Specific up-regulation of DNA polymerase by human papillomavirus 16.

Song-Nian Liu, Wu-Yun Bai, Russell M Frye, Lin Hou, Bo Zhang
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Abstract

Objective: To analyze how the infection of human papillomavirus 16 (HPV16) affects expression of DNA polymerase beta (DNA polB) with the aim of probing the mechanism of over-expression of DNA polB in human cancers.

Methods: Four fragments of human DNA polB promoter were amplified and constructed into luciferase reporter vector pGL-Basic, generating pGL-BP, pGL-BMH, pGL-BMS, and pGL-BAT constructs respectively, and co-transfected with HPV16 or HPV6 into Hep2 cells. Luciferase activity was assayed 48 hours after transfection. Semi-quantitative RT-PCR was used to measure mRNA expression of endogenous DNA polB. Immunohistochemistry and in situ hybridization were used to analyze DNA polB expression and HPV16 or HPV6 infection in 38 cases of cervical lesions respectively.

Results: With co-transfection of HPV16 and DNA polB promoter-driving reporters into Hep2 cells, pGL-BP reporter in full-length DNA polB promoter presented markedly elevated luciferase activities (P < 0.05). However, the other three mutant reporters: pGL-BMH, pGL-BMS, and pGL-BAT, generated no reporting activities in the presence of HPV16 (P > 0.05). On the contrary, all of polB promoter reporters were little stimulated in co-transfection of HPV6 (P > 0.05). The transfection of HPV16 could enhance the endogenous polB mRNA expression compared with that of HPV6 (3.42 vs. 0.80, P < 0.05). The DNA polB expression was found in 8 of 10 HPV16-positive cervical intraepithelial neoplasia grade III (CIN III) cases, while was only found in 3 of 11 HPV6-positive condyloma accuminatum cases, but was negative in all chronic cervicitis cases. The correlation of DNA polB expression with HPV16 infection in cervical lesions was significant (P < 0.05).

Conclusions: HPV16 is able to specifically stimulate the expression of DNA polB in human epithelial cells through interaction with the core upstream regulatory sequences of DNA polB promoter. Over-expression of DNA polB might be an explanation for the molecular mechanism underlying HPV-related human cancers.

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人乳头瘤病毒DNA聚合酶特异性上调
目的:分析人乳头瘤病毒16 (HPV16)感染对DNA聚合酶β (DNA polB)表达的影响,探讨DNA polB在人肿瘤组织中的过表达机制。方法:扩增人DNA polB启动子片段,构建荧光素酶报告载体pGL-Basic,分别生成pGL-BP、pGL-BMH、pGL-BMS和pGL-BAT构建体,与HPV16或HPV6共转染Hep2细胞。转染后48小时检测荧光素酶活性。采用半定量RT-PCR检测内源DNA polB mRNA表达量。应用免疫组织化学和原位杂交技术分别对38例宫颈病变的DNA polB表达和HPV16、HPV6感染情况进行了分析。结果:将HPV16与DNA polB启动子驱动报告子共转染Hep2细胞后,全长DNA polB启动子中pGL-BP报告子荧光素酶活性显著升高(P < 0.05)。而其他三个突变体报告基因:pGL-BMH、pGL-BMS和pGL-BAT在HPV16存在下没有报告活性(P > 0.05)。相反,共转染HPV6时,所有的polB启动子报告子几乎没有受到刺激(P > 0.05)。与HPV6相比,转染HPV16可提高内源性polB mRNA的表达量(3.42比0.80,P < 0.05)。DNA polB在10例hpv16阳性宫颈上皮内瘤变III级(CIN III)病例中有8例表达,而在11例hpv6阳性的尖锐湿疣病例中只有3例表达,而在所有慢性宫颈炎病例中均为阴性。DNA polB表达与宫颈HPV16感染有显著相关性(P < 0.05)。结论:HPV16可通过与DNA polB启动子上游核心调控序列相互作用,特异性刺激人上皮细胞中DNA polB的表达。DNA polB的过度表达可能是hpv相关人类癌症的分子机制的一个解释。
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