表达鸡传染性支气管炎病毒SD/97/01株S1蛋白的重组杆状病毒的构建

采用BAC－TO－BAC杆状病毒表达载体体系构建了表达鸡传染性支管炎病毒（IBV）呼吸型毒株SD／97／01S1蛋白的重组杆病病毒，含SD／97／01株S1基因原重组质粒p MDSD9701S1用BamHI和SalI双酶切后，回收的片段并克琶杆病病毒转座载体pFASTBACHTa中多角体基因启动子的下游，筛选出重组转座质粒pFASTSD9701S1U并转化大肠杆菌DH10BAC后,获得重组穿梭质粒rBacmidSD9701S1，用重组穿俊质粒DNA转染昆虫Sf9细胞，获得了含SD／97／01S1基因的重组杆状病毒rAcSD9701S1，重组病毒感染Sf9细胞后，用SDS－PAGE、Westernblot和IFA对细胞表达产物进行检测和分析。结果表明：构建的重组杆状病毒能够在昆虫细胞中表达SD／97／01的S1蛋白，该蛋白具有天然蛋白的抗原性。     

Construction and identification of reverse genetics system of Dengue type 2 virus isolated in China

Dengue (DEN) viruses, mosquito-borne pathogens of the Flavivirus genus, Flaviviridae family, are envel- oped RNA viruses that contain a single-stranded, posi- tive-sense, capped RNA genome of approximately 11 kb. Single polypeptide is co-translationlly pr…     

Cloning, construction of prokaryotic expression vector and expression ofEscherichia coli cytosine deaminase gene

Cytosine deaminase gene ofEscherichia coli strain H-30 was cloned, and its initiation codon of ‘GTG’ was mutated to ‘ATG’ by PCR. Prokaryotic recombinant expression vector pBV220-CD was constructed. Clone with high enzyme activity were selected by detecting their specific activity of cytosine deaminase. 5-FC(5-FC, 5-fluorocytosine) could induce the lethal toxicity to cells containing active CD gene. DNA sequence analysis indicated that there were 16 altered bases and 5 of them resulted in the alteration of amino acids in predicted peptide by comparing DNA sequence of the clone H-30-CD-11 with high enzyme activity with CD gene reported in Gene Bank.     

抗口蹄疫病毒phage-scFv及可溶性scFv的构建

利用重组DNA技术在抗口蹄疫病毒单克隆抗体1C 7 VH基因和VL基因之间导入一段连接肽[(G ly4Ser)3],采用重叠延伸拼接法,经聚合酶链反应(PCR)扩增获得scF v基因。将scF v基因克隆至噬菌粒pCANTAB 5E载体,转化E.coli TG 1,构建噬菌体抗体文库。用M 13KO 7辅助噬菌体挽救及固相口蹄疫病毒(FMDV)抗原对噬菌体抗体文库的三轮“吸附-洗脱-扩增”的淘洗,筛选出scFv阳性克隆。将阳性克隆转化E.coli BH 2151,通过异丙基硫代-β-D-半乳糖苷(IPTG)诱导可溶性scFv蛋白的表达。酶联免疫吸附实验(EL ISA)检测表明:scFv克隆表达的phage-scFv及可溶性scFv与FMDV亲和力高,特异性强。     

携带p53基因重组腺病毒载体的构建

将pCMVp53重组转移载体经BamHI和NheI酶切,得到p53基因cDNA,然后将cDNA片段克隆到转移载体pCMV5GFP,使其受CMV5启动子的调控,获得pCMV5p53重组转移载体.用该线状重组转移载体与腺病毒右臂DNA经磷酸钙共转染293细胞获得重组腺病毒,经酶联免疫吸附法(ELISA)测定p53蛋白含量,证明外源p53基因在含重组腺病毒的293细胞中得到表达.     

Ⅰ型单纯疱疹病毒包膜糖蛋白L基因片段的克隆及高效表达

 采用PCR方法扩增HSV-1病毒型特异性包膜糖蛋白L(gL)基因片段并克隆至原核表达载体pGEX-5X-1获得重组质粒pGEX-5X-1-gL,将重组质粒转化E.coli BL21表达菌后经IPTG诱导表达目的蛋白.SDS-PAGE蛋白检测表明,在分子质量56 ku处有HSV-1 GST-gL融合蛋白的高效表达,通过IPTG浓度筛选和诱导前表达菌扩增培养时间的比较分析对诱导条件进行了优化,GST-gL融合蛋白表达量可达到菌体蛋白总量的48.65%.Western blot中利用HSV-1灭活病毒获得的多克隆抗体确证所表达蛋白为HSV-1病毒组分.这一表达系统的建立和优化对进一步探讨HSV-1 gL蛋白功能及其免疫原性提供了有利条件.     

