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Efficient expression of exogenous genes in primary vascular cells using IRES-based retroviral vectors

机译:使用基于IRES的逆转录病毒载体在原代血管细胞中高效表达外源基因

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摘要

Analysis of gene function in primary vascular cells has been particularly limited by low transfection efficiencies. Using internal ribosomal entry site (IRES)-based retroviral vectors, we demonstrate efficient infection (range of 45%-95%) of primary human endothelial and smooth muscle cells with genes varying in size from 1.3 to 4.5 kb. Because IRES vectors are designed to allow the expression of two genes from a single mRNA, we can show excellent correlation between the expression of a reporter gene and an inserted gene of interest. Reporter gene expression allows rapid (24-48 h) and unambiguous identification of transduced cells. Additionally, reporter gene expression can be used to isolate subpopulations of cells that express distinct levels of cistron 1 genes by flow cytometry, and sorted cells maintain relative levels of gene expression over multiple passages in culture. Two examples of the usefulness of these vectors to characterize gene function in primary vascular cells include (i) the inhibition of endothelial cell inflammatory responses in a polyclonal population by the expression of a dominant negative inhibitor of nuclear factor-kappaB and (ii) monitoring the in vitro evolution of smooth muscle cells provided with a selective growth advantage by transduction with telomerase. Potential applications of retroviral expression strategies in vascular biology are also discussed.
机译:低转染效率特别限制了原代血管细胞基因功能的分析。使用基于内部核糖体进入位点(IRES)的逆转录病毒载体,我们证明有效感染(范围为45%-95%)的原代人内皮细胞和平滑肌细胞的基因大小从1.3到4.5 kb不等。因为IRES载体被设计为允许从单个mRNA表达两个基因,所以我们可以显示报告基因和感兴趣的插入基因之间的出色关联。报告基因的表达可以快速(24-48小时)和明确识别转导细胞。另外,报告基因表达可用于通过流式细胞术分离表达顺反子1基因水平不同的细胞亚群,分选的细胞在培养的多个传代中维持相对水平的基因表达。这些载体在原代血管细胞中表征基因功能的有用性的两个例子包括:(i)通过表达核因子-kappaB的显性负抑制剂抑制多克隆群体中的内皮细胞炎症反应,以及(ii)监测通过端粒酶的转导,平滑肌细胞的体外进化具有选择性的生长优势。还讨论了逆转录病毒表达策略在血管生物学中的潜在应用。

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