粟弯孢霉叶斑病菌G蛋白β亚基基因克隆及表达

doi:10.7668/hbnxb.2014.04.002

华北农学报 ›› 2014, Vol. 29 ›› Issue (4): 7-12. doi: 10.7668/hbnxb.2014.04.002

所属专题： 生物技术；

粟弯孢霉叶斑病菌G蛋白β亚基基因克隆及表达

司贺龙¹, 佟亚萌¹, 郝志敏¹, 李志勇², 王楠³, 董志平², 董金皋¹

1. 河北农业大学生命科学学院, 河北保定 071001;
2. 河北省农林科学院谷子研究所, 河北石家庄 050035;
3. 河北师范大学生命科学学院, 河北石家庄 050024

收稿日期:2014-05-12 出版日期:2014-08-28
通讯作者: 李志勇（1976-），男，河北邯郸人，副研究员，博士，主要从事分子植物病理学研究。董金皋（1963-），男，河北平乡人，教授，博士，主要从事分子植物病理学研究。
作者简介:司贺龙（1975-），男，河北蔚县人，在读博士，主要从事分子植物病理学研究。
基金资助:
谷子产业技术体系项目（CARS-07-12.5-A8）；国家自然科学基金项目（31271787；31301616）

Molecular Cloning and Expression of G Protein β Subunit Gene of Curvularia lunata

SI He-long¹, TONG Ya-meng¹, HAO Zhi-min¹, LI Zhi-yong², WANG Nan³, DONG Zhi-ping², DONG Jin-gao¹

1. College of Life Sciences, Agricultural University of Hebei, Baoding 071001, China;
2. Millet Institute, Hebei Academy of Agriculture and Forestry Sciences, Shijiazhuang 050035, China;
3. College of Life Science, Hebei Normal University, Shijiazhuang 050024, China

Received:2014-05-12 Published:2014-08-28

摘要/Abstract

摘要： 旨在获得粟弯孢霉叶斑病菌G蛋白β亚基基因，明确其表达模式，为阐明该基因对粟弯孢霉叶斑病菌致病性的调控机制奠定基础。运用SMART RACE RT-PCR技术，克隆粟弯孢霉叶斑病菌G蛋白β亚基基因 ClGβ 全长cDNA序列，以qRT-PCR 技术，对该基因在粟弯孢霉叶斑病菌不同生长时间的表达特征进行分析。结果表明，ClGβ 基因cDNA编码区为1 056 bp，DNA包含4个内含子和5个外显子，编码351个氨基酸。该基因的cDNA序列在GenBank中注册的登录号为JQ768316。qRT-PCR结果表明，Gβ 基因在菌株生长过程中表现出前期表达量较低而后期表达量明显升高的趋势。构建了pET28（a）-ClGβ 原核表达载体，经IPTG诱导，目的蛋白在宿主菌 E.coli BL21中获得表达，表达产物分子量与ClGβ蛋白计算分子量一致。

关键词: 粟弯孢病菌, G蛋白β亚基, qRT-PCR, 原核表达

Abstract: In order to make a foundation for illustrating the pathogenic mechanism of G protein beta-subunit in Curvularia lunata,this research focuses on acquiring the gene encoding Gβ subunit in C.lunata and exploring its expression pattern.The full-length cDNA of G-protein beta-subunit was cloned using SMART RACE RT-PCR,and the expression pattern of ClGβ gene was analyzed under different growth time using Real-time PCR.The full-length cDNA of ClGβ was 1 056 bp and encoded 351 amino acids,while its DNA contained 4 introns and 5 extrons.The cDNA sequence of ClGβ had been deposited in GenBank with accession number JQ768316.The results of Real-time PCR indicated that the gene expression level of G-protein beta-subunit is lower at early stage and higher at later stage.We constructed the prokaryotic expression vector pET28(a)-ClGβ,and E.coli BL21 was transformed by this recombinant construct and induced by IPTG.The molecular weight of the expression product was identical with the calculated molecular weight of ClGβ.

Key words: Curvularia lunata, G protein beta-subunit, Real-time quantitative PCR, Prokaryotic expression

中图分类号:

司贺龙, 佟亚萌, 郝志敏, 李志勇, 王楠, 董志平, 董金皋. 粟弯孢霉叶斑病菌G蛋白β亚基基因克隆及表达[J]. 华北农学报, 2014, 29(4): 7-12. doi: 10.7668/hbnxb.2014.04.002.

SI He-long, TONG Ya-meng, HAO Zhi-min, LI Zhi-yong, WANG Nan, DONG Zhi-ping, DONG Jin-gao. Molecular Cloning and Expression of G Protein β Subunit Gene of Curvularia lunata[J]. journal1, 2014, 29(4): 7-12. doi: 10.7668/hbnxb.2014.04.002.

http://www.hbnxb.net/CN/Y2014/V29/I4/7

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