猪输血传播病毒2型ORF1基因的原核表达及条件优化

doi:10.7668/hbnxb.2013.05.007

华北农学报 ›› 2013, Vol. 28 ›› Issue (5): 38-43. doi: 10.7668/hbnxb.2013.05.007

所属专题： 畜牧；生物技术；

猪输血传播病毒2型ORF1基因的原核表达及条件优化

王小敏¹, 何孔旺¹, 张文文^1,2, 王东田³, 周忠涛^1,2, 张雪寒¹, 周俊明¹, 汪伟¹, 倪艳秀¹, 温立斌¹

1 江苏省农业科学院兽医研究所农业部兽用生物制品工程技术重点实验室国家兽用生物制品工程技术研究中心江苏南京 210014;
2 南京农业大学动物医学院江苏南京 210095;
3 山东省蓬莱市村里集镇畜牧兽医工作站山东蓬莱 265604

收稿日期:2013-05-16 出版日期:2013-10-28
作者简介:王小敏(1983－),女,江苏盐城人,助理研究员,硕士,主要从事动物病毒学研究。
基金资助:
国家基金面上项目(31272574);江苏省自主创新专项(CX(11)2060)

Prokaryotic Expression and Optimization of Expression Conditions of Open Reading Frame 1 Gene of Porcine Torque Teno Virus Type 2

WANG Xiao-min¹, HE Kong-wang¹, ZHANG Wen-wen^1,2, WANG Dong-tian³, ZHOU Zhong-tao^1,2, ZHANG Xue-han¹, ZHOU Jun-ming¹, WANG Wei¹, NI Yan-xiu¹, WEN Li-bin¹

1 Institute of Veterinary Medicine, Jiangsu Academy of Agricultural Sciences, Key Laboratory of Veterinary Biological Engineering and Technology, Ministry of Agriculture, National Center for Engineering Research of Veterinary Bio-products, Nanjing 210014, China;
2 The College of Veterinary Medicine, Nanjing Agricultural University, Nanjing 210095, China;
3 Workstation of Animal Husbandry and Veterinary Medicine of Cunliji Town, Penglai 265604, China

Received:2013-05-16 Published:2013-10-28

摘要/Abstract

摘要： 为了克隆猪输血传播病毒2型(TTV2)ORF1基因,构建原核表达载体,在大肠杆菌BL21(DE3)中诱导表达猪TTV2 ORF1蛋白,并对其表达条件进行优化。利用普通PCR从猪TTV2阳性样本中扩增出TTV2 ORF1基因,利用分子克隆的方法将猪TTV2 ORF1基因克隆到原核表达载体pcoldI上,构建表达载体pcold-ORF1,在大肠杆菌中诱导表达带有6个组氨酸标签的ORF1融合蛋白。并对影响重组蛋白表达的3个因素,即诱导时间、诱导温度和IPTG浓度进行优化,确定了pcold-ORF1重组蛋白表达的最佳表达条件。SDS-PAGE分析结果表明,重组蛋白在BL21中高效表达,以包涵体形式表达为主,分子质量约为39 kDa。蛋白表达量随诱导时间增加而有所增加,在15℃时表达量最高,而IPTG浓度对蛋白的表达量没有显著影响。Western Blotting结果表明,重组蛋白与猪TTV2阳性血清特异性反应,具有很好的免疫原性。成功获得TTV2-ORF1基因,构建了原核表达载体并获得高效表达,为TTV的ELISA检测方法的建立提供抗原。且重组蛋白在15℃条件下,加入0.2 mmol/L浓度的IPTG,诱导24 h,表达条件最佳。

