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1.
Cellular insertions in the NS2-3 genome region of cytopathic bovine viral diarrhoea virus (BVDV) isolates 总被引:1,自引:0,他引:1
When compared to noncytopathic (ncp) bovine viral diarrhoea virus (BVDV), some cytopathic (cp) BVDV contain additional sequences in the NS2-3 genomic region. One of these insertions, which is 270 nucleotides long and of host origin (cINS), was first described for strain NADL. To find out how frequently this type of insertion occurs in other cp BVDV, 32 cp BVDV field isolates and the BVDV reference cp strain Indiana were screened using RT-PCR which detected cINS in NADL. For most cp viruses an RT-PCR product of 402bp indicated the presence of NS2-3 genes without insertions. In addition, one or two DNA fragments, around 600-850bp in size, were amplified from the genomes of 13 cp viruses indicating the presence of insertions. Sequencing of the PCR products, i.e. 402bp DNA fragment (with no insertion) and longer fragments (with insertion) revealed the location of the insertions in the NS2-3 coding region of eight cp BVDV genomes. All of the insertions were confirmed to be of the cINS type and were located in a very similar position to that found previously in the NADL genome. They were in the same reading frame as the viral polypeptide and they encoded 90-140 amino acids. The 5' and 3' ends of the insertions were different in most of the cp isolates studied. Interestingly, a 14-amino-acid stretch at the 5'-end of the insertion in the cp 5569 isolate as well as 15 amino acids at the 3'-end of the insertion in the cp 5.19516 isolate were not homologous to the cINS sequence. No significant matches for these stretches were found in the EMBL and Swissprot databases. 相似文献
2.
牛病毒性腹泻病毒P125基因重要区的比较与分析 总被引:11,自引:0,他引:11
根据牛病毒性腹泻病毒(BVDV)NADL株的序列,以计算机辅助设计,化学合成1对引物(W1/W2);应用RT-PCR对国内不同地区分离的4株BVDV的P125基因外源序列插入区进行了扩增,并将扩增的片段进行克隆和序列测定,同时以DNASIS和PROSIS计算机软件将测定的核苷酸序列及推导的氨基酸序列进行比较分析。结果证实,国内分离的4株BVDV在这一区域中既没有外源序列的插入,也没有基因重组、基因重排或基因缺失,但存在某些核苷酸和氨基酸的替换,表明病毒的致细胞病变作用除与外源序列的插入、基因重组、基因重排或基因缺失有关外,可能还存在其他机制。核苷酸序列的同源性及系统树分析的结果表明,国内的BVDV毒株存在Ia和Ib2个基因亚型,它们均属基因I型BVDV 相似文献
3.
Experimental infection of calves with two strains of bovine virus diarrhoea virus: virus recovery and clinical reactions 总被引:1,自引:0,他引:1
Fifteen calves were inoculated with a mixture of two strains of bovine virus diarrhoea virus (BVDV), the cytopathogenic NADL strain which had been passaged over 20 times n vitro, and the non-cytopathogenic FCS strain, passaged only once after isolation from fetal calf serum. In a second experiment, seven calves received the NADL strain, and eight the FCS strain. The clinical and virological results of the two experiments were compared. In dual infections, the NADL strain interfered with the replication of the FCS strain resulting in less severe disease than the FCS strain alone. The FCS-BVDV was recovered from nasopharyngeal swabs and buffy coat cells whereas the NADL-BVDV was recovered only from nasopharyngeal swabs. The cytopathogenicity of the two strains did not change after passage in vivo. The differences observed are discussed in relation to cultural history and cytopathogenicity. 相似文献
4.
