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CYP3A4基因原核表达质粒构建与诱导表达 总被引:1,自引:0,他引:1
以质粒pCWNF14为模板,采用PCR技术扩增出CYP3A4基因,并将其接入pET-22b(+)、pET-28b(+)和pET-32a(+)载体中,经PCR测序鉴定后,转化Rosetta(DE3)2pLysS细菌,并用IPTG诱导表达.采用考马斯亮蓝染色的方法检测重组蛋白表达,3个表达重组质粒中,只有pET-32a(+)-CYP3A4可以表达目的蛋白;在低浓度IPTG(50μmol/L)诱导6h,所表达的CYP3A4蛋白约占细菌总蛋白的40%。且该蛋白不溶于8mol/L的尿素,而溶于去污剂10mmol/L 3-((3-Cholamidopropyl)dimethvlammonio propanesulfonic acid(CHAPS))和0.3% lauroyl sarcosine(SKL).成功地使CYP3A4基因在原核系统中高效表达. 相似文献
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猪瘟病毒E2蛋白A3BCD主要抗原结构域的原核表达 总被引:2,自引:1,他引:1
目的:对猪瘟病毒E2蛋白A3BCD进行原核表达,以期获得具有抗原活性的表达产物。方法:利用反转录PCR(RT-PCR)和套式PCR(nPCR)技术从河南省近期流行猪瘟病毒野毒株中扩增得到E2基因,并将其克隆至pUCm-T载体,构建克隆载体pUCm-TE2;利用PCR方法扩增E2基因的主要抗原域A3BCD,克隆至pET-32a(+)载体,构建表达载体pET-32aE2-2,转化到大肠杆菌Rosetta(DE3)中,用IPTG进行诱导表达,对诱导产物进行SDS-PAGE和Western-blotting分析。结果:SDS-PAGE结果显示在相对分子质量约35000处出现预期条带,表达产物主要以包涵体形式存在;Western-blotting检测表明,表达产物能与猪瘟病毒阳性血清发生特异性反应,出现单一反应带;用8mol/L尿素(pH8.0)溶解包涵体,经Ni-NTA亲和层析法纯化,获得纯度较高的目的蛋白,ELISA检测表明能与猪瘟抗体阳性血清发生特异性反应。结论:重组质粒pET-32aE2-2转化大肠杆菌Rosetta(DE3),解除了由于稀有密码子造成的表达限制,表达量得到提高;表达产物为硫氧还蛋白和E2-2的融合蛋白,易于纯化,且具有活性,为研制猪瘟抗体ELISA检测试剂盒奠定了基础。 相似文献
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目的表达和纯化带多聚组氨酸(6×His)标签的Nono ( non-POU-domain-containing, octamer-binding protein )融合蛋白并制备抗Nono多克隆抗体。方法构建pET-28a(+)-Nono重组表达质粒,转入Rosetta(DE3)大肠埃希菌,以IPTG诱导6×His-Nono融合蛋白表达,经镍离子金属螯合树脂纯化后,用纯化出的蛋白免疫BALB/C小鼠制备多克隆抗体,并用ELISA检测多克隆抗体的效价,Western印迹检测多克隆抗体的特异性。结果在大肠埃希菌中诱导出高水平表达的His-Nono融合蛋白,经亲和树脂纯化后免疫小鼠,获得了高特异性的抗Nono抗血清。结论成功构建pET-28a(+)-Nono原核表达质粒,表达并纯化出高纯度的目标蛋白,制备出高滴度、高特异性的多克隆抗体。 相似文献
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目的:原核表达人类肥胖基因瘦素蛋白,方法:以携人类肥胖基因的pUC119-ob为模拟,PCR扩增瘦素蛋白基因片段,并克隆到pET-32a构建重组表达质粒pET-32a-ob,经酶切和测序鉴定后,转化至大肠埃希菌DH5α中表达,SDS-PAGE电泳鉴定表达产物。结果:测序和限制性分析均证明了pET-32a-ob的序列正确,转化的DH5α可高效表达一个30kD融合蛋白,与预期结果一致。结论:经pET-32a-ob转化的DH5α可有效表达重组人类瘦素蛋白,为进一步研究瘦素蛋白的生物活性提供了基础。 相似文献
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目的:克隆表达恶性疟原虫(Hasmodium falciparum,p.f)海南株(FCC1/HN)乳酸脱氢酶(LDH),并对其免疫原性进行鉴定.为制备抗LDH抗体用于胶体金法快速检测疟原虫奠定基础。方法:应用PCR技术对恶性疟原虫乳酸脱氢酶(LDHpf)基因进行特异性扩增,将扩增产物克隆入表达载体pET-32a(+),重组表达载体经鉴定后诱导表达;重组LDHpf(rLDHpf)经纯化后,免疫家兔制备兔抗rLDHpf免疫血清,间接免疫荧光和Western印迹鉴定表达产物的免疫原性。结果:构建了pET-32a/LDHpf重组表达载体,测序后同源性分析显示p.f不同株间LDH氨基酸序列同源性大于98%,不同种间同源性也在90%以上;间接免疫荧光和Western印迹分析显示rLDHpf具有较好的免疫原性。结论:LDHpf基因高度保守;rLDHpf得到高效表达并具有良好的免疫原性。 相似文献
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小鼠Klf4基因的克隆及原核表达分析 总被引:2,自引:1,他引:1
目的克隆Klf4基因并对其重组蛋白进行原核表达及分析。方法提取胎鼠皮肤mRNA后反转录为cDNA序列,用一对两端引入特定酶切位点引物,从该cDNA中扩增出Klf4基因编码区序列,将其克隆到pEasy-T3载体上。对质粒双酶切并回收其中Klf4基因片段后,克隆入pET-52b(+)载体后转化Origmai B(DE3)型大肠杆菌,用IPTG诱导表达,最后采用SDS-PAGE对重组蛋白进行鉴定及分析。结果对所克隆的Klf4mRNA蛋白编码区的DNA序列分析表明,klf4CDS区包括终止密码子在内为1452 bp,与参照序列对比仅有四处存在差异,不仅其同源性达到99.72%,且其氨基酸序列同源性为100%;在IPTG诱导下pET-52b(+)-Klf4重组质粒可表达与预期相符的约为57×103的蛋白质;经IPTG刺激后重组蛋白表达明显上调,其中IPTG为0.4 mol/L时效果最佳。结论从胎鼠皮肤中克隆的Klf4基因可在原核中表达。 相似文献
