人GDNF在甲醇酵母及家蚕幼虫中的表达

将人胶质细胞源性神经营养因子(GDNF)基因克隆入酵母分泌型表达载体pPIC9K中,酶切线性化后电穿孔导入酵母细胞进行整合,经G418筛选得到多拷贝转化子,甲醇诱导表达。将人GDNF基因克隆入昆虫病毒转移载体pBacPAK8中,与线性化Bm-BacPAK6修饰病毒基因组DNA共转染家蚕细胞,经体内重组,筛选到重组病毒。用重组病毒感染家蚕幼虫,5d后收集血淋巴。SDS-PAGE和蛋白质印迹杂交结果证实了酵母培养上清液及家蚕幼虫血淋巴中含有GDNF蛋白。活性研究表明,甲醇酵母及家蚕幼虫表达的GDNF蛋白能促进多巴胺能神经元的存活和突起生长。     

人白细胞介素-11基因在家蚕培养细胞和虫体内的表达

将缺少编码信号肽序列的人白细胞介素－11（hIL-11)546核苷酸cDNA,重组于质粒pBacPAK8构建重组转移载体pBacIL-11,与经线性化修饰的家蚕核型多角体病毒（BmBacPAK)DNA共转染家蚕培养细胞株BmN,获得了插入hIL-11基因的重组病毒。Southern杂交表明重组病毒基因组中含有hIL-11基因片段,RNA斑点杂交表明hIL-11基因得到了转录。重组病毒感BmN细胞株、家蚕幼虫和蛹,在细胞培养上清、细胞抽提物、幼虫和蛹的体液样品中,SDS－PAGE电泳分析都能检测得到表达产物的特异性条带;采用IL－11依赖细胞株B9－11和MTT法测定表达产物的生物活性,表明rIL-11基因分别在培养细胞和蚕体内得到了高效表达。     

人白细胞介素-11基因在家蚕培养细胞和虫体内的表达

将缺少编码信号肽序列的人白细胞介素 11(hIL 11) 5 46核苷酸cDNA ,重组于质粒pBacPAK8构建重组转移载体pBacIL 11,与经线性化修饰的家蚕核型多角体病毒 (BmBacPAK)DNA共转染家蚕培养细胞株BmN ,获得了插入hIL 11基因的重组病毒。Southern杂交表明重组病毒基因组中含有hIL 11基因片段 ,RNA斑点杂交表明hIL 11基因得到了转录。重组病毒感染BmN细胞株、家蚕幼虫和蛹 ,在细胞培养上清、细胞抽提物、幼虫和蛹的体液样品中 ,SDS PAGE电泳分析都能检测得到表达产物的特异性条带 ;采用IL 11依赖细胞株B9- 1 1 和MTT法测定表达产物的生物活性 ,表明hIL 11基因分别在培养细胞和蚕体内得到了高效表达     

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。     

用构建的新型BmNPV载体在家蚕高效表达人β-干扰素

家蚕核多角体病毒(Bombyx mori Nuclear Polyhedrosis Virus.BmNPV)和家蚕细胞已成功地用来大量生产具有生物活性的重组蛋白。但是BmNPV的通用载体的类型较少。因此,本实验构建了BmNPV新型载体pBm92,该载体将多角体蛋白基因的起始密码ATG改变为ATT,然后在多角体蛋白基因的 12位外连接有5个外源基因的克隆位点。将HuIFN-β基因克隆在多角体蛋白基因的 12位后,构建了pBmIFN 12;同时构建HuIFN-β克隆在-3位后的转移栽体pBmIFN-3。将两种转移载体DNA分别与BmNPV基因组DNA共转染Bm-N细胞。利用重组病毒不产生多角体蛋白的特征,筛选重组病毒。用HuIFN-β基因探针与重组病毒DNA进行杂交鉴定。重组病毒BmIFN 12感染Bm-N细胞,其上清IFN活性最高时可达2.0×10~6IU/ml,将BmIFN 12注射5龄家蚕虫体,表达水平为50×10~7IU/ml,是HuIFN-β基因克隆在多角体蛋白基因的-3位后获得的重组病毒的表达量的2～4倍。家蚕体生产的rHulFN-β为糖基化蛋白具有天然HuIFN-β的抗原性。     

