重组CHO细胞C_(28)株S基因序列的测定及分析

目的测定重组CHO细胞C28株S基因序列,研究其遗传稳定性,并与已全基因序列测定的乙型肝炎病毒的S基因序列进行比较分析,预测和揭示现有疫苗株对当前疾病流行株的防病效果。方法从C28株中选取第22代、24代2、5代2、7代、28代2、9代3、0代、31代3、2代3、3代和34代细胞,根据GenBank中C基因型adr亚型乙型肝炎病毒的全基因序列设计引物。采用酚-氯仿法抽提CHO细胞基因组DNA,用PCR法扩增各代次细胞的S基因,回收700 bp左右的目的片段,克隆至pMD18-T载体上进行序列测定。利用生物学软件MEGA4.1和BioEdit进行S基因序列同源性分析,绘制系统进化树,分析与其他HBV病毒株S基因的同源性。应用实验动物测定C28株生产的重组乙型肝炎疫苗的效价。结果 C28株十一个代次之间S基因序列核苷酸和氨基酸同源性均为100%;C28株十一个代次S基因与其他病毒株S基因比较,与C基因型乙型肝炎病毒同源性最高,与其他基因型乙型肝炎病毒的核苷酸同源性达91.4%～95.1%,氨基酸同源性达84.5%～93.3%。免疫NIH小鼠结果显示5批重组乙型肝炎疫苗的效价均符合标准。结论 C28株S基因在传代及保存过程中具有较高的稳定性,对当前疾病流行株有较好的防病效果。     

不同幽门螺杆菌菌株ureB和hspA基因同源性分析

目的研究不同来源幽门螺杆菌菌株的ureB基因和hspA基因的同源性。方法在GenBank中调取全球来源于幽门螺杆菌不同菌株的ureB基因序列23个和中国境内来源于幽门螺杆菌不同菌株的hspA基因序列20个,利用ClustalW2生物软件,分别对ureB基因和hspA基因序列进行同源性比较分析,并建立基因进化树,分析其特点。结果不同国家之间ureB基因序列并不一致,同一国家ureB基因序列相似性较高;中国境内hspA基因序列相似性程度很高。结论中国境内不同幽门螺杆菌菌株ureB基因序列和hspA基因序列的相似性程度都很高,都具有很高的同源性。     

猪圆环病毒2型福建株的全基因组克隆与序列分析

根据GenBank上公布的猪圆环病毒2型全基因序列设计一对扩增PCV-2全基因的引物,建立扩增PCV-2全序列的PCR方法,并应用此方法从福建省不同地区采集的疑似断奶仔猪多系统衰竭综合征(PMWS)的仔猪肺组织病料中扩增出PCV-2全基因组(1 767 bp),将此基因片段克隆入pMD 18-T载体,筛选获得重组质粒pMD-PCV-2,并对其进行序列测定,然后对全基因组进行同源性和遗传进化分析。结果表明,福建省不同地区采集的猪肺组织扩增出的PCV-2全序列与GenBank上公布的的全基因组同源性介于94.9%-99.8%之间,ORF1的同源性介于97.2%-99.9%,ORF2的同源性也很高,介于97.7%-99.8%之间。其中福州株、福清株和漳州株与中国农大报道的12株、郑州株5株、杭州4株、武汉株3株、上海株2株、扬州2株、南京1株和兰州1株共30株在一个进化分支上,同源性也高达99.3%。本研究有助于监测PCV-2的疫源和进化关系,为进一步深入研究福建省生猪猪圆环病毒来源奠定一定基础。     

狂犬病疫苗株病毒aG株全基因序列测定及特征分析

对我国狂犬病疫苗生产株aG株进行全基因序列测定分析,为完善aG株毒种的质量控制提供数据支持。将aG株病毒全基因组RNA分成8段进行RT-PCR分段扩增,其中基因组5′末端采取5′RACE方法,将PCR扩增产物分别克隆入pGEM-T载体中,测定序列并拼接获得病毒全基因序列;用DNAStar软件包中的相应软件对基因全序列进行分析,并与国内外主要狂犬病疫苗生产株进行基因同源性分析和主要抗原位点比较。aG株病毒基因组序列全长11 925bp(GenBank登录号为JN234411),属基因Ⅰ型狂犬病病毒;各疫苗株生物信息学分析表明,各株病毒存在同源性差异。本研究获得了aG株病毒全基因组序列,对aG株基因特征进行了分析并将其与国内外疫苗株进行了比较,为完善其质量控制提供了参考和数据支持。     

