家蚕浓核病毒 Bm DNV-3(中国株)VD1基因组结构与转录分析

为了进一步认识家蚕浓核病毒BmDNV-3(中国株)VD1基因组的结构和功能,VD1被分离、纯化、克隆到pUC119载体上,完成了基因组全序列的测定。序列分析显示VD1基因组全长为6543个核苷酸,末端拥有224个核苷酸反向重复序列(ITRs)。VD1基因组正链含有3个大的开放阅读框(ORF1-3),负链含有1个大的开放阅读框(ORF4)。比较BmDNV-3的VD1和BmDNV-2(Yamanashiisolate)的VD1基因组全序列,两者同源性为98.4%,并且有107个碱基的替代和1个碱基插入,氨基酸突变集中在VD1ORF3和VD1ORF4。Northern杂交结果显示VD1的左边正链上有1.1kb和1.5kb两个转录本,右边的负链上有一个3.3kb转录本。3′和5′-RACE结果显示1.1kb转录本开始于nt290,结束于nt1437;1.5kb转录本开始于nt1423,结束于nt2931;3.3kb转录本开始于nt6287,结束于nt2922。正链上1.5kb转录本和负链上3.3kb转录本拥有10个核苷酸的3′端的共同序列。研究结果显示该病毒基因转录与已报道的其它浓核病毒存在较大的差异性。     

家蚕浓核病毒Bm DNV-3（中国株）VD 1基因组结构与转录分析

为了进一步认识家蚕浓核病毒_BmDNV-3（中国株）VD₁基因组的结构和功能,VD1被分离、纯化、克隆到pUC119载体上,完成了基因组全序列的测定。序列分析显示VD₁基因组全长为6543个核苷酸,末端拥有224个核苷酸反向重复序列（ITRs）。VD₁基因组正链含有3个大的开放阅读框（ORF1-3）,负链含有1个大的开放阅读框（ORF4）。比较BmDNV-3的 VD₁和BmDNV2 (Yamanashi isolate) 的VD₁基因组全序列,两者同源性为98.4%,并且有107个碱基的替代和1个碱基插入,氨基酸突变集中在VD₁ ORF3和VD₁ORF4。Northern杂交结果显示：VD₁的左边正链上有1.1kb和1.5kb两个转录本,右边的负链上有一个3.3kb转录本。3′和5′-RACE结果显示：1.1kb转录本开始于nt 290,结束于nt 1437;1.5kb转录本开始于nt 1423,结束于nt 2931;3.3kb转录本开始于nt 6287,结束于nt 2922。 正链上15kb转录本和负链上3.3kb转录本拥有10个核苷酸的3′端的共同序列。研究结果显示该病毒基因转录与已报道的其它浓核病毒存在较大的差异性。     

一株雀纹天蛾核型多角体病毒的鉴定及其基因组序列分析

从自然死亡的雀纹天蛾幼虫分离到一株雀纹天蛾核型多角体病毒。通过扫描及切片透射电镜发现,该病毒为单粒包埋型核型多角体病毒,命名为ThjaSNPV(Theretra japonica single nucleopolyhedrovirus)。病毒全基因组重测序后拼接显示,该病毒基因组全长134 899 bp,GC含量37.28%,与豆天蛾单粒包埋型核型多角体病毒株DZ1基因组序列相似性高达96.24%。ThjaSNPV含有131个开放阅读框（ORF）其中55个为正链基因,76个为负链基因,与宿主同为天蛾科的豆天蛾单粒包埋型核型多角体基因组相比,雀纹天蛾单粒包埋型核型多角体病毒新注释到7个基因：chitin-binding protein(ORF9),ODV-E18(ORF11),lef-11(ORF27),hypothetical protein(ORF41),lef-10(ORF42),pif-6(ORF66),P6.9(ORF88)。ThjaSNPV的DNA光裂酶基因（DNA photolyase,ORF53）中不具有豆天蛾NPV中的1bp碱基的缺失,只编码一个大的完整DNA裂合酶。3...     

