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The 5'-untranslated region (5'-UTR) of the 'Giraffe' strain of pestivirus was sequenced for comparison with those of other pestiviruses from cattle, sheep, goats, and swine. A phylogenetic tree constructed with these strains suggested that the 'Giraffe' strain was allocated to a new taxon. This observation was also confirmed by a newly proposed method based on palindromic nucleotide substitutions (PNS) at the three variable regions in the 5'-UTR. Other reported pestivirus strains isolated from deer were assigned as bovine viral disease virus (BVDV)-1 according to the PNS as well as phylogenetic analysis, suggesting that BVDV-1 strains can cross-infect deer as well as cattle, sheep, goats, and swine, and that wild deer may serve as a reservoir of BVDV-1. We also identified the genovar of a deer isolate, SH9/11, as BVDV-1c by the PNS method. 相似文献
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The objective of this study was to determine the effect of BVD virus on the rabbit's endometrium. Six New Zealand White does (3-4 kg bwt) were used. Blood samples were obtained before treatment and euthanasia for determination of estrogen and progesterone. Does were anesthetized and both uterine horns identified through a midventral incision. Each horn was doubly-ligated at both cervical and ovarian ends. The right uterine horn (control) was injected with 1ml Eagle's MEM and the left (treated) with 1ml BVD virus (Singer strain, 10(3) CCID(50/ml)). Two does each were euthanized at 48h, 72h and 144h post-inoculation (PI) and uterine samples obtained for viral assay and light microscopic examination. Serum hormonal levels showed that all does were in the estrogenic phase before treatment and euthanasia. Viral isolation was negative for all samples taken. On each day examined, there were no histopathologic lesions in the control uterine horn. However, in the treated horn at 48h PI there was evidence of a purulent endometritis. At 72h and 144h PI there was mononuclear cell infiltration of the stratum compactum, but no other obvious lesions. A common feature in both treated and control uterine horns was mitosis of both endometrial and glandular epithelia. Results of this study suggest that BVD virus can induce histopathologic lesions of the rabbit's endometrium, the most obvious effect being at 48h PI. 相似文献
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BVDV(牛病毒性腹泻病毒)是一类有重要经济价值的病毒,其核酸为单链RNA。该病毒提纯以后.用苯酚-氯仿-异戊醇提取RNA.在提取的BVDy RNA中所含的DNA杂质用DNase I降解除去,然后进一步用oligo dT纤维素拄亲和层析,琼脂糖凝胶电泳等方法纯化。纯化的BVDV RNA在E.coli,poly A聚合酶的催化作用下,在3’羟基末端聚腺化。cDNA在逆向转录酶的作用下,用polyA接尾的BVDV RNA作模板,oligodT_12—18作引物合成。琼脂糖凝胶电泳结果说明它与BVDV RNA相似。该cDNA的探针用斑点杂交方法与BVDV RNA,HCV RNA和酵母tRNA杂交,BVDV RNA和HCVRNA显阳性反应,酵母tRNA显阴性反应,结果说明合成的cDNA为BVDV RNA的cDNA。BVDV和HCV同为披盖科疫病毒属成员,它们具有部分相同的抗原,因此编码病毒蛋白的RNA序列具有同源序列,本研究证实了这种假设。 相似文献
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目的:利用果蝇S2细胞表达牛病毒性腹泻病毒(BVDV)Erns-E2融合蛋白,并对其抗体结合能力进行鉴定。方法:用RT-PCR方法扩增BVDV NADL株Erns和E2蛋白的编码基因,利用(G4-S)3柔性15肽基因将扩增的2个基因连接,再与昆虫表达载体pMT/BiP/V5-His连接构建重组表达载体pMT/BiP/V5-His-Erns-E2,将后者与筛选质粒pCoBlast共转染果蝇S2细胞后表达Erns-E2融合蛋白,并对表达产物进行鉴定。结果:SDS-PAGE结果表明,融合蛋白相对分子质量为76800;Western blotting检测表明,该融合蛋白具有与BVDV抗体良好的结合能力。结论:BVDV的Erns-E2融合蛋白能在果蝇S2细胞中进行表达;经鉴定,表达产物具有良好的抗体结合能力,可用于抗原检测。 相似文献
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Contamination of animal-derived raw materials with viruses, mycoplasmas, bacteria and fungi is common. These contaminants
can interfere with the diagnosis of viral infection, and vaccines produced using infected cell cultures could lead to seroconversion
or disease in the vaccinated animal. The purity, safety and efficacy of viral vaccines requires testing of the ingredients,
cell substrates and final product. Methods for detection of viruses, especially bovine viral diarrhea virus, in nutrient serum,
cell cultures, seed viruses and viral vaccines, and the frequency of their detection at the Center for Veterinary Biologics
are discussed.
