首页> 美国卫生研究院文献>Journal of Virology >Analysis of extracellular West Nile virus particles produced by cell cultures from genetically resistant and susceptible mice indicates enhanced amplification of defective interfering particles by resistant cultures.
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Analysis of extracellular West Nile virus particles produced by cell cultures from genetically resistant and susceptible mice indicates enhanced amplification of defective interfering particles by resistant cultures.

机译:对来自具有遗传抗性和易感性的小鼠的细胞培养物产生的细胞外西尼罗河病毒颗粒的分析表明抗性培养物可增强缺陷性干扰颗粒的扩增。

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摘要

[3H]uridine-labeled extracellular West Nile virus (WNV) particles produced by cell cultures obtained from genetically resistant C3H/RV and congenic susceptible C3H/HE mice were compared by sucrose density gradient centrifugation as well as by analysis of the particle RNA. Defective interfering (DI) WNV particles were observed among progeny produced during acute infections in both C3H/RV and C3H/HE cells. Although only a partial separation of standard and DI particles was achieved, the DI particles were found to be more dense than the standard virions. Particles containing several species of small RNAs consistently constituted a major proportion of the total population of virus progeny produced by C3H/RV cells, but a minor proportion of the population produced by C3H/HE cells. Decreasing the multiplicity of infection or extensive plaque purification of the WNV inoculum decreased the proportion of small RNAs found in the progeny virus. The ratio of DI particles to standard virus observed in progeny virus was determined by the cell type used to grow the virus. The ratio could be shifted by passaging virus from one cell type to the other. Homologous interference could be demonstrated with WNV produced by C3H/RV cells but not with virus produced by C3H/HE cells. Continued passage of WNV in C3H/HE cells resulted in a cycling of infectivity. However, passage in C3H/RV cells resulted in the complete loss of infectious virus. Four size classes of small viral RNA, with sedimentation coefficients of about 8, 15, 26, and 34S, were observed in the extracellular particles. A preliminary analysis of these RNAs by oligonucleotide fingerprinting indicated that the smaller RNAs were less complex than the 40S RNA and differed from each other. The data are consistent with the conclusion that WNV DI particles interfere more effectively with standard virus replication and are amplified more efficiently in C3H/RV cells than in congenic C3H/HE cells. The relevance of these findings to the further understanding of genetically controlled resistance to flaviviruses is discussed.
机译:通过蔗糖密度梯度离心以及对颗粒RNA的分析,比较了从具有遗传抗性的C3H / RV和同基因易感的C3H / HE小鼠获得的细胞培养物中产生的[3H]尿苷标记的胞外西尼罗河病毒(WNV)颗粒。在C3H / RV和C3H / HE细胞的急性感染过程中产生的子代中均观察到了缺陷性干扰(DI)WNV颗粒。尽管仅实现了标准颗粒和DI颗粒的部分分离,但发现DI颗粒比标准病毒体更致密。包含数种小RNA的颗粒始终占C3H / RV细胞产生的病毒后代总数的主要部分,但占C3H / HE细胞产生的总数的次要部分。减少WNV接种物的感染多样性或广泛的噬菌斑纯化,会降低在子代病毒中发现的小RNA的比例。在子代病毒中观察到的DI颗粒与标准病毒的比例取决于用于繁殖该病毒的细胞类型。通过传代病毒可以将该比例从一种细胞类型转移到另一种细胞类型。同源干扰可以由C3H / RV细胞产生的WNV证明,而不能由C3H / HE细胞产生的病毒证明。 WNV在C3H / HE细胞中的持续传代导致感染力循环。但是,在C3H / RV细胞中传代会导致传染性病毒完全丧失。在细胞外颗粒中观察到四种大小的小病毒RNA,其沉降系数约为8、15、26和34S。通过寡核苷酸指纹图谱对这些RNA的初步分析表明,较小的RNA不如40S RNA复杂,并且彼此不同。数据与以下结论一致:WNV DI颗粒比标准C3H / HE细胞更有效地干扰标准病毒复制,并在C3H / RV细胞中更有效地扩增。讨论了这些发现与进一步了解黄病毒的基因控制抗性的相关性。

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