H9N2亚型禽流感病毒非结构蛋白（NS1）基因的克隆与表达

The nostructural protein (NS1) encoded by gene 8 of the Influenza virus is present in cells infected with Influenza virus. In this study, NS1 protein gene of the Chicken influenza virus A/chicken/Beijing/2/97 (H9N2) strain was amplified by PCR. The fragment contains EcoR Ⅰ and Xho Ⅰ restriction enzyme sites at the ends. The amplified product was cloned into the expression vector pET-30(c). Recombinant plasmid pET/NS 1 was transformed into E.coli BL21 (DE3) competent cells and induced with 0.4 mmol/L IPTG the target protein was produced, the molecular weight of the expressed protein was 30 kDa as expected. Western-blot test indicated that the expressed protein can react with the NS 1 monoclonal antibody of the influenza virus. This study laid an important foundation for H9N2 subtype avian influenza surveillance in China.     

一种可切除包装信号的重组1型单纯疱疹病毒的产生

A new kind of recombinant herpes simplex virus type 1 (HSV 1) was constructed. This recombinant, named HSV1 LaL, contained an unique packaging signal (“a" sequence) flanked by two loxP sites in parallel orientation, named LaL, while the original packaging signals of HSV 1 were deleted. Based on a set of cosmids containing the entire HSV 1 genome except the “a" sequence, the LaL was inserted into HSV 1 UL44 gene on one of the cosmids, cos56, generating cos56/LaL. By co transfecting cos56/LaL with the other cosmids, HSV1 LaL was generated in the cells by recombination. By introducing cos56/LaL or HSV1 LaL respectively into E.coli or BHK cells that expressed Cre recombinase, LaLs on both of them were excised by Cre, which was proved by PCR detection. To study the potential use as helper virus in packaging amplicon vector, HSV1 LaL was compared with a control virus HSV1 lacZ that contained a lacZ gene in the UL44 gene. The titer of amplicon virus generated from HSV1 LaL infected BHK/Cre cells was basically the same as that from HSV1 lacZ infected cells, however,the former contained about 10 fold less helper virus than the later, while HSV1 LaL showed the same replication rate as HSV1 lacZ on standard cells, like BHK 21.     

严重急性呼吸综合征(SARS)冠状病毒刺突蛋白基因片段的表达及其初步应用

SARS virus spike gene fra gment was expressed by Ecoli expr ession systemThe fragment enclose s major neutralization epitope of the virusThe expressed protein wa s purified and an ELISA method was set upBy using the recombinant,tw elve patients' sera were detected The recombinant SARS coronavirus s pike protein offers an efficient wa y for serological diagnosis and is useful for epidemiological survey and vaccin e development     

中国株HIV-1外膜蛋白真核表达载体的构建与表达

To construct the eukaryotic expression vector of HIV-1 gp120 gene and observe its expression in vitro, the recombinant expression vector pVAX1GP120 was constructed by inserting the gp120 gene into the eukaryotic expression vector pVAX1. The pVAX1GP120 was transfected into Vero cells by lipofectamine and the expressed product was detected by indirect immunofluore- scence.Restriction enzymes digestion analysis and sequencing results revealed that the recombinant expression vector pVAX1GP120 has been constructed successfully. The indirect immunofluorescence result showed green fluorescence on the membrane of transfected cells. The constructed eukaryotic expression vector of HIV-1 gp120 can be expressed in vitro, which lay the foundation for the further study of HIV-1 DNA vaccine.     

人载脂蛋白AⅠ基因的克隆表达及功能

To identify, clone ,sequence and highly express the mature peptide gene of ApoA Ⅰ, total RNA was prepared from human fetal liver tissue. cDNA fragment encoding human ApoA Ⅰ was amplified by RT-PCR using specific primers, and then was inserted in pGEM-T vector. DNA sequencing indicates that the fragment is 729 base pairs in length and has 100% nucleotide homology with that of reported ApoA Ⅰ cDNA gene previously. The ApoA Ⅰ gene was cloned into pGEX 5X-1.The recombinant protein was expressed in E.coli DH5α, purified by glutathione-Sepharose 4B affinity chromatography and confirmed by SDS-PAGE. It was shown that the recombinant ApoA Ⅰ was expressed in E.coli, and the target protein amounted to 36% of total bacteria proteins. Cholesteryl ester transfer experiment showed that the recombinant ApoA Ⅰ was capable of promoting transfer of CE from HDL to LDL. Western blotting showed that the protein could react specifically with anti-ApoA Ⅰ antibodies.     