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甘油脱水酶再激活酶的克隆表达及活性鉴定 总被引:1,自引:1,他引:0
运用PCR技术从克雷伯氏菌的基因组中分别扩增得到了编码甘油脱水酶再激活酶α、β两个亚基的基因gdrA、gdrB。将gdrA、gdrB克隆至pMD-18T载体上,构建克隆载体pMD-gdrAB。经测序正确后,将gdrAB亚克隆至表达载体pET-28a( )上构建表达质粒pET-28gdrAB。利用双抗生素筛选法,将pET-28gdrAB与连有甘油脱水酶基因的表达载体pET-32gldABC在大肠杆菌菌株BL21(DE3)中共表达,鉴定了甘油脱水酶再激活酶的活性。 相似文献
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目的:合成胆汁三烯结合蛋白(BBP)基因并在大肠杆菌中表达,获得重组BBP纯化制品。方法:根据天然BBP的基因序列和大肠杆菌偏好密码子设计并合成BBP基因的引物,PCR扩增优化的BBP基因序列,克隆至载体pEasy-T3;测序正确后,将该序列克隆至表达载体pET-32a上,构建表达质粒,转化至大肠杆菌BL21(DE3)pLysS,在IPTG诱导下表达融合蛋白;采用Ni柱纯化融合蛋白。结果:PCR扩增获得了优化后的BBP基因序列,构建了表达载体pET-32a-BBP;SDS-PAGE分析表明表达的融合蛋白相对分子质量为20×10^3,以包涵体形式存在,占全菌蛋白的40%以上;变性、复性后经Ni2+柱纯化,获得纯度达98%以上的重组蛋白。结论:优化并合成了BBP全基因序列,获得了高纯度重组融合蛋白,为进一步鉴定其生物活性及筛选小分子的研究奠定了基础。 相似文献
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根据类球红菌(Rhodobacter sphaeroides2.4.1)自诱导物合成酶基因cerⅠ的序列,设计并合成了1对特异性引物,在引物的5′和3′分别加入含有HindⅢ和XhoⅠ限制性酶切位点的序列,以类球红细菌Rhodobactersphaeroides基因组为模板扩增了cerⅠ基因序列。将PCR产物与pMD18-T载体连接,转化大肠杆菌DH5α。鉴定成功获得目的片段,经HindⅢ和XhoⅠ双酶切后与载体pET-28a(+)连接,构建原核表达质粒pET-28a(+)-cerⅠ,并将其转化宿主菌BL21(DE3),用IPTG诱导其表达。SDS-PAGE分析表明,重组载体pET-28a(+)-cerⅠ可成功地在大肠杆菌中表达cerⅠ蛋白。 相似文献
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Expression of gloshedobin,a thrombin-like enzyme from the venom of Gloydius shedaoensis,in Escherichia coli 总被引:2,自引:0,他引:2
Gloshedobin, a thrombin-like enzyme from the venom of Gloydius shedaoensis, was expressed in Escherichia coli using expression vector pET-32a(+). The gene was expressed under T7 promotor with a fusion partner of Thx.Tag and a 6xHis.Tag at its 5 terminal. After induction by IPTG for 6 h, the recombinant enzyme was expressed in the cytoplasm. Expression at 25°C gave twice the amount of recombinant gloshedobin in cytoplasm than at 37°C. 相似文献
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目的构建SDF-1α基因与绿色荧光蛋白的融合蛋白表达载体,进而观察SDF-1α基因编码蛋白在细胞内的定位情况。方法用EcoRI内切酶从pMD-T18一SDF-1α重组载体中酶切分离SDF-1α基因的完整ORF,构建pEGFP-C1-SDF-1α的融合表达载体,脂质体转染COS-7细胞,并在荧光显微镜下观察表达的融合蛋白。结果SDF-1α基因在COS-7细胞中高效表达,激光共聚焦的结果显示,SDF-1α基因定位在细胞质内。结论成功构建了pEGFP-C1-SDF-1α的融合表达载体,SDF-1α基因主要在细胞质中表达。 相似文献
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Abstract. A set of cell lines was constructed by infection of established murine fibroblasts with recombinant retroviruses encoding the simian virus 40 large T antigen (Tag) gene. By immunofluorescence flow cytometry, it was shown that these cell lines expressed Tag over at least a 20-fold concentration range. Using these cells, the dose-response relationship between Tag concentration and a phenotype detected by flow cytometry that measures the rate at which proliferating cells transit the cell cycle (i.e. cell-cycling phenotype) was