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shRNA Expression Plasmids Generated by a Novel Method Efficiently Induce Gene-Specific Knockdown in a Silkworm Cell Line

机译:通过一种新方法生成的shRNA表达质粒可有效诱导家蚕细胞系中的基因特异性敲低

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摘要

RNAi knockdown by using shRNA expression plasmids is widely used to determine the function of individual genes in mammals. Here we developed a simple method to create an IR DNA in a U6 small nuclear RNA promoter-based parent vector using a single-stranded IR DNA with short hairpin structure and Bst DNA polymerase. Furthermore, we demonstrated that the shRNA expression plasmids constructed by our method effectively induced target-specific RNAi in the silkworm cell line. We also found that sequence preference in the silkworm cell line was much lower than in mammalian cells and shRNA-induced RNAi was influenced by the length of the stem region.
机译:通过使用shRNA表达质粒进行RNAi敲除已广泛用于确定哺乳动物中单个基因的功能。在这里,我们开发了一种简单的方法,可以使用具有短发夹结构的单链IR DNA和Bst DNA聚合酶在基于U6小核RNA启动子的亲本载体中创建IR DNA。此外,我们证明了通过我们的方法构建的shRNA表达质粒可在蚕细胞系中有效诱导靶标特异性RNAi。我们还发现,家蚕细胞系中的序列优先级比哺乳动物细胞中的低得多,并且shRNA诱导的RNAi受茎区长度的影响。

著录项

  • 来源
    《Molecular Biotechnology》 |2009年第2期|173-179|共7页
  • 作者单位

    Innate Immunity Research Unit National Institute of Agrobiological Sciences Ibaraki 305-8634 Japan;

    Innate Immunity Research Unit National Institute of Agrobiological Sciences Ibaraki 305-8634 Japan;

    Innate Immunity Research Unit National Institute of Agrobiological Sciences Ibaraki 305-8634 Japan;

    Innate Immunity Research Unit National Institute of Agrobiological Sciences Ibaraki 305-8634 Japan;

    Genebank National Institute of Agrobiological Sciences Ibaraki 305-8634 Japan;

    Innate Immunity Research Unit National Institute of Agrobiological Sciences Ibaraki 305-8634 Japan;

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  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

    RNA interference; Bombyx mori; Short hairpin RNA; U6 promoter; Bst DNA polymerase;

    机译:RNA干扰;桑蚕;短发夹RNA;U6启动子;Bst DNA聚合酶;

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