Subcellular Localization Analysis of Bovine Foamy Virus Borfl Protein

The Borfl protein is encoded by an immediate-early gene of the bovine foamy virus （BFV） and plays a key role in the viral life cycle. Borfl is a DNA binding protein which can transactivate both the long terminal repeat （LTR） and the internal promoter （IP） of BFV by specifically binding to the transactivation responsive element （TRE）. To analyze the subcellular localization of Borfl during the BFV life cycle, this gene was cloned into a prokaryotic expression vector and expressed in a soluble form. After the purification and immunization, we raised the mouse anti-Borfl serum with a high titer based on ELISA results. Western blot analysis showed that the antiserum could specifically recognize the Borfl protein that was expressed in 293T cells. With this specific serum, we revealed the nuclear and cytoplasmic localization of Borfl in HeLa cells that was transfected with Borfl. Moreover, the immuno-fluorescence assay also showed that the localization of Borfl during the infection and transfection of BFV was identical.     

Expression of HSV-1 ICP0 Antigen Peptide in Prokaryotic Cells and Preparation of Specific Antibody

As an immediate-early protein of herpes simplex virus, infected-cell polypeptide 0 (ICP0) exhibits complicated interactions with host cells, and its regulatory function on gene expression is of great importance. Since the ICP0 encoding sequence contains many rare codons which are absent in E.coli, and ICP0 is highly unstable in prokaryotic cells, expression of entire ICP0 in prokaryotic cells has never been reported. In order to further investigate the function of ICP0, a recombinant plasmid was constructed by subcloning a cDNA fragment encoding an amino-terminal of 105 residues of the ICP0 protein into pGEX-5x-1 vector. The resulting GST-105 fusion antigen peptide was expressed with high efficiency in E.coli. Antibodies prepared after the immunization of mice with purified fusion protein can recognize not only the denatured ICP0 protein, but also the native ICP0 protein with normal biological conformation.     

严重急性呼吸综合征(SARS)冠状病毒N蛋白基因的表达及其初步应用

SARS coronavirus N gene w as expressed by Ecoli expression systemThe expressed protein was p urified and an ELISA method was se t up for detection of SARS virus i nfected patient's serum antibodyT he recombinant SARS coronavirus N protein offers an efficient way fo r serological diagnosis and is use ful for epidemiological study and vaccine development     

插入CpG序列的汉坦病毒S基因真核表达载体的构建及表达

To improve the effect of the gene immunization against Hantaan virus, we constructed the eukaryotic expression vector pTARGET-hans(ISS) containing Hantaan Virus S gene coding region and CpG motif by cloning S gene segment with CpG motif into eukaryotic expression vector pTARGET^TM.After conformed by enzyme analysis, the recombinant expression vector pTARGET-hans(ISS) was transferred into Vero-E6 cells by electroporation and the transient expression of Hantaan virus nucleocapsid protein was detected by indirect immunofluorescence assay(IFA). In some transferred Vero-E6, the green fluorescence was showed, thus we can conclude that the eukaryotic expression vector pTARGET-hans(ISS) was successfully constructed and expressed in vitro,which will lay a foundation for further animal vaccination.     