This revised version was published online in August 2006 with corrections to the Cover Date. 相似文献
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对梅花鹿源BVDV基因E0进行了克隆和序列分析。结果表明,梅花鹿源BVDV基因E0的大小为681bp,与报道9株BVDV(VEDEVAC、Bega、C24V、ILLC、NADL、OSLOSS、R1935、SD-1、Y546)和7株猪瘟病毒(ALD、Bres-cia、c、GPE、JL、LN9912、SM)及3株羊边界病毒(BD31、C413、BDVX818)相比,核苷酸序列的同源性依次为98.6%~84.8%、76.1%~74.7%、77.0%~76.7%。梅花鹿源BVDV为Ιb基因亚型。 相似文献
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以DNAStar5.01软件,对鹿源BVDV基因E0蛋白特性进行了分析。结果表明E0蛋白由227个残基构成,等电点为7.61。E0蛋白中有与地衣类植物核苷酸酶的保守区域相似序列,维持催化活性所必需的氨基酸残基区域在28-40和71-89处,催化活性的氨基酸为His30、His79,且该序列高度保守。E0蛋白氨基酸亲水性与抗原性指数成平行相关,BVDV各毒株间非常相似,亲水性与抗原性指数都较高的区域有8-16,23-29,59-67,70-81,96-109,114-122,127-134,137-143,165-172,186-198和213-221,适合研制亚单位基因工程疫苗。 相似文献
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试验首先根据GenBank上所发表的狂犬病病毒CVS-24株糖蛋白基因序列,设计并合成一对特异性引物,通过反转录 聚合酶链式反应(RT-PCR),获得糖蛋白全长cDNA,连接在pMD18-T载体上,测序证明克隆的正确性后,将其插入真核表达载体pIRES1neo,构建了糖蛋白单一表达载体pICG,表达质粒通过脂质体转染BHK-21细胞,在G418抗性压力下出现细胞克隆,通过PCR检测,确定启动子与糖蛋白基因在细胞基因组中共同整合。借助Western blot检测,证明所表达的糖蛋白与狂犬病抗血清有特异的反应性。采用间接ELISA法,筛选出3株高效表达糖蛋白的细胞株,分别命名为ICG1、ICG2、ICG3。 相似文献
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【目的】牛病毒性腹泻病毒(bovine viral diarrhea virus, BVDV)是引起牛病毒性腹泻-黏膜病的关键病毒。BVDV的结构蛋白Erns可在病毒感染的初期削弱宿主的免疫防御,引发牛群炎症反应。核苷酸寡聚化结构域样受体(nucleotide-binding oligomerization domain, NOD)热蛋白结构域相关蛋白3 (NLRP3)炎症小体是NOD样受体(NOD-like receptor, NLRs)家族重要成员,调控炎症性疾病的发生发展,同时激活的NLRP3炎症小体能够引起宿主细胞焦亡,进而诱发级联放大的炎症反应。但BVDV Erns蛋白在BVDV感染诱发炎症反应的分子机制尚不清楚。【方法】为进一步探索Erns蛋白对BVDV感染激活NLRP3炎症小体诱发细胞焦亡的影响,构建了BVDV Erns蛋白的真核表达质粒pCMV-HA-Erns,过表达BVDV Erns蛋白,检测BVDV感染细胞中NLRP3炎症小体组分[半胱氨酸蛋白酶(caspase-1)、凋亡相关斑点样蛋白(apoptosis-associated speck-like protein, ASC)和NLRP3]、IL-1β的mRNA转录水平和蛋白表达水平,以及细胞死亡调节蛋白(gasdermin D, GSDMD)的基因表达和蛋白剪切情况,并通过扫描电镜观察牛睾丸(bovine testis, BT)细胞膜成孔及BT细胞内容物释放情况,以分析Erns蛋白诱导BT细胞产生细胞焦亡。【结果】Erns蛋白能够显著引起NLRP3炎症小体活化进而激活caspase-1,活化的caspase-1一方面切割GSDMD,形成有活性的GSDMD-N端并在BT细胞膜形成孔洞,释放内容物,诱导BT细胞发生细胞焦亡;另一方面活化的caspase-1切割pro-IL-1β,形成有活性的IL-1β,并释放到BT细胞外,引起BT细胞上清中IL-1β水平上升。【结论】系统解析了BVDV Erns蛋白激活NLRP3炎症小体介导细胞焦亡的产生,对疫苗及治疗药物的研制具有重要指导意义。 相似文献
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牛病毒性腹泻病毒RT-LAMP检测方法的建立 总被引:4,自引:0,他引:4
