the crude enzyme extracts by treatment with the cross-linked antibody-protein A-MCMS, resulting in a high level of L-cysteine production. The conversion rate of DL-2-amino-Delta2-thiazoline-4-carboxylic acid (DL-ATC) to L-cysteine increased significantly from 61.9 to 96.2%. The cross-linked antibody-protein A-MCMS showed its durability after repetitive use, maintaining a constant binding capacity for CD during five cycles. This study may lead to a convenient and cost-efficient method to produce L-cysteine by enzymatic conversions.     

猪白细胞介素18成熟蛋白基因的克隆与表达

目的克隆猪白细胞介素18(pIL-18)成熟蛋白基因,并在植物乳杆菌(Lb.plantarum)NC8中进行表达。方法通过RT-PCR方法从猪脾脏细胞中扩增出pIL-18成熟蛋白基因,克隆到T载体pMD18-T后测序;将阳性基因片段克隆至大肠埃希菌-乳酸菌穿梭表达载体pSIP-409构建重组表达载体pSIP-409-IL-18,进行酶切和PCR鉴定;应用电穿孔技术将其转化至Lb.plantarum NC8中,经SppIP诱导表达后,进行SDS-PAGE及Western-blot分析。结果经测序,pIL-18成熟蛋白基因核苷酸长度为579 bp,编码193个核苷酸;酶切和PCR鉴定证明成功构建了重组表达载体pSIP-409-IL-18;SDS-PAGE及Western-blot分析表明重组菌表达了18 kD的融合蛋白,该重组蛋白可以与鼠抗猪IL-18多克隆抗体反应。结论成功克隆了pIL-18成熟蛋白基因,并获得有生物活性的pIL-18重组乳酸菌,为研制开发IL-18重组乳酸菌制剂奠定基础。     

Cd1-型亚硝酸盐还原酶脱氮工程菌的构建与表达

目的用基因工程技术将铜绿假单胞菌PAO1中nirS基因定向克隆至表达载体pQE-30上,使nirS基因得到高效表达。方法根据GenBank公布的nirS碱基序列和表达载体pQE-30的多克隆位点设计引物,以铜绿假单胞菌PAO1的基因组DNA为模板,应用PCR技术扩增目的片段nirS;之后经过BamH I和HindⅢ双酶切,定向克隆到pQE-30上,化学转化DH5α,构建含有重组质粒的转化子pQE30-nirS-DH5α;经酶切和测序鉴定,扩增产物的碱基序列与GenBank公布的序列完全吻合,再将重组质粒pQE30-nirS转化表达菌株SG13009构建脱氮基因工程菌pQE30-nirS-SG-13009（PNS）。最后用SDS-PAGE（IPTG浓度：0．05mmol／L;诱导温度：25℃;诱导时间：2～3h）和His-tag in-gel Stain鉴定cd1-型亚硝酸盐还原酶的分子量与特异性。结果构建了高效表达cd1-型亚硝酸盐还原酶的脱氮基因工程菌PNS。结论Cd1-型亚硝酸盐还原酶能够在脱氮基因工程菌PNS中得到正确和高效的表达。     

Effect of cysteine desulfhydrase gene disruption on L-cysteine overproduction in Escherichia coli

In Escherichia coli, the enzyme called cysteine desulfhydrase (CD), which is responsible for L-cysteine degradation, was investigated by native-PAGE and CD activity staining of crude cell extracts. Analyses with gene-disrupted mutants showed that CD activity resulted from two enzymes: tryptophanase (TNase) encoded by tnaA and cystathionine beta-lyase (CBL) encoded by metC. It was also found that TNase synthesis was induced by the presence of L-cysteine. The tnaA and metC mutants transformed with the plasmid containing the gene for feedback-insensitive serine acetyltransferase exhibited higher L-cysteine productivity than the wild-type strain carrying the same plasmid. These results indicated that TNase and CBL did act on L-cysteine degradation in E. coli cells.     

Cloning, expression and characterization of L-cysteine desulfhydrase gene from Pseudomonas sp. TS1138

L-cysteine desulfhydrase (CD) plays an important role in L-cysteine decomposition. To identify the CD gene in Pseudomonas sp. TS1138 and investigate its effect on the L-cysteine biosynthetic pathway, the CD gene was cloned from Pseudomonas sp. TS1138 by polymerase chain reaction (PCR) method. The nucleotide sequence of CD gene was determined to be 1,215 bp, and its homology with other sequences encoding CD was analyzed. Then the CD gene was subcloned into pET-21a(+) vector and expressed in Escherichia coli (E. coli) by isopropyl-β-D-thiogalactopyranoside (IPTG) inducement. The recombinant CD was purified by Ni-NTA His-Bind resin, and its activity was identified by the CD activity staining. The enzymatic properties of the recombinant CD were characterized and its critical role involved in the L-cysteine biosynthetic pathway was also discussed. __________ Translated from Microbiology, 2006, 33(4): 21–26 [译自: 微生物学通报]     

PPARγ基因真核表达载体的构建及其在乳腺癌MDA—MB-231细胞中的表达

目的：构建以绿色荧光蛋白（GFP）为报告基因的重组表达质粒pEGFP—C1—PPARγ,观察小鼠PPARγ基因在MDA-MB-231细胞中的表达及定位。方法：采用克隆和亚克隆技术构建小鼠PPARγ基因真核表达载体,脂质体Lip2000介导转染MDA—MB-231细胞,real—time PCR和western—blot验证其mRNA和蛋白的表达,荧光显微镜观察该基因亚细胞定位。结果：酶切和测序结果证实重组质粒含有PPAIh编码区序列且插入方向正确,转染后观察该基因亚细胞定位于胞核,胞质有弥散分布。结论：成功构建了小鼠PPARγ基因真核表达载体,该基因在MDA—MB-231细胞中成功表达,PPARγ基因主要集中表达于胞核。     

C型产气荚膜梭菌α毒素基因的克隆与表达

利用PCR技术,从C型产气荚膜梭菌染色体基因组中扩增了1．2kb的α毒素基因,将纯化的PCR产物与载体pGEM-T连接,转化至受体菌JM109中,经NcoI／EcoRI和BamHI／EcoRI酶切鉴定及核苷酸序列测定证实,重组质粒pXCPAl中含有α毒素全基因。随后用NcoI／EcoRI酶切质粒pXCPAl,回收α毒素基因片段,插入到事先经同样酶切处理的载体pET-28c中相应酶切位点,构建了表达质粒pETXAl,经NcoI／EcoRI和BamHI／EcoRI酶切鉴定及核苷酸序列测定证实,表达质粒含有α毒素基因且基因序列和阅读框架正确。重组菌株BL21(DE3)(pETXAl)表达产物经ELISA检测和SDS-PAGE分析,重组菌株表达的α毒素蛋白能够被α毒素单抗识别,其表达量占菌体总蛋白相对含量的16．28％。