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首页> 美国卫生研究院文献>Journal of Virology >Comparing transcriptional activation and autostimulation by ZEBRA and ZEBRA/c-Fos chimeras.
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Comparing transcriptional activation and autostimulation by ZEBRA and ZEBRA/c-Fos chimeras.

机译:比较ZEBRA和ZEBRA / c-Fos嵌合体的转录激活和自动刺激。

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摘要

The lytic cycle of Epstein-Barr virus (EBV) can be activated by transfection of the gene for ZEBRA, a viral basic-zipper (bZip) transcriptional activator. ZEBRA and cellular AP-1 bZip activators, such as c-Fos, have homologous DNA-binding domains, and their DNA-binding specificities overlap. Moreover, EBV latency can also be disrupted by phorbol esters, which act, in part, through AP-1 activators. It is not known whether ZEBRA and AP-1 factors play equivalent roles in the initial stages of reactivation. Here the contribution of ZEBRA's basic DNA recognition domain to disruption of latency was analyzed by comparing ZEBRA with chimeric mutants in which the DNA recognition domain of ZEBRA was replaced with the analogous domain of c-Fos. Chimeric ZEBRA/c-Fos proteins overexpressed in Escherichia coli bound DNA with the specificity of c-Fos; they bound a heptamer AP-1 site and an octamer TPA response element (TRE). ZEBRA bound the AP-1 site and an array of ZEBRA response elements (ZREs). In assays with reporter genes, both ZEBRA and ZEBRA/c-Fos chimeric mutants activated transcription from Zp, a promoter of the ZEBRA gene (BZLF1) that contains the TRE and multiple ZREs. However, despite their capacity to activate reporters bearing Zp, neither ZEBRA nor the c-Fos chimeras activated transcription from Zp in the context of the intact latent viral genome. In contrast, ZEBRA but not ZEBRA/c-Fos chimeras activated Rp, a second viral promoter that controls ZEBRA expression. Hence, transcriptional autostimulation by transfected ZEBRA occurred preferentially at Rp. Both ZEBRA and the ZEBRA/c-Fos chimeras activated transcription from reporters with multimerized AP-1 sites. However, in the context of the virus, only ZEBRA activated the promoters of two early lytic cycle genes, BMRF1 and BMLF1, that contain an AP-1 site. Thus, overexpression of an activator that recognized AP-1 and TRE sites was not sufficient to activate EBV early lytic cycle genes.
机译:可通过转染病毒基本拉链(bZip)转录激活因子ZEBRA的基因来激活爱泼斯坦-巴尔病毒(EBV)的裂解周期。 ZEBRA和细胞AP-1 bZip激活剂(例如c-Fos)具有同源的DNA结合结构域,并且它们的DNA结合特异性重叠。此外,佛波酯还可以破坏EBV潜伏期,其部分通过AP-1激活剂起作用。尚不知道ZEBRA和AP-1因子在再激活的初始阶段是否起相同的作用。在这里,通过比较ZEBRA与嵌合突变体(其中ZEBRA的DNA识别结构域被c-Fos的类似结构域替代)的嵌合突变体,分析了ZEBRA的基本DNA识别结构域对延迟潜伏性的影响。在大肠杆菌结合的DNA中过表达的嵌合ZEBRA / c-Fos蛋白具有c-Fos的特异性;它们结合了七聚体AP-1位点和八聚体TPA反应元件(TRE)。 ZEBRA绑定了AP-1站点和一系列ZEBRA响应元素(ZRE)。在带有报告基因的分析中,ZEBRA和ZEBRA / c-Fos嵌合突变体均激活了Zp的转录,Zp是包含TRE和多个ZRE的ZEBRA基因(BZLF1)的启动子。然而,尽管它们具有激活携带Zp的报告基因的能力,但在完整的潜伏病毒基因组中,ZEBRA和c-Fos嵌合体均未激活Zp的转录。相反,ZEBRA而非ZEBRA / c-Fos嵌合体激活Rp,后者是控制ZEBRA表达的第二种病毒启动子。因此,转染的ZEBRA转录自动刺激优先发生在Rp。 ZEBRA和ZEBRA / c-Fos嵌合体均激活了具有多聚AP-1位点的报告基因的转录。但是,在这种病毒的情况下,只有ZEBRA激活了两个早期裂解周期基因BMRF1和BMLF1的启动子,它们含有一个AP-1位点。因此,识别AP-1和TRE位点的激活剂的过表达不足以激活EBV早期裂解周期基因。

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