中国南瓜曲叶病毒DNAA的克隆及其全序列

对引起我国南瓜曲叶病的病毒分离物DNA的克隆和序列分析表明,中国南瓜曲叶病毒DNA A由2741个核苷酸组成,共编码6个开放阅读框(ORF),其中病毒链有2个ORF：AV1(256aa)和AV2(140aa),AV1为外壳蛋白基因;病毒链的互补链有4个ORF,AC1(243aa)编码复制酶基因,AC2(134aa)编码反式激活蛋白,AC3(136aa)和AC4(172aa),该病毒属于旧世界Begomoviruses,是一个粉虱传播的联体病毒。     

福建一例HAstV-5型星状病毒的全基因组测序与重组分析

为了探究一例福建省检出的HAstV-5型星状病毒2013/Fuzhou/85毒株基因组分子结构特点,本研究采用PCR分段扩增、测序、拼接的方法,获得2013/Fuzhou/85毒株基因组序列全长6 803bp:5’端和3’端均有85bp非编码区;中间3个开放阅读框:ORF1a长2 802bp(86～2 887nt),编码非结构蛋白丝氨酸蛋白酶;ORF1b长1 548bp(2 827～4 374nt),编码非结构蛋白RNA聚合酶;ORF2长2 352bp(4 367～6 718nt),编码结构蛋白衣壳蛋白前体。目前,GenBank中仅有两株HAstV-5型星状病毒全基因组序列:中国辽宁毒株(JQ403108)和巴西哥亚尼亚毒株(DQ028633),2013/Fuzhou/85毒株和中国辽宁毒株核苷酸相似度最高,达94.4%。对该HAstV-5型星状病毒3个开放阅读框分别构建系统进化树,发现ORF1a与HAstV-1(JF327666)相似度最高,ORF1b和ORF2与HAstV-5(JQ403108)相似度最高,提示其有可能存在重组,用Simplot软件进行重组分析,重组位点位于2 741bp,在ORF1a和ORF1b重叠区的上游。本研究中对2013/Fuzhou/85毒株的全基因组测序和重组分析,可以为星状病毒的重组和遗传进化规律研究提供参考。     

大麦黄矮病毒GAV基因组全序列测定及其结构分析

测定了在中国分离得到由麦二叉蚜和麦长管蚜传播的大麦黄矮病毒GAV的基因组核苷酸全序列, 该病毒分离物的RNA由5685个核苷酸组成, 内含6个开放阅读框架(ORF)和4个非编码区(UTR), 基因组大小和结构与黄症病毒属(Luteovirus)的大麦黄矮病毒PAV(BYDV-PAV)和MAV(BYDV-MAV)相似. 序列分析表明, 它与BYDV-MAV的PS1分离物基因组序列的同源性最高. 在6个开放阅读框架中, 除ORF6核苷酸序列同源性为72.0%外, 其他ORF的核苷酸序列同源性均大于90%. 两者全基因组的同源性为90.4%. 推导的编码产物氨基酸序列同源性除P6和通读蛋白(RTP)分别为67.4%和87.4%外, 其他均大于90%, 其中外壳蛋白(CP)为95.5%. 根据与BYDV-MAV的相似性, BYDV-GAV应是一种与BYDV-MAV类似的病毒.     

水稻黑条矮缩病毒基因组片段S7的cDNA克隆及全序列分析

应用RTPCR技术克隆了2个水稻黑条矮缩病毒 (rice blackstreaked dwarf virus,RBSDV)中国分离物,即浙江分离物和河北分离物的基因组片段S7,并测定了他们的全序列。结果表明：RBSDV浙江分离物(RBSDVZj)基因组片段S7全长2193nts(EMBL登录号为AJ297427),RBSDV河北分离物基因组片段S7全长2190nts(EMBL登录号为AJ297428),二者均含有两个开放阅读框(open reading frame,ORF),分别编码约41kD和36kD多肽,2个中国分离物核苷酸同源性高达99%,相应的ORF编码的多肽同源性分别为100%和94.4%,与日本RBSDV基因组片段S7核苷酸同源性为93.4%和93.8%,相应ORF编码的多肽同源性分别为98.1%(ORF1)、96.5%和97.8%(ORF2),与意大利MRDV S6核苷酸同源性为85.1%和85.3%,相应多肽同源性分别为92.3%(ORF1)、85.5%和86.8%(ORF2)。     

