人A组轮状病毒地方株外壳蛋白VP4的原核表达

目的：制备轮状病毒外壳蛋白VP4。方法：从病人粪便中分离的毒株中提取病毒dsRNA为模板,经RT—PCR获得编码VP4截短蛋白基因片段cDNA(1—1253bp),将VP4基因片段克隆于pGEX-4T-2融合表达载体中,经dot印迹筛出阳性重组子,重组质粒转化大肠杆菌BL21(DE3)。工程菌经IPTG诱导,11％聚丙烯酰胺凝胶电泳。结果：Western印迹分析表明,工程菌能正确表达VP4蛋白片段,且具有良好的抗原性。结论：为研制轮状病毒重组疫苗、亚单组疫苗、转基因植物口服疫苗做了前期准备。     

轮状病毒外壳蛋白VP7在转基因番茄果实中的特异表达

将轮状病毒外壳蛋白VP7基因克隆到含有番茄果实特异性启动子TFP的植物表达载体pTF ,并转化到根癌农杆菌 (Agrobacteriumtumefaciens)菌株EHA10 5中 ,采用叶盘转化法转化番茄 (LycopersiconesculentumMill.)栽培品种TX0 0 14 ,获得了转基因植株。经PCR、PCR Southernblot和Southernblot分析表明VP7基因已整合到转基因番茄植株的核基因组中 ,RT PCR、Westernblot结果表明VP7蛋白在果实中获得了特异表达     

高粱花叶病毒外壳蛋白的原核表达及其抗血清制备

高粱花叶病毒(Sorghum mosaic virus,SrMV)是世界上分布最广的侵染甘蔗的病毒之一,引起甘蔗花叶病,对甘蔗产业危害很大。根据SrMV外壳蛋白(coat protein,CP)基因序列合成一对引物,以海南(SrMV-HN)染病植株总RNA为材料,采用RT-PCR方法克隆了长约987 bp的目的片段。将CP基因与质粒pET32a(+)连接,构建了含SrMV CP基因的融合蛋白原核表达载体pET32a-SrMVCP。然后用正确的重组质粒转化大肠杆菌Rosetta(DE3),经IPTG诱导后,SDS-PAGE检测出一条约36kD的特异融合蛋白表达谱带。融合蛋白主要以可溶性蛋白形式稳定表达。通过优化诱导条件,确立了CP基因表达的最佳条件:IPTG终浓度为0.1 mmol/L,诱导时间为4 h,诱导温度为30℃。用Ni2+-NTA琼脂糖亲和层析纯化融合蛋白,免疫家兔制备出抗血清。通过酶联法(ID-ELISA)测定本试验制备的SrMV CP抗血清工作浓度为1∶1 000,Western blotting检测结果表明,抗血清与SrMV-HN诱导表达的CP蛋白发生特异性反应。对田间25个甘蔗样品进行检测,结果表明该抗血清的效价高、灵敏度高、特异性强,可以应用于田间样品的检测。     

甘蔗黄叶病毒外壳蛋白基因原核表达研究

本研究主要目的是构建ScYLV-CP基因的原核表达载体,表达ScYLV-CP蛋白。采用PCR扩增出CP基因的蛋白编码序列,克隆到中间载体中,再经双酶切、亚克隆到表达载体中,构建该基因的表达载体pET-29 a-CP,在大肠杆菌中用IPTG诱导表达,SDS-PAGE电泳。酶切鉴定表明表达载体内插入片段正确,在大肠杆菌中诱导后,出现一条分子量约为22 kDa蛋白带,与CP基因开放阅读框架的理论推算值21.719 kDa相符。研究表明甘蔗黄叶病毒外壳蛋白能在原核细胞中高效表达,为建立甘蔗黄叶病毒血清学快速检测技术奠定基础。     

马铃薯S病毒外壳蛋白基因的克隆与原核表达

依据马铃薯S病毒(Potato virus S,PVS)外壳蛋白(CP)基因序列(885bp)设计合成了两对 引物,通过RT-PCR扩增得到长0.8kb的目的片段,将目的片段转入大肠杆菌,酶切鉴定证明 得到了含有目的片段的重组子,测定序列结果与其他PVS分离物CP基因的序列比较,发现其核苷酸同源性达95%左右;构建了含PVS CP基因的融合蛋白原核表达载体,并在大肠杆菌中得到表达,SDS-PAGE测定融合蛋白的分子量为58kD.     

