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本文引用的文献

1
Use of a dialyzable short-chain phospholipid for efficient solubilization and reconstitution of influenza virus envelopes.使用可透析的短链磷脂实现流感病毒包膜的高效溶解和重组。
Biochim Biophys Acta. 2006 Apr;1758(4):527-36. doi: 10.1016/j.bbamem.2006.03.011. Epub 2006 Apr 3.
2
Reconstituted influenza virus envelopes as an efficient carrier system for cellular delivery of small-interfering RNAs.重组流感病毒包膜作为一种用于细胞递送小干扰RNA的高效载体系统。
Gene Ther. 2006 Mar;13(5):400-11. doi: 10.1038/sj.gt.3302673.
3
The many mechanisms of viral membrane fusion proteins.病毒膜融合蛋白的多种机制。
Curr Top Microbiol Immunol. 2005;285:25-66. doi: 10.1007/3-540-26764-6_2.
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Virosomes for antigen and DNA delivery.用于抗原和DNA递送的病毒体。
Adv Drug Deliv Rev. 2005 Jan 10;57(3):451-63. doi: 10.1016/j.addr.2004.09.005.
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Use of the nuclease inhibitor aurintricarboxylic acid (ATA) for improved non-viral intratumoral in vivo gene transfer by jet-injection.使用核酸酶抑制剂金精三羧酸(ATA)通过喷射注射改善非病毒瘤内体内基因转移。
J Gene Med. 2005 Apr;7(4):477-85. doi: 10.1002/jgm.690.
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Lipoplex-mediated delivery of nucleic acids: factors affecting in vivo transfection.脂质体介导的核酸递送:影响体内转染的因素
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Preparation of virosomes coated with the vesicular stomatitis virus glycoprotein as efficient gene transfer vehicles for animal cells.制备包被有水泡性口炎病毒糖蛋白的病毒体作为动物细胞高效基因转移载体。
Microbiol Immunol. 2004;48(3):163-74. doi: 10.1111/j.1348-0421.2004.tb03502.x.
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Efficient delivery of DNA to dendritic cells mediated by influenza virosomes.流感病毒体介导的DNA向树突状细胞的高效递送。
Vaccine. 2004 Jan 26;22(5-6):735-9. doi: 10.1016/j.vaccine.2003.08.024.
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Virology: a class act.病毒学:一门卓越的学科。
Nature. 2004 Jan 22;427(6972):307-8. doi: 10.1038/427307a.
10
LMO2-associated clonal T cell proliferation in two patients after gene therapy for SCID-X1.两名接受X连锁重症联合免疫缺陷(SCID-X1)基因治疗的患者中与LMO2相关的克隆性T细胞增殖。
Science. 2003 Oct 17;302(5644):415-9. doi: 10.1126/science.1088547.

由包裹有质粒DNA的流感病毒体介导的细胞基因转移。

Cellular gene transfer mediated by influenza virosomes with encapsulated plasmid DNA.

作者信息

de Jonge Jørgen, Leenhouts Johanna M, Holtrop Marijke, Schoen Pieter, Scherrer Peter, Cullis Pieter R, Wilschut Jan, Huckriede Anke

机构信息

Department of Medical Microbiology, Molecular Virology Section, University Medical Center Groningen and University of Groningen, Groningen, The Netherlands.

出版信息

Biochem J. 2007 Jul 1;405(1):41-9. doi: 10.1042/BJ20061756.

DOI:10.1042/BJ20061756
PMID:17355227
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1925238/
Abstract

Reconstituted influenza virosomes (virus membrane envelopes) have been used previously to deliver pDNA (plasmid DNA) bound to their external surface to a variety of target cells. Although high transfection efficiencies can be obtained with these complexes in vitro, the virosome-associated DNA is readily accessible to nucleases and could therefore be prone to rapid degradation under in vivo conditions. In the present study, we show a new method for the production of DNA-virosomes resulting in complete protection of the DNA from nucleases. This method relies on the use of the short-chain phospholipid DCPC (dicaproylphosphatidylcholine) for solubilization of the viral membrane. The solubilized viral membrane components are mixed with pDNA and cationic lipid. Reconstitution of the viral envelopes and simultaneous encapsulation of pDNA is achieved by removal of the DCPC from the mixture through dialysis. Analysis by linear sucrose density-gradient centrifugation revealed that protein, phospholipid and pDNA physically associated to particles, which appeared as vesicles with spike proteins inserted in their membranes when analysed by electron microscopy. The DNA-virosomes retained the membrane fusion properties of the native influenza virus. The virosome-associated pDNA was completely protected from degradation by nucleases, providing evidence for the DNA being highly condensed and encapsulated in the lumen of the virosomes. DNA-virosomes, containing reporter gene constructs, transfected a variety of cell lines, with efficiencies approaching 90%. Transfection was completely dependent on the fusogenic properties of the viral spike protein haemagglutinin. Thus, DNA-virosomes prepared by the new procedure are highly efficient vehicles for DNA delivery, offering the advantage of complete DNA protection, which is especially important for future in vivo applications.

摘要

重组流感病毒体(病毒膜包膜)此前已被用于将结合在其外表面的质粒DNA(pDNA)递送至多种靶细胞。尽管这些复合物在体外可获得较高的转染效率,但病毒体相关的DNA很容易被核酸酶识别,因此在体内条件下可能易于快速降解。在本研究中,我们展示了一种生产DNA-病毒体的新方法,可使DNA完全免受核酸酶的降解。该方法依赖于使用短链磷脂DCPC(二癸酰磷脂酰胆碱)来溶解病毒膜。将溶解的病毒膜成分与pDNA和阳离子脂质混合。通过透析从混合物中去除DCPC,从而实现病毒包膜的重构以及pDNA的同时包封。线性蔗糖密度梯度离心分析表明,蛋白质、磷脂和pDNA与颗粒物理结合,通过电子显微镜分析时,这些颗粒表现为膜上插入有刺突蛋白的囊泡。DNA-病毒体保留了天然流感病毒的膜融合特性。病毒体相关的pDNA完全免受核酸酶的降解,这为DNA高度浓缩并包封在病毒体腔内提供了证据。含有报告基因构建体的DNA-病毒体转染了多种细胞系,转染效率接近90%。转染完全依赖于病毒刺突蛋白血凝素的融合特性。因此,通过新方法制备的DNA-病毒体是高效的DNA递送载体,具有DNA完全保护的优势,这对于未来的体内应用尤为重要。