关键词: 猪输血传播病毒2型, 基因克隆, 原核表达

Abstract: To clone the open reading frame 1(ORF1)gene of porcine torque teno virus type 2 and construct a prokaryotic expression vector. TTV2 ORF1 recombinant protein was expressed in Escherichia coli and optimal ex-pression was performed.The ORF1 gene of TTV2 was amplified from the TTV2 positive samples and sub-cloned in a prokaryotic expression vector pcoldI. The constructed recombinant plasmid pcold-ORF1 was transformed to E.coli BL21 for expression the ORF1 fusion protein with six histidine-tag under induction of IPTG. The induction time,in-duction in different temperature and IPTG concentrations were optimized. The recombinant fusion protein had high expression level in BL21(DE3),and SDS-PAGE analysis showed the exogenous gene was mainly expressed as in-clusion bodies and its molecular weight was about 39 kDa.The induction time were positively related trends with re-combinant protein expression,the best induction temperature was 15 ℃,whereas IPTG concentration had no signifi-To clone the open reading frame 1(ORF1)gene of porcine torque teno virus type 2 and construct a prokaryotic expression vector. TTV2 ORF1 recombinant protein was expressed in Escherichia coli and optimal ex-pression was performed.The ORF1 gene of TTV2 was amplified from the TTV2 positive samples and sub-cloned in a prokaryotic expression vector pcoldI. The constructed recombinant plasmid pcold-ORF1 was transformed to E.coli BL21 for expression the ORF1 fusion protein with six histidine-tag under induction of IPTG. The induction time,in-duction in different temperature and IPTG concentrations were optimized. The recombinant fusion protein had high expression level in BL21(DE3),and SDS-PAGE analysis showed the exogenous gene was mainly expressed as in-clusion bodies and its molecular weight was about 39 kDa.The induction time were positively related trends with re-combinant protein expression,the best induction temperature was 15 ℃,whereas IPTG concentration had no signifi- cant impact on protein expression. Western Blotting revealed that the recombinant protein reacted positively with TTV2 positive serum and had a good immunogenicity. The ORF1 gene of TTV2 was successfully cloned and ex-pressed in prokaryotic cells, which provides the immunogen for ELISA. Adding IPTG to a final concentration of 0. 2 mmol/L and shaking the culture at 15 ℃,and then the optimal expression of ORF1 fusion protein were accu-mulated after 24 h.

Key words: Torque teno virus type 2( TTV2), Gene cloning, Prokaryotic expression

中图分类号:

S852.65

王小敏, 何孔旺, 张文文, 王东田, 周忠涛, 张雪寒, 周俊明, 汪伟, 倪艳秀, 温立斌. 猪输血传播病毒2型ORF1基因的原核表达及条件优化[J]. 华北农学报, 2013, 28(5): 38-43. doi: 10.7668/hbnxb.2013.05.007.

WANG Xiao-min, HE Kong-wang, ZHANG Wen-wen, WANG Dong-tian, ZHOU Zhong-tao, ZHANG Xue-han, ZHOU Jun-ming, WANG Wei, NI Yan-xiu, WEN Li-bin. Prokaryotic Expression and Optimization of Expression Conditions of Open Reading Frame 1 Gene of Porcine Torque Teno Virus Type 2[J]. ACTA AGRICULTURAE BOREALI-SINICA, 2013, 28(5): 38-43. doi: 10.7668/hbnxb.2013.05.007.

