人乳头瘤病毒16型L1/E7嵌合基因的克隆及其在毕赤酵母中的表达  

作　　者：宋衍燕[1] 李秀玲[1] 何薇薇[1] 张中洋[1] 许丽锋[1] 

机构地区：[1]北京生物制品研究所病毒室,北京100024

出　　处：《中国生物制品学杂志》2006年第4期355-361,共7页Chinese Journal of Biologicals

摘　　要：目的 克隆人乳头状瘤病毒16型（HPV16）L1／E7嵌合蛋白基因，并在毕赤酵母中表达。方法 PCR扩增HPV16L1／E7基因，并克隆至毕赤酵母表达载体pPIC-3．5K和pPIC-9K中，构建含HPV16L1／E7基因的pPIC3．5K—HPV16L1／E7和pPIC9K—HPV16L1／E7重组表达载体，经测序证实插入的外源基因读码框正确后，分别转入GS115和KM71菌株中，筛选阳性转化菌株，经PCR鉴定，甲醇诱导表达HPV16L1／E7嵌合蛋白，经SDS—PAGE和Western blot鉴定，电镜观察，并经离心法纯化VLPs。结果 HPV16LI／E7基因已成功插入pPIC-3．5K和pPIC-9K载体中，共获得6株KM71HPV16L1／E7-pPIC3．5K、5铢GS115HPV16L1／E7-pPIC3．5K、1株KM71HPV16L1／E7-pPIC9K和2株GS115HPV16L1／E7-pPIC9K阳性转化菌株，并可表达相对分子质量约为69000的蛋白，与预期值一致。表达量约为0．35～1．04mg／ml。Western blot显示该蛋白可与抗-HPV16L1蛋白和抗-HPV16E7蛋白的单克隆抗体特异性结合。在透射电镜下可观察到VLPs的形成，其形态与HPV16天然病毒颗粒相似。经纯化的目的蛋白纯度接近100％。结论 已成功构建了pPIC3．5K—HPV16L1／E7和pPIC9K—HPV16L1／E7重组表达载体，阳性转化菌株可表达结构与野生型HPV16一致的VLPs。Objective To clone the L1/E7 chimeric gene of human papillomavirus type 16 and express in Pichia pastoris. Methods Amplify HPV16 L1/E7 gene by PCR and clone into expression vectors pPIC-3.5K and pPIC-9K to construct recombinant plasmids pPIC3.5K-HPV16 L1/E7 and pPIC9K-HPV16 L1/E7 respectively. Identify the recombinant plasmids by sequencing and transform to GS115 and KM71 strains of Pichia pastoris separately. Screen positive recombinants and identify by PCR, then express HPV16 L1/E7 chimeric protein in vitro under induction of methanol. Identify the expressed produet by SDS-PAGE and Western blot. Observe the formation of vires-like partieles（VLPs） by electron miemseopy and purify by cesium chloride density gradient eentrifugation. Results HPV16 L1/E7 gene was suceessfuUy inserted into vectors pPIC-3.5K and pPIC-9K. Six recombinant KM71 strains with HPV16 L1/E7-pPIC3.5K,five recombinant GS115 strains with HPV16 L1/E7-pPIC3. 5K,one recombinant KMT1 strain with HPV16 L1/E7-pPIC9K and two recombinant GS115 strains with HPV16 L1/E7-pPIC9K were obtained. The expressed produet with a relative molecular weight of 69 000, whieh was eonsistent with that expected, eontained 0. 35-1.04 mg/ml protein. Western blot showed specific bindings of the expressed protein to the MeAbs against HPV16 L1 and HPV16 E7 proteins. The VLPs with similar appearanee to that of natural HPV16 particles were observed under electron microscope and reached a purity of nearly 100% after purification. Conclusion Recombinant plasmids pPIC3.5K-HPV16 L1/E7 and pPIC9K-HPV16 L1/E7 were successfully eonstrueted and used for the expression of VLPs with identieal strueture to that of wild HPV16.

关 键 词：人乳头瘤病毒 毕赤酵母 基因表达 

分 类 号：R392-33[医药卫生—免疫学] R373[医药卫生—基础医学]