辣椒脉斑驳病毒文昌分离物基因组测序及分析

辣椒脉斑驳病毒(Chilli veinal mottle virus,ChiVMV)近年来严重危害海南黄灯笼辣椒的产量,开展针对该病毒的研究以求达到对其有效防控迫在眉睫.本研究分7段克隆了ChiVMV文昌分离物(ChiVMV Wenchang isolate,ChiVMV-WC)的基因组.分段克隆的测序结果通过拼接,共获得ChiVMV-WC基因组9 717个核苷酸(nt)序列(GenBank登录号:GQ981316).在核苷酸序列的第164位~第9 270位存在一个大的开放阅读框(ORF),编码一个多聚蛋白(分子量为350.44 kD).近年来被证实的马铃薯Y病毒科的一个新的ORF (pretty interesting potyviridae ORF,PIPO)存在于ChiVMV-WC基因组核苷酸序列的第2 892位~第3 110位,编码一个由72个氨基酸聚合而成的多肽(分子量为8.26 kD).ChiVMV-WC与ChiVMV其它分离物的基因组核苷酸序列比较发现该病毒存在着较高的变异率.本研究通过与同属内病毒的同源性分析以及系统进化树分析,确定了ChiVMV-WC在生物进化史上的地位.     

慢性蜜蜂麻痹病毒Ch1株的编码区测序及其序列的分析

对中国分离株慢性蜜蜂麻痹病毒(Chronic bee paralysis virus,CBPV)Ch1编码区全基因序列进行克隆、测序、分析。利用RT-PCR方法和生物信息学软件,对本实验室分离到的Ch1株CBPV编码区的基因序列进行克隆,测序,与GenBank收录的CBPV毒株进行同源性比较,并以RdRp为靶基因构建了遗传进化树。结果显示,CBPV Ch1株的编码区由RNA1(GenBank No.KU950353)和RNA2(GenBank No.KU950354)两部分构成,全长5 979个核苷酸。其中RNA1片段全长3 674个核苷酸,编码3个开放阅读框,RNA2片段全长2 305个核苷酸,编码4个开放阅读框,RNA2片段中ORF2和ORF3,可能编码两个结构蛋白,分别命名为SP1和SP2。RNA1和RNA2核苷酸序列与2005年法国分离株Fr2核苷酸序列同源性最高,分别为96.1%和95.5%,但预测蛋白SP1核苷酸序列同源性与2006年乌拉圭分离株Ur1核苷酸序列同源性最高(96.9%)。基于RdRp为靶基因进行了遗传进化分析表明,Ch1株与Fr2株位于同一分支,且在该区域,Ch1株与Fr2株的核苷酸序列同源性最高(96.5%)。本实验成功分离到一株CBPV(KU950353,KU950354),并命名为Ch1株,完成了Ch1株CBPV的编码区的序列测定以及核苷酸序列与推导的氨基酸序列同源性比较及遗传进化分析,为研究CBPV的致病机制和免疫机制提供重要信息。     

一种简单高效扩增人杯状病毒ORF2区RT-PCR方法的建立及其意义

人杯状病毒(human calicivirus,HuCV)属于杯状病毒科(Caliciviridae),是单股正链RNA病毒,长约7·5 kb,其3′末端有poly(A)结构。它可分为两个属:诺如病毒(Norovirus)和札如病毒(Sapovirus)[1],根据病毒抗原性和核苷酸序列的多样性,目前将诺如病毒和札如病毒分别划分为三个遗传组(group),每一遗传组依据RNA多聚酶及衣壳蛋白区域序列的差异,可进一步划分为不同群或基因型(cluster or genotype)。病毒基因组包括3个开放读码框(open reading frame,ORF),5′端和3′端各有一个小的非编码区。ORF1编码非结构蛋白的前体聚蛋白,其中包括RNA…     

Complete Genome Sequence of Recombinant Porcine Circovirus Type 2 Strain SD-3

We report here the genome sequence of a recombinant porcine circovirus type 2 strain SD-3, isolated from a commercial swine farm with an outbreak of postweaning multisystemic wasting syndrome (PMWS) in pigs in Shandong Province of China. The complete circular genome of this isolate is 1,767 nucleotides in length. This recombinant isolate has the ORF1 regions from PCV2a viruses and ORF2 regions from PCV2b. The findings will help us to understand the molecular evolution of porcine circovirus type 2 and the relationship between porcine circovirus type 2 and disease.     

The 160,000-Mr virion protein encoded at the right end of the herpesvirus saimiri genome is homologous to the 140,000-Mr membrane antigen encoded at the left end of the Epstein-Barr virus genome.

