重组家蚕病毒表达系统转移载体的构建和β—半乳糖苷酶的表达

本文从中国农科院蚕业研究所提供的我国家蚕核多角体病毒镇江株中获得了多角体蛋白的强启动子,用此启动子构建了家蚕病毒表达系统的转移载体。外源基因能在此启动了控制下在家蚕细胞和虫体中进行高效表达。用此载体我们首先成功地在家蚕虫体中高效表达了β－半乳糖苷酶,表达量达到５８０μｇ／条蚕,从而证实我们构建的载体是可靠的,有效的,可用于家蚕重组病毒表达外源基因的研究。     

乙肝病毒s基因在家蚕细胞及蚕体内高效表达

把人乙型肝炎病毒(adr)的表面抗原S基因插入到家蚕核型多角体病毒基因组中,构建了重组病毒BmNPVS。用重组病毒感染家蚕细胞,测得每毫升培养物(1×10⁶细胞)HBsAg表达量达35．5μg;感染家蚕幼虫和蛹,经检测表明HBSAg产量平均为每头蚕约750μg,每只蛹约为690μg。初步纯化的表达产物经Westefn blotting和电镜观察证实,表达产物是直径为22nm的颗粒,并主要以糖基化形式存在。表达产物的浮力密度为1．2g／ml,与病人血清的HBsAg一致。     

江浙蝮蛇神经生长因子在家蚕幼虫中的表达

江浙蝮蛇神经生长因子（ＮＧＦ）基因克隆于昆虫病毒转移栽体ｐＢａｃＰＡＫ８中,获得重组转移栽体ｐＢａｃ－ＰＡＫ－ＮＧ〈与线性化Ｂｍ－ＡａｃＰＡＫ６修饰病基因组ＤＮＡ共转染家蚕细胞,经过体内重组,筛选到重组病毒。用重组病毒洒家蚕幼虫,５天后收集血淋巴,经ＳＤＳ－ＰＡＧＥ检测及利用ＰＣ１２细胞进行ＮＧＦ生物活力测定证明,神经生长因子在家蚕幼虫中得到较高表达,且表达产物具有良好的生物学活性     

家蚕核型多角体病毒ORF 75基因的克隆和表达

河南农业大学植保学院尹新明、安世恒、江志伟、胡鹏等博士、教授根据GenBank序列L33180设计引物用PCR技术扩增了编码家蚕核型多角体病毒bombyx mori nueleopolyhedrovirus,BmNPVORF75基因的DNA片段,将其连接至PMD18-T载体上,获得了该基因的成熟蛋白阅读框序列,用设计的酶切位点将目的基因从克隆载体上切下,     

家蚕病毒的表面增强拉曼光谱研究

得到并分析了家蚕核型多角体病毒（ＢｏｍｂｙｘｍｏｒｉＮｏｃｌｅａｒＰｏｌｙｈｅｄｒｏｓｉｓＶｉｒｕｓ缩写为ＢｍＮＰＶ）和质型多角体病毒（ＢｏｍｂｙｘｍｏｒｉｃｙｔｏｐｌａｓｍｉｃＰｏｌｙｈｅｄｒｏｓｉｓＶｉｒｕｓ缩写为ＢｍＣＰＶ）包涵体（即核型多角体ＢｍＮＰＢ和质型多角体ＢｍＣＰＢ）在银胶溶液中的表面增强拉曼散射（ＳＥＲＳ）光谱。ＢｍＮＰＢ和ＢｍＣＰＢ通过氨基酸残基侧链的Ｓ原子、ＣＯＯ－（ＣＯＯＨ）和ＮＨ２（ＮＨ）基团以及蛋白质分子的Ｎ－末端与银表面相作用。Ｔｒｐ残基金部或大部处于疏水环境中。ＢｍＮＰＢ中蛋氨酸残基侧链的Ｓ－ＣＨ２和ＣＨ２－ＣＨ２链分别为扭曲和扭曲式构型。ＢｍＣＰＢ中的Ｓ－ＣＨ２和ＣＨ２－ＣＨ２链则分别属于反式和扭曲构型;Ｃ－Ｃ－Ｓ－Ｓ－Ｃ－Ｃ链为反式－扭曲－反式结构。     

用杆状病毒载体在家蚕细胞中表达HBeAg基因

以ＰＣＲ技术扩增含有ＰｒｅＣ信号肽序列及完整的ＨＢｅＡｇ基因的序列（即ＨＢｃＡｇ基因５′端４４７ｂｐ）,在５′端加上合适的酶切位点,克隆到家蚕核多角体病毒转移载体ｐＢｍ０３０上,与野生型ＢｍＮＰＶＤＮＡ共转染家蚕ＢｍＮ细胞,空斑纯化后得到多角体基因失活的重组病毒。ＥＬＩＳＡ法测定表明培养液上清中ＨＢｅＡｇ效价达１∶３２０００,细胞内ＨＢｅＡｇ效价为１∶２０００,培养液及细胞内的ＨＢｃＡｇ含量极低（＜１∶１６０）。研究结果表明,ＢｍＮ细胞能正确识别与切割ＨＢｅＡｇ信号肽序列,所表达的ＨＢｅＡｇ效价高,纯度好,明显优于大肠杆菌表达系统     

