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Genotyping of Endosperms to Determine Seed Dormancy Genes Regulating Germination Through Embryonic Endospermic or Maternal Tissues in Rice

机译:胚乳的基因分型以确定调节通过胚胚乳或母体组织发芽的种子休眠基因

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摘要

Seed dormancy is imposed by one or more of the embryo, endosperm, and maternal tissues that belong to two generations and represent two ploidy levels. Many quantitative trait loci (QTL) have been identified for seed dormancy as measured by gross effects on reduced germination rate or delayed germination in crop or model plants. This research developed an endosperm genotype−based genetic approach to determine specific tissues through which a mapped QTL regulates germination using rice as a model. This approach involves testing germination velocity for partially after-ripened seeds harvested from single plants heterozygous for a tested QTL and genotyping endosperms from individual germinated and nongerminated seeds with a codominant DNA marker located on the QTL peak region. Information collected about the QTL includes genotypic frequencies in germinated and/or nongerminated subpopulations; allelic frequency distributions during a germination period; endosperm or embryo genotypic differences in germination velocity; and genotypic frequencies for gametes involved in the double fertilization to form the sampled seeds. Using this approach, the seed dormancy loci SD12, SD1-2, and SD7-1 were determined to regulate germination through the embryo, endosperm, and maternal tissues, respectively; SD12 and SD1-2 acted additively on germination velocity in the offspring tissues; and SD12 also was associated with the preferential fertilization of male gametes in rice. This new genetic approach can be used to characterize mapped genes/QTL for tissue-specific functions in endospermic seeds and for marker-assisted selection of QTL alleles before or immediately after germination in crop breeding.
机译:种子休眠是由属于两个世代并代表两个倍性水平的一个或多个胚胎,胚乳和母体组织施加的。根据对作物或模型植物发芽率降低或发芽延迟的总体影响,可以确定许多休眠的数量性状位点(QTL)。这项研究开发了一种基于胚乳基因型的遗传方法,以水稻为模型,通过映射的QTL来确定特定组织来调控发芽。该方法涉及测试从单株杂合子中收获的部分后成熟种子的发芽速度,以测试QTL,并使用位于QTL峰值区域的显性DNA标记对单个发芽和未发芽种子的胚乳进行基因分型。收集的有关QTL的信息包括发芽和/或未发芽亚群的基因型频率;萌发期间的等位基因频率分布;胚乳或胚芽发芽速度的基因型差异;配子受精形成双倍受精的基因型频率。使用这种方法,确定了种子休眠位点SD12,SD1-2和SD7-1分别调节通过胚胎,胚乳和母体组织的发芽。 SD12和SD1-2对后代组织中的萌发速度有累加作用。 SD12也与水稻中雄配子的优先受精有关。这种新的遗传方法可用于表征映射的基因/ QTL,用于胚乳种子中组织特有的功能,以及在作物育种中发芽之前或之后立即进行QTL等位基因的标记辅助选择。

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