The sequence of 4.4 kilobase pairs (kbp) from the conventional right terminus of the A + T-rich light-DNA (L-DNA) sequences of the herpesvirus saimiri (HVS) genome contains a leftward-directed open reading frame (ORF) for a 1,299-residue protein. The molecular weight predicted for the protein (143,000) is in good agreement with the estimates of 150,000 to 160,000 for the major nonglycosylated polypeptide of the virion tegument (the 160K polypeptide), previously shown to be encoded by this region of the genome. The first initiation codon of the ORF is only 250 nucleotides from the junction of the L-DNA component with the G + C-rich terminal reiterations (i.e., heavy or H-DNA) of the genome. An unusually A + T-rich sequence (43 of 45 nucleotides are A or T, relative to a mean composition of 40% G + C for the ORF) occurs some 75 bp 5' to this initiation codon, and the first adenylation signal (AATAAA) on this DNA strand occurs 18 bp 3' to the termination codon. The amino acid sequence predicted for the 160K protein of HVS is homologous over most of its length to the 1,318-residue protein encoded by the leftmost major ORF of the G + C-rich genome of Epstein-Barr virus (BNRF1, the 140K nonglycosylated membrane antigen). No homology to either of these proteins is evident among the products predicted from the complete sequence of the alpha herpesvirus varicella-zoster virus. Thus gamma herpesviruses with coding sequences which differ in mean nucleotide composition by some 20% G + C have homologous proteins encoded at similar positions with respect to genome termini, with the right end of HVS being homologous to the left end of Epstein-Barr virus.     

Complete sequences of the highly rearranged molluscan mitochondrial genomes of the Scaphopod Graptacme eborea and the bivalve Mytilus edulis

We have determined the complete sequence of the mitochondrial genome of the scaphopod mollusk Graptacme eborea (14,492 nts) and completed the sequence of the mitochondrial genome of the bivalve mollusk Mytilus edulis (16,740 nts). (The name Graptacme eborea is a revision of the species formerly known as Dentalium eboreum.) G. eborea mtDNA contains the 37 genes that are typically found and has the genes divided about evenly between the two strands, but M. edulis contains an extra trnM and is missing atp8, and it has all genes on the same strand. Each has a highly rearranged gene order relative to each other and to all other studied mtDNAs. G. eborea mtDNA has almost no strand skew, but the coding strand of M. edulis mtDNA is very rich in G and T. This is reflected in differential codon usage patterns and even in amino acid compositions. G. eborea mtDNA has fewer noncoding nucleotides than any other mtDNA studied to date, with the largest noncoding region only 24 nt long. Phylogenetic analysis using 2,420 aligned amino acid positions of concatenated proteins weakly supports an association of the scaphopod with gastropods to the exclusion of Bivalvia, Cephalopoda, and Polyplacophora, but it is generally unable to convincingly resolve the relationships among major groups of the Lophotrochozoa, in contrast to the good resolution seen for several other major metazoan groups.     

家蚕浓核病毒 (中国镇江株)在不同感受性宿主体内的复制

家蚕浓核病毒中国镇江株是一株双生浓核病毒(bidensovirus)。其宿主感染后的病症与典型的家蚕浓核病毒(BmDNV-1伊那株)表现相似,病蚕软化,中肠的圆筒型细胞呈浓核症。该病毒的最大特点是基因组中含有二套DNA分子(VD1,VD2),这两种核酸分子以单链( VD1,-VD1, VD2,-VD2)线型方式被分开包装在各自的衣壳蛋白中,成为四种病毒体,而且它自身编码DNA聚合酶。有部分蚕品种对该病毒表现完全抗性,即不发病。分别对敏感性家蚕品种(华八35)和抗性家蚕品种(秋丰d)的幼虫进行经口接种病毒。在接种后,从2h到96h分9个时间点,对中肠组织进行取样。以家蚕细胞质肌动蛋白A3(actinA3)基因作为参比基因,用来标定取样组织细胞数。针对VD1和VD2分别设计特异引物,用荧光定量PCR的方法分别检测各个时间点的样品中的病毒基因组VD1和VD2拷贝数。结果表明:无论是在感性还是在抗性宿主体内,家蚕浓核病毒中国株的基因组VD1和VD2在各时间点拷贝数相近,表现出VD1和VD2是同步复制的;病毒侵入两种宿主中肠的初始量(接种后2h)基本相等,每个细胞约为6~10拷贝数。在敏感性宿主体内病毒感染过程表现为潜伏期,指数增长期,平台期。从接种后2h到12h为病毒潜伏期;12h到36h为指数增长期,倍增时间为1·71h,大约扩增15次;36h到96h为平台期,进入平台期病毒的拷贝数达到20万个。在抗性宿主体内病毒处于一种极低水平的增殖,从添毒后2h的6~10拷贝数到96h的150~200拷贝数,病毒复制倍增时间分别为3h和12h,大约扩增5次。推测家蚕对浓核病毒中国株的抗病性,只是一种慢性的带毒不发病的表现。     