The bovine viral diarrhea virus (BVDV) strains exist as two biotypes, cytopathic (cp) and noncytopathic (ncp), according to their effects on tissue culture cells. It has been previously reported that cell death associated to cp BVDV in vitro is mediated by apoptosis. Here, experiments were conducted to determine the involvement of the NS3 protein in the induction of apoptosis. The NS3- and NS3Delta50 (deleted from the NH2-terminal 50 amino acids)-cDNA encoding sequences of BVDV NADL cp reference strain were cloned into adenoviral vectors (AdV) from which the BVDV gene of interest could be expressed from a tetracycline-responsive promoter. A549tTA cells infected in vitro with NS3 or NS3Delta50-expressing AdV showed cytopathic changes characterized by cell rounding and detachment, and nucleus chromatin condensation. DNA fragmentation assays, cytochrome c release, and activation of cellular caspases performed on these infected cells clearly correlated with the observed cytopathic changes with apoptosis. The BVDV NS3Delta50-induced apoptotic process was inhibited by caspase-8- and -9-specific peptide inhibitors (Z-IETD-FMK and Z-LEHD-FMK). Furthermore, apoptosis was inhibited in cells expressing the R1 subunit of herpes simplex virus type 2 ribonucleotide reductase (HSV2-R1) or hsp70, two proteins which are known to inhibit apoptosis associated with caspase-8 activation and cytochrome c release-dependent caspase-9 activation, respectively. Given that HSV2-R1, a specific inhibitor of the caspase-8 activation pathway, efficiently suppressed apoptosis and also prevented caspase-9 activation, the overall results indicate that the BVDV NS3/NS3Delta50 induces apoptosis initiated by caspase-8 activation and subsequent cytochrome c release-dependent caspase-9 activation. 相似文献
5.
从疑似猪瘟病料中检出牛病毒性腹泻病毒 总被引:22,自引:1,他引:22
根据牛病毒性腹泻病毒(BVDV)NADL株和猪瘟病毒(HCV)Alfort株的核苷酸序列,设计合成了1对BVDV引物和3对HCV引物。以从吉林、长春、哲盟3个地区经临床及病理学诊断为猪瘟的病料中提取的RNA为模板,采用反转录-聚合酶链反应(RT-PCR),分别以BVDV和HCV引物进行扩增。结果,用BVDV引物从哲盟地区的疑似猪瘟病料中扩增出大小约400bp的片段,而用3对HCV引物在不同的条件下均未从该病料中扩增出相应大小的HCV基因片段。此外,用HCV的PE0/PE4引物从吉林、长春的病料中扩增出了HCV的基因片段,但用BVDV引物从这两个地区的病料中均未扩增出BVDV的基因片段。从哲盟疑似猪瘟病料中扩增出的片段经克隆、序列测定及计算机分析证实,该片段的核苷酸序列和氨基酸序列与BVDV的同源性明显高于与HCV的同源性。将哲盟病料接种于MDBK传代细胞,出现典型而规律的BVDV样细胞病变。由此证明,从哲盟疑似猪瘟病料中检测出的是BVDV而不是HCV 相似文献
6.
从长春地区某牛场发生疑似为牛病毒性腹泻-黏膜病的病牛粪样中分离到1株病毒,经序列测定为牛病毒性腹泻病毒命名为BVDV CC13B株。核苷酸序列的测定结果显示,CC13B毒株的完全基因组序列由12 265个核苷酸组成,其中5′端非编码区包含380个核苷酸,3′端非编码区包含188个核苷酸。病毒基因组含有1个大的读码框架,编码1个由3 898个氨基酸组成的前体多聚蛋白。序列对比结果显示,CC13B毒株的核苷酸和氨基酸序列与国外CP-5A毒株同源性最高,分别为为96.2%和97.3%;而与国内分离株JZ05-1的同源性最低,分别为69.8%和71.0%。系统进化树分析结果表明,CC13B毒株与国内分离的长春184、Xinjiang-3156和H等分离株归类为BVDV基因Ⅰ型的Ib基因亚型。结果表明,长春地区近年发生的牛病毒性腹泻-黏膜病依然主要由BVDV基因Ⅰ型毒株引起。 相似文献
7.