新城疫病毒TL1株P、NP、L蛋白基因表达载体的构建及鉴定

将新城疫病毒TL1株的P、NP、L基因通过RT-PCR方法从尿囊液中扩增后分别克隆进pGEM-Teasy载体,再分别亚克隆到真核表达载体pCI-neo上,命名为pCI-P、pCI-NP、pCI-L,通过酶切、PCR和测序验证克隆正确.纯化后的重组质粒单独转染BHK-21细胞,经间接免疫荧光试验检测到了P、NP、L蛋白的表达.新城疫病毒TL1株的P、NP、L基因的克隆成功,为即将进行的新城疫病毒的反向遗传操作奠定了基础.     

香石竹斑驳病毒（CarMVsh）外壳蛋白基因克隆及原核表达

香石竹斑驳病毒上海分离株是从上海地区栽培的香石竹上分离并鉴定的,以提纯的病毒为材料,ＳＤＳ－酚法纯化的基因组ＲＮＡ作为模板,ＲＴ－ＰＣＲ合成并扩增外壳蛋白基因ｃＤＮＡ,ｃＤＮＡ克隆于ｐＧＥＭ－Ｔ ｅａｓｙ ｖｅｃｔｏｒ,转化为Ｅ．ｃｏｌｉＪＭ１０９。阳笥克隆ｐＴＣａＣＰ经序列分析,证明带有全长ＣＰ基因。     

新基因Splt137在大肠杆菌中的表达及抗体制备

用PCR的方法扩增得到斜纹夜蛾核多角体病毒 (SpltMNPV)ORF137全长基因 (Splt137)。将其克隆到原核表达载体pQE30上 ,并转化大肠杆菌M15 ,在IPTG诱导下表达了与预期相对分子质量相符的一个 2 7× 10 7的蛋白质 ,经过聚丙烯酰氨凝胶电泳纯化 ,免疫家兔制备了抗Splt137抗体。Western免疫印迹分析表明 ,该抗体适合用作Splt137蛋白的进一步分析。     

Combined immunity of DNA vector and recombinant vaccinia virus expressing Gag proteins of equine infectious anemia virus

In order to develop a new vaccine candidate for equine infectious anemia virus (EIAV), gag gene of Chinese donkey leukocyte attenuated strain (EIAV DLV) and its parental virulent strain (EIAV LN) were inserted respectively into the TK region of the Tiantan strain (VV) of vaccinia virus by homologous recombination and the positive clone was confirmed by blue plaque assay. Protein expression was examined by Western blot. Prime and prime-boost procedures were used to immunize mice with two DNA vectors and two recombinant vaccinia viruses expressing EIAV Gag proteins. The results showed that the specific lysis of CTL responses in the DNA rVV groups was stronger than those in the DNA groups, amounting to 31%. Although the levels of specific antibodies were not significantly different, we could conclude that the recombinant vaccinia virus could boost the cellular responses following DNA vector priming. There was no detectable difference between the immune responses induced by DLV and LN Gag proteins. This data demonstrates that the combined immunity of DNA vector and recombinant vaccinia virus expressing EIAV gag proteins, utilizing the prime-boost procedure, can drive immunized mice to produce powerful cellular responses. These results lay an important foundation for the development of a new EIAV genetic engineering vaccine.     

Construction of transposon-mediated baculovirus vector and expression of green fluorescent protein in insect cells and larvae

A transposon-shuttle vector Hanpvid was constructed by using wild-type genomic DNA fromHeliothis armigera nuclear polyhedrosis virus (HaNPV). It could replicate inE. coli cells as a large plasmid and remain infectious when being induced into insect cells. Hanpvid comprises HaNPV DNA and a transposon cassette which includes a miniF replicon, a kanamycin resistance gene (kan), lacZa and an attachment site for Tn7 (attTn7). Recombinant virus rHa-FaGP was obtained after transposition of a donor plasmid carrying green fluorescent protein gene (gfp) and polyhedrin gene (ocu) into attTn7. SDS-PAGE analysis shows that both gfp and ocu genes were highly expressed inHeliothis armigera cells. Green Hemolymphocytes can be seen under a fluorescent microscope 4 d after recombinant virus rHa-FaGP infected the third-instar larvae. The infected larvae show strong green fluorescence 6 d post infection.     

