[1]邹晶晶,陆玲,曾祥玲,等.桂花DAD-1基因克隆与表达分析[J].北方园艺,2017,41(08):96-102.[doi:10.11937/bfyy.201708022]
　ZOU Jingjing,LU Ling,ZENG Xiangling,et al.Cloning and Expression Analysis of DAD-1 Gene in Osmanthus fragrans[J].Northern Horticulture,2017,41(08):96-102.[doi:10.11937/bfyy.201708022]

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桂花DAD-1基因克隆与表达分析

《北方园艺》[ISSN:1001-0009/CN:23-1247/S] 卷: 第41卷期数: 2017年08 页码: 96-102 栏目: 出版日期: 2017-04-30

Title:: Cloning and Expression Analysis of DAD-1 Gene in Osmanthus fragrans

作者:: 邹晶晶1; 陆玲2; 曾祥玲1; 王彩云3; （1.湖北科技学院核技术与化学生物学院，湖北咸宁 437100；2.孝感市农业科学院蔬菜研究所，湖北孝感 432000； 3.华中农业大学园艺植物生物学教育部重点实验室，湖北武汉 430070）

Author(s):: ZOU Jingjing1; LU Ling2; ZENG Xiangling1; WANG Caiyun3; (1.School of Nuclear Technology and Chemistry & Biology，Hubei University of Science and Technology，Xianning，Hubei 437100;2.Institute of Vegetables,Xiaogan Academy of Agricultural Sciences，Xiaogan,Hubei 432000;3.Key Laboratory for Biology of Horticultural Plants，Ministry of Education，Huazhong Agricultural University,Wuhan,Hubei 430070)

关键词:: 桂花; DAD-1基因; 细胞程序性死亡; 花瓣衰老

Keywords:: Osmanthus fragrans; DAD-1 gene; program cell death; flower senescence

DOI:: 10.11937/bfyy.201708022

文献标志码:: A

摘要:: 以“柳叶金桂”桂花(Osmanthus fragrans ‘Liuye Jingui’)为试材，采用TAIL-PCR技术，克隆了“柳叶金桂”花瓣中DAD-1基因的全长序列，并分析了其在桂花不同组织部位及开花阶段的时空表达模式，以期为研究该基因在桂花花瓣衰老过程中的功能提供参考依据。结果表明：DAD-1基因由560个碱基组成，包含一个351 bp的完整开放阅读框和一个3′-Poly A尾巴；DAD-1基因编码的蛋白包含116个氨基酸，其结构预测表明DAD-1蛋白属于疏水性膜整合蛋白，通过3个α-螺旋构成的跨膜区行使功能。半定量PCR结果表明，该基因在“柳叶金桂”的根、茎、叶、花等各组织器官中均有表达，且在花苞、新叶等幼嫩组织器官中相对表达量较高，在老叶等成熟组织器官中相对表达量较低。实时荧光定量PCR结果表明，在“柳叶金桂”花瓣衰老过程中，DAD-1基因在铃梗期开始显著下调表达。

Abstract:: Osmanthus fragrans ‘Liuye Jingui’ was used as tested material.The complete coding sequence (CDS) of DAD-1 gene was cloned by the method of thermal asymmetric interlaced PCR (TAIL-PCR)，and its expression patterns in different organs and different flowering stages in O.fragrans were analyzed，to provide reference for studying the function of this gene during the flower senescence.The results showed that the length of DAD-1 gene was constituted of 560 bases with an open reading frame of 351 bp and a 3′-Poly A.The DAD-1 protein encoded 116 amino acids，and it was a hydrophobic integration membrane protein with three alpha-helixs in the structure.The results of semi-quantitative reverse transcription-polymerase chain reaction (RT-PCR) showed that DAD-1 expressed in most tissues of sweet Osmanthus，such as the stem，root，flower and leaf，and it was higher in the young organs such as young flowers and new leaves，but lower in old organs such as the old leaves.The results of quantitative real-time polymerase chain reaction (real-time PCR) showed that DAD-1 abundance rapidly decreased at the initial flowering stage，much earlier than the visible senescence symptoms.

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备注/Memo

第一作者简介：邹晶晶（1985-），女，博士，讲师，研究方向为观赏植物采后生理与分子生物学。E-mail：xingxingzou@163.com.责任作者：王彩云（1963-），女，博士，教授，研究方向为观赏植物栽培及采后生理。E-mail：248361509@qq.com.基金项目：湖北省教育厅科学技术研究资助项目（Q20162805）；湖北科技学院博士启动基金资助项目（BK1429）。

更新日期/Last Update: 2017-05-05