http://www.hbnxb.net/CN/Y2013/V28/I5/38

参考文献

[1] Nishizawa T,Okamoto H,Konishi K, et al. A Novel DNA Virus( TTV) associated with elevated transaminase levels in posttransfusion hepatitis of unknown etiology[J]. Biochem Biophys Res Commun,1997,241( 1) : 92-97.
[2] 庄辉. TT 病毒的研究现状及展望[J]. 中华内科杂志, 1999,38( 11) : 727-728.
[3] Leary T P,Erker J C,Chalmers M L, et al. Improved detection systems for TT virus reveal high prevalence in humans,non-human primates and farm animals[J]. J Gen Virol,1999,80( 8) : 2115-2120.
[4] Biagini P,de Micco P,de Lamballerie X. Identification of a third member of the Anellovirus genus( "small anellovirus") in French blood donors[J]. Arch Virol,2006,151( 2) : 405-408.
[5] Niel C,Diniz-Mendes L,Devalle S. Rolling-circle amplification of Torque teno virus( TTV) complete genomes from human and swine sera and identification of a novel swine TTV genogroup[J]. J Gen Virol,2005,86 ( 5) : 1343 －1347.
[6] Segales J,Martinez-Guino L,Cortey M, et al. Retrospective study on swine Torque teno virus genogroups 1 and 2 infection from 1985 to 2005 in Spain[J]. Vet Microbiol,2009,134: 199-207.
[7] Martinez L,Kekarainen T,Sibila M, et al. Torque teno virus(TTV) is highly prevalent in the European wild boar( susscrofa) [J]. Vet Microbiol,2006,118 ( 324) : 223 －229.
[8] 王礞礞,周艳君,陈宗艳,等. 我国猪群中TTV 的鉴定及其分子流行病学分析[J]. 中国预防兽医学报, 2009,31( 10) : 751-755.
[9] Kekarainen T,Sibila M,Segales J. Prevalence of swine Torque teno virus in post-weaning multisystemic wasting syndrome( PMWS) -affected and non-PMWS-affected pigs in Spain[J]. J Gen Virol,2006,87( 4) : 833-837.
[10] 刘建波,郭龙军,危艳武,等. 猪输血传播病毒( TTV)与猪圆环病毒混合感染的检测及TTV 遗传变异分析[J]. 中国预防兽医学报, 2011,33( 1) : 6-10.
[11] Okamoto H. TT viruses in animals[J]. Curt Top Microbiol Immunol,2009,33( 1) : 35-52.
[12] Mohammad Irshad,Shiwani Singh,Khushboo Irshad,et al. Torque teno virus: Its prevalence and isotypes in North India[J]. World J Gastroenterol,2008,14( 39) :6044-6051.
[13] Andreas G,Stefan P,Wiebke S E, et al. Porcine Torque teno virus: Determination of viral genomic loads by genogroup- specic multiplex rt-PCR detection of frequent multiple infections with geno groups 1 or 2,and establishment of viral full-length sequences[J]. Vet Microbiol, 2010,143( 2-4) : 202-212.
[14] Huang Y W,Dryman B A,Harrall K K, et al. Development of SYBR green-based real-time PCR and duplex nested PCR assays for quantitation and differential detection of species-or type-specific porcine Torque teno viruses[J]. Jornal Virological Methods,2010,170: 140-146.
[15] 侯军委,周艳君,王礞礞,等. 猪源TTVTaqman 实时荧光定量PCR 检测方法的建立和应用[J]. 中国动物传染病学报, 2011,19( 2) : 13-19.
[16] 陈欣,符芳,王伟,等. TTV1 与TTV2 SYBRGreenⅠ实时荧光PCR 检测方法的建立和应用[J].中国预防兽医学报, 2010,32( 12) : 948-951.
[17] Sambrook J,Fritsch E F,Maniatis T. Molecular cloning: a laboratory manual[M]. 3rd eds. Cold Spring Harbor: Cold Spring Harbor Laboratory Press,2002:934

选择文件类型/文献管理软件名称

选择包含的内容

猪输血传播病毒2型ORF1基因的原核表达及条件优化

Prokaryotic Expression and Optimization of Expression Conditions of Open Reading Frame 1 Gene of Porcine Torque Teno Virus Type 2