determined. This relationship between Tag concentration and phenotype was not linear. Instead, the cell-cycling phenotype became saturated at relatively low Tag concentrations, i.e. a further increase in Tag concentration did not change the phenotype. The dose-response relationship between Tag and a second phenotype, colony formation in soft agar, was also determined. Colony formation in soft agar is a measurement of cell transformation. In contrast to the cell-cycling phenotype, transformation was linearly related to Tag over the entire 20-fold Tag concentration range. This phenotype did not saturate at high Tag concentrations. Therefore, the dose-response relationship between Tag concentration and the cell-cycling phenotype was different from that between Tag concentration and cellular transformation. Since the Tag gene is comprised of multiple genetic domains that independently affect cellular proliferation, one possibility is that the differences in dose-response of the two phenotypes indicate that different genetic domains of the gene are necessary for production of each phenotype. 相似文献
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Dey S 《Indian journal of experimental biology》1999,37(8):787-792
A partial genomic library was prepared in E. coli JM109 using pBR322 as vector and 2.4 kb Sau 3A I chromosomal fragment, encoding a nitroaryl reductase (nbr A) gene, from Streptomyces aminophilus strain MCMB 411. From the library, 2.4 kb fragment was recloned in E. coli JM109 and S. lividans TK64 using pUC18 and pIJ702 as vectors respectively. The recombinant plasmids pSD103 and pSD105 expressed the reductase gene and exported the enzyme in periplasmic space of E. coli and in cytoplasm of S. lividans TK64. The proteins expressed by E. coli and S. lividans had the same molecular mass (70 kD) as that expressed by parent strain, which suggested that the enzyme was processed similarly by all strains. Activities of the enzymes cloned in E. coli JM109 and S. lividans TK64 containing recombinant plasmids pSD103 and pSD105 respectively were optimum at 30 degrees C and pH 9 and requirement of cofactors was same as that of the parent strain. 相似文献
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构建登革 3型病毒 prM E基因的真核表达重组质粒 ,并进行体外表达 ,为登革DNA疫苗的研究奠定基础。用RT -PCR法获得 prM -E基因片段 ,然后将其克隆到真核表达载体中。用电穿孔法将重组质粒DNA转入BHK细胞 ,通过免疫荧光法检测外源基因在真核细胞中的表达。结果 ,通过酶切和序列测定证实了构建的重组质粒DNA含序列正确的 prM- E基因。用免疫荧光法检测到转染了重组质粒DNA的BHK细胞的胞浆中有登革 3型病毒特异蛋白的表达。说明含有登革 3型病毒prM -E基因的真核表达重组质粒可以在BHK细胞中表达 ,该结果为观察该重组质粒的免疫原性奠定了基础。 相似文献
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Braud S Belin P Dassa J Pardo L Mourier G Caruana A Priest BT Dulski P Garcia ML Ménez A Boulain JC Gasparini S 《Protein expression and purification》2004,38(1):69-78
