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用脂精胺包被的DNA进行基因转移优化。

Gene transfer optimization with lipospermine-coated DNA.

作者信息

Barthel F, Remy J S, Loeffler J P, Behr J P

机构信息

Institut de Physiologie, URA 1446 du CNRS, Strasbourg, France.

出版信息

DNA Cell Biol. 1993 Jul-Aug;12(6):553-60. doi: 10.1089/dna.1993.12.553.

Abstract

Designed synthetic DNA carriers represent an attractive alternative to the widely used calcium phosphate gene transfer technique. In this context, we developed a class of nucleic acid binding lipids, the lipopolyamines, which spontaneously condense DNA on a cationic lipid layer. The resulting nucleolipidic particles transfect most animal cells efficiently. However, compaction depends on many experimental factors, some of which have been varied here to give optimal transfection efficiency. When plasmid condensation by the lipospermine is performed in the absence of competing polyions or serum proteins, or when the gene of interest is diluted into carrier DNA, transfection efficiency is increased by 2-3 orders of magnitude. With these improvements, chloramphenicol acetyl transferase activity resulting from transfection of as little as 25 ng could easily be detected by a nonradioactive ELISA test.

摘要

设计合成的DNA载体是广泛使用的磷酸钙基因转移技术的一种有吸引力的替代方法。在这种情况下,我们开发了一类核酸结合脂质,即脂多胺,它能在阳离子脂质层上自发地浓缩DNA。由此产生的核脂质颗粒能有效地转染大多数动物细胞。然而,压实作用取决于许多实验因素,这里对其中一些因素进行了改变以获得最佳转染效率。当在没有竞争性聚离子或血清蛋白的情况下进行脂精胺对质粒的浓缩时,或者当将感兴趣的基因稀释到载体DNA中时,转染效率提高2至3个数量级。通过这些改进,用非放射性ELISA试验可以很容易地检测到低至25 ng转染所产生的氯霉素乙酰转移酶活性。

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