转录因子E2F1抑制CREG表达调控体外培养的人血管平滑肌细胞分化

为探讨转录因子E2F1在血管平滑肌细胞(vascular smooth muscle cells,VSMCs)表型转化中的作用及其对E1A激活基因阻遏子(cellular repressor of E1A-stimulated genes,CREG)表达调控的分子机制,应用生物信息学方法,定位人CREG(hCREG)基因启动子并确定转录因子E2F1在hCREG启动子区的结合位点,PCR方法克隆并构建hCREG基因启动子绿色荧光报告基因载体,以hCREG启动子区E2F1结合位点为模板,化学合成E2F1寡聚脱氧核苷酸(ODN)和错配E2F1ODN,利用转录因子"诱骗(Decoy)"策略,用E2F1ODN转染体外培养的VSMCs以阻断E2F1与hCREG基因启动子区的结合,蛋白质印迹(Western blot)分析检测阻断前后细胞内hCREG蛋白、报告基因绿色荧光蛋白(green fluorescent protein,GFP)和平滑肌细胞分化标志蛋白SMα-actin表达变化.结果显示:分化表型HITASY细胞中E2F1表达下调伴出核转位,而增殖表型的HITASY细胞中E2F1蛋白表达明显增加且定位于核内.进一步应用FuGene6瞬时转染E2F1ODN和错配E2F1ODN于体外培养HITASY细胞中,蛋白质印迹分析发现,转染E2F1ODN后,HITASY细胞中hCREG、SMα-actin和GFP表达均较未阻断组及错配组细胞明显增加.上述研究结果证实,E2F1是hCREG基因转录的重要调控因子,能够直接结合于hCREG启动子区阻遏hCREG表达,参与hCREG蛋白对VSMCs表型转化的调控作用.     

人HTR1E基因在不同细胞系和多种组织中的表达及其功能

人的HTR1E基因是五羟色胺受体（HTR）家族中的一员．这个家族里面的基因都和精神分裂症、抑郁症以及人的自杀活动有关．但是对于其具体的作用机制目前研究不多．采用实时定量PCR方法分析了HTR1E基因在各个组织和不同细胞系中的表达情况．亚细胞定位发现HTR1E位于细胞膜上,萤光素酶实验分析确定HTR1E可以抑制原癌基因erbB2启动子的转录活性．这些研究结果为进一步研究HTR1E基因在疾病发生中的作用奠定了一定的基础．     

E1A激活基因阻遏子表达与小鼠胚胎血管发生的关系

目的探讨E1A激活基因阻遏子(CREG)蛋白表达与小鼠动脉形态学发生的关系,了解CREG蛋白在血管发育中的生物学作用。方法制备E9.5d-E18.5d胎鼠、新生1d、28d和2月成鼠不同脏器功能血管的石蜡组织切片,观察主动脉发生过程中的形态学变化;采用免疫组化染色法观察不同发育时相的血管细胞中CREG蛋白和血管平滑肌细胞(vascular smooth muscle cells,VSMCs)标记物肌动蛋白(SMα-actin)的表达变化。结果HE染色显示E9.5d的胚胎血管由单层血管内皮细胞构成,免疫组化显示CREG表达阳性,主要定位于血管壁的单层内皮细胞中,SMα-actin表达为阴性;E10.5d的胚胎血管内皮细胞周围开始出现少量SMα-actin表达阳性的原始VSMCs,同时CREG蛋白表达,定位与SMα-ac-tin蛋白一致。自E12.5d开始SMα-actin蛋白在血管中膜VSMCs中表达增强并持续至成年。CREG蛋白在三层结构的血管细胞中均为阳性表达,其表达强度在E15.5d达到最高,E18.5d表达下降并维持至成年。进一步分析CREG蛋白在成年鼠心、肺、脾和肾等多个脏器血管中的分布,发现所有脏器血管细胞均表达CREG,但表达丰度明显不同,在储存血管和分配血管中CREG蛋白呈高表达,在调节血管中低表达。结论CREG蛋白在小鼠胚胎血管发育早期、持续表达的特点及其在不同脏器功能血管中表达的差异,提示CREG蛋白可能通过调控并维持血管细胞,特别是VSMCs的分化,参与了胚胎血管发生的调控。     