人血管抑素（k1—3）在家蚕细胞和幼虫中的表达及活性测定

将人血管抑素 (angiostatin)基因重组于家蚕杆状病毒转移载体 pBacPAK8中 ,获得重组转移载体pBacPAK angiostatin ,并与被线性化的Bm BacPAK6病毒DNA共转染家蚕细胞 ,获得重组病毒BacPAK angiostatin。DNA点杂交结果表明重组病毒基因组中含有血管抑素基因。重组病毒以MOI=10感染家蚕细胞 (2×10 6个细胞 /瓶 )和家蚕 5龄幼虫 ,表达产物用体外培养的人脐静脉血管内皮细胞 (ECV30 4 )及体内鸡胚尿囊膜(CAM)新生血管实验检测其抑制活性 ,测得血管抑素可明显抑制体外培养的内皮细胞增殖 ,家蚕细胞的产物活性在表达 72h达到最高值 ,在 2× 10 6个细胞中的表达量约 2 2u ;在家蚕体内表达 14 4h生物活性达到最高值 ,表达量约 15 9u/ml。2 .5u/ml的血管抑素能使ECV30 4细胞在 2 4h发生明显凋亡 ;可使CAM新生血管化率明显下降。此外 ,用ELISA、Western印迹方法测定了表达产物的免疫反应性。     

传染性法氏囊病病毒多聚蛋白基因在家蚕中的表达

将传染性法氏囊病病毒(IBDV)细胞致弱株(JD1株)的基因组A节段基因重组于家蚕杆状病毒转移载体pAcHLT-C中,获得的重组转移载体pAcHLT-C-A与线性化病毒Bm-BacPAK6 DNA共转染家蚕培养细胞,获得重组病毒BacPAK-A。DIG标记的DNA点杂交证实重组病毒基因组中含有A节段基因,重组病毒感染家蚕5龄幼虫进行表达, ELISA和Western blotting等结果表明多聚蛋白基因在蚕体内得到了表达,表达产物具有免疫反应性,表达量在感染后5～6 d达到最高。家蚕生物反应器表达IBDV多聚蛋白具有我国的资源优势,为今后研制低成本、实用化的IBDV基因工程疫苗打下基础。     

中国人促红细胞生成素cDNA的克隆及其在COS—7细胞中的表达

利用PCR技术,以中国人促红细胞生成素(EPO)次全基因组为模板,进行了基因修补和重组,克隆出EPO cDNA全序列。同时发现中国人EPO cDNA与国外的克隆比较有一个核苷酸的差异,导致第62位氨基酸是丝氨酸,不是亮氨酸。将人EPO cDNA基因插入表达载体pSV2-dhfr中的不同克隆位点,构建了6种不同的转移载体质粒,即pSV2-dhfr/F1,pSV2/N2,pSV2-dhfr/F3,pSV2-dhfr/P4,pSV2-dhfr/G1和pSV2-dhfr/G3。将它们分别转染导入COS-7细胞,结果表明6种转移载体质粒转染的细胞上清液都有明显的EPO活性。人EPO cDNA基因转移载体质粒在COS-7细胞中的表达水平高于人次全EPO基因组转移载体质粒。     

中国人促红细胞生成素cDNA的克隆及其在COS-7细胞中的表达

利用PCR技术。以中国人促红细胞生成素(EPO)次全基因组为模板,进行了基因修补和重组．克隆出EPO cDNA全序列。同时发现中国人EPO cDNA与国外的克隆比较有一个核苷酸的差异,导致第62位氨基酸是丝氨酸．不是亮氨酸。将人EPO cDNA基因插入表达载体pSV2-dhfr中的不同克隆位点,构建了6种不同的转移载体质粒,即psV2 dhfr／F1,pSV2／F2,pSV2 dbfT／F3,pSV2 dhfr／F4,pSV2-dhfr／G1和psV2 dhfr／G3。将它们分别转染导人COS-7细胞,结果表明6种转移载体质粒转染的细胞上清液都有明显的EPO活性。人EPO cDNA基因转移载体质粒在COS-7细胞中的表达水平高于人次全EPO基因组转移载体质粒。     