Complete Genome of a Novel Porcine Astrovirus

Astroviruses have been widely described in mammalian and avian species. Here, we report a complete genome sequence of a novel porcine astrovirus (PoAstV) isolated from a porcine fecal sample in China. The genome consists of 6,611 nucleotides, excluding the 3′ poly(A) tail, and has two open reading frames (ORFs). ORF1 maps between nucleotide positions 19 and 4211 and encodes a 1,396-amino-acid (aa) polyprotein precursor consisting of nonstructural protein and putative RNA-dependent RNA polymerase, and ORF2 maps between nucleotide positions 4202 and 6531 and encodes a 775-aa polyprotein which is a capsid precursor protein. The genome sequence of the virus was distinct enough from those of the known PoAstVs to be considered a novel sequence. Phylogenetic analysis based on the predicted amino acid sequence of the complete capsid region showed that this strain may be a novel porcine astrovirus.     

Completion of the Nucleotide Sequence of a Brazilian Isolate of Southern bean mosaic virus

The sequence of the central part (ORF2) of a Brazilian isolate of Southern bean mosaic virus (SBMV^SP) is described. This ORF is 2888 nt long and together with the previously-sequenced 5' and 3' ends provides the complete nucleotide sequence of this virus isolate. The SBMV^SP RNA encodes four overlapping open reading frames (ORF1, ORF2a, ORF2b, ORF4) and has a genome organization similar to that of the Cocksfoot mottle sobemovirus .     

Genomic characterization of the filamentous integrative bacteriophages {phi}RSS1 and {phi}RSM1, which infect Ralstonia solanacearum

The genomic DNA sequences were determined for two filamentous integrative bacteriophages, phiRSS1 and phiRSM1, of the phytopathogen Ralstonia solanacearum. The 6,662-base sequence of phiRSS1 contained 11 open reading frames (ORFs). In the databases, this sequence showed high homology (95% identity) to the circular double-stranded DNA plasmid pJTPS1 (6,633 bp) isolated from a spontaneously occurring avirulent mutant of R. solanacearum. Two major differences between the two sequences were observed within phiRSS1 ORF7, corresponding to pIII, a minor coat protein required for host adsorption, and at the phiRSS1 intergenic (IG) region. The 9,004-base sequence of phiRSM1 showed 12 ORFs located on the same strand (plus strand) and 2 ORFs on the opposite strand. Compared with Ff-type phages, two insertions are obvious in the phiRSM1 replication module. Genomic DNA fragments containing the phiRSM integration junctions were cloned and sequenced from phiRSM lysogenic strain R. solanacearum MAFF211270. The att core sequence was identified as 5'-TGGCGGAGAGGGT-3', corresponding to the 3' end of the serine tRNA (UCG) gene. Interestingly, ORF14, located next to the attP site on the phiRSM1 genome, showed high amino acid sequence homology with bacterial DNA recombinases and resolvases, different from XerCD recombinases. attP of phiRSS1 is within a sequence element of the IG region.     

Complete Genomic Sequence of a Chinese Isolate of Duck Hepatitis Virus

The complete genomic sequence of Duck hepatitis virus 1(DHV-1) ZJ-V isolate was sequenced and determined to be 7 691 nucleotides(nt) in length with a 5'-terminal un-translated region(UTR) of 626 nt and a 3'-terminal UTR of 315 nt(not including the poly(A) tail).One large open reading frame(ORF) was found within the genome(nt 627 to 7 373) coding for a polypeptide of 2 249 amino acids.Our data also showed that the poly(A) tail of DHV-1 has at least 22 A's.Sequence comparison revealed significant homology(from 91.9% to 95.7%) between the protein sequences of the ZJ-V isolate and those of 21 reference isolates.Although DHV-1 has been classified as an unassigned virus in the Picornaviridae family,its genome showed some unique characteristics.DHV-1 contains 3 copies of the 2A gene and only 1 copy of the 3B gene,and its 3'-NCR is longer than those of other picornaviruses.Phylogenetic analysis to do sequence homology based on the VP1 protein sequences showed that the ZJ-V isolate shares high sequence homology with the reported DHV-1 isolates(from 92.9% to 99.2%),indicating that DHV-1 is genetically stable.