陕西省9株乙脑病毒的分离及E基因序列分析

分析陕西省分离的9株乙脑病毒基因组序列特征。使用乙脑病毒全基因组序列测定引物进行RT-PCR扩增,扩增产物进行测序,拼接后获得基因组序列。利用MEGA 4.1、MegAlin、MEGA7.0等软件进行毒株的系统进化分析,并与P3株、减毒活疫苗SA14-14-2株及覆盖5个基因型别的其他乙脑病毒进行E基因序列比对。9株分离株3株分离自猪舍、6株分离自羊舍,其中4株获得全基因组序列,5株测得E基因序列。基于E基因序列进行毒株核苷酸、氨基酸同源性比较,结果显示分离株均与基因I型GI-b亚型毒株核苷酸和氨基酸同源性最高,核苷酸同源性范围为96.5%～99.7%、氨基酸同源性范围99.2%～100.0%;与SA14-14-2株核苷酸同源性范围为87.5%～88.9%、氨基酸同源性范围96.3%～97.2%;与P3株核苷酸同源性范围为87.6%～88.1%、氨基酸同源性范围96.7%～97.6%。分析09年（陕南地区）分离株与18年（关中地区）分离株的E基因核苷酸差异率为1.8%～2.9%、氨基酸差异率为0%～0.8%。陕西省自然界中循环的乙脑病毒以基因Ⅰ型为主,与P3株在抗原毒力关键位点无差异,...     

鲤春病毒糖蛋白(G)基因的分离及同源性比较

通过RT-PCR和巢氏PCR方法从疑似鲤春病毒(SVCV)侵染的镜鲤肝组织中获得了鲤春病毒糖蛋白(G)基因。通过序列测定与分析,所获得的鲤春病毒糖蛋白(G)基因由606个核苷酸组成,编码一个由202个氨基酸组成的糖蛋白。通过NCBIblast与9个来自不同国家或地区的鲤春病毒糖蛋白(G)基因序列比对分析,发现获得的鲤鱼春季病毒糖蛋白G基因DNA序列与美国分离的AY527273株同源性最高为99.8%,与中国分离的AY842485株同源性次高为98.7%,与英国分离的两个序列SVI538065和SVI538066株的同源性为98.2%,而与其它国家的分离株如SVU18101、SVI318079、SVI538061、SVI538062、SVI538063的同源性最差,仅为89.4%~90.0%。氨基酸同源性分析结果与DNA同源性分析结果一致,所获得的鲤春病毒糖蛋白G基因氨基酸推导序列与其它9个分离株的氨基酸同源性在89.6%~99.5%之间。对SVCV不同分离株遗传变异和进化关系的分析为下一步开展SVCV快速诊断方法的研究和疫苗的研制奠定了基础。     

西藏部分地区12株藏族人群C/D重组型乙型肝炎病毒全基因序列分析

为了解藏族人群中流行的乙型肝炎病毒(HBV)基因型及基因重组状况,收集藏族人群HBsAg阳性样本,提取HBV DNA并用巢氏PCR的方法扩增HBV全长序列,测序后用DNAstar软件拼接全基因序列,进一步利用MEGA6和Simplot软件进行序列同源性和系统进化分析。应用该方法获得12株藏族人群HBV全基因序列,分析结果显示12株样本为C/D重组型,其中9株样本的重组位点位于nt750,3株样本的重组位点位于nt 1526,以此可分为两种重组方式,分别命名为C/Da和C/Db;从总体序列同源性来分析12株样本均属于C基因型,且与现有的C1-C15亚型的核苷酸差异均大于4%,与C1亚型最为接近。从地理分布来看,C/Da来自西藏中部和北部的拉萨市、阿里和林芝地区,C/Db均来自西藏南部的山南地区,提示两种重组型C/Da和C/Db在西藏地区的地理分布具有一定规律。研究结果可为西藏地区特殊HBV基因重组、基因特征分析、病毒进化研究以及当地乙肝防控提供参考。     

