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Selective targeting of human cells by a chimeric adenovirus vector containing a modified fiber protein.

机译:通过含有修饰的纤维蛋白的嵌合腺病毒载体对人细胞的选择性靶向。

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摘要

The adenovirus fiber protein is responsible for attachment of the virion to unidentified cell surface receptors. There are at least two distinct adenovirus fiber receptors which interact with the group B (Ad3) and group C (Ad5) adenoviruses. We have previously shown by using expressed adenovirus fiber proteins that it is possible to change the specificity of the fiber protein by exchanging the head domain with another serotype which recognizes a different receptor (S. C. Stevenson et al., J. Virol. 69:2850-2857, 1995). A chimeric fiber cDNA containing the Ad3 fiber head domain fused to the Ad5 fiber tail and shaft was incorporated into the genome of an adenovirus vector with E1 and E3 deleted encoding beta-galactosidase to generate Av9LacZ4, an adenovirus particle which contains a chimeric fiber protein. Western blot analysis of the chimeric fiber vector confirmed expression of the chimeric fiber protein and its association with the adenovirus capsid. Transduction experiments with fiber protein competitors demonstrated the altered receptor tropism of the chimeric fiber vector compared to that of the parental Av1LacZ4 vector. Transduction of a panel of human cell lines with the chimeric and parental vectors provided evidence for a different cellular distribution of the Ad5 and Ad3 receptors. Three cell lines (THP-1, MRC-5, and FaDu) were more efficiently transduced by the vector containing the Ad3 fiber head than by the Ad5 fiber vector. In contrast, human coronary artery endothelial cells were transduced more readily with the vector containing the Ad5 fiber than with the chimeric fiber vector. HeLa and human umbilical vein endothelial cells were transduced at equivalent levels compared with human diploid fibroblasts, which were refractory to transduction with both vectors. These results provide evidence for the differential expression of the Ad5 and Ad3 receptors on human cell lines derived from clinically relevant target tissues. Furthermore, we show that exchange of the fiber head domain is a viable approach to the production of adenovirus vectors with cell-type-selective transduction properties. It may be possible to extend this approach to the use of ligands for a range of different cellular receptors in order to target gene transfer to specific cell types at the level of transduction.
机译:腺病毒纤维蛋白负责将病毒体附着到未鉴定的细胞表面受体上。至少有两种不同的腺病毒纤维受体与B组(Ad3)和C组(Ad5)腺病毒相互作用。我们以前已经证明,通过使用表达的腺病毒纤维蛋白,可以通过将头部结构域与识别不同受体的另一种血清型交换来改变纤维蛋白的特异性(SC Stevenson等人,J。Virol。69:2850- 2857,1995)。将含有与Ad5纤维尾巴和轴融合的Ad3纤维头部结构域的嵌合纤维cDNA掺入腺病毒载体的基因组中,其中E1和E3缺失编码β-半乳糖苷酶,以生成Av9LacZ4(一种含有嵌合纤维蛋白的腺病毒颗粒)。嵌合纤维载体的蛋白质印迹分析证实了嵌合纤维蛋白的表达及其与腺病毒衣壳的关系。纤维蛋白竞争者的转导实验表明,与亲本Av1LacZ4载体相比,嵌合纤维载体的受体向性发生了变化。用嵌合和亲本载体转导一组人类细胞系为Ad5和Ad3受体的不同细胞分布提供了证据。包含Ad3纤维头的载体比通过Ad5纤维载体更有效地转导了三种细胞系(THP-1,MRC-5和FaDu)。相反,与含有嵌合纤维的载体相比,含有Ad5纤维的载体更容易转导人冠状动脉内皮细胞。与人二倍体成纤维细胞相比,HeLa和人脐静脉内皮细胞的转导水平相同,后者对两种载体均难以转导。这些结果为来自临床相关靶组织的人细胞系上Ad5和Ad3受体的差异表达提供了证据。此外,我们表明纤维头域的交换是一种具有细胞类型选择性转导特性的腺病毒载体生产的可行方法。可能有可能将此方法扩展为将配体用于一系列不同的细胞受体,以便在转导水平上将基因转移靶向特定细胞类型。

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