广东番茄黄化曲叶病毒AC2基因的原核表达及抗血清制备

利用PCR方法从广东番茄黄化曲叶病毒分离物G3(TomatoyellowleafcurlGuangdongvirus-[G3],TYLCGuV-[G3])全长序列的重组质粒上扩增该病毒的AC2基因,将其构建至原核表达载体pET-28b(+)上,经IPTG诱导,在大肠埃希菌Rosetta(DE3)Ⅲ中高效表达.SDS—PAGE电泳结果显示,目的融合蛋白与预期大小一致,相对分子质量约为19500.以诱导的融合蛋白为抗原,免疫注射新西兰大耳白兔制备抗血清,间接ELISA测定抗血清效价为1:16384.Western—blotting检测结果表明,制备的抗血清有较好的抗原-抗体识别反应,为专化性抗血清...

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Bibliographic Details
Published in华南农业大学学报 Vol. 32; no. 4; pp. 53 - 56
Main Author 赵芹 李华平 何自福 佘小曼 谢大森 何晓明 彭庆务
Format Journal Article
LanguageChinese
Published 广东省农业科学院蔬菜研究所,广东广州,510640%华南农业大学植物病毒研究室,广东广州,510642%广东省农业科学院植物保护研究所,广东广州,510640 2011
Subjects
AC2基因
原核表达
广东番茄黄化曲叶病毒
抗血清制备
AC2基因
广东番茄黄化曲叶病毒
抗血清制备
原核表达
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ISSN1001-411X
DOI10.3969/j.issn.1001-411X.2011.04.012

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Summary:利用PCR方法从广东番茄黄化曲叶病毒分离物G3(TomatoyellowleafcurlGuangdongvirus-[G3],TYLCGuV-[G3])全长序列的重组质粒上扩增该病毒的AC2基因,将其构建至原核表达载体pET-28b(+)上,经IPTG诱导,在大肠埃希菌Rosetta(DE3)Ⅲ中高效表达.SDS—PAGE电泳结果显示,目的融合蛋白与预期大小一致,相对分子质量约为19500.以诱导的融合蛋白为抗原,免疫注射新西兰大耳白兔制备抗血清,间接ELISA测定抗血清效价为1:16384.Western—blotting检测结果表明,制备的抗血清有较好的抗原-抗体识别反应,为专化性抗血清.
Bibliography:AC2 gene of Tomato yellow leaf curl Guangdong virus isolate G3 ( TYLCGuV- [ G3 ] ) was amplified from its recombinant plasmid by PCR, and the gene was cloned into prokaryote expression vector pET-28b( + ). The expressed fusion protein was highly expressed in Escherichia coli Rosetta( DE3 )Ⅲ induced by IPTG, and the molecular mass was about 19 500 by SDS-PAGE analysis. The fusion protein was used as an antigen to immunize the healthy rabbit and the antiserum of AC2 was prepared. The titer measured by ELISA was about 1:16 384. Western-blotting analysis indicated that the antiserum could serologically react with AC2 protein of TYLCGuV-[ G3 ].
44-1110/S
Tomato yellow leaf curl Guangdong virus; AC2 gene ; prokaryotic expression; antiserumpreparation
ZHAO Qin, LI Hua-ping , HE Zi-fu, SHE Xiao-man , XIE Da-sen , HE Xiao-ming , PENG Qing-wu ( 1 Vegetable Research Institute, Gnangdong Academy of Agricultural Sciences, Guangzhou 510640, China; 2 Laboratory of Plant Virology, South China Agricultural University, Guangzhou
ISSN:1001-411X
DOI:10.3969/j.issn.1001-411X.2011.04.012