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Cell-specific nuclear import of plasmid DNA in smooth muscle requires tissue-specific transcription factors and DNA sequences.

机译:平滑肌中质粒DNA的细胞特异性核输入需要组织特异性转录因子和DNA序列。

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Two shortcomings of nonviral gene therapy are a lack of tissue-specific targeting of vectors and low levels of gene transfer. Our laboratory has begun to address these limitations by designing plasmids that enter the nucleus of specific cell types in the absence of cell division, thereby enhancing expression in a controlled manner. We have shown that a 176 bp portion of the smooth muscle gamma-actin (SMGA) promoter can mediate plasmid nuclear import specifically in smooth muscle cells (SMCs). Here, we demonstrate that the binding sites for serum response factor (SRF) and NKX3-1/3-2 within this DNA nuclear targeting sequence (DTS) are required for plasmid nuclear import. Knockdown of these factors with siRNA abrogates plasmid nuclear import, indicating that they are necessary cofactors. In addition, coinjection of recombinant SRF and Nkx3.2 with the vector in TC7 epithelial cells rescues import. Finally, we show that the SRF nuclear localization sequence (NLS) is required for vector nuclear import. We propose that SRF and NKX3-1/3-2 bind the SMGA DTS in the cytoplasm, thus coating the plasmid with NLSs that mediate translocation across the nuclear pore complex. This discovery could aid in the development of more efficient nonviral vectors for gene transfer to SMCs.
机译:非病毒基因治疗的两个缺点是缺乏载体的组织特异性靶向和低水平的基因转移。我们的实验室已开始通过设计在不存在细胞分裂的情况下进入特定细胞类型的细胞核的质粒来解决这些局限性,从而以受控方式增强表达。我们已经表明,平滑肌γ-肌动蛋白(SMGA)启动子的176 bp部分可以介导质粒核导入,特别是在平滑肌细胞(SMC)中。在这里,我们证明了在质粒DNA导入中需要血清反应因子(SRF)和NKX3-1 / 3-2在该DNA核靶向序列(DTS)中的结合位点。用siRNA敲除这些因子可消除质粒的核输入,表明它们是必需的辅因子。另外,重组载体SRF和Nkx3.2与载体在TC7上皮细胞中的共注射可以挽救进口。最后,我们表明载体核导入需要SRF核定位序列(NLS)。我们建议SRF和NKX3-1 / 3-2结合SMGA DTS在细胞质中,从而用介导跨核孔复合体易位的NLSs覆盖质粒。这一发现可能有助于开发更有效的非病毒载体,以将基因转移至SMC。

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