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水稻光温敏核不育系的ISSR和SSR遗传分析比较
引用本文:李进波,江良荣,李春海,牟同敏.水稻光温敏核不育系的ISSR和SSR遗传分析比较[J].分子植物育种,2003,1(1):42-47.
作者姓名:李进波  江良荣  李春海  牟同敏
作者单位:1. 湖北省农科院杂交水稻工程技术研究中心,武汉,430070;海南省农作物分子育种重点实验室,三亚,572025
2. 海南省农作物分子育种重点实验室,三亚,572025
3. 华中农业大学作物遗传改良国家重点实验室,武汉,430070
基金项目:国家高技术研究发展计划(863计划),海南省自然科学基金,海南省科学事业费项目,2001AA211091,3003,,,,
摘    要:本研究应用ISSR和SSR技术建立了24个水稻光温敏核不育系的DNA指纹图谱,利用13个ISSR引物和20对SSR引物,分别获得174个多态性片段和62个多态性片段,平均每个ISSR引物检测到13.38个多态性片段,远远高于SSR引物的检测率。根据遗传距离进行的聚类分析表明,利用这两种标记所得的聚类结果十分相似,24个材料被聚为粳型,偏籼型和籼型三个类群,在籼型不育系类群内,又可明显的分成三个亚类群,其中7个安农S-1衍生的不育系聚为一类,与农垦58S衍生的不育系有明显的遗传差异。根据两种标记计算的遗传距离及其遗传关系,所得的结果仍有一些差异,但总体趋势是一致。研究结果表明,ISSR和SSR标记适用于构建DNA指纹图谱,进行分类鉴定和遗传分析。

关 键 词:水稻  光温敏核不育系  ISSR  SSR  遗传分析  遗传标记  DNA指纹图谱

Comparisons of Genetic Analysis Based on ISSR and SSR in PGMS and TGMS Rice Lines
Li Jinbo , Jiang Liangrong Li Chunhai Mou tongmin National Key Laboratory of Crop Genetic Improvement,Huazhong Agricultural University,Wuhan, Hybrid Rice Research and Development Center,Hubei Academy of Agricultural Sciences,Wuhan, Hainan Provincial Key Laboratory of Crop Molecular Breeding,Sanya.Comparisons of Genetic Analysis Based on ISSR and SSR in PGMS and TGMS Rice Lines[J].Molecular Plant Breeding,2003,1(1):42-47.
Authors:Li Jinbo  Jiang Liangrong Li Chunhai Mou tongmin National Key Laboratory of Crop Genetic Improvement  Huazhong Agricultural University  Wuhan  Hybrid Rice Research and Development Center  Hubei Academy of Agricultural Sciences  Wuhan  Hainan Provincial Key Laboratory of Crop Molecular Breeding  Sanya
Institution:Li Jinbo 2,3 Jiang Liangrong 3 Li Chunhai 1 Mou tongmin 1* 1 National Key Laboratory of Crop Genetic Improvement,Huazhong Agricultural University,Wuhan,430070 2 Hybrid Rice Research and Development Center,Hubei Academy of Agricultural Sciences,Wuhan,430070 3 Hainan Provincial Key Laboratory of Crop Molecular Breeding,Sanya,572025
Abstract:In this study, DNA fingerprints of 24 elite photoperiod sensitive genic male sterile (PGMS) and thermo sensitive genic male sterile (TGMS ) rice lines were established using inter simple sequence repeats (ISSR) markers and simple sequence repeats (SSR) markers. 13 ISSR primers could amplify 174 polymorphic bands and 20 SSR primers could amplify 62 polymorphic bands. The numbers of average polymorphic bands produced by per ISSR primer are 13 38 more than those produced by per pair of SSR primer. The results showed that clustering analysis based on ISSR data is very similar to that based on SSR data. These 24 sterile lines used in this research were divided into three groups, indica group, indica like and japonica group. In the indicagroup, 19 sterile lines were also clustered into three subgroups. 7 sterile lines derived from Annong S 1 were clustered together, which show obviously genetic differences compared to 11 indica sterile lines derived from Nongken 58S. There are a little differences in genetic distance and genetic relationship of tested sterile lines calculated by depending on data from ISSR or SSR. The results of this research demonstrated that it is more suitable for using ISSR and SSR as marker to do DNA fingerprint construction, classification and genetic analysis.
Keywords:Rice  PGMS  TGMS  ISSR  SSR  Genetic analysis
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