PDF

可视化

被引次数

摘要/Abstract

引用本文

使用本文

参考文献

相关文章 15

编辑推荐

Metrics

本文评价

[1]	肖士奎, 李芳, 张文婷, 吕淑芳, 史国安, 吴疆, 范丙友. *芍药ACS基因的克隆及其蛋白质原核表达*[J]. 华北农学报, 2022, 37(5): 36-44.
[2]	侯瑞泽, 侯玉翔, 许小勇, 李璿, 李梅兰. 普通白菜CYP同源基因克隆与表达分析[J]. 华北农学报, 2022, 37(5): 45-51.
[3]	金一锋, 高岩松, 王琦, 王萌萌, 赵迪, 熊毅, 陈阳. *草地早熟禾蛋白激酶SnRK2.4* 基因克隆及非生物胁迫响应分析**[J]. 华北农学报, 2022, 37(5): 9-15.
[4]	张冬梅, 冯亚艳, 修志君, 杨春芳, 杜美娥, 李得宙, 张笑宇. *硅酸钠诱导的马铃薯抗黑痣病StWRKY11基因克隆及生物信息学分析*[J]. 华北农学报, 2022, 37(5): 194-203.
[5]	郑玉斯, 王培, 郭颖, 白丽蓉, 喻达辉, 赵森. *合浦珠母贝PfCLEC17A* 基因的克隆及表达分析**[J]. 华北农学报, 2022, 37(5): 230-238.
[6]	王亚男, 梁岩岩, 严文培, 张银萍, 李强, 吴秀菊. *北细辛AhOMT1基因的克隆及原核表达分析*[J]. 华北农学报, 2022, 37(4): 62-70.
[7]	贾志强, 许云玉, 高雪, 陶宏征, 陈增敏, 刘雅婷, 李永忠. *辣椒CaWRKY30转录因子的克隆、亚细胞定位及番茄斑萎病毒侵染下的表达分析*[J]. 华北农学报, 2022, 37(3): 186-192.
[8]	程春红, 游经番, 蔡兆明, 叶春宏, 陈丽. *茎瘤芥BjuEAR1-1的克隆与表达分析*[J]. 华北农学报, 2022, 37(3): 37-43.
[9]	唐忠丽, 逯晓楠, 赵蕊, 刘庆华, 李梅兰, 雷逢进, 许小勇. *黄皮西葫芦类胡萝卜素合成酶基因的鉴定及PSY1和LCYE2克隆分析*[J]. 华北农学报, 2022, 37(3): 60-67.
[10]	赵惠英, 杨光凯, 高燕, 张小军, 郝燕燕. *苹果MdSGR2基因克隆及植物超表达载体构建*[J]. 华北农学报, 2022, 37(2): 42-48.
[11]	贾伟哲, 焦博, 王娇, 陈文烨, 杨帆, 刘永伟, 董福双, 赵立群, 周硕. *小麦类钙调素TaCML8-A基因的克隆和表达分析*[J]. 华北农学报, 2022, 37(1): 1-8.
[12]	唐文芳, 徐升胜, 段延碧, 龙雯虹, 杨荣萍, 张雪梅, 孟金贵. 山药DoIPTs基因克隆及珠芽发芽期表达分析[J]. 华北农学报, 2022, 37(1): 27-34.
[13]	陈龙正, 刘静, 刘之洋, 夏彭飞, 袁希汉, 宁宇. *苦瓜白粉病响应基因McMLO1的克隆及表达分析*[J]. 华北农学报, 2022, 37(1): 165-171.
[14]	连凯琪, 纪爽, 周玲玲, 时志琪, 王飞, 张元臣. 黏虫clip型丝氨酸蛋白酶基因的克隆及原核表达[J]. 华北农学报, 2022, 37(1): 195-201.
[15]	李琪, 杨昌恒, 王永, 林亚秋, 向华, 朱江江. 山羊CIDE家族基因克隆分析及互作蛋白预测鉴定[J]. 华北农学报, 2022, 37(1): 211-221.

模态框（Modal）标题

选择文件类型/文献管理软件名称

选择包含的内容

猪输血传播病毒2型ORF1基因的原核表达及条件优化

Prokaryotic Expression and Optimization of Expression Conditions of Open Reading Frame 1 Gene of Porcine Torque Teno Virus Type 2

PDF

可视化

被引次数

摘要/Abstract

引用本文

使用本文

参考文献

相关文章 15

编辑推荐

Metrics

本文评价