拟南芥抗病相关基因<em>T1N6_22</em>的原核表达分析

doi:10.7668/hbnxb.2015.01.012

华北农学报 ›› 2015, Vol. 30 ›› Issue (1): 73-76. doi: 10.7668/hbnxb.2015.01.012

所属专题： 生物技术；

拟南芥抗病相关基因T1N6_22的原核表达分析

蒋琛茜¹, 瓮巧云², 樊锦涛¹, 王冠宇¹, 董丽萍¹, 邢继红¹, 董金皋¹

1. 河北农业大学, 真菌毒素与植物分子病理学实验室, 河北保定 071001;
2. 河北北方学院农林科技学院, 河北张家口 075000

收稿日期:2014-11-26 出版日期:2015-02-28
通讯作者: 邢继红(1977-),女,河北东光人,教授,博士,主要从事植物与病原物互作研究。董金皋(1963-),男,河北邢台人,教授,博士,博士生导师,主要从事植物病理学研究。
作者简介:蒋琛茜(1988-),男,河北石家庄人,在读硕士,主要从事植物抗病研究。
基金资助:
国家自然科学基金项目(31200203);河北省自然科学基金项目(C2012204032;C2014405010);高等学校博士学科点专项科研基金项目(20121302120007)

Prokaryotic Expression Analysis of Resistance-related Gene T1N6_22 from Arabidopsis thaliana

JIANG Chen-xi¹, WENG Qiao-yun², FAN Jin-tao¹, WANG Guan-yu¹, DONG Li-ping¹, XING Ji-hong¹, DONG Jin-gao¹

1. Mycotoxin and Molecular Plant Pathology Laboratory, Agricultural University of Hebei, Baoding 071001, China;
2. College of Agriculture and Forestry Science and Technology, Hebei North University, Zhangjiakou 075000, China

Received:2014-11-26 Published:2015-02-28

摘要/Abstract

摘要： 为构建拟南芥抗病相关 T1N6_22 基因的原核表达载体并进行高效表达,获得纯化的T1N6_22蛋白,以拟南芥Col-0的cDNA为模板,扩增获得了 T1N6_22 基因CDS,对其进行克隆、测序后与含有GST标签蛋白的pGEX4T-1载体相连,构建 T1N6_22 的原核表达载体pGEX4T-1- T1N6_22 -GST。经酶切和测序鉴定正确后,将构建好的载体及空载体转化大肠杆菌BL21。结果表明,在大肠杆菌BL21菌株中成功表达了与标签蛋白融合的T1N6_22蛋白,大小约57 kDa。SDS-PAGE分析表明,高效表达的诱导条件为0.1 mmol/L IPTG诱导培养3 h。研究结果为进一步T1N6_22互作蛋白的筛选及其调控拟南芥抗病分子机制的研究奠定了基础。

关键词: 拟南芥, T1N6_22, 原核表达, 纯化

Abstract: This study was aimed to construct prokaryotic expression vector of resistance-related gene T1N6_22 from Arabidopsis thaliana and obtain the purified protein T1N6_22 with high-efficiency expression.The CDS of T1N6_22 was amplified by RT-PCR technology using the cDNA of the Arabidopsis Col-0 and was fused into a prokaryotic expression vector pGEX4T-1.Restriction enzyme digestion and sequencing showed that the recombinant vector pGEX4T-1- T1N6_22 -GST was successfully constructed and transformed into E.coli BL21 cells.The results indicated that the pGEX4T-1- T1N6_22 -GST with the predicted molecular weight of about 57 kDa was successfully expressed in E.coli BL21 strain.SDS-PAGE indicated that the best expression quantity was induced with 0.1 mmol/L IPTG treatment for 3 h.These results would provide basis for screening interacting proteins of T1N6_22 and the regulation mechanism in Arabidopsis resistance.

Key words: Arabidopsis thaliana, T1N6_22, Prokaryotic expression, Purification

中图分类号:

S432.1
Q78

蒋琛茜, 瓮巧云, 樊锦涛, 王冠宇, 董丽萍, 邢继红, 董金皋. 拟南芥抗病相关基因T1N6_22的原核表达分析[J]. 华北农学报, 2015, 30(1): 73-76. doi: 10.7668/hbnxb.2015.01.012.

JIANG Chen-xi, WENG Qiao-yun, FAN Jin-tao, WANG Guan-yu, DONG Li-ping, XING Ji-hong, DONG Jin-gao. Prokaryotic Expression Analysis of Resistance-related Gene T1N6_22 from Arabidopsis thaliana[J]. ACTA AGRICULTURAE BOREALI-SINICA, 2015, 30(1): 73-76. doi: 10.7668/hbnxb.2015.01.012.

http://www.hbnxb.net/CN/Y2015/V30/I1/73

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拟南芥抗病相关基因T1N6_22的原核表达分析

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