1株牛病毒性腹泻病毒分离毒株的基因组特征 总被引:3,自引:3,他引:0
旨在从宁夏某奶牛群持续感染牛分离牛源牛病毒性腹泻病毒(BVDV),并解析其基因组特征,为研究我国不同地区BVDV分离株遗传演化规律提供理论依据。利用BVDV抗原检测试剂盒检测宁夏回族自治区银川市某示范区的240头高产奶牛间隔两周的双份抗凝血,筛选持续感染牛,分离血液淋巴细胞制备裂解液接种牛肾细胞(MDBK),分离鉴定获得BVDV株,克隆测序获得全基因组序列,比较分析其遗传演化关系。从该示范区高产奶牛筛选获得2头持续感染牛,分离获得1株非致细胞病变型BVDV,命名为NX2019/01。测序获得基因组全序列(12 107 nt),其中ORF长11 703 nt,编码3 898个氨基酸。在基因组水平,NX2019/01株与我国SD-15、ZM-95、XC、LN-1等1m亚型分离株相似性较高(92.17%~93.84%),但Erns、E1以及E2基因存在较大差异。示范区同群牛急性感染BVDV时,毒株E2蛋白N端编码区核苷酸突变可导致第9位或第67位氨基酸变异。重组分析表明,NX2019/01株E2基因179—288位核苷酸区段以及ZM-95株E1基因168位—E2基因332位核苷酸区段存在相似的重组信号,可能由主要亲本SD-15株与次要亲本LN-1株重组形成,表明NX2019/01株、ZM-95株在演化进程中与SD-15株以及LN-1株或早期流行的高度相似毒株存在密切关联。本研究从持续感染高产奶牛分离获得了牛源BVDV-1m亚型毒株,在基因组水平厘清了BVDV-1m亚型毒株的进化关系,并首次发现同亚型BVDV毒株基因同源重组,为进一步研究BVDV在我国的演化规律奠定了基础。 相似文献
8.
The genetic basis for cytopathogenicity of pestiviruses 总被引:8,自引:0,他引:8
Two biotypes of pestiviruses, cytopathogenic (cp) and noncp viruses, can be distinguished by their effects on tissue culture cells. Identification of cp bovine viral diarrhea virus (BVDV) has been frequently reported since antigenically closely related noncp and cp BVDV can be isolated from cattle with fatal mucosal disease (MD) and are called a virus pair. In contrast to the BVDV system, only few cp border disease virus (BDV) and cp classical swine fever virus (CSFV) strains have been described. Serological analyses and sequence comparison studies showed that cp pestiviruses arise from noncp viruses by mutation. Elaborate studies during the last 10 years revealed that in most cases RNA recombination is responsible for the generation of the cp viruses. Recent results showed a second way for the development of a cp pestivirus which is based on the introduction of a set of point mutations within the NS2 gene. 相似文献
9.
根据已发表的鸡传染性支气管炎病毒S1基因,设计并合成了一对引物,经RT-PCR扩增后获得全长约为1700bp的核苷酸序列。序列分析表明,S1基因的最大开放阅读框位于12位~1685位碱基之间,编码557个氨基酸;KIBVXJ株S1基因序列在19位~292位点的氨基酸区域内有较多的氨基酸置换、插入和与缺失现象;S1的裂解位点的序列为HRRRR,具有我国地方流行株的特征。KIBVXJ株的S1基因与国内外疫苗株的同源性分析表明,核苷酸同源率为73.8%~74.2%,氨基酸同源率为74.9%~76.0%。遗传进化分析表明,KIBVXJ株与国内外的主要疫苗株亲缘关系最远,与国内近年来分离的A2株、LX4株和QXIBV株的亲缘关系最近。 相似文献
10.
A region of genome from the NADL strain of BVDV corresponding to the coding sequence for the E2 glycoprotein has been molecularly cloned using RT-PCR. The viral cDNA sequence was used to construct vaccinia virus recombinants that expressed either the entire E2 coding sequence or fragments of it. These recombinants were used to immunise mice of three H-2 haplotypes to investigate their ability to elicit a neutralising antibody response against BVDV. Sera from mice immunised with the recombinant expressing full length E2 contained high levels of virus neutralising antibodies that in addition to giving neutralisation of the homologous NADL strain were also able to neutralise the Oregon C24V reference strain. These sera failed to give any neutralisation of the Osloss reference strain providing evidence for the division of BVDV isolates into at least two distinct E2 serotypes. These results were confirmed in gnotobiotic lambs. Expression of E2 fragments revealed the presence of at least two distinct neutralising epitopes, one of which was localised within the carboxy terminal 90 amino acids of the protein. 相似文献
11.