目的:建立牛病毒性腹泻病毒(BVDv)的环介导体外等温扩增(LAMP)快速检测方法。方法:根据BVDv的5'端非编码区序列,在保守区的8个位点设计LAMP特异性引物(2对特异性引物和1对环引物),对反应条件和试剂浓度进行优化,建立恒温(63.5℃)、快速(65min)的检测方法。结果:建立的方法特异性好,检测其他对照病毒均为阴性;灵敏度高,最低可检测到1个拷贝的阳性质粒,可通过观察浑浊度或加入染料后直接判定扩增结果。结论:建立了用于检测BVDv的LAMP方法,该方法简便、快速、特异性好、灵敏度高,适合基层和现场检测。 相似文献
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牛病毒性腹泻病毒NS3基因的序列分析、表达与抗原性鉴定 总被引:1,自引:0,他引:1
本研究应用套式RT-PCR方法扩增出牛病毒性腹泻病毒VEDEVAC株编码NS3蛋白的基因,克隆至表达载体pET-30a(+),并进行测序。对瘟病毒属病毒NS3基因进行氨基酸差异性分析,显示平均P-distance为0.07,系统进化树分析表明VEDEVAC株隶属于BVDV1型。将构建成功的重组质粒转化大肠埃希氏菌Rosetta(DE3),在IPTG诱导下表达NS3重组蛋白,经Ni-NTA亲和层析纯化和尿素梯度透析后进行反应原性鉴定。Western blotting结果显示表达的重组蛋白可以与牛病毒性腹泻病毒阳性血清反应,并与猪瘟阳性血清有交叉反应,ELISA结果显示该重组蛋白具有良好的反应原性。所获得的蛋白为建立针对NS3抗体的ELISA检测方法奠定了基础。 相似文献
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Duarte L. Martins Jure Sencar Nikolaus Hammerschmidt Bjrn Tille Johanna Kinderman Thomas R. Kreil Alois Jungbauer 《Biotechnology journal》2019,14(8)
Continuous virus inactivation (VI) remains one of the missing pieces while the biopharma industry moves toward continuous manufacturing. The challenges of adapting VI to the continuous operation are two‐fold: 1) achieving fluid homogeneity and 2) a narrow residence time distribution (RTD) for fluid incubation. To address these challenges, a dynamic active in‐line mixer and a packed‐bed continuous virus inactivation reactor (CVIR) are implemented, which act as a narrow RTD incubation chamber. The developed concept is applied using solvent/detergent (S/D) treatment for inactivation of two commonly used model viruses. The in‐line mixer is characterized and enables mixing of the viscous S/D chemicals to ±1.0% of the target concentration in a small dead volume. The reactor's RTD is characterized and additional control experiments confirm that the VI is due to the S/D action and not induced by system components. The CVIR setup achieves steady state rapidly before two reactor volumes and the logarithmic reduction values of the continuous inactivation process are identical to those obtained by the traditional batch operation. The packed‐bed reactor for continuous VI unites fully continuous processing with very low‐pressure drop and scalability. 相似文献