临床和实验医学杂志
臨床和實驗醫學雜誌
림상화실험의학잡지
JOURNAL OF CLINICAL AND EXPERIMENTAL MEDICINE
2014年
16期
1329-1331
,共3页
丙型肝炎病毒%病毒核心蛋白质类%酵母双杂交技术
丙型肝炎病毒%病毒覈心蛋白質類%酵母雙雜交技術
병형간염병독%병독핵심단백질류%효모쌍잡교기술
Hepatitis C virus%Viral core proteins%Two-hybrid system techniques
目的构建含丙型肝炎病毒( hepatitis C virus,HCV)核心( core,C)蛋白基因的酵母双杂交诱饵载体,为C蛋白与宿主蛋白相互作用机制研究奠定基础。方法聚合酶链反应( PCR)法扩增HCV 1b基因型C蛋白基因,经EcoR I和Pst I双酶切后插入到诱饵载体pGBKT7中,构建含HCV C蛋白基因的酵母双杂交诱饵载体pGBKT7-Core,经酶切分析及核酸测序分析加以鉴定。醋酸锂法将pGBKT7-Core转化入酵母菌株Y2HGold,蛋白印迹法检测C蛋白的表达,通过表型筛选检测诱饵蛋白对酵母细胞的毒性作用及对报告基因的激活作用。结果重组质粒pGBKT7-Core中的C蛋白基因为576 bp,经核酸测序分析与NCBI中注册的HCV 1b基因型C蛋白基因序列一致;转化酵母菌后检测到C蛋白的表达;HCV C蛋白对酵母菌Y2HGold无毒性,且对报告基因无激活作用。结论含HCV C蛋白基因的酵母双杂交诱饵载体构建成功,表达稳定。
目的構建含丙型肝炎病毒( hepatitis C virus,HCV)覈心( core,C)蛋白基因的酵母雙雜交誘餌載體,為C蛋白與宿主蛋白相互作用機製研究奠定基礎。方法聚閤酶鏈反應( PCR)法擴增HCV 1b基因型C蛋白基因,經EcoR I和Pst I雙酶切後插入到誘餌載體pGBKT7中,構建含HCV C蛋白基因的酵母雙雜交誘餌載體pGBKT7-Core,經酶切分析及覈痠測序分析加以鑒定。醋痠鋰法將pGBKT7-Core轉化入酵母菌株Y2HGold,蛋白印跡法檢測C蛋白的錶達,通過錶型篩選檢測誘餌蛋白對酵母細胞的毒性作用及對報告基因的激活作用。結果重組質粒pGBKT7-Core中的C蛋白基因為576 bp,經覈痠測序分析與NCBI中註冊的HCV 1b基因型C蛋白基因序列一緻;轉化酵母菌後檢測到C蛋白的錶達;HCV C蛋白對酵母菌Y2HGold無毒性,且對報告基因無激活作用。結論含HCV C蛋白基因的酵母雙雜交誘餌載體構建成功,錶達穩定。
목적구건함병형간염병독( hepatitis C virus,HCV)핵심( core,C)단백기인적효모쌍잡교유이재체,위C단백여숙주단백상호작용궤제연구전정기출。방법취합매련반응( PCR)법확증HCV 1b기인형C단백기인,경EcoR I화Pst I쌍매절후삽입도유이재체pGBKT7중,구건함HCV C단백기인적효모쌍잡교유이재체pGBKT7-Core,경매절분석급핵산측서분석가이감정。작산리법장pGBKT7-Core전화입효모균주Y2HGold,단백인적법검측C단백적표체,통과표형사선검측유이단백대효모세포적독성작용급대보고기인적격활작용。결과중조질립pGBKT7-Core중적C단백기인위576 bp,경핵산측서분석여NCBI중주책적HCV 1b기인형C단백기인서렬일치;전화효모균후검측도C단백적표체;HCV C단백대효모균Y2HGold무독성,차대보고기인무격활작용。결론함HCV C단백기인적효모쌍잡교유이재체구건성공,표체은정。
Objective To construct a bait vector containing the gene encoding hepatitis C virus(HCV)core(C)protein in yeast two - hybrid system,laying the foundation for further study of the mechanism of interaction between C protein and host proteins. Methods The cDNA fragment encoding C protein of HCV 1b genotype was amplified by PCR,then digested by EcoR I/ Pst I and cloned into the bait vector pGBKT7 to construct recombinant bait plasmid pGBKT7 - Core. Then right fragment of recombinant plasmid pGBKT7 - Core was tested by both restriction endonuclease analysis. The sequence analysis was transformed into the yeast strain Y2HGold by LiAc method. The expression of C protein was detected by Western blot. The toxicity and autoactivation of bait protein was tested by phenotype assay. Results The gene encoding HCV C protein in the recombinant plasmid pGBKT7 - Core was 576bp and consistent with that of HCV 1b genotype registered in NCBI. The expression of C protein was detected by Western blot after being transformed into the yeast cell. HCV C protein was not toxic to the yeast strain Y2HGold,and could not be activate the reporter genes. Conclusion The bait vector containing the gene encoding HCV C protein was constructed successfully and expressed stably.