农学学报
農學學報
농학학보
Chinese Countryside Well-off Technology
2011年
10期
18-24
,共7页
薛艺敏%何天友%黄宇%荣俊冬%陈礼光%郑郁善
薛藝敏%何天友%黃宇%榮俊鼕%陳禮光%鄭鬱善
설예민%하천우%황우%영준동%진례광%정욱선
九节茶%ISSR分子标记%多态性%遗传多样性
九節茶%ISSR分子標記%多態性%遺傳多樣性
구절다%ISSR분자표기%다태성%유전다양성
Sarcandra glabra (Thunb.) Nakai%ISSR Molecular Markers%Polymorphism%Genetic Diversity
为进一步研究九节茶的遗传特性,为育种工作提供理论指导,利用ISSR分子标记试验方法研究了37个九节茶种源的遗传多样性,从100条引物中筛选出17条引物,分别利用POPGENE1.32软件及NTSYS软件对九节茶种源进行了基于ISSR的遗传多样性分析及种源聚类分析。结果表明:17条引物共扩增出105个位点,其中多态性位点87个,多态性位点百分率65.71%;37个种源间遗传多样性较低,福建、广东、江西、浙江和广西5个种群之间的遗传多样性为0.1770,种内遗传多样性为0.0990,基因分化系数为0.4405,即种群间遗传变异占种群遗传变异的44.05%,55.95%的遗传变异在种内进行。由种群间的遗传分化系数计算的基因流Nm=0.6350。遗传相似系数为0.7048~0.9143,平均0.8096。聚类分析表明,在遗传相似系数为0.81处,37个种源可以分为5类,聚类结果并不能完全反映出种源的地理分布,但可以部分反映地理分布的特点,为种质资源的鉴定打下良好基础。
為進一步研究九節茶的遺傳特性,為育種工作提供理論指導,利用ISSR分子標記試驗方法研究瞭37箇九節茶種源的遺傳多樣性,從100條引物中篩選齣17條引物,分彆利用POPGENE1.32軟件及NTSYS軟件對九節茶種源進行瞭基于ISSR的遺傳多樣性分析及種源聚類分析。結果錶明:17條引物共擴增齣105箇位點,其中多態性位點87箇,多態性位點百分率65.71%;37箇種源間遺傳多樣性較低,福建、廣東、江西、浙江和廣西5箇種群之間的遺傳多樣性為0.1770,種內遺傳多樣性為0.0990,基因分化繫數為0.4405,即種群間遺傳變異佔種群遺傳變異的44.05%,55.95%的遺傳變異在種內進行。由種群間的遺傳分化繫數計算的基因流Nm=0.6350。遺傳相似繫數為0.7048~0.9143,平均0.8096。聚類分析錶明,在遺傳相似繫數為0.81處,37箇種源可以分為5類,聚類結果併不能完全反映齣種源的地理分佈,但可以部分反映地理分佈的特點,為種質資源的鑒定打下良好基礎。
위진일보연구구절다적유전특성,위육충공작제공이론지도,이용ISSR분자표기시험방법연구료37개구절다충원적유전다양성,종100조인물중사선출17조인물,분별이용POPGENE1.32연건급NTSYS연건대구절다충원진행료기우ISSR적유전다양성분석급충원취류분석。결과표명:17조인물공확증출105개위점,기중다태성위점87개,다태성위점백분솔65.71%;37개충원간유전다양성교저,복건、엄동、강서、절강화엄서5개충군지간적유전다양성위0.1770,충내유전다양성위0.0990,기인분화계수위0.4405,즉충군간유전변이점충군유전변이적44.05%,55.95%적유전변이재충내진행。유충군간적유전분화계수계산적기인류Nm=0.6350。유전상사계수위0.7048~0.9143,평균0.8096。취류분석표명,재유전상사계수위0.81처,37개충원가이분위5류,취류결과병불능완전반영출충원적지리분포,단가이부분반영지리분포적특점,위충질자원적감정타하량호기출。
In order to further study the genetic characteristics of Sarcandra glabra (Thunb.) Nakai,ISSR markers were involved to analyze genetic diversity in 37 accessions of Sarcandra glabra (Thunb.) Nakai germplasms.Among the 100 ISSR molecular markers,there were 17 primers showing good diversity and clear bands.The genetic diversity analysis and cluster analysis were based on the amplification results with POPGENE 1.32 and NTSYS software.It was found that the 105 sites were found by 17 primers,and 87 sites showed polymorphism,the percentage of polymorphic loci was 65.71%,the genetic diversity of the tested 5 populations in the Fujian,Guangdong,Jiangxi,Zhejiang and Guangxi,was 0.1770,and the intra species genetic diversity was 0.0990.The coefficient of gene differentiation (Gst) was 0.4405,and the gene flow Nm was 0.6350.It was indicated that 44.05% population variation came from the interspecific variation,and the others came from intraspecific variation.The variance range of genetic similarity coefficient was 0.7048-0.9143,with an average of 0.8096.Cluster analysis showed that 37 kinds of species could be clustered into 5 groups at a genetic distance coefficient of 0.81.The cluster result indicated that the genetic distance between each small population was related to the environment in which different population of Sarcandra glabra (Thunb.) Nakai grew.However,the genetic distance had no correlation with geographic distance.
