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首页> 外文期刊>Virology >Cellular factors are required to activate bovine papillomavirus-1 early gene transcription and to establish viral plasmid persistence but are not required for cellular transformation.
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Cellular factors are required to activate bovine papillomavirus-1 early gene transcription and to establish viral plasmid persistence but are not required for cellular transformation.

机译:细胞因子是激活牛乳头瘤病毒-1早期基因转录和建立病毒质粒持久性所必需的,但细胞转化并不是必需的。

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摘要

Transcription from the major upstream early gene promoter, P89, of bovine papillomavirus (BPV)-1 is detectable in transfected cells lacking viral gene products yet also responds to viral E2 proteins. In contrast to human papillomaviruses (HPVs), the BPV upstream regulatory region (URR) functions as a transcriptional enhancer in epithelial cells and fibroblasts of bovine, murine or human origin. Mutations of Sp1 and/or two novel transcriptional enhancer factor (TEF)-1 sites within the 5' URR of the intact BPV-1 genome dramatically reduced P89-initiated mRNA levels, leading to decreased BPV-1 plasmid amplification and inefficient formation of transformed cell foci. However, cell lines transformed with wt or mutant BPV-1 genomes contained similar levels of unintegrated BPV-1 DNA, P89 mRNA and E2-dependent transactivation. We conclude that cellular factors necessary for activating viral early gene transcription, establishment of viral plasmid replication and cell immortalization are not required during the maintenance phase of BPV-1 infection.
机译:牛乳头瘤病毒(BPV)-1的主要上游早期基因启动子P89的转录在缺乏病毒基因产物但也对病毒E2蛋白有反应的转染细胞中可检测到。与人乳头瘤病毒(HPV)相比,BPV上游调节区(URR)在牛,鼠或人来源的上皮细胞和成纤维细胞中作为转录增强子。 Sp1和/或完整BPV-1基因组5'URR内两个新的转录增强因子(TEF)-1位点的突变显着降低了P89启动的mRNA水平,从而导致BPV-1质粒扩增降低和转化子形成效率低下细胞灶。然而,用野生型或突变型BPV-1基因组转化的细胞系包含相似水平的未整合BPV-1 DNA,P89 mRNA和E2依赖性反式激活。我们得出结论,在BPV-1感染的维持阶段,不需要激活病毒早期基因转录,建立病毒质粒复制和永生化所需的细胞因子。

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