以家蚕核型多角体病毒为载体高效表达天花粉蛋白基因

本文报道以家蚕核型多角体病毒为载体,在家蚕体内高效表达天花粉蛋白基因的结果。天花粉蛋白基因是用ＰＣＲ技术从栝楼基因组中分离的,该基因被插入到家蚕核型多角体病毒转移载体质粒ｐＢｍ-１的多角体蛋白基因启动子下游,构建成重组质粒ｐＢｍＴＣＳ。将重组质粒ＤＮＡ和野生型ＢｍＮＰＶＤＮＡ共转染家蚕培养细胞,通过在家蚕培养细胞中进行同源重组和筛选,获得了无多角体的重组病毒ＢｍＴＣＳ。采用ＰＣＲ技术对重组病毒进行了鉴定,证实重组病毒合天花粉蛋白基因。重组病毒对家蚕的感染性不及野生病毒,提示表达产物对病毒的增殖有抑制作用。对重组病毒感染的家蚕血淋巴进行了ＳＤＳ-ＰＡＧＥ和免疫印迹分析,结果显示在蚕体血淋巴中的表达产物天花粉蛋白占总蛋白的５％。本实验为利用基因工程方法大量生产天花粉蛋白提供了又一条新的途径。     

表达barnase基因的重组棉铃虫核型多角体病毒的构建及其杀虫活性研究

将含有 barnase基因与杆状病毒多角体基因 ( ph)的重组转座载体 p Fb- Bar在大肠杆菌中与含有棉铃虫核型多角体病毒 ( Ha NPV)的穿梭载体 Hanpvid转座并提取重组穿梭载体 DNA转染棉铃虫细胞 ,得到重组棉铃虫病毒 r Ha- Bar.其分子杂交证明 ,昆虫细胞中有 r Ha- Bar的 bar基因转录本存在 ,并能表达产生 33k D的多角体蛋白和 1 2 k D的 barnase.在平板上 ,barnase能降解RNA,出现清晰的降解圈 .r Ha- Bar对三龄棉铃虫幼虫的毒力比野生型 Ha NPV的 LD50 减少 2 0 % ,LT50 减少 30 % .用 barnase的拮抗基因 barstar构建了具有 Neo抗性、并能稳定表达 barstar的棉铃虫转化细胞 AM1 - NB.以携带 barnase基因的重组病毒 r Ha- Bar分别感染转化细胞和正常细胞 ,48h子代病毒在转化细胞中的产量比在正常细胞中高 2 3倍 ,72 h高 1 60倍 .     

A high efficient method of constructing recombinant Bombyx mori (silkworm) multiple nucleopolyhedrovirus based on zero‐background Tn7‐mediated transposition in Escherichia coli

A high efficient way for generation of recombinant Bombyx mori (silkworm) multiple nucleopolyhedrovirus by Tn7‐mediated transposition in Escherichia coli was performed. The new system consists of a conditional replication donor vector pRCDM and an attTn7 site blocked E. coli containing BmNPV‐Bacmid. The donor vector contains a replication origin derived from R6Kγ, which propagated only in host cells with pir gene expression decreased in the transposition background greatly. Compared with original vector derived from pUC, the transposition efficiency increased from 5.7 to 66% (≈10 fold) when using conditional replication vector pRCDM transposition into original BmDH10Bac. A further effort to decrease the transposition background was made by blocking the attTn7 site in host E. coli genome. The resulting attTn7 occupied BmDH10BacΔTn7 resulted in a significant increase from 5.7 to 23% (≈4 fold) in the efficacy of generate recombinant BmNPV Bacmid by transposition. Furthermore, the transposition of BmDH10BacΔTn7 with pRCDM resulted typically in 100% white colonies, and it indicated that a zero transposition background was accomplished. This high efficient and zero background transposition system provides a new simple and rapid method for construction of recombinant BmNPV used to express target genes or produce gene‐delivery virus particles in silkworm. © 2009 American Institute of Chemical Engineers Biotechnol. Prog., 2009     

Genomic Sequence Analysis of Bombyx mori Nucleopolyhedrovirus Isolated from Yunnan Sericulture Region,China

