| 猪瘟病毒糖蛋白E0基因的克隆及及表达研究 |
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| 引用本文: | 周鹏程,陈建国.猪瘟病毒糖蛋白E0基因的克隆及及表达研究[J].微生物学通报,2000,27(3):165-170. |
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| 作者姓名: | 周鹏程 陈建国 |
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| 作者单位: | 周鹏程(北京大学生命科学学院细胞及遗传学系北京 100871);陈建国(北京大学生命科学学院细胞及遗传学系北京 100871);翟中和(北京大学生命科学学院细胞及遗传学系北京 100871);丁明孝(北京大学生命科学学院细胞及遗传学系北京 100871) |
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| 基金项目: | 国家攀登计划B类项目资助 |
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| 摘 要: | 用RT-PCR方法扩增分别获得了中国猪瘟病毒强毒石门株和兔化弱毒株糖蛋白E0基因cDNA,并克隆到pGEM T载体中测定其核苷酸序列和推导出其对应氨基酸序列,结果表明这两个毒 间的E0基因核苷酸序列同源性为95.3%,氨基酸序列同源性为94%,有14个殖基的差异;与几个代表毒株ALD株、GPE株、Brescia株、Alfort株和国外测得的兔化弱毒C株相应序列进行比较,所测石门病毒核苷酸序列与上述
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| 关 键 词: | 猪瘟病毒 糖蛋白E0 基因克隆 基因表达 致病机制 |
| 文章编号: | 0253-2654(2000)03-0165-06 |
| 修稿时间: | 1999年2月25日 |
Molecular Cloning and Expression of E0 Gene of the Chinese Classical Swine Fever Virus and Its Locali
zation in Host Cells |
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| ZHOU Peng-Cheng,CHEN Jian-Guo,ZHAI Zhong-He,DING Ming-Xiao.Molecular Cloning and Expression of E0 Gene of the Chinese Classical Swine Fever Virus and Its Locali
zation in Host Cells[J].Microbiology,2000,27(3):165-170. |
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| Authors: | ZHOU Peng-Cheng CHEN Jian-Guo ZHAI Zhong-He DING Ming-Xiao |
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| Abstract: | EO gene fragments of chinese classical swine fever virus (CSFV) Shimen strain (a standard virulent strain) and hog cholera lapinized vaccine(HCLV) strain, was amplified by RT-PCR from total RNA of cell cultures infected by CSFV, and cloned into pGEM T vector, respectively. The nucleotide sequences of two fragments were sequenced by Sanger's method and the amino acid sequences were deduced. Sequence analysis shows the homologies of the nucleotide sequence and the deduced amino acid of EO gene between Shimen strain and HCLV were 95.3% and 94%, respectively. Compared with the corresponding regions of ALD. GEP. Brescia. Alfort strain and C strain sequenced by K J. M. Moormann, the nucleotide sequence homology of Shimen strain EO gene is 98.0%, 97.l%, 92.7%, 86.8% and 95.4%, and the amino acid sequence 97.4%, 96.l%, 95.3%, 92.7% and 94.4%, respectively; similarly, the nucleotide sequence homology of HCLV EO gene compared with above mentioned strains is 95.2%, 94.6%, 91.3%, 85.l% and 99%, and the amino acid sequence 93.l%, 92.3%, 91.4%, 90.5% and 98.7%, respectively. It has also been found that above mentioned strain's EO RNases, belonging to the RNases family consisting of several fungal and plant RNases, contain two conserved streches of 8 amino acids each, SLHGIWPX (X for G or E) and EWNKHGWC, which are spaced by 38 nonhomologous amino acids and which form the RNase active site, Histidine residues in both streches is essential for RNase catalysis. We subcloned 696bp of EO gene cDNA into baculovirus transfer vector and constructed successfully recombinant baculovirus expressing GST-EO by homologous recombination in Sf9 cells. Furthermore, we also constructed recombinant eukaryotic expression vector pEGry-EO containing EO gene in frame and transfected PK-15 cell by lipofectamine, the fluorescene microscopy detection indicated expressed EO protein mainly locate in plasma of PK-15 cells, which is the same as the results when PK-15 cells are infected by CSFV. |
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| Keywords: | classical swine fever virus Glycoprotein EO Clone and expression |
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