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1、中国水稻科学(ChinJRiceSci),2016,30(3):232-238http://www.ricesci.cn232DOI:10.16819/j.1001G7216.2016.5156水稻迟抽穗突变体dth9的遗传分析与基因定位叶卫军1,2,#胡时开2,3,#吴立文2郭龙彪2钱前2,3,∗(1浙江大学农业与生物技术学院,杭州310058;2中国水稻研究所,杭州310006;3中国农业科学院深圳农业基因组研究所,广东深圳518120;#共同第一作者;∗通讯联系人,EGmail:qianqian188@
2、hotmail.com)GeneticAnalysisandGeneMappingofaHeadingGdelayedMutantdth9inRice(OryzasativaL.)YEWeiGjun1,2,#,HUShiGkai2,3,#,WULiGwen2,GUOLongGbiao2,QIANQian2,3,∗(1CollegeofAgriculture&Biotechnology,ZhejiangUniversity,Hangzhou310058,China;2ChinaNationalRiceResea
3、rchInstiGtute,Hangzhou310006,China;2AgriculturalGenomicsInstitute,ChineseAcademyofAgriculturalSciences,Shenzhen518120,China;#Theseauthorscontributedequallytothiswork;∗Correspondingauthor,EGmail:qianqian188@hotmailc.om)YEWeijun,HUShikai,WULiwen,etal.Genetica
4、nalysisandgenemappingofaheadingGdelayedmutantdth9inrice(OryzasativaL.).ChinJRiceSci,2016,30(3):232G238.Abstract:AheadingGdelayedmutant,dth9(daystoheading9)wasidentifiedfromanethylmethylsulfonate(EMS)Ginduced93G11mutantlibrary.Theheadingdateofdth9delayedabou
5、t50dayscomparedtothewildGtypeandtherewasnosignificantdifferenceinotheragronomictraits.Geneticanalysisshowedthatthephenotypeofdth9wascontrolledbyasinglerecessivenucleargene.Tomapthisgene,twoF2populationsweregeneratedbycrossingthedth9mutantwithNipponbareorWuy
6、unjing7asmappingpopulations.ByusingSSRmarkersandeightnewdesignedInDelmarkers,DTH9wasnarrowedtoa240kbintervalbetweenthemarkersD9G9andD9G17nearthecentromereofchromosome9,therewerenoreportsaboutgenesassociatedwithheadingdateinthisinterval.Inaddition,theexpress
7、ionlevelsofgenesrelatedtoheadingdateweresignificantlydecreasedindth9byquantitativerealGtimePCRanalysis.Keywords:rice;headingdate;geneticanalysis;genemapping叶卫军,胡时开,吴立文,等.水稻迟抽穗突变体dth9的遗传分析与基因定位.中国水稻科学,2016,30(3):232G238.摘要:在EMS诱变的93G11突变体库中筛选到一个稳定遗传的迟抽穗突变体dt
8、h9(daystoheading9).该突变体的抽穗期比野生型延长了50d左右,其他农艺性状基本无异.遗传分析表明迟抽穗性状受一个隐性核基因控制.以突变体dth9与日本晴和武运粳7号杂交构建的F2分离群体作为定位群体,利用SSR标记和新开发的8个InDel标记,将DTH9定位在第9染色体着丝粒附近D9G9和D9G17之间240kb的区间内,该区域尚未发现与抽穗期有关的基因.此外,实时荧光定量PCR结
