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| 构建及鉴定携带角蛋白启动子和人乳头瘤病毒16E6/E7基因的重组腺病毒 | |
| 引用本文: | 潘巍巍,赖国旗,易发平,成海恩,张溢,左国伟,李成华,马永平,宋方洲.构建及鉴定携带角蛋白启动子和人乳头瘤病毒16E6/E7基因的重组腺病毒[J].西安交通大学学报(医学版),2006,27(5):421-425. |
| 作者姓名: | 潘巍巍 赖国旗 易发平 成海恩 张溢 左国伟 李成华 马永平 宋方洲 |
| 作者单位: | 1. 重庆医科大学,生物化学与分子生物学教研室,重庆,400016;重庆医科大学,重庆市生物化学与分子药理学重点实验室,重庆,400016 2. 重庆医科大学,实验动物中心,重庆,400016 3. 重庆医科大学,生物化学与分子生物学教研室,重庆,400016;重庆医科大学,教育部临床检验诊断学重点实验室,重庆,400016;重庆医科大学,重庆市生物化学与分子药理学重点实验室,重庆,400016 |
| 基金项目: | 国家自然科学基金资助项目(No.30371479),教育部“春晖计划”资助项目(No.Z2004-1-55103) |
| 摘 要: | 目的利用AdEasy系统构建携带人角蛋白启动子的人乳头瘤病毒-16(HPV-16)E6/E7基因重组腺病毒,并通过RT-PCR方法检测E6/E7基因的表达。方法应用PCR方法从含有HPV-16全基因序列的质粒上扩增E6/E7基因,构建pCDNA3.1(-)-K14-E6/E7-polA载体,扩增、酶切获得K14-E6/E7-polA片段插入腺病毒穿梭载体质粒pAdTrack上,构建重组穿梭载体pAdTrack-K14-E6/E7-polA,线性化后与骨架载体AdEasy-1在细菌BJ5183内同源重组得到腺病毒质粒pAd-K14-E6/E7-polA,经人胚肾293细胞包装后得到重组腺病毒pAd-K14-E6/E7-polA。氢化铯(CsCl)梯度离心纯化病毒,提取病毒再感染后的293细胞总RNA,通过RT-PCR方法检测E6/E7基因的表达。结果通过同源重组的方法构建了腺病毒pAd-K14-E6/E7-polA载体,经酶切和测序鉴定该质粒构建成功。293细胞包装3d后观察到绿色荧光蛋白(GFP)表达,CsCl梯度离心纯化最终获得7.2×1010pfu/mL滴度的重组病毒;用该滴度病毒重新感染293细胞3d后,提取细胞总RNA,RT-PCR检测E6/E7有表达。结论利用新型腺病毒载体AdEasy系统可在短期内制备同时表达GFP和E6/E7的重组腺病毒pAd-K14-E6/E7-polA。这将为进一步研究HPV-16E6/E7基因功能及利用基因治疗女性宫颈癌奠定了基础。 |
| 关 键 词: | 人乳头瘤病毒 腺病毒 角蛋白启动子 |
| 文章编号: | 1671-8259(2006)05-0421-05 |
| 收稿时间: | 2006-02-20 |
| 修稿时间: | 2006年2月20日 |
Construction and identification of recombinant adenoviruses carrying cytokeratin promoters 14 and HPV-16 E6/E7 |
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| Pan Weiwei,Lai Guoqi,Yi Faping,Cheng Haien,Zhang Yi,Zuo Guowei,Li Chenghua,Ma Yongping,Song Fangzhou.Construction and identification of recombinant adenoviruses carrying cytokeratin promoters 14 and HPV-16 E6/E7[J].Journal of Xi‘an Jiaotong University:Medical Sciences,2006,27(5):421-425. | |
| Authors: | Pan Weiwei Lai Guoqi Yi Faping Cheng Haien Zhang Yi Zuo Guowei Li Chenghua Ma Yongping Song Fangzhou |
| Abstract: | Objective To construct the recombinant adenoviruses carrying cytokeratin promoters and HPV-16 E6/E7 gene by AdEasy system and to identify the expression of E6/E7 mRNA by RT-PCR. Methods HPV-16 E6/E7 was amplified by polymerase chain reaction(PCR) from vectors that contained all sequence of HPV16, and the pcDNA3.1(-)-K14-E6/E7-polA vector was constructed. The oligo K14-E6/E7-polA was obtained by amplifying and digesting the pcDNA3.1(-)-K14-E6/E7-polA vector. The shuttle plasmid pAdTrack-K14-E6/E7-polA was constructed by inserting the K14-E6/E7-polA into the pAdTrack vector. Then the linearized shuttle plasmids were co-transformed into bacteria containing AdEasy-1 backbone vector for homologous recombination and obtaining the recombinant adenoviral plasmid pAd-K14-E6/E7-polA. The recombined adenovirus DNA was transfected into 293 cells for packing of Ad-K14-E6/E7-polA virus, and the virus was purified by CsCl density gradient centrifugation. The expression of E6/E7 was determined by RT-PCR after infection of Ad-K14-E6/E7-polA in 293 cells. Results The recombinant plasmid pAd-K14-E6/E7-polA was successfully constructed and confirmed by restriction endonuclease digestion and sequencing. GFP expression could be observed on the 3rd day after the package of linearized pAd-K14-E6/E7-polA in the 293 cells. The titer of pAd-K14-E6/E7-polA was 7.2×10~ 10 pfu/mL by CsCl gradient purification. Total RNA in 293 cells was collected 3 days after the 293 cells were re-infected with the pAd-K14-E6/E7-polA virus with the titer being 7.2×10~ 10 pfu/mL. The RT-PCR results indicated that E6/E7 could be detected in the transfected 293 cells. Conclusion The recombinant adenoviruses Ad-K14-E6/E7-polA expressing GFP and E6/E7 simultaneously could be generated in a short time by using the AdEasy system. The construction of recombinant adenoviruses Ad-K14-E6/E7-polA provides a base for further study of the gene function of HPV-16 E6/E7 and gene therapy of female cervical carcinoma. |
| Keywords: | human papillomavirus adenovirus cytokeratin promoter |
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