Molecular cloning and expression of Pfu DNA polymerase gene and its application in long-distance PCR

A 2.3 kb DNA fragment containing Pfu DNA polA gene was amplified by PCR from total DNA of Pyrococcus furiosus and cloned into a pGEM-T vector. The recombinant clone pT-pfu was digested with Nco I and Xho I and the fragment was inserted into an expression vector pET3d-X. The Pfu polA gene was expressed in Escherichia coli BL21 (DE3). The gene product (Pfu) was purified with heat denaturation, polyethylenemine (PEI) precipitation and Bio-rex 70 ion-exchange chromatography. The recombinant Pfu was verified by protein N-terminal sequencing. With the recombinant Pfu, large λ DNA fragments were successfully amplified in long-distance PCR.     

嗜酸乳杆菌亚油酸异构酶基因的克隆与表达

利用分子生物学方法对嗜酸乳杆菌AS1.1854菌株的亚油酸异构酶基因进行克隆与表达.培养菌体后提取总DNA,用PCR法扩增其亚油酸异构酶基因,再将其克隆到pET30a载体上,转入到大肠杆菌BL21株中表达,在低温下诱导表达出重组蛋白,并用Ni2 金属鳌合层析对重组蛋白进行分离和纯化.通过实验,得到了亚油酸异构酶的基因,成功转入到载体中,表达出了可溶性的重组蛋白,并对其进行了纯化.实验表明,在原核细胞中可以表达出可溶性重组亚油酸异构酶,以200 mmol/L的咪唑洗脱液进行洗脱可以获得目标蛋白.     

乙型肝炎病毒HBX基因的克隆、表达和蛋白的纯化

克隆乙肝病毒X基因,并在大肠杆菌中进行表达和纯化。用PCR方法从结乙肝病毒基因组扩增出HBX基因片段,克隆至pMD18-T载体中。序列测定正确后,将其亚克隆到表达载体pProExHTa并在大肠杆菌BL21中表达。表达蛋白经SDS-PAG及Western-blot分析后,亲和层析法纯化蛋白。结果成功克隆了HBX基因,并对其在E.coli中进行了表达。SDS-PAGE及Western blot分析表明表达产物正确。通过IMAC纯化系统获得17 kD纯化蛋白,与文献报道相符。结果成功获得了纯化的HBX蛋白,为进一步研究HBX蛋白与宿主蛋白之间的相互作用奠定基础。     

汉滩病毒囊膜糖蛋白g2基因重组腺病毒的构建与表达

获得汉滩病毒G2 基因 ,构建其重组腺病毒并在HEK2 93细胞中包装表达 ,为研究汉滩病毒基因疫苗提供了实验基础。设计引物采用PCR从含汉滩病毒 \|76 1 1 8株M基因的M5 6质粒扩增出糖蛋白G2 基因片段 ,并将其克隆入腺病毒载体Adeno XviralDNA ,筛选获得重组腺病毒DNA ,转染HEK2 93细胞 ,包装、扩增后得到汉滩病毒G2 基因重组腺病毒原种 ;并在感染细胞内初步表达 ,用ELISA检测表达产物。得到了含汉滩病毒G2 基因的重组腺病毒 ,其滴度约为 1 0 10 pfu/mL ,同时在感染的HEK2 93细胞中检测到汉滩病毒糖蛋白G2 的表达。含汉滩病毒糖蛋白G2 基因重组腺病毒的成功构建 ,为研究汉滩病毒基因疫苗提供了实验基础     

Function of resveratrol derived from transgenic plant expressing resveratrol synthase gene

Two genes from grapevine coding for resveratrol synthase, named RS1 and RS2, were cloned by RT-PCR. AnEscherichia coli expression vector was constructed by insertion of RS1 into pBV221. A specific protein with the same molecular weight (42 ku) as the resveratrol synthase was expressed and used to prepare the rabbit antiserum. A plant expression vector was constructed by inserting the RS1 gene into pBin438 downstream of the doubled CaMV 35S promoter and TMV-Ω fragment. PCR-positive transgenic tobacco plants were obtained after transformation withAgrobacterium tumefaciens LBA4404 harboring the plant expression vector. Southern blot analysis demonstrated that the foreign gene was integrated into the tobacco genome. The results of RT-PCR and Western blot indicated that the RS1 gene was transcribed and expressed. Formation of resveratrol in transgenic tobacco was further determined by thin-layer chromatography of silica gel and HPLC. Increased accumulation of human breast adenocarcinoma cells in G₀ and G₁ phases of cell cycle was observed in cells treated with resveratrol purified from transgenic tobacco as compared to the untreated cells.     