中国国内首次发现Ⅰ基因型乙型肝炎病毒基因序列

对云南省参加健康体检人员中一份乙肝表面抗原阳性标本S区基因序列测定,以了解其分子生物学特点。利用巢式PCR扩增HBV S基因片段,并对扩增产物进行序列测定,将基因序列提交到GenBank上进行BLAST搜索,同时运用Mega软件进行同源性分析,并构建基因树,并将其核苷酸和氨基酸与已报道的A~I基因型参考株的同源性进行比较。核苷酸和氨基酸比较结果证明,此标本病毒基因型为HBV I基因型。本文所发现的I基因型标本为国内首次报道。     

中国国内首次发现Ⅰ基因型乙型肝炎病毒基因序列

对云南省参加健康体检人员中一份乙肝表面抗原阳性标本S区基因序列测定,以了解其分子生物学特点。利用巢式PCR扩增HBV S基因片段,并对扩增产物进行序列测定,将基因序列提交到GenBank上进行BLAST搜索,同时运用Mega软件进行同源性分析,并构建基因树,并将其核苷酸和氨基酸与已报道的A~I基因型参考株的同源性进行比较。核苷酸和氨基酸比较结果证明,此标本病毒基因型为HBV I基因型。本文所发现的I基因型标本为国内首次报道。     

四株不同宿主来源的Class I基因3型新城疫病毒全基因组序列测定及比较分析

为了解析基因型相同但宿主来源不同的新城疫病毒的全基因组差异。本文采用RT-PCR方法分别获得4株（JS/3/09/Ch,ZJ/3/10/Ch,AH/2/10/Du,JS/9/08/Go）Class I 基因3型病毒的全基因组核苷酸序列,并与GenBank中已公布的Class I基因3型病毒全基因组序列进行比对分析。本实验4株病毒的基因组长度均为15198bp,在基因组1607～1608位有6碱基的缺失,在2381～2382位有12碱基的插入,裂解位点为112EQ/RQE/GRL117是标准弱毒特征。5株Class I基因3型病毒之间全基因组同源性超过93%;而与Class II弱毒株同源性最低只有72.2%;比较6个结构蛋白基因的同源性,NP基因的同源性最高(98.3%～96.4%),而P基因最低(96.1%～91.9%)。结果表明不同宿主来源的Class I基因3型新城疫病毒在遗传信息方面差异不大,但NP/F/L基因的变异幅度较P/M/HN基因明显。     

乙型肝炎病毒全基因序列的测定

测定７ 例慢性 Ｈ Ｂ Ｖ 携带者 Ｈ Ｂ Ｖ 基因组全序列,经同源性比较,确定基因型。２ 例基因型为 Ｂ 型,余均为 Ｃ 型;血清型ａｄｒ ４ 例,ａｄｗ ３ 例。各序列间 Ｘ 基因差异最大。未见 Ａ１８９６ 、 Ｔ１７６２ Ａ１７６４等重要位点的变异。结合已有的２ 株 Ｈ Ｂ Ｖ 中国流行株全基因序列,初步建立以中国流行株序列为基础的 Ｈ Ｂ Ｖ 标准序列,该标准序列与国外标准序列仅有２２ 个位点的差异     

乙型肝炎病毒全基因序列的测定

Seven cases of chronic hepatitis B virus carriers were included for sequencing of whole gene sequences of hepatitis B virus (HBV). The serotype of 4 strains of HBV were adr, and 3 strains were adw. Two strains were classified to genotype B, and the other 5 strains to genotype C. No significant mutations, such as A¹⁸⁹⁶, T¹⁷⁶²A¹⁷⁶⁴ were present. With other reported 2 complete sequences of HBV strains prevailing in mainland China, 7 strains of HBV whole sequences of genotype C from mainland China were analyzed to produce the consensus sequence of HBV of China. Comparing of the consensus sequence with that from Genbank, there were only 22 sites with different nucleotides.     

