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Inhibition of simian immunodeficiency virus by foamy virus vectors expressing siRNAs.

机译:表达siRNA的泡沫病毒载体对猿猴免疫缺陷病毒的抑制作用。

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摘要

Viral vectors available for gene therapy are either inefficient or suffer from safety concerns for human applications. Foamy viruses are non-pathogenic retroviruses that offer several unique opportunities for gene transfer in various cell types from different species. In this report, we describe the use of simian foamy virus type 1 (SFV-1) vector to examine the efficacy of therapeutic genes. Hairpin short-interfering RNA (siRNA) that targets the simian immunodeficiency virus (SIV) rev/env was placed under the control of the PolIII U6 snRNA promoter for expression and screened for silencing target genes using cognate target-reporter fusions. We have identified an effective siRNA (designated R2) which reduces the rev and env gene expression by 89% and 95%, respectively. Using the simian foamy virus type 1 (SFV-1) based vector, we delivered the PolIII expressed R2 siRNA into cultured cells and challenged with SIV. The results show that the R2 siRNA is a potent inhibitor of SIV replication as determined byp27 expression and reverse transcriptase assays. Vectors based on a non-pathogenic SFV-1 vector may provide a safe and efficient alternative to currently available vectors, and the SIV model will help devise protocols for effective anti-HIV gene therapy.
机译:可用于基因治疗的病毒载体效率低下或存在人类应用的安全隐患。泡沫病毒是非致病性逆转录病毒,为来自不同物种的各种细胞类型的基因转移提供了几种独特的机会。在此报告中,我们描述了使用猿猴泡沫病毒1型(SFV-1)载体来检查治疗性基因的功效。将靶向猿猴免疫缺陷病毒(SIV)rev / env的发夹短干扰RNA(siRNA)置于PolIII U6 snRNA启动子的控制下进行表达,并使用同源靶标-报告子融合蛋白筛选沉默的靶标基因。我们已经鉴定出有效的siRNA(称为R2),可将rev和env基因表达分别降低89%和95%。使用基于猿猴泡沫病毒1型(SFV-1)的载体,我们将PolIII表达的R2 siRNA递送到培养细胞中并用SIV攻击。结果表明,根据p27表达和逆转录酶分析,R2 siRNA是SIV复制的有效抑制剂。基于非致病性SFV-1载体的载体可为当前可用载体提供安全有效的替代方法,SIV模型将有助于设计有效的抗HIV基因治疗方案。

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