甘蔗花叶病毒E株系外壳蛋白基因原核表达载体的构建与表达

目的:用原核表达的方法获取大量带6个His标记的甘蔗花叶病毒E株系(ScMV-E)外壳蛋白(CP)。方法:用带有BamHⅠ和SalⅠ酶切位点的特异引物,以带有多个基因的重组质粒pNUSCP为模板,扩增出片段长度为942bp的ScMV-E外壳蛋白基因,亚克隆到pMD18-T载体上,转化E.coliDH5α,经双酶切检测获得阳性克隆。BamHⅠ和SalⅠ双酶切阳性克隆质粒,回收目的片段ScMV-E的CP基因。把目的片段插入表达载体pET29a( ),转化E.coliBL21(DE3),测序。结果:阳性质粒pET29a-CP在E.coliBL21(DE3)中得到大量特异表达。SDS-PAGE分析表明,该蛋白的相对分子质量约36000,与预测一致。结论:以上方法可以得到带6个His标记的目的蛋白,有利于纯化并获取高纯度的ScMV-E的外壳蛋白。     

马铃薯S病毒外壳蛋白基因的克隆与原核表达

依据马铃薯S病毒 (PotatovirusS ,PVS)外壳蛋白 (CP)基因序列 (885bp)设计合成了两对引物 ,通过RT PCR扩增得到长 0 .8kb的目的片段 ,将目的片段转入大肠杆菌 ,酶切鉴定证明得到了含有目的片段的重组子 ,测定序列结果与其他PVS分离物CP基因的序列比较 ,发现其核苷酸同源性达 95 %左右 ;构建了含PVSCP基因的融合蛋白原核表达载体 ,并在大肠杆菌中得到表达 ,SDS PAGE测定融合蛋白的分子量为 5 8kD。     

A组人轮状病毒VP6基因克隆及在大肠杆菌中的高效表达

轮状病毒(rotavirus RV) 结构蛋白VP6位于病毒三层衣壳结构的中间层,在病毒粒子的形成过程中起重要的作用。从临床样品中分离的人轮状病毒TB-Chen株VP6基因通过RT-PCR得到扩增产物。以pET作为表达载体,将VP6蛋白编码基因序列插入到质粒pET中成功构建原核表达质粒pET-VP6。实验表明,带有pET-VP6质粒的大肠杆菌BL21(DE3)可以高效表达目的蛋白VP6,重组表达产物VP6占菌体总蛋白的27.4%, 其分子量约为45 kDa,并且能被豚鼠抗SA11血清抗体识别（Western blot）。这一结果为进一步研究VP6的结构和功能奠定了重要的物质基础。     

猪轮状病毒vp4基因在大肠杆菌中的表达

以猪轮状病毒JL94株核酸为模板扩增该病毒vp4全基因,对扩增产物进行测序及序列比较;根据VP4的5’端(1bp-750bp)特异片段主要决定其活性的观点,再设计一对引物扩增该主要抗原位点基因,将此主要抗原位点基因同pGEX-6P-1载体连接并转化入E．coli．BL2l(DE3)plays,经IPTG诱导表达出蛋白质;对表达的蛋白进行Westernblot分析、纯化和血清中和抗体试验。结果表明：JL94株与国外分离株CRW．8株、BEN．307株vp4全基因片段氨基酸同源性分别为96．98％和98．05％,说明JL94株与CRW．8株、BEN．307株属于同-vP4血清型;经IPTG诱导VP4主要抗原位点基因获得了高效表达,表达量占菌体蛋白的26％;Westernblot结果和所表达的融合蛋白免疫小鼠产生的中和抗体能阻断JL94在MAl04细胞上引起的细胞病变,说明所表达蛋白有良好的生物学活性。     

在昆虫细胞中表达G2型轮状病毒地方株VP7基因

Ａ组轮状病毒是导致婴幼儿重症腹泻的最主要病毒病原,ＶＰ７是病毒外壳上的主要糖蛋白,它具有中和抗原活性,与病毒的毒力及免疫保护性有关,也是划分病毒血清型的最主要标志之一〔１〕。ＶＰ７基因及其编码蛋白一直是人们研究的主要对象,很多研究工作和诊断试剂都需大...     