乙型肝炎病毒逆转录酶区基因序列准种与变异特点

乙型肝炎病毒(Hepatitis B Virus,HBV)P基因编码产物从功能上分为末端蛋白(1～178aa)、间隔区(179～336aa)、逆转录酶区(337～682aa)和RNA酶H区(683～816aa),各区有相应的生物学功能;逆转录酶区包含S基因主蛋白编码区.近年来的研究提出HBV感染者体内存在有准种[1,2]的假说.我们以逆转录酶区序列为研究靶区域,应用聚合酶链反应(PCR)技术扩增慢性乙型肝炎患者血清中的靶基因序列,随机选择克隆测序,比较其结果,证明了HBV准种特点的存在,并发现多种基因突变形式.     

Rare Detection of Occult Hepatitis B Virus Infection in Children of Mothers with Positive Hepatitis B Surface Antigen

The prevalence of occult Hepatitis B virus (HBV) infection in children was considerably varied from 0.1–64% in different reports. In this study we aimed to investigate the prevalence of occult HBV infection among the children born to mothers with positive hepatitis B surface antigen (HBsAg) in Jiangsu, China. Serum samples were collected from 210 children of 207 mothers with positive HBsAg. HBV serological markers were detected by ELISA and HBV DNA was detected by nested PCR. Homology comparison of HBV sequences recovered from the child and mother was used to define the infection. Three children (1.43%) were positive for HBsAg, in whom the HBV pre S and S gene sequence in each child was identical to that in her mother. Of the 207 HBsAg-negative children, nine displayed HBV DNA positive by two nested PCR assays using primers derived from S and C genes. However, the sequence alignment showed that the sequences in each child were considerably different from those in his/her mother. Therefore, the sequences amplified from the children were very likely resultant from the cross-contaminations. Furthermore, the nine children with ‘positive HBV DNA’ were all negative for anti-HBc, and one had anti-HBs 3.42 mIU/ml and eight others had anti-HBs from 72 to >1000 mIU/ml, indicating that the nine children were less likely infected with HBV. Therefore, none of the 207 HBsAg-negative children of HBV-infected mothers was found to have occult HBV infection. We conclude that the prevalence of occult HBV infection in vaccinated children born to HBsAg positive mothers should be extremely low. We recommend that homology comparison of sequences recovered from the child and mother be used to define the occult HBV infection in children born to HBV infected mothers.     

Genotyping of hepatitis B virus in Malaysia based on the nucleotide sequence of preS and S genes

Hepatitis B virus (HBV) has been classified into eight genotypes, designated A-H. These genotypes are known to have distinct geographic distributions. The clinical importance of genotype-related differences in the pathogenicity of HBV has been revealed recently. In Malaysia, the current distribution of HBV remains unclear. The aim of this study was to determine the genotypes and subtypes of HBV by using PCR, followed by DNA sequencing, as well as to analyse the mutations in the immunodominant region of preS and S proteins. The S gene sequence was determined from HBV DNA of four apparently healthy blood donors' sera and three sera from asymptomatic chronic hepatitis B carriers. Of this batch of sera, the preS gene sequence was obtained from HBV DNA from three out of the four blood donors and two out of the three chronic carriers. Due to insufficient sera, we had to resort to using sera from another blood donor to make up for the sixth DNA sequence of the preS gene. Based on the comparative analysis of the preS sequences with the reported sequences in the GenBank database, HBV DNA from two normal carriers was classified as genotype C. Genotype B was assigned to HBV from one blood donor and two hepatitis B chronic carriers, whereas HBV of one chronic carrier was of genotype D. Based on the S gene sequences, HBV from three blood donors was of genotype C, that of one blood donor and one chronic carrier was of genotype B, and the remaining, of genotype D. In the five cases where both preS and S gene sequences were determined, the genotypes assigned based on either the preS or S gene sequences were in concordance. The nature of the deduced amino acid (aa) sequences at positions 125, 127, 134, 143, 159, 161 and 168 of the S gene enabled the classification of these sequences into subtypes, namely, adrq+, adw2 and ayw2. The clustering of our DNA sequences into genotype groups corresponded to their respective subtype, that is, adw2 in genotype B, adrq in genotype C and ayw in genotype D. Analysis of the point mutations revealed that five of the sequences contained aa substitutions at immunodominant epitopes involved in B or/and T cell recognition. In conclusion, despite the low numbers of samples studied, due to budget constraints, these data are still worthwhile reporting, as it is important for the control of HBV infections. In addition, the genotype and mutational data obtained in this study may be useful for designing new treatment regimes for HBV patients.     