The blood pathogens of grasserie caused by Bombyx mori nucleopolyhedrovirus BmNPV have a serious impact on the sericulture industry. To understand the genetic status of BmNPV endemic strains in the Yunnan sericulture region, the structure and complete genome sequence of BmNPV isolated from Baoshan city of Yunnan Province were described and compared to known strains. The BmNPV-Baoshan isolate was a nucleopolyhedrovirus parasitized in silkworm larvae. Its genome has 128, 452 bp with a G + C content of 40.4%. Phylogenetic analysis clustered the virus with China BmNPV isolates; BmNPV-Baoshan was closely related to BomaNPV-S1 (both strains originated from the same ancestor). BmNPV-Baoshan strain has bro-b gene deletion, hr1 missing 4 repeat units of 30-bp palindrome structure compared to BmNPV-T3 strain. The aim of this study was to elucidate the evolution of the virus further and provide insights for the protection of virus-induced hematologic sepsis.     

Construction of the Bac-to-Bac System of Bombyx mori Nucleopolyhedroviru

To construct the Bac-to-Bac expression system of Bombyx mori nucleopolyhedrovirus(BmNPV),a transfer vector was constructed which contained an Escherichia coli(E.coli)mini-F replicon and a lacZ:attTN7:lacZ cassette within the upstream and downstream regions of the BmNPV polyhedrin gene.B.mori larvae were cotransfected with wild-type BmNPV genomic DNA and the transfer vector through subcutaneous injection to generate recombinant viruses by homologous recombination in vivo.The genomic DNA of budded viruses extracted from the hemolymph of the transfected larvae was used to transform E.coli DH10B.Recombinant bacmids were screened by kanamycin resistance,PCR and restriction enzyme(REN)digestion.One of the bacmid colonies,BmBacJS13,which had similar REN profiles to that of wild-type BmNPV,was selected for further research.To investigate the infectivity of BmBacJS13,the polyhedrin gene was introduced into the bacmid and the resultant recombinant(BmBacJS13-ph)was transfected to BmN cells.The budded viruses were collected from the supernatant of the transfected cells and used for infecting BmN cells.Growth curve analysis indicated that BmBacJS13-ph had a similar growth curve to that of wild-type BmNPV.Bio-assays indicated that BmBacJS13-ph was also infectious to B.mori larvae.     

Construction of the Bac-to-Bac System of Bombyx mori Nucleopolyhedroviru

To construct the Bac-to-Bac expression system of Bombyx mori nucleopolyhedrovirus (BmNPV), a transfer vector was constructed which contained an Escherichia coli (E. coli) mini-F replicon and a lacZ: attTN7: lacZ cassette within the upstream and downstream regions of the BmNPV polyhedrin gene. B. mori larvae were cotransfected with wild-type BmNPV genomic DNA and the transfer vector through subcutaneous injection to generate recombinant viruses by homologous recombination in vivo. The genomic DNA of budded viruses extracted from the hemolymph of the transfected larvae was used to transform E. coli DH10B. Recombinant bacmids were screened by kanamycin resistance, PCR and restriction enzyme (REN) digestion. One of the bacmid colonies, BmBacJS13, which had similar REN profiles to that of wild-type BmNPV, was selected for further research. To investigate the infectivity of BmBacJS13, the polyhedrin gene was introduced into the bacmid and the resultant recombinant (BmBacJS13-ph) was transfected to BmN cells. The budded viruses were collected from the supernatant of the transfected cells and used for infecting BmN cells. Growth curve analysis indicated that BmBacJS13-ph had a similar growth curve to that of wild-type BmNPV. Bio-assays indicated that BmBacJS13-ph was also infectious to B. mori larvae.     

家蚕核型多角体病毒BmNPV囊膜蛋白P74膜外区克隆和原核表达

通过PCR扩增家蚕核型多角体病毒(Bombyx mori nucleopolyhedrovirus,BmNPV)囊膜蛋白p74基因膜外区片段,对切胶纯化得到的DNA目的片段与原核表达载体pET28a进行连接,通过不同浓度的IPTG对含有pET28a-p74重组质粒的大肠杆菌BL21(DE3)进行诱导,对诱导产物进行SDS-PAGE电泳.结果表明p74基因膜外区获得了表达;通过His单抗对原核表达产物进行Western blotting分析,其结果证实诱导蛋白带为融合有组氧酸的目的蛋白.对割胶获得的P74蛋白和免疫佐剂进行克分研磨,以研磨后的匀浆液对昆明小鼠进行皮下多点注射,通过收获的抗血清对BmNPV ODV病毒粒子进行Westem blotting分析,检测到一条分子量大小为74 kD的特异杂交带,表明获得的多抗可用于P74蛋白功能的进一步研究.     