猪细小病毒SY-99株非结构蛋白NS1基因的克隆及序列分析 总被引:12,自引:0,他引:12
猪细小病毒(Porcine parvovirus,PPV)SY-99株由本室分离,提取SY-99株的基因组DNA,利用PCR扩增出全长NS1基因,将该基因克隆到 核表达载体pET28a中并测序。结果表明,NS1基因全长1989bp,编码662个氨基酸,氨基酸序列中含有PP 制过程中发挥重要作用的保守基序GKRN,并有3个潜在的糖基化位点,分别位于356-359、446-449、513-516位氨基酸处,SY-99株NS1基因与其它PPV毒株NADL2-1、NADL2-2、Kresse株核苷酸同源性分别为98%、99%、99%,氨基酸同源性分别为97%、99%、995。SN1基因的克隆为研究NS1在PPV的复制中所发挥的功能及利用人工表达的NS1来制备诊断抗原提供了可能。 相似文献
12.
鸡传染性支气管炎病毒国内分离D971株 5a、5b及核蛋白基因的分子特征 总被引:12,自引:0,他引:12
13.
猪源牛病毒性腹泻病毒的流行初探 总被引:7,自引:0,他引:7
根据牛病毒性腹泻病毒(BVDV)代表株NADL的NS5B基因序列,设计合成2对引物进行套式PCR,检测从浙江、安徽、湖南、江西、广西、辽宁等地采集的43份猪病料中BVDV的流行情况,结果有7份病料可以扩增出360bp的特异性条带,阳性率为16.3%。为追踪BVDV在猪体中的流行来源,我们又对细胞培养用国产及进口犊牛血清进行了检测,结果也能扩增到目的条带。对这些病料和血清中扩增出的目的条带进行克隆、测序,并用DNASTAR软件分析,结果表明这些目的片段均为BVDV序列,这些不同BVDV序列可以分为两个亚群,ZJ133、HN386、LN247、NCS-J属于BVDV-Ⅰa亚型,ZJ114、AH138、JX60、GX96、NCS-G、DZ属于BVDV-Ⅰb亚型。这些毒株与BVDVI型间的同源性为80.3%-98.6%,与BVDV-Ⅱ型的同源性为72.2%-74.4%。本文研究结果说明我国猪群中BVDV感染情况已经比较严重,应该予以重视。 相似文献
14.
为了解1株圈养小熊猫源犬瘟热病毒(CDV)GD-1的遗传变异情况,通过RT-PCR方法对该株CDV进行H、F基因的克隆、测序及序列分析。结果显示:该分离株的H基因序列与GenBank中丹麦报道的登录号为GU266280的犬源CDV毒株的核苷酸序列相似性最高,为96%;F基因序列与巴西报道的登录号为KY057355的犬源CDV的核苷酸序列相似性最高,为95.7%。下载CDV代表毒株序列进行遗传演化、氨基酸序列比对及分子特征分析。结果显示:H蛋白共有8个潜在的N-糖基化位点,分别位于19、149、309、391、422、456、587、603位点;H蛋白的SLAM受体结合位点氨基酸序列与欧亚野生型毒株一致,与疫苗株相比,530、549位氨基酸不同,与其他CDV参考毒株H蛋白相比还存在24、41等9处氨基酸位点发生明显变异,与标准强毒株A75/17的氨基酸相似性为95.2%,与Onderstepoort、Convac等5株疫苗株的氨基酸序列相似性为88.2%~89.3%;F蛋白共有6个N-糖基化位点,分别位于62、108、141、173、179、517位,与Onderstepoort等疫苗株氨基酸相似性为89.1%~89.7%;与其他参考毒株相比还存在115、130等11处氨基酸发生变异;构建基于H、F基因的遗传进化树,结果显示:该毒株位于Asia-4型的一个小的进化分支,这与目前我国流行毒株主要位于Asia-1型存在明显不同。本研究首次报道了小熊猫源的Asia-4基因型CDV野毒株,并对毒株的H及F基因进行了序列分析,对于了解我国CDV流行株的遗传变异情况、流行病学调查、疾病防控及疫苗研发等具有重要意义。 相似文献
15.