Expression of Rotavirus Capsid Protein VP6 in Transgenic Potato and Its Oral Immunogenicity in Mice

Murine rotavirus gene six encoding the 41 kDa group specific capsid structural protein VP6 was stably inserted into the Solanum tuberosum genome by Agrobacterium tumefaciens mediated transformation. The molecular mass of plant synthesized VP6 capsid protein determined by immunoblot was similar to the size of both purified virus VP6 monomeric peptides and partially assembled virus-like particles. The amount of VP6 protein synthesized in transgenic potato leaf and tuber was determined by enzyme-linked immunosorbent assay to be approximately 0.01% of total soluble protein. Oral immunization of CD-1 mice with transformed potato tuber tissues containing VP6 capsid protein generated measurable titers of both anti-VP6 serum IgG and intestinal IgA antibodies. The presence of detectable humoral and intestinal antibody responses against the rotavirus capsid protein following mucosal immunization provides an optimistic basis for the development of edible plant vaccines against enteric viral pathogens.     

肠道病毒71型外壳蛋白VP1全长在大肠杆菌中的高效表达及初步活性测定

目的:重组表达肠道病毒71型(EV71)外壳蛋白VP1全长,用于研制血清学检测试剂和疫苗研发。方法:在获得EV71全长基因并测序正确的基础上,将外壳蛋白VP1全长基因克隆到表达载体pET28a(+)上,构建重组表达质粒pET28a(+)/VP1,转化大肠杆菌BL21,IPTG诱导表达,利用Ni2+亲和层析柱对重组蛋白进行纯化,采用双抗原夹心检测技术评价重组抗原与27份EV71抗体阳性血清和18份阴性血清的反应情况。结果:重组EV71-VP1蛋白在大肠杆菌中诱导6 h后可获得高效表达,能与27份EV71抗体阳性血清中的21份发生阳性反应,EV71双抗原夹心检测与中和血清测试结果具有很好的一致性(P0.05)。结论:实现了肠道病毒71型外壳蛋白VP1的高效表达,为肠道病毒71型诊断试剂和疫苗的研究奠定了基础。     

High Level Expression of Grass Carp Reovirus VP7 Protein in Prokaryotic Cells

Sequences analysis revealed Grass carp reovirus （GCRV） s10 was 909 nucleotides coding a 34 kDa protein denoted as VP7, which was determined to be a viral outer capsid protein （OCP）. To obtain expressed OCP in vitro, a full length VP7 gene was produced by RT-PCR amplification, and the amplified fragment was cloned into T7 promoted prokaryotic expression vector pRSET. The recombinant plasmid, which was named as pR/GCRV-VP7, was then transformed into E.coli BL21 host cells. The data indicated that the expressed recombinant was in frame with the N-terminal fusion peptide. The over-expressed fusion protein was produced by inducing with IPTG, and its molecular weight was about 37kDa, which was consistent with its predicted size. In addition, the fusion protein was produced in the form of the inclusion body with their yield remaining steady at more than 60% of total bacterial protein. Moreover, the expressed protein was able to bind immunologically to anti-his-tag monoclonal antibody （mouse） and anti-GCRV serum （rabbit）. This work provides a research basis for further structure and function studies of GCRV during entry into cells     

登革2型病毒衣壳蛋白在哺乳动物细胞中的表达与鉴定

从构建的重组质粒pLEX—C中高保真PCR获得编码登革2型病毒43株C基／E／（D2C）DNA片段,通过基因重组的方法将其克隆入真核表达载体pcDNA6／V5-His获得了重组真核表达载体pc／D2C。经电穿孔的方法转染BHK21细胞后,分别通过RT—PCR、免疫荧光和western印迹鉴定表达的蛋白。结果重组蛋白在BHK21细胞中获得表达,表达的蛋自主要存在于胞浆中,并具有较好的抗原性,能够被抗登革病毒衣壳蛋白单克隆抗体特异识别。此研究为深入了解登革病毒衣壳蛋白在病毒复制及组装过程中的生物学功能奠定了基础。     

Expression and Immunoreactivity of a Human Group A Rotavirus Vp4

Rotavirus capsid protein Vp4 plays an important role in the virus adhering and entering the cells. In this study, a Vp4 gene cloned from a rotavirus strain TB-Chen was highly expressed in E.coli BL21 (DE3). The results of the Western blot showed that the protein possesses specific immuno-reactivities and can be specifically recognized by guinea pig antibodies against rotavirus strain SA11 or Wa. Some Vp4 dimers were formed during renaturation. These data obtained from this study provide a strong basis for further study on the structure and function of the Vp4.     