家蚕血淋巴体外黑化观察及相关黑色素合成催化酶基因

观察不同生长期家蚕幼虫血淋巴在体外的黑化速度和对大肠杆菌生长的影响结果显示,随食桑生长幼虫血淋巴的黑化速度逐渐变快,对大肠杆菌生长的抑制作用逐渐增强。RT-PCR实验显示,黑色素合成催化酶Bm Tan、Bm Po-1、Bm Yellow-f和Bm Ddc等的基因在家蚕5 L 3 d血淋巴中表达量高,Bm Black、Bm Yellow和Bm Pah等的基因也有明显表达。q PCR分析显示,黑化病蚕中Bmtan、Bmddc、Bmyellow、Bmebony和Bmblack,尤其Bmddc表达发生了显著上调。与对照相比,Ddc酶的抑制剂能显著抑制脂多糖对血淋巴的诱导黑化作用。用大肠杆菌注射家蚕幼虫,血淋巴中多巴和多巴胺的含量明显上升。这些表明家蚕幼虫血淋巴黑化与防御免疫有关,Bmddc很可能在幼虫血淋巴的免疫黑化中发挥作用。     

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。     

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.     

Biosynthesis of recombinant human hepatitis B M-HBsAg in silkworm larvae

The middle surface antigen (M-HBsAg) of human hepatitis B virus is virus envelope protein. It's used as a basis for development of vaccine and test-system for detecting of hepatitis B virus. The cDNA of M-HBsAg was inserted into transfer vector pBK273 under the polyhedron promoter with obtaining of recombinant plasmid DNA pBHep-2. As a result of cotransfection pBHep-2 with wild type BmNPV the recombinant baculovirus rBmNPVHep which included the cDNA of M-HBsAg under the polyhedron promoter was obtained. Infection of silkworm larvae Bombyx mori with recombinant virus resulted in expression of foreign gene and accumulation of middle surface antigen of human hepatitis B virus mostly (>90%) in fat bodies of silkworm 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.     

High-level expression of secreted complex glycosylated recombinant human erythropoietin in the Physcomitrella Delta-fuc-t Delta-xyl-t mutant

The highly glycosylated peptide hormone erythropoietin (EPO) plays a key role in the regulation of erythrocyte maturation. Currently, marketed EPO is produced by recombinant technology in mammalian cell cultures. The complementary DNA (cDNA) for human EPO (hEPO) was transiently and stably expressed in the moss Physcomitrella patens wild-type and Δ-fuc-t Δ-xyl-t mutant, the latter containing N -glycans lacking the plant-specific, core-bound α1,3-fucose and β1,2-xylose. New expression vectors were designed based on a Physcomitrella ubiquitin gene-derived promoter for the expression of hEPO cDNA. Transient expression in protoplasts was much stronger at 10 than at 20 °C. In Western blot analysis, the molecular size of moss-produced recombinant human EPO (rhEPO) was identified to be 30 kDa, and it accumulated in the medium of transiently transformed protoplasts to high levels around 0.5 µg/mL. Transgenic Physcomitrella Δ-fuc-t Δ-xyl-t mutant lines expressing EPO cDNA showed secretion of rhEPO through the cell wall to the culture medium. In 5- and 10-L photobioreactor cultures, secreted rhEPO accumulated to high levels above 250 µg/g dry weight of moss material after 6 days. Silver staining of rhEPO on sodium dodecylsulphate-polyacrylamide gel electrophoresis (SDS-PAGE) taken from the bioreactor culture demonstrated a high purity of the over-expressed secreted rhEPO, with a very low background of endogenous moss proteins. Peptide mapping of rhEPO produced by the Physcomitrella Δ-fuc-t Δ-xyl-t mutant indicated correct processing of the plant-derived signal peptide. All three N -glycosylation sites of rhEPO were occupied by complex-type N -glycans completely devoid of the plant-specific core sugar residues fucose and xylose.     

