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Informative ISSR Markers Help Identify Genetically Distinct Accessions of Oryza rufipogon in Yield Improvement

机译:信息性ISSR标记有助于鉴定在增产中红毛猩猩的遗传不同种质

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Inter simple sequence repeat (ISSR) polymorphism was used to determine genetic diversity and phylogenetic relationships in 90 genotypes of wild and cultivated species of Oryza from different geographical regions of the world. In all the 17 primers used in ISSR-PCR, a total of 11 464 bands were amplified at 253 band positions/loci. The primer UBC-809 amplified the maximum bands (1 059) at 21 band positions. UBC-810 and UBC-835 amplified the minimum of 391 bands each at 7 and 14 band positions, respectively. The mean polymorphism information content ranged from 0.44 to 0.84 and resolving power ranged from 8.69 to 23.53. Un-weighted pair group method with arithmetic mean dendrogram and population structure based on the 17 primers separated all genotypes into 4 major clusters with a genetic similarity of 53%–100%. The first two clusters consisted of 30 O. rufipogon accessions each. In the third cluster, O. nivara and O. longistaminata grouped as one sub-cluster and all other O. nivara accessions and cultivars grouped as another sub-cluster. The fourth cluster had only five O. rufipogon accessions which can be a source of new genes. Four sub-populations were identified within O. rufipogon and two sub-populations within O. nivara at K = 7. A subset of six primers with high resolving power values were the most informative and grouped all genotypes almost similarly as the 17 primers did. Use of these six highly informative primers in ISSR-PCR is a cost effective and robust method for assessing genetic diversity in large germplasm collections of wild rice species.
机译:间简单序列重复(ISSR)多态性用于确定来自世界不同地理区域的90种野生和栽培稻的基因型的遗传多样性和系统发育关系。在ISSR-PCR中使用的所有17种引物中,在253个条带位置/位点上总共扩增了11464个条带。引物UBC-809在21个条带位置扩增了最大条带(1059)。 UBC-810和UBC-835分别在7和14个频段位置分别扩增了至少391个频段。平均多态性信息含量为0.44至0.84,分辨力为8.69至23.53。基于17个引物的算术平均树状图和种群结构的非加权对分组方法将所有基因型分为4个主要簇,遗传相似性为53%–100%。前两个簇每个由30个红景天种质组成。在第三个集群中,O。nivara和O. longistaminata分组为一个子集群,而所有其他O. nivara品种和栽培品种分组为另一个子集群。第四个簇只有五个麦冬麦芽孢杆菌种质,它们可能是新基因的来源。在K = 7时,在O. rufipogon中鉴定出四个亚群,在O. nivara中鉴定出两个亚群。六个具有高分辨力值的引物的子集提供的信息最多,并且将所有基因型分组,与17个引物几乎相似。在ISSR-PCR中使用这六种高度信息量的引物是一种经济高效且可靠的方法,可用于评估野生稻物种的大型种质资源中的遗传多样性。

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