重组人肝细胞生长因子真核表达的定性及定量检测

将人肝细胞生长因子（human hepatocyte growth factor hHGF)全长cDNA重组入pEE14真稳定表达质粒,用lipofectin脂质体将pEE14/rhHGF转染入CHO－K1细胞,蛋氨酸亚氨基代砜（methionine sulfoximine,MSX)筛选出阳性细胞克隆,利用RT－PCR检测rhHGF mRNA的表达通过ELISA法测定rhHGF的蛋白表达,3H掺入法检测培养上清液对大鼠原代培养肝细胞DNA合成的影响,结果表明转染pEE14/rhHGF的细胞可扩增出hHGF特异的396bp RT-PCR片段,培养上清液明显促进大鼠肝细胞DNA的合成,ELISA法测出上清液中,rhHGF的含量在8ug/L以上,显示rhHGF在CHO细胞中以活性形式得到表达。     

Construction and Co-expression of Grass Carp Reovirus VP6 Protein and Enhanced Green Fluorescence Protein in the Insect Cells

Grass carp reovirus(GCRV),a disaster agent to aquatic animals,belongs to Genus Aquareovirus of family Reoviridea.Sequence analysis revealed GCRV genome segment 8(s8) was 1 296 bp nucleotides in length encoding an inner capsid protein VP6 of about 43kDa.To obtain in vitro non-fusion expression of a GCRV VP6 protein containing a molecular of fluorescence reporter,the recombinant baculovirus,which contained the GCRVs8 and eGFP(enhanced green fluorescence protein) genes,was constructed by using the Bac-to-Bac insect expression system.In this study,the whole GCRVs8 and eGFP genes,amplified by PCR,were constructed into a pFastBacDual vector under polyhedron(PH) and p10 promoters,respectively.The constructed dual recombinant plasmid(pFbDGCRVs8/eGFP) was transformed into DH10Bac cells to obtain recombinant Bacmid(AcGCRVs8/eGFP) by transposition.Finally,the recombinant bacluovirus(vAcGCRVs8/eGFP) was obtained from transfected Sf9 insect cells.The green fluorescence that was expressed by transfected Sf9 cells was initially observed 3 days post transfection,and gradually enhanced and extended around 5 days culture in P1(Passage1) stock.The stable high level expression of recombinant protein was observed in P2 and subsequent passage budding virus(BV) stock.Additionally,PCR amplification from P1 and amplified P2 BV stock further confirmed the validity of the dual-recombinant baculovirus.Our results provide a foundation for expression and assembly of the GCRV structural protein in vitro.     

猪轮状病毒JL94株vp4全基因克隆及原核表达载体构建

根据GenBank已发表的猪轮状病毒vp4基因保守序列,设计一对引物扩增猪轮状病毒地方株JL94株vp4全基因;将扩增产物与载体pMD-18T连接进行序列测定并将测序结果同国外分离株进行序列比较。用限制性内切酶BamHI和SalI将vp4基因从pMD-18T-vp4切下;同样用BamHI和SalI双酶切表达载体pGEX-6P-1;将这2个双酶切产物连接并转化,通过酶切鉴定和PCR鉴定证明完成了vp4原核表达载体的构建。测序结果表明:vp4全基因长2362bp,JL94株同国外分离株BEN307株、Gottfried株vp4全基因片段核苷酸同源性分别为93.44%和69.43%;氨基酸同源性分别为96.06%和71.88%。说明JL94株同BEN-307株属同一VP4血清型,而同Gottfried株属于不同血清型。重组原核表达载体pGEX-6P1-vp4的构建为表达VP4蛋白,研制诊断性抗原和病毒重组活载体疫苗奠定了基础。     

Morphological Study of the Role of Calcium in the Assembly of the Rotavirus Outer Capsid Protein VP7

Maturation of rotavirus occurs in the endoplasmic reticulum (ER), a site of intracellular calcium storage. It was demonstrated previously that calcium plays an important role in the maturation of bovine rotavirus. We used protein A colloidal gold conjugated to an antibody to localize VP7, the outer capsid protein of the simian rotavius SA11, in permeabilized infected cells in the presence and absence of calcium in the culture medium. In medium containing calcium, VP7 was associated with nonenveloped double-shelled particles and membranous structures of the ER. In calcium-free medium, gold particles were not associated with the ER or with virus particles. Gold particles were distributed through the cytoplasm and were mainly associated with granular structures, but did not assemble onto virus particles. Our data suggest that in calcium-free medium, VP7 is synthesized, but does not remain incorporated, in the ER.