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Remnant cationic dendrimers block RNA migration in electrophoresis after monophasic lysis

机译:单相裂解后,残留的阳离子树状聚合物可阻止电泳中的RNA迁移

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Cationic dendrimers such as poly(amidoamine) (PAMAM) and poly(propyleneimine) (PPI) have attractive characteristics for the delivery of nucleic acid and various biomedical applications. Most studies have focused on cationic dendrimer-based intracellular delivery, and very few studies have focused on the non-specific interaction of remnant cationic dendrimers with total RNA after isolation directly from cells in vitro. We examined RNA isolation using the common method of monophasic lysis from human macrophage-like cells (U937) and mouse fibroblast cells (NIH/3T3) that had been exposed to dendrimers and DNA/dendrimer complexes using gel electrophoresis. We found that PAMAM and PPI dendrimers strongly altered the mobility of RNA in the gels. In addition, the extent of dendrimer-induced alteration in RNA mobility was directly dendrimer-generation-dependent: the alteration was greater with higher-generation dendrimers. We also found that DNA/dendrimer complexes at higher dendrimer to DNA ratios interacted with RNA after isolation while gene expression was maintained. The interactions between RNA and remnant dendrimers after isolation were caused by electrostatic bindings, and we recovered total RNA using high ionic strength solvents (2M NaCl solution) to disrupt the electrostatic forces binding dendrimers to RNA. Because RNA isolation is routinely used for biological applications, such dendrimer-induced alteration in RNA mobility should be accounted for in the further processing of RNA-related applications.
机译:阳离子树状聚合物,例如聚(酰胺基胺)(PAMAM)和聚(丙烯亚胺)(PPI)具有吸引人的特性,可用于核酸的输送和各种生物医学应用。大多数研究集中于基于阳离子树状聚合物的细胞内递送,很少研究集中于直接从细胞中分离后残留阳离子树状聚合物与总RNA的非特异性相互作用。我们使用单相裂解的常规方法从人巨噬细胞样细胞(U937)和小鼠成纤维细胞(NIH / 3T3)中使用凝胶电泳暴露于树状大分子和DNA /树状大分子复合物,研究了RNA的分离。我们发现PAMAM和PPI树状聚合物强烈改变了凝胶中RNA的迁移率。此外,树枝状大分子诱导的RNA迁移率变化的程度直接取决于树枝状大分子的生成:较高年龄的树枝状大分子的变化更大。我们还发现,在保持基因表达不变的情况下,分离后较高的树状体与DNA比率的DNA /树状体复合物与RNA相互作用。分离后,RNA与残余树状聚合物之间的相互作用是由静电结合引起的,我们使用高离子强度溶剂(2M NaCl溶液)回收了破坏总树状分子与RNA的静电力,从而回收了总RNA。由于RNA分离通常用于生物学应用,因此在进一步处理RNA相关应用时应考虑到树枝状大分子诱导的RNA迁移率变化。

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