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人乳头瘤病毒18型E7蛋白与c-Myc结合并介导其转录活性。

HPV-18 E7 conjugates to c-Myc and mediates its transcriptional activity.

作者信息

Wang Yi-Wei, Chang Hung-Shu, Lin Ching-Hui, Yu Winston C Y

机构信息

National Health Research Institutes, 35, Keyan Road, Zhunan Town, Miaoli County 350, Taiwan, ROC.

出版信息

Int J Biochem Cell Biol. 2007;39(2):402-12. doi: 10.1016/j.biocel.2006.09.006. Epub 2006 Oct 4.

DOI:10.1016/j.biocel.2006.09.006
PMID:17070091
Abstract

Several reports in the literature have indicated that the E6 not only elevates the level of c-Myc level but that the protein also associates with the Myc complex and activates Myc-responsive genes. There would seem to be a mechanism by which this oncogene can modulate cell proliferation and differentiation. Furthermore, an increase in c-Myc levels has also observed during ectopic expression of HPV E7 alone. Using the yeast two-hybrid system, we further found that the c-Myc interacts and forms a specific complex with HPV-16E7. In this study, we have demonstrated that E7 does indeed interact with c-Myc and a sequential deletion analysis of E7 maps the c-Myc interaction site to the carboxyl-terminal region. We determined two HPV-18 E7 binding sites on c-Myc involving the amino acids regions 1-100 and 367-439. The interaction of the high-risk type HPV E7 with c-Myc can augment c-Myc transactivation activity but this does not occur with low-risk type HPV E7. Deletion within the Cys-X-X-Cys repeat motif at the C-terminus of HPV-18 E7 leads to a lost of association with c-Myc and also abolishes the enhancement of c-Myc's transactivation activity. Furthermore, the interaction of HPV-18 E7 with c-Myc functionally promotes c-Myc's DNA-binding ability. Using the hTERT promoter as a model, enhanced c-Myc binding ability to the hTERT promoter as measured by immunoprecipitation assay was observed and occurred in an E7 dose-dependent manner. Taken together, these results provide significant new insights into the association of c-Myc with E7 and the possible involvement of high-risk E7 in oncogenesis.

摘要

文献中的几篇报道指出,E6不仅能提高c-Myc的水平,而且该蛋白还能与Myc复合物结合并激活Myc反应基因。似乎存在一种机制,通过该机制这种癌基因可以调节细胞增殖和分化。此外,在单独异位表达HPV E7的过程中也观察到了c-Myc水平的升高。利用酵母双杂交系统,我们进一步发现c-Myc与HPV-16E7相互作用并形成特定复合物。在本研究中,我们已经证明E7确实与c-Myc相互作用,并且对E7进行的序列缺失分析将c-Myc相互作用位点定位到羧基末端区域。我们确定了c-Myc上两个HPV-18 E7结合位点,涉及氨基酸区域1-100和367-439。高危型HPV E7与c-Myc的相互作用可以增强c-Myc的反式激活活性,但低危型HPV E7则不会。HPV-18 E7 C末端的Cys-X-X-Cys重复基序内的缺失导致与c-Myc的结合丧失,也消除了对c-Myc反式激活活性的增强作用。此外,HPV-18 E7与c-Myc的相互作用在功能上促进了c-Myc的DNA结合能力。以hTERT启动子为模型,通过免疫沉淀试验观察到c-Myc与hTERT启动子的结合能力增强,且呈E7剂量依赖性。综上所述,这些结果为c-Myc与E7的关联以及高危E7在肿瘤发生中的可能作用提供了重要的新见解。

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