Genomic analysis of anti-hepatitis B virus (HBV) activity by small interfering RNA and lamivudine in stable HBV-producing cells

Hepatitis B virus (HBV) causes acute and chronic hepatitis and hepatocellular carcinoma. Small interfering RNA (siRNA) and lamivudine have been shown to have anti-HBV effects through different mechanisms. However, assessment of the genome-wide effects of siRNA and lamivudine on HBV-producing cell lines has not been reported, which may provide a clue to interrogate the HBV-cell interaction and to evaluate the siRNA's side effect as a potential drug. In the present study, we designed seven siRNAs based on the conserved HBV sequences and tested their effects on the expression of HBV genes following sorting of siRNA-positive cells. Among these seven siRNAs, siRNA-1 and siRNA-7 were found to effectively suppress HBV gene expression. We further addressed the global gene expression changes in stable HBV-producing cells induced by siRNA-1 and siRNA-7 by use of human genome-wide oligonucleotide microarrays. Data from the gene expression profiling indicated that siRNA-1 and siRNA-7 altered the expression of 54 and 499 genes, respectively, in HepG2.2.15 cells, which revealed that different siRNAs had various patterns of gene expression profiles and suggested a complicated influence of siRNAs on host cells. We further observed that 18 of these genes were suppressed by both siRNA-1 and siRNA-7. Interestingly, seven of these genes were originally activated by HBV, which suggested that these seven genes might be involved in the HBV-host cell interaction. Finally, we have compared the effects of siRNA and lamivudine on HBV and host cells, which revealed that siRNA is more effective at inhibiting HBV expression at the mRNA and protein level in vitro, and the gene expression profile of HepG2.2.15 cells treated by lamivudine is totally different from that seen with siRNA.     

Comparative Analysis of CpG Islands among HBV Genotypes

DNA methylation is being increasingly recognized to play a role in regulation of hepatitis B virus (HBV) gene expression. The aim of this study was to compare the CpG island distribution among different HBV genotypes. We analyzed 176 full-length HBV genomic sequences obtained from the GenBank database, belonging to genotypes A through J, to identify the CpG islands in the HBV genomes. Our results showed that while 79 out of 176 sequences contained three conventional CpG islands (I–III) as previously described, 83 HBV sequences harbored only two of the three known islands. Novel CpG islands were identified in the remaining 14 HBV isolates and named as CpG island IV, V, and VI. Among the eight known HBV genotypes and two putative genotypes, while HBV genomes containing three CpG islands were predominant in genotypes A, B, D, E, and I; genotypes C, F, G, and H tended to contain only two CpG islands (II and III). In conclusion, the CpG islands, which are potential targets for DNA methylation mediated by the host functions, differ among HBV genotypes, and these genotype-specific differences in CpG island distribution could provide new insights into the understanding of epigenetic regulation of HBV gene expression and hepatitis B disease outcome.     

Rearrangement of the surface antigen gene of hepatitis B virus integrated in the human hepatoma cell lines.

The rearrangement of integrated HBV DNA sequences in three different hepatoma cell lines, huH-1, huH-2, KG-55-T from Japanese patients, were studied by blot hybridization using whole HBV genome or a HBsAg or HBcAg DNA as a probe. The characteristic existence of multiple integration sites of HBV DNA sequences in each HindIII-restricted hepatoma cell DNA was revealed by the HBV genome probe. Detection of the isolated HBsAg gene in the HindIII fragment indicates that the integration of HBV DNA was not always related to the maintenance of the whole viral genome, and that movement of the HBsAg gene to another location occurred by rearrangement. On the other hand, the presence of the HBV DNA sequence without the intact HBcAg gene was shown in some of the HindIII fragments, when the HBcAg gene, probe was used, but a HindIII fragment, containing only the HBcAg gene, was not detected so far. The absence of the intact HBcAg gene suggests that the viral genome may lose a part of the HBcAg gene in the process of integration. This is consistent with recent findings of Ogston et al. (1982) that in Woodchuck hepatocellular carcinoma viral sequences are extensively rearranged.