猪瘟病毒兔化弱毒株cDNA片段的克隆及序列分析被引量：2

MOLECULAR CLONE AND SEQUENCE ANALYSIS OF cDNA FRAGMENTS OF HOG CHOLERA VIRUS STRAIN C 

下载PDF

导出

摘要 The 5′ nonencoding region, p23 and p14 encoding region and E1 gene of hog cholera virus (HCV) strain C were amplified from total RNA extracted from HCV strain C infected rabbit spleen by reverse transcription and nested or half\_nested PCR. The PCR products were cloned into pGEM\|T vector. Nucleotide sequencing was performed using an ABI PRISM sequencing device; based on the incorporation of fluoresect labelled dideoxynuclotide teminators. The obtained sequences on 5′ noncoding region and part of p23 and p14 encoding region were compared with HCV strains Shimen and C sequenced in Moormann’s lab. The result showed that the homology between HCV strains C sequenced in this report and in Moormann’s lab was 99.19%, and the homology between HCV strains Shimen, the standard virulent HCV strain in China, and C sequenced in this report was 94.69%. It was also discovered that the base C at 244 of the genome of HCV strains Shimen and C sequenced in this report was absent at the genome of C strain sequenced in Moormann’s lab et al. The 5′ nonencoding region, p23 and p14 encoding region and E1 gene of hog cholera virus (HCV) strain C were amplified from total RNA extracted from HCV strain C infected rabbit spleen by reverse transcription and nested or half\_nested PCR. The PCR products were cloned into pGEM\|T vector. Nucleotide sequencing was performed using an ABI PRISM sequencing device; based on the incorporation of fluoresect labelled dideoxynuclotide teminators. The obtained sequences on 5′ noncoding region and part of p23 and p14 encoding region were compared with HCV strains Shimen and C sequenced in Moormann's lab. The result showed that the homology between HCV strains C sequenced in this report and in Moormann's lab was 99.19%, and the homology between HCV strains Shimen, the standard virulent HCV strain in China, and C sequenced in this report was 94.69%. It was also discovered that the base C at 244 of the genome of HCV strains Shimen and C sequenced in this report was absent at the genome of C strain sequenced in Moormann's lab et al.

作者李红卫刘湘涛李小兵韩雪清涂长春殷震

机构地区长春农牧大学兰州兽医研究所

出处《微生物学报》 CAS CSCD 北大核心 1999年第6期554-558,共5页 Acta Microbiologica Sinica

基金国家攀登计划B 类项目资助课题

关键词 cDNA 克隆序列分析 HCLV 猪瘟疫苗 Hog cholera virus strain C, cDNA fragments, Cloning, Sequencing

分类号 S858.285.3 [农业科学—临床兽医学] Q78 [生物学—分子生物学]

引文网络
相关文献

同被引文献98

1黄茜华,张楚瑜,王家富,付烈振,王宁,朱燕,怀济森,张玮,于建石,许晖.猪瘟病毒石门株全基因组cDNA文库构建、序列测定及分析[J].科学通报,1999,44(17):1823-1826. 被引量：7
2肖昌,涂长春.猪瘟病毒E0、E2蛋白抗原表位的研究进展[J].畜牧兽医科技信息,2002,4(9):19-21. 被引量：1
3Martin B O, Thomas B R, Preben N,et al. Determination of the sequence of the complete open reading frame and the 5'NTR of the Paderborn isolate of classical swine fever virus[J].J Veter Microbiol, 2003, 92:311-325.
4Ruggli N, Tratschin J, Mittelholzer C,et al. Nucleotide sequence of classical swine fever virus strain alfort/187 and transcription of infectious RNA stably cloned full-length cDNA [J]. J Virol, 1996, 70:3478-3487.
5Van Gennip H G P, Van-Rijn P A, Moormann R J M. Chimeric classical swine fever viruses containing envelop protein ERNs or E2 of bovine viral diarrhea virus protect pigs against challenge with CSFV and induce a distinguishable antibody response[J]. Vaccine, 2001, 19:447-459.
6Ishikawa K, Nagai H, Katayama K. Comparison of the entire nucleotide and deduced amino acid sequences of the attenuated hog cholera vaccine strain GPE and the wild type parental strain ALD[J]. Arch Virol, 1995, 140:1385-1391.
7Simon P, Richard J. Pestivirus Internal Ribosome Entry Site(IRES) Structure and Function:Elements in the 5'Untranslated Region Important for IRES Function[J]. Virology, 2002,5:5024-5033.
8Vilcek S, Belak S. Organization and diversityi of the 3'-noncoding region of classical swine fever virus genome[J]. Virus Genes, 1997, 15:181-186.
9Klumpp S, Krieglstein J. Serine/Threonine protein phosphatases in apoptosis[J]. Curren Opinion in Pharmacology, 2002.2:458-462.
10Werten P J, Remigy H W. Progress in the analysis of membrane protein structure and function[J]. FEBS Letter, 2002,529:65-72.