Recognition of signal peptide by protein translocation machinery in middle silk gland of silkworm Bombyx mori

To investigate the functions of signal peptide in protein secretion in the middle silk gland of silkworm Bombyx mori, a series of recombinant Autographa californica multiple nucleopolyhedroviruses containing enhanced green fluorescent protein （egfp） gene, led by sericin-1 promoter and mutated signal peptide coding sequences, were constructed by region-deletions or single amino acid residue deletions. The recombinant Autographa californica multiple nucleopolyhedroviruses were injected into the hemocoele of newly ecdysed fifth-instar silkworm larvae. The expression and secretion of EGFP in the middle silk gland were examined by fluorescence microscopy and Western blot analysis. Results showed that even with a large part （up to 14 amino acid residues） of the ser-1 signal peptide deleted, the expressed EGFP could still be secreted into the cavity of the silk gland. Western blot analysis showed that shortening of the signal peptide from the C-terminal suppressed the maturation of pro-EGFP to EGFP. When 8 amino acid residues were deleted from the C-terminal of the signal peptide （mutant 13 aa）, the secretion of EGFP was incomplete, implicating the importance of proper coupling of the h-region and c-region. The deletion of amino acid residue（s） in the h-region did not affect the secretion of EGFP, indicating that the recognition of signal peptide by translocation machinery was mainly by a structural domain, but not by special amino acid residue（s）. Furthermore, the deletion ofArg^2 or replacement with Asp in the n-region of the signal peptide did not influence secretion of EGFP, suggesting that a positive charge is not crucial.     

重组家蚕病毒表达传染性法氏囊病病毒VP2蛋白

将传染性囊病病毒ＨＺ９６株主要宿主保护性抗原ＶＰ２的ｃＤＮＡ基因克隆到杆状病毒转移载体ｐＢａｃ－ＰＡＫ８中,获得重组转移载体ｐＢａｃＰＡＫ－ＶＰ２,载体ｐＢａｃＰＡＫ－ＶＰ２与修饰病毒Ｂｍ－ＢａｃＰＡＫ６线性化基因组ＤＮＡ共转染单层家蚕Ｂｏｍｂｙｘ ｍｏｒｉ（Ｂｍ）Ｎ细胞,经细胞内同源重组,筛选到重组病毒。ＥＬＩＳＡ和Ｗｅｓｔｅｒｎ免疫鲩迹结果表明,ＶＰ２在家蚕培养细胞和家蚕幼虫中均得到了表达。     

家蚕CPV感染离体细胞的电镜观察

本文报道了BmCPV感染家蚕细胞系后的电镜观察。病毒感染早期,细胞质内形成电子致密的病毒发生基质,由病毒发生基质形成BmCPV球状病毒粒子;病毒感染48小时后,多角体在病毒发生基质周围形成,大量的病毒粒子随机包埋在多角体内;病毒接种后96小时,多角体数目增多,其形状有三角,四角,五角及六角形,细胞质内充盈多角体致使细胞核被挤向细胞一侧并伴有形态的改变,受染细胞约为40％。     

家蚕近交系遗传纯度的RAPD检测

目的分析家蚕近交系IS-c108A的遗传纯度,为家蚕实验动物化的培育工作提供指导。方法应用经过筛选的20条随机引物对家蚕近交系IS-c108A(F10)的3个蛾区各30个个体和该近交系的亲本系统c108、对照实用化品种871各30个个体的基因组DNA进行RAPD扩增,计算个体间和蛾区间的相似系数及遗传距离。结果家蚕近交系IS-c108A(F10)的3个蛾区内的多态性带频率分别为1.807%、1.841%、1.841%,平均为1.830%;起点亲本c108个体间多态性带频率为7.207%,对照品种871个体间的多态性带频率为7.08%;而近交系IS-c108A与c108之间的多态性带频率为49.20%,c108和871品种之间的多态性带频率为58.33%。家蚕近交系IS-c108A10的3个蛾区内个体之间遗传相似系数的平均值分别为0.99581、0.99555、0.99551,总平均为0.99562。结论家蚕近交系IS-c108A(F10)已具有较高的遗传纯合度,家蚕具有易于获得高纯的有利条件。     

激光诱发家蚕孤雌生殖的研究

采用 CO2激光扩束辐照诱发家蚕孤雌生殖,获得着色卵率约60%,转青卵率约31%,孵化率只占转青率的1.85%,全是雌蚕,其发育机制属非减数分裂型,没有出现畸形蚕,茧质未下降。从激光诱发的孤雌生殖的后代中,初步选出两个新类型的可作育种材料。 Abstrect:In order to induce silkworm(Bombyx mori)parthenogenesis,we irradiated eggs by Co2 laser.The results showed,60% colored eggs,31% average bluish eggs,only 1.85% hatchavility among the bluish eggs,all female from those eggs and so an ameiosis parthenogenesis;no malformed worm,thus similar constitution and quality to their parents;and finally two new strains which can be used to breed new strains and furhther studies.