植物学报 ›› 2011, Vol. 46 ›› Issue (4): 386-395.DOI: 10.3724/SP.J.1259.2011.00386

• 研究报告 • 上一篇    下一篇

棉花叶绿体基因RNA编辑位点的测定及分析

江媛1, 范术丽2, 宋美珍2, 俞嘉宁1*, 喻树迅2*   

  1. 1陕西师范大学生命科学学院, 西安 710062
    2中国农业科学院棉花研究所/农业部棉花遗传改良重点实验室, 安阳 455000
  • 收稿日期:2010-11-18 修回日期:2011-04-12 出版日期:2011-07-01 发布日期:2011-07-01
  • 通讯作者: 俞嘉宁;喻树迅
  • 基金资助:

    转基因生物新品种培育

Identification and Analysis of RNA Editing Sites in Chloroplast Transcripts of Gossypium hirsutum

Yuan Jiang1, Shuli Fan2, Meizhen Song2, Jianing Yu1*, Shuxun Yu2*   

  1. 1College of Life Science, Shaanxi Normal University, Xi’an 710062, China;

    2Key Laboratory of Cotton Genetics Improvement, Ministry of Agriculture/Cotton Research Institute of the Chinese Academy of Agricultural Sciences, Anyang 455000, China
  • Received:2010-11-18 Revised:2011-04-12 Online:2011-07-01 Published:2011-07-01
  • Contact: Jianing Yu; Shuxun Yu

摘要: 陆生植物叶绿体RNA编辑是转录后基因表达调控的一种重要方式。该文在预测棉花(Gossypium hirsutum)叶绿体基因RNA编辑位点的基础上, 选取中棉10 (CRRI 10)为实验材料, 采用PCR、RT-PCR及测序等方法, 确定CRRI 10的27个叶绿体蛋白编码基因共有55个编辑位点, 均是C→U的转换。与棉种柯字310(C310)的编辑位点比对后发现, CRRI 10多出accD-468和rpoC1-163两个编辑位点, 同时缺失psbN-10。利用生物信息学分析这3个位点, rpoC1-163和psbN-10的编辑可能会改变各自蛋白的二级结构。对CRRI 10中55个编辑位点上游的顺式作用元件(−30–−1)分析显示, 共有8组顺式作用元件的相似性达到60%或以上, 推测各组中的编辑位点可能由相同的反式作用因子来识别。

Abstract: RNA editing is one of the post-transcriptional modification processes in which the bases of a RNA molecule are altered by the addition, deletion and alteration of nucleotides. In most higher plants, RNA editing mainly occurs in mitochondria and plastids and converts from C to U, very rarely from U to C. We investigated RNA editing sites in chloroplasts of Gossypium hirsutum ‘CRRI 10’ by PCR, RT-PCR and sequence alignment. We identified 55 editing sites in 27 protein-coding genes all of which were C-to-U conversion. By comparing editing sites between CRRI 10 and Coker310FR, CRRI 10 had two novel editing sites, accD-468 and rpoC1-163, whereas site psbN-10 was absent. Bioinformatics analysis of the 3 sites revealed that rpoC1-163 and psbN-10 editing might affect the secondary structure of the corresponding protein. Comparison among upstream regions (−30 to −1) of the 55 editing sites of CRRI 10 revealed that 8 pairs share more than 60% sequence similarity suggesting that the sites in each pair may be recognized by the same trans-acting factors.