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影响核定位序列肽增强非病毒基因递送能力的因素。

Factors influencing the ability of nuclear localization sequence peptides to enhance nonviral gene delivery.

作者信息

Bremner K Helen, Seymour Leonard W, Logan Ann, Read Martin L

机构信息

Cancer Research UK Institute for Cancer Studies, University of Birmingham, Birmingham, B15 2TH, UK.

出版信息

Bioconjug Chem. 2004 Jan-Feb;15(1):152-61. doi: 10.1021/bc034140k.

DOI:10.1021/bc034140k
PMID:14733595
Abstract

Nonviral gene delivery is limited by inefficient transfer of DNA from the cytoplasm to the nucleus. Nuclear localization sequence (NLS) peptides have been widely used to exploit intracellular transport mechanisms and promote nuclear uptake of DNA. However, the exact conditions to successfully utilize the properties of NLS peptides are still unclear. In the present study a panel of NLS peptides that bind different transport receptors were compared for their ability to enhance nonviral gene transfer. Several factors such as method of incorporating the NLS peptide, type of NLS peptide, DNA morphology, and proper characterization of NLS peptide/DNA conjugates were identified as important considerations in utilizing NLS peptides to enhance gene transfer. In particular, it was shown that a peptide derived from human T cell leukaemia virus type 1 (HTLV) was able to effectively condense DNA into discrete particles and mediate levels of transgene expression up to 32-fold greater than polylysine-based polyplexes. This is the first study to demonstrate efficient transfection mediated by an importin beta-binding peptide based on the HTLV sequence. Promising results were also achieved with a 7-fold increase in gene expression using a NLS peptide/DNA conjugate formed by site-specific linkage of an extended SV40 peptide via a peptide nucleic acid (PNA) clamp. Altogether, the results from this study should help to define the requirements for successful NLS-enhanced transfection.

摘要

非病毒基因递送受到DNA从细胞质向细胞核低效转运的限制。核定位序列(NLS)肽已被广泛用于利用细胞内运输机制并促进DNA的核摄取。然而,成功利用NLS肽特性的确切条件仍不清楚。在本研究中,比较了一组结合不同转运受体的NLS肽增强非病毒基因转移的能力。在利用NLS肽增强基因转移方面,确定了几个重要的考虑因素,如NLS肽的掺入方法、NLS肽的类型、DNA形态以及NLS肽/DNA缀合物的适当表征。特别是,研究表明,源自人类1型T细胞白血病病毒(HTLV)的一种肽能够有效地将DNA浓缩成离散颗粒,并介导转基因表达水平比基于聚赖氨酸的多聚体高出32倍。这是第一项证明基于HTLV序列的输入蛋白β结合肽介导高效转染的研究。使用通过肽核酸(PNA)夹将延伸的SV40肽进行位点特异性连接形成的NLS肽/DNA缀合物,基因表达增加了7倍,也取得了有前景的结果。总之,本研究的结果应有助于确定成功进行NLS增强转染的要求。

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