牛病毒性腹泻病毒P20和P14基因的克隆及序列分析 总被引:5,自引:0,他引:5
参考GenBank中BVDV Oregon C24V株的基因组序列设计两对引物,利用套式PCR方法扩增P20基因,扩增出预期525 bp的目的片段.扩增产物克隆至pMD18-T载体,经酶切鉴定获得阳性重组质粒并对其进行测序.测序结果与参考序列Oregon C24V比较,二者的核苷酸同源性仅为80.95%,推导氨基酸同源性为87.50%.测序结果经NCBI上的Blast(Http:/www.ncbi.nlm.nih.gov/BLAST/)同源性比较,克隆得到的基因与Osloss株同源性最高,核苷酸同源性为93.65%,推导氨基酸同源性为95.83%.根据P20的测序结果,参照GenBank中BVDV Osloss株设计一对引物,扩增P14基因,经同源性比较,扩增的P14基因与Osloss株核苷酸同源性为94.77%,推导氨基酸同源性为95.10%,通过系统发生分析,推测P20基因和P14基因与Osloss株在进化上比较接近. 相似文献
16.
17.
【目的】利用原核表达系统体外表达牛病毒性腹泻病毒(Bovine viral diarrhea virus,BVDV)NS5A基因,获得非结构蛋白NS5A,对其进行核苷酸、氨基酸序列分析,以解析BVDV非结构蛋白NS5A的功能。【方法】参考BVDV-1型毒株V006的NS5A基因序列(GenBank登录号:KX170647)设计并合成1对特异性引物,以分离到的牦牛BVDV GSTZ毒株cDNA为模板,PCR扩增NS5A基因片段,并克隆至表达载体pET-28a (+)中,构建重组原核表达载体pET28a-NS5A。经酶切初步鉴定及测序鉴定正确后,转化大肠杆菌BL21(DE3)感受态细胞,然后利用IPTG诱导表达。经10% SDS-PAGE电泳及Western blotting分析鉴定重组蛋白的表达,并根据NS5A基因的序列构建遗传发育进化树,利用DNAStar软件预测NS5A蛋白的亲水性、表面可塑性和抗原性等特性,并结合二级结构的预测对NS5A蛋白的B细胞抗原表位进行预测。【结果】PCR扩增NS5A目的基因片段为1 488 bp,双酶切和测序鉴定结果证明,重组质粒pET28a-NS5A构建成功。经10% SDS-PAGE电泳及Western blotting鉴定重组蛋白,表达出了大小为55 ku的目的蛋白,大小与预期结果相符。通过对不同BVDV毒株NS5A基因序列构建遗传发育进化树,显示GSTZ毒株NS5A在遗传进化特征上属于BVDV-1型。NS5A蛋白的亲水性主要位于12—21、32—69、75—113、120—135、143—147、152—163、165—180、215—230、265—274、296—340、348—378、389—447、455—463、469—495位氨基酸处,表面可塑性主要位于14—18、37—42、76—81、86—109、154—160、169—178、218—228、297—309、348—358、365—373、414—442、430—437、454—460位氨基酸处,柔性区域较多,主要位于14—21、37—43、67—82、86—93、97—110、152—158、169—179、218—231、240—255、296—310、313—328、344—359、364—373、413—422和472—483位氨基酸处。NS5A蛋白的B细胞抗原表位主要位于15—18、76—81、154—158、169—178、218—228、297—309、348—358、365—373和414—422位氨基酸处。【结论】成功表达并鉴定了牦牛源BVDV的非结构蛋白NS5A,系统发育进化树表明BVDV GSTZ株基因型属于BVDV-1型,NS5A蛋白具有良好的抗原性,为深入解析BVDV非结构蛋白NS5A的自身结构功能、免疫学特性以及进一步研究非结构蛋白对病毒复制的影响提供参考。 相似文献
18.