植酸酶基因在家蚕—杆状病毒表达系统中的表达及其酶学特性

将从黑曲霉菌株Aspergillusniger 96 3克隆并经改造后的植酸酶基因在昆虫 -杆状病毒表达系统中表达 ,SDS PAGE电泳检测蚕体和蛹的表达量分别达到 1.4 3g L血淋巴液和 1.90g L血淋巴液。酶活性测定结果表明 ,在蚕体和蛹的表达活性分别为 4 .6 7× 10 8u L血淋巴液和 5 .99× 10 8u L血淋巴液。该酶活性的最适温度范围为 5 0～6 0℃ ,最适pH值为 5 .5～ 5 .0和 2 .5。研究表明杆状病毒系统表达的植酸酶具有耐酸性和抗高温的特性 ,可以用于生产饲用植酸酶。     

Expression of post-translational processing of preprocecropin A using a baculovirus vector.

A cDNA fragment encoding preprocecropin A was inserted into the baculovirus Autographa californica nuclear polyhedrosis virus downstream of the polyhedrin promoter. The gene was expressed in recombinant-infected last instar larvae of Trichoplusia ni and in diapausing pupae of Hyalophora cecropia. The identity of the recombinant product was established by electrophoresis with detection of antibacterial activity and mass spectrometry. The prepropeptide had been correctly processed including removal of signal peptide and pro-part. Biologically active and amidated cecropin A was exported to the hemolymph. The yield of recombinant protein in H. cecropia reached a level of 600 micrograms/ml hemolymph and about 70% of the material was amidated.     

High-level expression of orange fluorescent protein in the silkworm larvae by the Bac-to-Bac system

This novel orange fluorescent protein (OFP) emits brilliant orange fluorescent light. OFP has high fluorescence quantum yield, fast maturation rate, and stability, which imply this protein should be the most favorable biotechnological tools used to investigate the function of target gene by visualizing, monitoring, and quantifying in living cells. B. mori, silkworm has been used as an important bioreactor for the production of recombinant proteins through baculovirus expression system (BES). In this paper, we used infection technique which introduced the baculovirus DNA into silkworms using a cationic lipofectin reagent instead of directly injecting the virus, and demonstrated a high-level expression of the orange fluorescent protein (OFP) gene in the Bombyx mori, silkworm larvae. When recombinant rBacmid/BmNPV/OFP DNA ranging from 50–100 ng/larval was injected, a sufficient OFP expression in hemolymph was harvested. The recombinant viruses could be obtained from the hemolymph of infected larvae and stored as seed which could be used for the large-scale expression. This procedure omitted the costly and labor-consumed insect cell culture. Further investigation of OFP should provide us with more insight in unlocking the mystery of the mechanisms of autocatalytic bioluminescence and its utilization in biotechnology.     

Improvement of recombinant baculovirus infection efficiency to express manganese superoxide dismutase in silkworm larvae through dual promoters of Pph and Pp10

The silkworm, Bombyx mori, has been used as an important bioreactor for the production of recombinant proteins through baculovirus expression system (BES). There are several problems which will probably be the bottleneck for practical and industrial utilization of silkworm bioreactor. Traditionally, the recombinant virus should infect the larvae through individual dorsal injection by a syringe. This is a time- and labor-consuming procedure. This drawback has become a bottleneck for practical and industrial utilization of baculovirus expression system in the silkworm bioreactor. In this paper, we constructed a dual expression baculovirus to express the renovated polyhedron and target manganese superoxide dismutase (SOD) gene under P10 and polyhedron promoters, respectively, through oral infection. The results showed that the direct injection of recombinant rBacmid/BmNPV/SOD DNA with cellfectin reagent infected the silkworm larvae partially. When next batches of larvae were fed orally with hemolymph, which was collected from first batch of injected and infected larvae, the obvious symptom of infection was found and high target SOD was expressed. These results imply it is feasible to express target genes through combination of recombinant bacmid DNA injection and oral feeding by a dual expression bacmid baculovirus.