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Improved transfection using epithelial cell line-selected ligands and fusogenic peptides

机译:使用上皮细胞系选择的配体和融合肽改善转染

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Synthetic gene transfer vectors can be optimised by combining DNA-binding peptides, cell surface receptor ligands, and fusogenic and nuclear localisation peptides. We have used the phage display technique to identify ligands of the tracheal epithelial cell line CFT-2. The peptides harboured by two phages were selected for transfection studies: peptide 7 (GRGDGDV) that contained the integrin-binding motif RGD, and peptide 9 (RFDSLKV) that was found in six out of 24 phages analysed. Both peptides, fused with the DNA-binding peptide P2 (SPKRSPKRSPKR), enhanced transfection efficiency in cell lines CFT-2, NT-1, NIH-3T3 and ECV-304. In particular, peptide P2-7 increased transfection efficiency from 36.5% to 44.8% in NIH-3T3 cells and from 10.9% to 14.4% in CFT-2 cells, when compared to transfections performed with peptide P2. Two fusogenic peptides, HA (GLFEAIAEFIEGGWEGLIEGC) and JTS-1 (GLFEALLELLESLWELLLEA), were then added to the complexes and shown to improve transfection efficiency to the same extent. For instance, when combined to peptide P2-7, transfection levels of 54.1% and 55.2% were attained in NIH-3T3 cells with HA and JTS-1, respectively. The addition of the ligands and fusogenic peptides thus allowed us to construct greatly improved transfection reagents.
机译:合成基因转移载体可以通过结合DNA结合肽,细胞表面受体配体以及融合和核定位肽来优化。我们已经使用噬菌体展示技术来鉴定气管上皮细胞系CFT-2的配体。选择了两个噬菌体所具有的肽进行转染研究:包含整联蛋白结合基序RGD的肽7(GRGDGDV),以及在分析的24个噬菌体中的六个中发现的肽9(RFDSLKV)。两种肽都与DNA结合肽P2(SPKRSPKRSPKR)融合,可增强细胞系CFT-2,NT-1,NIH-3T3和ECV-304的转染效率。尤其是,与用肽P2进行转染相比,肽P2-7在NIH-3T3细胞中的转染效率从36.5%增至44.8%,在CFT-2细胞中从10.9%增至14.4%。然后将两个融合肽HA(GLFEAIAEFIEGGWEGLIEGC)和JTS-1(GLFEALLELLESLWELLLEA)添加到复合物中,并显示出一定程度地提高了转染效率。例如,当与肽P2-7结合时,在具有HA和JTS-1的NIH-3T3细胞中,转染水平分别达到54.1%和55.2%。因此,配体和融合肽的添加使我们能够构建大大改进的转染试剂。

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