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Direct Repeat 6 from Human Herpesvirus-6B Encodes a Nuclear Protein that Forms a Complex with the Viral DNA Processivity Factor p41

机译:来自人类疱疹病毒6B的直接重复6编码一种核蛋白,该核蛋白与病毒DNA生产力因子p41形成复合体

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摘要

The SalI-L fragment from human herpesvirus 6A (HHV-6A) encodes a protein DR7 that has been reported to produce fibrosarcomas when injected into nude mice, to transform NIH3T3 cells, and to interact with and inhibit the function of p53. The homologous gene in HHV-6B is dr6. Since p53 is deregulated in both HHV-6A and -6B, we characterized the expression of dr6 mRNA and the localization of the translated protein during HHV-6B infection of HCT116 cells. Expression of mRNA from dr6 was inhibited by cycloheximide and partly by phosphonoacetic acid, a known characteristic of herpesvirus early/late genes. DR6 could be detected as a nuclear protein at 24 hpi and accumulated to high levels at 48 and 72 hpi. DR6 located in dots resembling viral replication compartments. Furthermore, a novel interaction between DR6 and the viral DNA processivity factor, p41, could be detected by confocal microscopy and by co-immunoprecipitation analysis. In contrast, DR6 and p53 were found at distinct subcellular locations. Together, our data imply a novel function of DR6 during HHV-6B replication.
机译:来自人类疱疹病毒6A(HHV-6A)的SalI-L片段编码一种蛋白质DR7,据报道,该蛋白质被注射到裸鼠体内时会产生纤维肉瘤,转化NIH3T3细胞,并与p53相互作用并抑制其功能。 HHV-6B中的同源基因是dr6。由于p53在HHV-6A和-6B中均失控,因此我们在HCT116细胞感染HHV-6B的过程中表征了dr6 mRNA的表达和翻译蛋白的定位。 dr6 mRNA的表达被环己酰亚胺抑制,部分被膦酰乙酸抑制,这是疱疹病毒早期/晚期基因的已知特征。 DR6可以在24 hpi时被检测为核蛋白,并在48和72 hpi时积累到高水平。 DR6位于类似于病毒复制区室的点中。此外,可以通过共聚焦显微镜和免疫共沉淀分析检测DR6和病毒DNA合成因子p41之间的新型相互作用。相反,DR6和p53被发现在不同的亚细胞位置。总之,我们的数据暗示在HHV-6B复制过程中DR6具有新功能。

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