甘薯IbTPS1基因的克隆与活性鉴定
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  • 英文篇名:Cloning and identification of IbTPS1 from Ipomoea batatas
  • 作者:王文斌 ; 于欢 ; 杨燕新 ; 邱相坡
  • 英文作者:Wang Wenbin;Yu Huan;Yang Yanxin;Qiu Xiangpo;College of Life Sciences,Shanxi Agricultural University;College of Arts and Sciences,Shanxi Agricultural University;
  • 关键词:甘薯 ; 海藻糖-6-磷酸合成酶基因(TPS1) ; 基因克隆
  • 英文关键词:Ipomoease batatas;;Trehalose-6-phosphate synthase gene;;Gene cloning
  • 中文刊名:SXNY
  • 英文刊名:Journal of Shanxi Agricultural University(Natural Science Edition)
  • 机构:山西农业大学生命科学学院;山西农业大学文理学院;
  • 出版日期:2019-06-13 09:21
  • 出版单位:山西农业大学学报(自然科学版)
  • 年:2019
  • 期:v.39
  • 基金:山西省基础研究计划(201801D121204);; 山西农业大学国家自然科学基金培育项目(2017GPY06);山西农业大学科技创新基金(2018yz003);山西农业大学博士科研启动基金(XB2009002)
  • 语种:中文;
  • 页:SXNY201904003
  • 页数:7
  • CN:04
  • ISSN:14-1306/N
  • 分类号:23-29
摘要
[目的]发掘植物海藻糖合成途径关键酶基因,探究其编码蛋白TPS活性,为作物遗传改良抗多种胁迫提供优良的候选基因。[方法]本研究基于干旱条件下从甘薯转录组数据库中得到一条与拟南芥AtTPS1基因高度同源的Unigene序列,通过RT-PCR技术克隆了甘薯TPS基因。利用生物信息学软件分析序列特征,酵母互补试验鉴定编码蛋白TPS活性。[结果]IbTPS1基因cDNA序列全长2 811bp,编码936个氨基酸,且具有典型的GT1-TPS和HAD-TPP结构域;生物信息学预测表明IbTPS1编码的蛋白是一个不稳定亲水性蛋白,无信号肽,定位于细胞质中;二级结构元件多以无规则卷曲和α-螺旋为主;酵母互补实验证明表达IbTPS1基因的TPS突变酵母菌株(tps1Δ)和TPS,TPP双突变酵母菌株(tps1Δtps2Δ),以葡萄糖为唯一碳源的尿嘧啶缺失培养基上可恢复生长。[结论]证实甘薯IbTPS1基因的编码蛋白具有生物活性。
        [Objectives]Present study was conducted to explore key enzymatic genes which involved in plant trehalose synthesis,to determine the activity of trehalose-6-phosphate synthase gene,and to provide an excellent candidate gene for crop genetic improvement with resistance to multiple stresses.[Methods]A sweet potato trehalose-6-phosphate synthase gene(IbTPS1)which has high homology with AtTPS1,was screened from the transcriptome database under drought stress conditions,and was amplified by RT-PCR.The bioinformatics software was used to analyze the sequence characteristics,and the yeast complementation assay was used to identify the TPS activity.[Results]The cDNA full-length of IbTPS1 was 2 811 bp that encoded 936 amino acid.IbTPS1 protein contained a typical GT1-TPS structure domain and HAD-TPP structure domain.Biological information analysis showed that IbTPS1 belonged to the unstable and hydrophilic protein without signal peptide,and localized in the cytoplasm.The secondary structural elements were mostly composed of random coils andα-helices.Yeast complementation assay results demonstrated that yeast TPS mutant(tps1Δ)and TPS/TPP mutant(tps1Δtps2Δ)expressing IbTPS1 gene could restore growth on the medium supplemented with glucose.[Conclusion]The result indicated that sweetpotao IbTPS1 protein is an activetive trehalose-6-phosphate synthase.
引文
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