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首页> 外文期刊>Journal of Virological Methods >Construction and characterization of a stable subgenomic replicon system of a Brazilian dengue virus type 3 strain (BR DEN3 290-02)
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Construction and characterization of a stable subgenomic replicon system of a Brazilian dengue virus type 3 strain (BR DEN3 290-02)

机译:巴西登革热病毒3型病毒株(BR DEN3 290-02)的稳定亚基因组复制子系统的构建和表征

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摘要

Dengue viruses (DENV) cause the most common arboviral disease afflicting men. Clinical manifestations range from asymptomatic to dengue hemorrhagic fever/dengue shock syndrome (DHF/DSS). The mechanisms involved in the disease pathogenesis are not fully understood. The severity of the disease seems to be influenced by both viral and host factors. Subgenomic replicons of DENV can be used to study viral replication mechanisms and evaluate the effects of antiviral drugs on viral replication. The objective was to generate and characterize biologically a replicon from a clinical isolate of DENV-3, as part of our studies to understand how this new isolate interacts with cells. To obtain this replicon several RT-PCR fragments encoding the non-structural proteins genes were cloned in high-copy vectors, and used to assemble the replicon in a BAC plasmid vector containing a synthetic DNA molecule encoding the 5' and 31 ends of a viral cDNA with a T7 DNA-dependent RNA polymerase promoter and a ribozyme. In vitro transcribed RNA recovered from this BAC plasmid was transfected into C6/36 mosquito cells, and dengue virus protein expression was assessed by indirect immunofluorescence using polyclonal antibodies. The results showed that the replicon was replicated efficiently in cells, demonstrating successful assembly of a DENV-3 replicon.
机译:登革热病毒(DENV)是困扰男性的最常见的虫媒病毒疾病。临床表现从无症状到登革出血热/登革热休克综合征(DHF / DSS)。尚未完全了解疾病发病机理的机制。该疾病的严重程度似乎受到病毒和宿主因素的影响。 DENV的亚基因组复制子可用于研究病毒复制机制并评估抗病毒药物对病毒复制的影响。目的是从DENV-3的临床分离株中生成复制子并对其进行生物学表征,这是我们了解该新分离株如何与细胞相互作用的研究的一部分。为了获得该复制子,将几个编码非结构蛋白基因的RT-PCR片段克隆到高拷贝载体中,并用于在包含编码病毒5'和31末端合成DNA分子的BAC质粒载体中组装复制子。具有T7 DNA依赖性RNA聚合酶启动子和核酶的cDNA。从该BAC质粒中回收的体外转录RNA被转染到C6 / 36蚊子细胞中,并使用多克隆抗体通过间接免疫荧光法评估了登革热病毒蛋白的表达。结果表明,该复制子在细胞中被有效复制,表明DENV-3复制子的成功组装。

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