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首页> 外文期刊>ACS nano >Peptide dendrimer/lipid hybrid systems are efficient DNA transfection reagents: Structure-activity relationships highlight the role of charge distribution across dendrimer generations
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Peptide dendrimer/lipid hybrid systems are efficient DNA transfection reagents: Structure-activity relationships highlight the role of charge distribution across dendrimer generations

机译:肽树状聚合物/脂质杂合系统是有效的DNA转染试剂:结构-活性关系突显了树状聚合物各代之间电荷分布的作用

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Efficient DNA delivery into cells is the prerequisite of the genetic manipulation of organisms in molecular and cellular biology as well as, ultimately, in nonviral gene therapy. Current reagents, however, are relatively inefficient, and structure-activity relationships to guide their improvement are hard to come by. We now explore peptide dendrimers as a new type of transfection reagent and provide a quantitative framework for their evaluation. A collection of dendrimers with cationic and hydrophobic amino acid motifs (such as KK, KA, KH, KL, and LL) distributed across three dendrimer generations was synthesized by a solid-phase protocol that provides ready access to dendrimers in milligram quantities. In conjunction with a lipid component (DOTMA/DOPE), the best reagent, G1,2,3-KL ((LysLeu)8(LysLysLeu)4(LysLysLeu) 2LysGlySerCys-NH2), improves transfection by 6-10-fold over commercial reagents under their respective optimal conditions. Emerging structure-activity relationships show that dendrimers with cationic and hydrophobic residues distributed in each generation are transfecting most efficiently. The trigenerational dendritic structure has an advantage over a linear analogue worth up to an order of magnitude. The success of placing the decisive cationic charge patterns in inner shells rather than previously on the surface of macromolecules suggests that this class of dendrimers significantly differs from existing transfection reagents. In the future, this platform may be tuned further and coupled to cell-targeting moieties to enhance transfection and cell specificity.
机译:有效地将DNA传递到细胞中是在分子和细胞生物学以及最终在非病毒基因治疗中对生物进行基因操作的前提。然而,当前的试剂效率相对较低,并且难以获得指导其改进的结构-活性关系。现在,我们探索肽树状聚合物作为新型转染试剂,并为其评估提供定量框架。通过固相规程合成了分布在三个树状聚合物世代中的具有阳离子和疏水性氨基酸基序(例如KK,KA,KH,KL和LL)的树状聚合物的集合,该方案可以方便地获取毫克量的树状聚合物。与脂质成分(DOTMA / DOPE)结合使用时,最好的试剂G1,2,3-KL((LysLeu)8(LysLysLeu)4(LysLysLeu)2LysGlySerCys-NH2)的转染效果比市售产品提高6-10倍试剂在各自的最佳条件下。新兴的结构-活性关系表明,在每一代中分布有阳离子和疏水残基的树枝状聚合物的转染效率最高。三代树突状结构具有优于线性模拟物的优势,其价值高达一个数量级。将决定性的阳离子电荷模式置于内壳而不是先前在大分子表面上的成功表明,这类树状聚合物与现有的转染试剂有很大不同。将来,可以进一步调整该平台并将其与细胞靶向部分偶联,以增强转染和细胞特异性。

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