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首页> 外文期刊>Virology >Establishment and characterization of plasmid-driven minigenome rescue systems for Nipah virus: RNA polymerase I- and T7-catalyzed generation of functional paramyxoviral RNA.
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Establishment and characterization of plasmid-driven minigenome rescue systems for Nipah virus: RNA polymerase I- and T7-catalyzed generation of functional paramyxoviral RNA.

机译:Nipah病毒的质粒驱动微型基因组拯救系统的建立和表征:RNA聚合酶I和T7催化的功能性副粘病毒RNA的产生。

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摘要

In this study we report the development and optimization of two minigenome rescue systems for Nipah virus, a member of the Paramyxoviridae family. One is mediated by the T7 RNA polymerase supplied either by a constitutively expressing cell line or by transfection of expression plasmids and is thus independent from infection with a helper virus. The other approach is based on RNA polymerase I-driven transcription, a unique approach for paramyxovirus reverse genetics technology. Minigenome rescue was evaluated by reporter gene activities of (i) the two different minigenome transcription systems, (ii) genomic versus antigenomic-oriented minigenomes, (iii) different ratios of the viral protein expression plasmids, and (iv) time course experiments. The high efficiency and reliability of the established systems allowed for downscaling to 96-well plates. This served as a basis for the development of a high-throughput screening system for potential antivirals that target replication and transcription of Nipah virus without the need of high bio-containment. Using this system we were able to identify two compounds that reduced minigenome activity.
机译:在这项研究中,我们报告了副粘病毒科成员Nipah病毒的两个小型基因组拯救系统的开发和优化。一种是由组成型表达细胞系或表达质粒的转染提供的T7 RNA聚合酶介导的,因此独立于辅助病毒的感染。另一种方法是基于RNA聚合酶I驱动的转录,这是副粘病毒逆向遗传技术的独特方法。通过(i)两种不同的微型基因组转录系统,(ii)基因组与反基因组导向的微型基因组,(iii)不同比例的病毒蛋白表达质粒和(iv)时程实验的报告基因活性评估了微型基因组的拯救。已建立系统的高效率和可靠性允许将其规模缩小至96孔板。这为开发针对潜在的抗病毒药物的高通量筛选系统奠定了基础,这些抗病毒剂的目标是尼帕病毒的复制和转录,而无需高度的生物污染。使用该系统,我们能够鉴定出两种降低最小基因组活性的化合物。

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