番鸭细小病毒国内分离株主要结构蛋白基因的克隆和序列分析 总被引:4,自引:0,他引:4
根据国外已发表的番鸭细小病毒 (MPV) FM株基因组核苷酸序列 ,设计了 1对引物 ,分别对国内 2株番鸭细小病毒分离株 MPV扬州 (YZ)株和 MPV佛山 (FS)株主要结构蛋白 (VP2和 VP3)基因进行 PCR扩增 ,并克隆到p CR3.1T载体 ,经酶切鉴定筛选出阳性克隆质粒并进行核苷酸序列分析比较。结果表明 ,MPV YZ和 MPV FS的VP2 - VP3基因大小均为 176 4bp,编码 5 88个氨基酸。 MPV YZ、MPV FS与 MPV FM核苷酸序列同源性分别为98.5 %和 98.6 % ,氨基酸序列同源性为 97.1%和 97.8% ;MPV YZ与 MPV FS核苷酸序列的同源性为 99.5 % ,氨基酸序列同源性为 98.8%。 相似文献
19.
Evaluation of multiple immune parameters after vaccination with modified live or killed bovine viral diarrhea virus vaccines 总被引:1,自引:0,他引:1
Reber AJ Tanner M Okinaga T Woolums AR Williams S Ensley DT Hurley DJ 《Comparative immunology, microbiology and infectious diseases》2006,29(1):61-77
The development of immunity to vaccine antigen was examined using three prime/boost strategies and the progression of immune activities was evaluated over the course of 8 weeks. Calves were vaccinated and multiple immune parameters were evaluated using several methods to assess humoral or cellular immunity from the same samples in parallel. The three vaccination protocols used were a killed vaccine followed by a killed boost (killed/killed), MLV vaccine and boost (MLV/MLV), or a MLV vaccine and killed boost (MLV/killed). All the vaccines used included modified live IBR/PI3 viruses to make the bystander context as similar as possible. The Singer strain of BVDV was used as the source antigen in the killed vaccine, and the NADL strain of BVDV was used in the MLV vaccine. Controls received a vaccine containing only MLV IBR/PI3. The assessment panel measured SN titers, as well as lymphocyte proliferation, cytokine mRNA expression, intracellular cytokine production, and released IFN-gamma after in vitro stimulation with three strains of BVDV virus. MLV/MLV and MLV/killed groups developed significant SN titers to the type 1 BVDV virus strains, Singer and NADL, and low crossover titers were also seen to the type 2 strain, 890 over the evaluation period. These two groups showed significant proliferation in response to the NADL virus as compared to controls. Multiple immune assessments were conducted simultaneously to attempt to provide a broader, more in depth evaluation of immune response to these BVDV vaccination protocols. We observed that the correlation among most of the assays conducted were weak; the correlation between SN titers and cellular proliferation assays demonstrated a moderate correlation. 相似文献
20.
新城疫病毒(长春株)F蛋白基因的克隆和序列分析 总被引:15,自引:6,他引:15
新城疫病毒(NDV)长春株在鸡胚增殖后纯化,提取RNA,然后利用特异性引物,经RT-PCR一次性扩增出了NDV长春株的全长F基因。将该F基因插入pKS(-)后,进行了序列测定。序列分析表明,该F基因核苷酸长度为1758bp,编码553个氨基酸,序列中有6个糖基化位点,13个半胱氨酸残基,裂解位点区(112~117)氨基酸序列为Gly-Arg-Gln-Gly-Arg-Leu,与所有弱毒株在这一区域的序列(Gly-Arg/Lys-Gln-Gly/Ser-Arg-Leu)相符,证明长春株为弱毒株。同源性分析表明,长春株F基因与目前国外发表的其他NDVF基因相比,核苷酸序列同源性在88%~99%之间,推导的氨基酸序列同源性在90%~98%之间 相似文献