| 人巨细胞病毒gp52蛋白基因片段的克隆及表达 |
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| 引用本文: | 李越希,汪兴太,陶开华,李长贵,周宗安. 人巨细胞病毒gp52蛋白基因片段的克隆及表达[J]. 中国生物制品学杂志, 2000, 13(1): 9-12 |
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| 作者姓名: | 李越希 汪兴太 陶开华 李长贵 周宗安 |
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| 作者单位: | [1]南京军区军事医学研究所,南京 [2]中国药品生物制品检定所,北京 |
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| 摘 要: | 目的为获得高表达人巨细胞病毒 gp52蛋白基因的工程菌。方法通过计算机分析,筛选出巨细 胞病毒蛋白gp52中优势抗原决定簇,用PCR技术扩增克隆了含强抗原决定簇的基因片段。将克隆的基因片段插 入表达载体pET28(a)内,转化大肠杆菌BL21,经Sepharery1 S-200分子筛及Ni-NTA Sepharose螯合层析进行纯化。结 果获得的工程菌所表达的 gp52蛋白片段相对分子质量约为 21 000,约占菌体可溶性蛋白的 28%。获得的表达蛋 白纯度达95%,电泳显示单一条蛋白带,ELISA分析证实有较强的抗原性和较好的特异性。结论本研究对人巨细 胞病毒感染,尤其是对孕妇及献血员等感染的检测有重要意义。
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| 关 键 词: | 人巨细胞病毒 gp52蛋白 基因克隆 基因表达 |
Cloning and Expression of Human Cytomegavirus gp52 Gene in E. coli |
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| Li Yuexi,Wang Xingtai,Tao Kaihua. Cloning and Expression of Human Cytomegavirus gp52 Gene in E. coli[J]. Chinese Journal of Bilogicals, 2000, 13(1): 9-12 |
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| Authors: | Li Yuexi Wang Xingtai Tao Kaihua |
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| Affiliation: | Li Yuexi,Wang Xingtai,Tao Kaihua(East-China Research Institute for Medical Biotechniques, Nanjing 210002) |
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| Abstract: | Objective To obtain engineering E. coli for the high expression of human cytomegavirus gp52 gene. Methods The human cytomegalovirus (HCMV) gp52 gene fragment containing 2 dominant antigen dormains confirmed by computer analysis was cloned by PCR and inserted into plasmid vector pET28(a),then the recombinant plasmid was transformed to E. coli BL21 and purified by Sephacry1 S-200 and Ni-NTA Sepharose chromatographies. Results About 28% of ed soluble somatic proteins were expressed, the molecular weight of the expressed gp52 protein was abaut 21 000. After being purified, the purity of it reached 95%. SDS-PAGE profile showed a single protein band,and ELISA showed good antigenicity and specificity of the expressed protein. Conclusion The study is of great signficance in examination of HCMV, especially in pregnant women and blood donors. |
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| Keywords: | Human cytomegalovims gp52 protein Gene cloning Gene expression |
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