[1]林苏霞,王晓梅,刘志刚,等.大豆主要过敏原GlymBd30K的抗原表位区基因的克隆表达、纯化及免疫原性鉴定[J].大豆科学,2010,29(02):186-190.[doi:10.11861/j.issn.1000-9841.2010.02.0186]
 LIN Su-xia,WANG Xiao-mei,LIU Zhi-gang,et al.Cloning and Expression of the Antigenic Epitope of Gly m Bd 30K Protein from Soybean and Purification and Identification of Expressed Product[J].Soybean Science,2010,29(02):186-190.[doi:10.11861/j.issn.1000-9841.2010.02.0186]
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大豆主要过敏原GlymBd30K的抗原表位区基因的克隆表达、纯化及免疫原性鉴定

《大豆科学》[ISSN:1000-9841/CN:23-1227/S] 卷: 第29卷 期数: 2010年02期 页码: 186-190 栏目: 出版日期: 2010-04-25
Title:
Cloning and Expression of the Antigenic Epitope of Gly m Bd 30K Protein from Soybean and Purification and Identification of Expressed Product
文章编号:
1000-9841(2010)02-0186-05
作者:
林苏霞12王晓梅3刘志刚13曾梦雅1吴 研1陈家杰1
1.呼吸疾病国家重点实验室,深圳大学变态反应分室,广东深圳518060;
2.深圳大学生命科学学院,广东深圳518060;
3.深圳大学医学院,广东深圳518060
Author(s):
LIN Su-xia12 WANG Xiao-mei3 LIU Zhi-gang13 ZENG Meng-ya1WU Yan1CHEN Jia-jie1
1.State Key Laboratory of Respiratory Disease for Allergy, Shenzhen University, Shenzhen 518060;
2.College of Life Science , Shenzhen University, Shenzhen 518060;
3.Medical College, Shenzhen University, Shenzhen 518060, Guangdong, China
关键词:
大豆主要过敏原GlymBd30k抗原表位区基因克隆
Keywords:
The major allergens of soybean Gly m Bd 30k Epitope Cloning
分类号:
S565.1
DOI:
10.11861/j.issn.1000-9841.2010.02.0186
文献标志码:
A
摘要:
根据文献并结合生物信息学方法选取大豆主要过敏原GlymBd30k的抗原表位区,采用PCR方法扩增出该抗原表位区基因片段,并通过酶切连接分别构建单体的pET表达载体(pET-sGly)和二聚体的pET表达载体(pET-dGly),重组质粒转化到大肠杆菌BL21(DE3)plysS,经IPTG诱导后进行SDS-PAGE分析;同时用Ni2+离子亲和层析柱纯化表达的sGly和dGly抗原表位蛋白,用western-blotting和ELISA检测重组蛋白的免疫原性。结果表明:表达的单体sGly蛋白以可溶性表达为主,而其二聚体dGly蛋白以包涵体形式存在,纯化的sGly和dGly蛋白都具有较好的免疫原性,重组蛋白sGly的抗原性更佳。成功构建的大豆主要过敏原GlymBd30k蛋白的抗原表位区单体sGly蛋白及其二聚体dGly蛋白的工程菌,为研制大豆主要过敏原的单克隆抗体以制备用于大豆主要过敏原检测的试剂奠定了基础。
Abstract:
Through reviewing the literatures combined with bioinformatics predication, the antigenic epitope of Gly m Bd 30k allergen was selected. And the gene was amplified by PCR. The pET expression vector for the monomer protein (pET-sGly) and the dimer (pET-dGly) were constructed. The recombinant proteins were expressed in E.coli BL21 (DE3) plysS by IPTG, analyzed by SDS-PAGE, and then purified by metal (Ni2+) chelating affinity chromatography.The immunogenicity was tested by western-blotting and ELISA. Results shows that the monomer protein sGly was mainly expressed as soluble protein, while the dimer protein dGly as inclusion bodies. Purified protein sGly and dGly both have good immunogenicity, and sGly is better. The prokaryotic expression vectors for the monomer protein and dimer of the antigenic epitope of Gly m Bd 30k protein of soybean will make great foundations for developing the monoclonal antibodies and the detection kit of the major allergens of soybean.

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备注/Memo

基金项目:广东省科技计划资助项目(2003A3080502);深港创新圈计划资助项目(200701)。

第一作者简介:林苏霞(1987-),女,在读硕士,研究方向为食物过敏原的分子生物学。E-mail:525yunyi@163.com。
通讯作者:刘志刚,教授,博士生导师。E-mail:lzg@szu.edu.cn。

更新日期/Last Update: 2014-09-13