BgK, a sea anemone peptide consisting of 37 amino acid residues and 3 disulfide bonds, blocks voltage-gated potassium (Kv1) channels. Here, we report a method for producing tagged BgK in Escherichia coli, as a soluble cytoplasmic protein. First, using peptidic synthesis, we show that addition of a 15 residue peptide (S.Tag) at the BgK C-terminus does not affect its biological activity. Then, a synthetic DNA sequence encoding BgK was constructed and cloned to produce a BgK-S.Tag hybrid in the cytoplasm of E. coli. The presence of S.Tag did not only facilitate detection, quantification, and purification of the recombinant protein, but also increased the production yield by more than two orders of magnitude. Moreover, use of an E. coli OrigamiB(DE3)pLacI strain also increased production; up to 5.8-7.5mg of BgK-S.Tag or mutated BgK(F6A)-S.Tag was produced per liter of culture and could be functionally characterized in crude extracts. Using a two-step purification procedure (affinity chromatography and RP-HPLC), we obtained 1.8-2.8mg of purified recombinant protein per liter of culture. The recombinant peptides displayed functional properties similar to those of native BgK or BgK(F6A). 相似文献
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A critical stage in pollen development is the dissolution of tetrads into free microspores. Tetrads are surrounded by a wall composed primarily of beta-1,3-glucan. At the completion of meiosis, tetrads are released into the anther locule after hydrolysis of the callose by a beta-1,3-glucanase complex. The cDNA corresponding to a beta-1,3-glucanase cloned from tobacco (Tag 1) represents a gene that is highly similar to other beta-1,3-glucanases and is expressed exclusively in anthers from the tetrad to free microspore stage of pollen development. Tag 1 protein was overexpressed in E. coli, accumulating in insoluble inclusion bodies. Polyclonal antibodies against Tag 1 recombinant protein identify a single 33 kD protein accumulating only in anthers at tetrad and free microspore stages where beta-1,3-glucanase activity is present. Transgenic plants expressing Tag 1 antisense RNA were produced. Although Tag 1 RNA and protein levels were greatly reduced, tetrad dissolution and pollen development were normal. These data indicate that under the conditions these tobacco plants were grown, wild type levels of Tag 1 protein are not necessary for male fertility. 相似文献
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口蹄疫是由口蹄疫病毒引起的世界上最重要的畜牧疾病之一,严重影响世界畜牧业的发展,而疫苗免疫仍然是对疫情预防和控制的最有效手段。铁蛋白具有自组装和生物修饰的特性,在纳米疫苗等领域具有广阔的应用前景。选用O型口蹄疫病毒的vp1基因和幽门螺杆菌铁蛋白基因,通过融合PCR将vp1基因构建到铁蛋白亚基基因前端,在大肠杆菌中表达后通过His标签进行镍柱亲和层析纯化。将纯化好的重组蛋白进行Western blotting检测、质谱分析和透射电镜观察,发现重组蛋白VP1-Ferritin在大肠杆菌中获得表达,并可自组装成纳米颗粒。 相似文献