Enhanced virulence of influenza A viruses with the haemagglutinin of the 1918 pandemic virus

The 'Spanish' influenza pandemic of 1918-19 was the most devastating outbreak of infectious disease in recorded history. At least 20 million people died from their illness, which was characterized by an unusually severe and rapid clinical course. The complete sequencing of several genes of the 1918 influenza virus has made it possible to study the functions of the proteins encoded by these genes in viruses generated by reverse genetics, a technique that permits the generation of infectious viruses entirely from cloned complementary DNA. Thus, to identify properties of the 1918 pandemic influenza A strain that might be related to its extraordinary virulence, viruses were produced containing the viral haemagglutinin (HA) and neuraminidase (NA) genes of the 1918 strain. The HA of this strain supports the pathogenicity of a mouse-adapted virus in this animal. Here we demonstrate that the HA of the 1918 virus confers enhanced pathogenicity in mice to recent human viruses that are otherwise non-pathogenic in this host. Moreover, these highly virulent recombinant viruses expressing the 1918 viral HA could infect the entire lung and induce high levels of macrophage-derived chemokines and cytokines, which resulted in infiltration of inflammatory cells and severe haemorrhage, hallmarks of the illness produced during the original pandemic.     

Expression of human β-subunit nerve growth factor (hNGFB) in yeast Pichia pastoris and E. coli

The gene hNGFB encoding the β subunit of human nerve growth factor (hNGF) was cloned intoP. pastoris secretive expression vector pHIL-S1 andE. coli expression vector pET-15b. The recombinant hNGFB vectors pSNGF and pET15b-NGF were transformed intoP. pastoris host cell GS115 (Mut⁺, His⁻) andE. coli strain BL21 (DE3) respectively. Expression and secretion of hNGFB inP. pastoris was attempted under the direction of the AOX1 promoter and PHO1 signal sequence. The positive colonies growing on medium without histidine were further selected by PCR. The yield of rehNGFB in GS115 was about 14.4% of total cellular secretive protein. The secreted protein was immunological active on Western blotting with rabbit anti-mNGFB antibodies. The fusion protein yield of rehNGFB inE. coli BL21 (DE3) was about 10.3% of total cellular protein after IPTG induction. Western blot detection showed its immunological activity.     

Construction of DNA damage response gene pprI functiondeficient and function-complementary mutants in Deinococcus radiodurans

PprI, a DNA damage response factor from the extraordinary radioresistant bacterium Deinococcus radiodurans, plays a central regulatory role in multiple DNA damage repair. In this study, a fusion DNA fragment carrying kanamycin resistance gene with the D. radiodurans groEL promoter was cloned by PCR amplification and reversely inserted into the pprl locus in the genome of the wild-type strain R1. The resultingpprl-deficient strain, designated YR1,was very sensitive to ionizing radiation. Meanwhile, the recombinant DNA fragment was cloned into the shuttle vector pRADZ3, and resulted in plasmid pRADK with kanamycin resistance in D. radiodurans. The fragments containing complete pprl gene and 3‘-terminal deletion pprIΔ were cloned into plasmid pRADK. The resulted plasmids designated pRADKpprI and pRADKpprIΔ were then transformed to YR1. Results show that YR1 carrying pRADKpprI was able to fully restore the extreme radioresistance to the same level as the wild-type D. raiodurans R1, whereas YR1 pRADKpprIΔ failed to do so. Construction of DNA repair switch PprI function-deficient and function-complementary mutants in D. radiodurans is not only useful to elucidating the relationship between domains and functions of PprI protein, but also opens the door to the further studies of the biological functions of PprI protein in vivo.     

结核分枝杆菌Rv2450基因真核表达质粒的构建及表达

构建结核分枝杆菌Rv2450基因真核表达载体.PCR扩增Rv2450基因,测序正确后克隆入真核表达载体pCDNA3.1（-）,重组质粒酶切鉴定正确后以阳离子聚合物转染P815细胞,分别以RT-PCR方法检测mRNA表达和间接免疫荧光技术检测目的蛋白的表达.结果构建了重组质粒pCDNA-Rv2450,RT-PCR结果证明Rv2450可在P815细胞中转录,用间接免疫荧光检测,表达有Rv2450蛋白的细胞着染.成功构建了结核分枝杆菌Rv2450基因的真核表达载体pCDNA-Rv2450,Rv2450基因可以在P815细胞中表达.