高危型HPV 复制相关蛋白在宫颈组织中的研究

人乳头瘤病毒(Human Papillomavirus,HPV)复制机制的研究,对复制与宫颈病变的相关性可提供重要的依据。HPV是有衣壳包裹的小型环状双链DNA病毒。其基因组可分早期及晚期蛋白编码区和一个调控区。高危型HPV通过E1、E2蛋白及Ori序列启动复制。高危型HPV在宫颈上皮细胞中的复制是分化依赖型的,在高危型HPV感染的成熟的宫颈表皮细胞中,HPV E7蛋白使细胞再次进入增殖分裂期,HPV-DNA得以复制,但同时E7蛋白亦会诱发宿主细胞染色体不稳定,增加癌变风险。由此推理,高危型HPV的复制与宫颈癌的发病有一定相关性。目前有学者对高危型HPV的复制机制,复制与致癌的关系方面正开展相关研究。     

草鱼肝细胞中CYP2E1活性的诱导研究

CYP2E1为代谢大部分药物及环境巾毒物的关键酶。以草鱼肝细胞（Ctenopharyngodon idellus hepatocyte）为反应体系,选取氯唑沙宗（CZX）为底物,采用反相高效液相色谱（RP-HPLC）法测定其产物6-OH-氯唑沙宗（HCZX）的量,Lowry法测定肝细胞巾蛋白的浓度从而反映CYP2E1活性,并采用该酶特异性诱导剂乙醇对其进行诱导,观察其酶活变化及CZX在细胞中代谢情况。结果表明,CZX在草鱼肝细胞中的基础代谢较低,经过对CYP2E1诱导条件的优化及筛选,得到最佳诱导剂剂量为4μg／mL、诱导时间为24h、底物浓度为50μg／mL并且孵育时间为1h时,其酶活达到最高,约为0．47μg／min·mg。对照组和诱导组的草鱼肝细胞中CZX的消除半衰期（t。）分别为202．10h和28．75h,差异极显著,表明乙醇诱导的CYP2E1能够加快底物的代谢。酶促反应动力学参数表明乙醇诱导的CYP2E1与底物的亲和力较高,酶促反应强度较大。该结果能够为CYP2E1代谢的药物及环境毒物的研究提供理论依据。     

Induction of cell death by adenoviruses

Adenoviruses have proved to be excellent tools for gaining insight into the regulation, and deregulation, of the mammalian cell cycle. With the widespread clinical use of gene therapy fast approaching, there comes a need for a better understanding of how the cell death process is regulated. A greater understanding will allow the development of therapeutic approaches that both maximise transgene expression while minimising cytotoxicity to the target cell. Consequently, much adenovirus research has centered on understanding the mechanisms governing adenovirus induced cell death or apoptosis. This review discusses recent advances in the field of adenovirus cell death regulation and evaluates the roles of implicated gene products and their respective data. The data suggest the existence of multiple virus gene products involved in cell death regulation and point towards several distinct, yet related, cell death pathways. A discussion of the shortcomings of current adenoviral research, along with a proposed model based upon the data is also given.     

一种新的重组腺病毒的构建及其对人肿瘤细胞的影响

腺病毒E1A基因诱导细胞凋亡．E1B19K基因及E1B55K基因抑制细胞凋亡,前者被克隆到腺病毒转移载体pCA13的HCMVIE启动子下游．构建成转移载体pCAE1A。采用lipofectin法将PCAE1A和含腺病毒基因组（E1、E3区缺失）的质粒pBHG11共转染293细胞,7～10d后得到重组病毒v5Ad4。用v5Ad4感染人肺腺癌细胞系A549,结果表明v5Ad4有明显杀伤和裂解肿瘤细胞功能。在人胚肺正常二倍体细胞中,v5Ad4没有表现出可见的细胞毒效应。     

ENSO事件的发生对马尾松毛虫发生的影响

迈过对２０多年来ＥＮＳＯ事件的发生与马尾松毛虫发生关系的研究．探讨全球气侯异常对马尾松毛虫发生和种群发展动态的影响．结果表明：在厄尔尼诺或反厄尔尼诺事件的当年,连江县马尾松毛虫书为中到大发生年;南方涛动｜ΣＳＯＩ｜≤０．９的当年,为马尾松毛虫大发生年;在南方涛动０．９＜｜ΣＳＯＩ｜＜１．９的当年,为马尾松毛虫轻发生年．