引证文献2

1徐卓菲,钱平,李祥敏,郭东春,姚清侠,陈焕春.猪瘟弱毒C81株全基因组测序及分子结构预测[J].中国病毒学,2005,20(4):413-419.
2仇华吉,童光志,沈荣显.猪瘟兔化弱毒疫苗——半个世纪的回顾[J].中国农业科学,2005,38(8):1675-1685. 被引量：83

二级引证文献83

1王遵宝,贺笋,李俊辉,刘宏,豆智华,郑侃,李森江,寇春.昆虫细胞-杆状病毒系统分泌表达的猪瘟病毒E2蛋白及其免疫原性研究[J].中国预防兽医学报,2020,42(4):383-388. 被引量：9
2王继英,牛晓艳,郝小静,赵红梅,尼桂琰,张勤.21日龄猪瘟疫苗首次免疫前后仔猪抗体水平变化[J].华北农学报,2011,26(S1):283-286. 被引量：4
3朱妍,史子学,涂长春.免疫压力下猪瘟病毒遗传稳定性研究[J].中国动物传染病学报,2013,21(4).
4马秋明,张建安,王强,朱小甫,王文江,何维明.陕西省猪瘟病毒流行毒株E2基因变异分析初报[J].西北农林科技大学学报（自然科学版）,2007,35(5):19-23. 被引量：2
5梁润娴,黎敏,徐一洲,唐灼能,李耀灿,杜建兴.佛山市禅城区规模化猪场猪瘟抗体水平血清学调查[J].广东农业科学,2008,35(7):116-117. 被引量：2
6刘萍.猪瘟疫苗的研究进展[J].中国畜牧兽医,2008,35(7):95-98. 被引量：8
7周绪斌,丹尼.猪群免疫和猪场疫苗应用[J].养猪,2008(6):49-55. 被引量：1
8徐彦召,张彦明,何雷,唐青海,代晨,王静,杨小云.猪瘟病毒囊膜蛋白E2基因真核分泌型表达载体的构建及其表达[J].西北农林科技大学学报（自然科学版）,2009,37(5):7-11. 被引量：3
9王向鹏,孙元,杨增岐,仇华吉.检测猪瘟病毒野毒株胶体金免疫层析方法的建立[J].中国预防兽医学报,2010,32(6):441-445. 被引量：28
10刘大伟,张小飞,胡来根,李郁,尹秀凤,毛火云.猪瘟兔化弱毒疫苗株TaqMan荧光定量RT-PCR检测方法的建立及初步应用[J].中国预防兽医学报,2010,32(6):446-450. 被引量：6

1赵耘,秦玉明,张广川,赵启祖,宁宜宝,戴志红,谢磊.猪瘟病毒猪细小病毒猪繁殖与呼吸综合征病毒猪伪狂犬病病毒多重PCR方法的建立以及初步应用[J].中国兽医杂志,2007,43(2):3-6. 被引量：22
2张启敬,徐伟,李继庚,王桂敏,丁庆猷.猪肺炎霉形体兔化弱毒株的超微结构及致病性研究——1.兔化弱毒株的超微结构[J].电子显微学报,1989,8(4):13-18. 被引量：4
3高纪振,毕振兴.猪群免疫猪瘟疫苗后免疫效果不理想的原因及应对措施[J].兽药市场指南,2012(11):31-32. 被引量：2
4张启敬,徐伟,李继庚,丁庆猷,王桂敏.猪肺炎霉形体兔化弱毒株的超微结构及致病性研究——Ⅱ.兔化弱毒株的致病性[J].电子显微学报,1990,9(1):5-9. 被引量：7
5王欢.猪瘟兔化弱毒株克隆化的研究[J].中国兽医科技,1989(6):3-5.
6白同臣,曲海波.接种猪瘟疫苗时如何消除母源抗体干扰和仔猪的过敏反应[J].畜牧兽医科技信息,2006,22(11):25-25. 被引量：1
7“文易宁”猪瘟弱毒活疫苗[J].动物保健,2005(9):29-29.
8陆增荣,张民秀,肖雄,王艺,刘芳,刘欢,卢冰霞,刘磊,郭旋,黎木兰,黄福标,黄伟坚.广西猪瘟病毒E2基因克隆及序列分析[J].南方农业学报,2012,43(4):528-531. 被引量：5
9黄宗洲,李继庚,王桂敏,丁庆猷,张贤,鲍恩东.猪肺炎支原体兔化弱毒株与强毒济南株感染乳兔和断奶仔猪的肺脏病理组织学观察[J].中国兽药杂志,1989,23(3):10-14.
10丁庆猷,王桂敏,李继庚,朴永哲,张启敬,刘付启荣.猪喘气病弱毒苗的研究 2.冻干大兔苗的研制和应用[J].中国兽医杂志,1989,15(7):2-4. 被引量：9

微生物学报

1999年第6期

浏览历史

内容加载中请稍等...

猪瘟病毒兔化弱毒株cDNA片段的克隆及序列分析被引量：2

同被引文献98

引证文献2

二级引证文献83

相关作者

相关机构

相关主题

浏览历史

猪瘟病毒兔化弱毒株cDNA片段的克隆及序列分析 被引量：2

同被引文献98

引证文献2

二级引证文献83

相关作者

相关机构

相关主题

浏览历史

猪瘟病毒兔化弱毒株cDNA片段的克隆及序列分析被引量：2