菘蓝ItSnRK2.1基因的克隆及其序列特性分析

doi:10.13560/j.cnki.biotech.bull.1985.2017-0692

生物技术通报 ›› 2018, Vol. 34 ›› Issue (1): 119-128.doi: 10.13560/j.cnki.biotech.bull.1985.2017-0692

菘蓝ItSnRK2.1基因的克隆及其序列特性分析

张春兰¹, 满丽莉¹, 向殿军², 包乌日娜², 刘鹏²

1. 内蒙古民族大学生命科学学院,通辽 028042;
2. 内蒙古民族大学农学院,通辽 028042

收稿日期:2017-08-22 出版日期:2018-01-26 发布日期:2018-01-22
作者简介:张春兰,女,实验师,研究方向：作物生物技术;E-mail：xiangman05@126.com;满丽莉为本文共同第一作者
基金资助:
牡丹江市科学技术计划项目（G2013n0012）

Cloning and Characteristics Analysis of Gene ItSnRK2.1 from Isatis tinctoria

ZHANG Chun-lan¹, MAN Li-li¹, XIANG Dian-jun², Winner², LIU Peng²

1. College of Life Science,Inner Mongolia University for Nationalities,Tongliao 028042;
2. College of Agriculture,Inner Mongolia University for Nationalities,Tongliao 028042

Received:2017-08-22 Published:2018-01-26 Online:2018-01-22

摘要/Abstract

摘要： SnRK2是ABA通路中至关重要的蛋白激酶,可通过调节下游相关蛋白质的活性来调节胁迫响应基因的表达,显著改进植物对高盐和干旱等非生物胁迫的抗性。基于SnRK2成员cDNA的UTR保守区域设计兼并引物,利用RT-PCR方法从菘蓝中克隆得到一个SnRK2全长cDNA序列,命名为ItSnRK2.1。测序显示该基因长度为1 305 bp,包含一个1 071 bp的完整开放阅读框,编码356个氨基酸,在GenBank数据库的登录号为 MF423122。ItSnRK2.1蛋白激酶理论等电点为5.64,理论分子量为40.6 kD,属于亲水性蛋白,存在二个显著跨膜结构域,含有42处磷酸化位点,没有信号肽,最可能定位的位置是在细胞质上。ItSnRK2.1蛋白激酶的二级结构具有151个α-螺旋、109个无规则卷曲、66个延伸链和30个β-转角。ItSnRK2.1蛋白包含一个ATP结合位点和一个丝氨酸/苏氨酸酶活结构域,同AtSnRK2.1、AtSnRK2.5和StSnRK2.6蛋白亲缘关系最近,处在同一进化分枝。实时定量RT-PCR检测结果显示,ItSnRK2.1基因在菘蓝幼苗的根部表达量最高,其次是叶,茎的表达量最低;ItSnRK2.1基因积极参与高盐和干旱胁迫应答反应,但对ABA胁迫不敏感,表明该基因可能与植物抗逆境胁迫有关,且不依赖ABA调控通路。

关键词: 菘蓝, ItSnRK2.1基因, 克隆, 特性分析

Abstract: As crucial protein kinase in ABA pathway,SnRK2 regulates the expressions of stress responsive genes by regulating the activity of downstream related proteins,and which then significantly improves the resistance of plants to abiotic stresses such as high salinity and drought. The degenerate primers were designed according to the conserved sequences of UTR domains from SnRK2 cDNA sequences. And a full-length cDNA sequence of SnRK2,named as ItSnRK2.1,was cloned from Isatis tinctoria by RT-PCR method. The length of full-length cDNA（GenBank accession number：MF423122）was 1 305 bp containing a complete open reading frame of 1 071 bp and encoding 356 amino acids. The theoretical isoelectric point and putative molecular weight of the ItSnRK2.1 protein were 5.64 and 30.60 kD,respectively. The ItSnRK2.1 was a hydrophilic protein with 42 phosphorylation sites,contained two significant transmembrane domains and no signal peptide,and played a physiological role in the cytoplasm. The secondary structure of the ItSnRK2.1 protein contained 151 α-helixes,109 random coils,66 extended strands,and 30 β-turns. The ItSnRK2.1 protein contained an ATP binding site and a serine/threonine enzyme activity domain,and was at the same evolutionary branch with AtSnRK2.1,AtSnRK2.5 and StSnRK2.6. RT-PCR results showed that ItSnRK2.1 gene expressed mostly in roots,following in leaves,and marginally in stems of I. tinctoria seedlings. In conclusion,ItSnRK2.1 gene actively involved in the responses to high salt and drought stresses,but not sensitive to ABA stress,suggesting that the function of this gene was possibly associated with plant stress resistance,and independent of ABA regulatory pathway.

Key words: Isatis tinctoria, ItSnRK2.1 gene, cloning, characterization analysis

张春兰, 满丽莉, 向殿军, 包乌日娜, 刘鹏. 菘蓝ItSnRK2.1基因的克隆及其序列特性分析[J]. 生物技术通报, 2018, 34(1): 119-128.

ZHANG Chun-lan, MAN Li-li, XIANG Dian-jun, Winner, LIU Peng. Cloning and Characteristics Analysis of Gene ItSnRK2.1 from Isatis tinctoria[J]. Biotechnology Bulletin, 2018, 34(1): 119-128.

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菘蓝ItSnRK2.1基因的克隆及其序列特性分析

Cloning and Characteristics Analysis of Gene ItSnRK2.1 from Isatis tinctoria

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