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首页> 外文期刊>Molecular Breeding >Development of retrotransposon-based molecular markers and their application in genetic mapping in chokecherry (Prunus virginiana L.)
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Development of retrotransposon-based molecular markers and their application in genetic mapping in chokecherry (Prunus virginiana L.)

机译:基于反转录转座子的分子标记的开发及其在拟南芥(Prunus virginiana L.)遗传图谱中的应用

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摘要

Retrotransposons are the largest group of transposable elements (TEs) that are ubiquitous and well dispersed in plant genomes. Transposition/insertion of TEs on chromosomes often generates unique repeat junctions (RJs) between TEs and their flanking sequences. Long terminal repeats (LTR) are well conserved and abundant in plant genomes, making LTR retrotransposons valuable for development of TE junction-based markers. In this study, LTR retrotransposons and their RJs were detected from chokecherry genome sequences generated by Roche 454 sequencing. A total of 1246 LTR retrotransposons were identified, and 338 polymerase chain reaction primer pairs were designed. Of those, 336 were used to amplify DNA from chokecherry and other rosaceous species. An average of 283 of 336 (84.2 %) LTR primer pairs effectively amplified DNA from chokecherries. One hundred and seventeen chokecherry LTR primers also produced amplification in other Prunus (99) or rosaceous species (19). A total of 59 of 78 polymorphic LTR markers were qualified for linkage map construction according to the segregation distortion Chi-square (chi(2)) test. Forty-eight LTR markers were successfully located on a previously constructed chokecherry map. The majority of the LTR markers were mapped on LG XI of the chokecherry map. Our results suggest that LTR marker development using random genome sequences is rapid and cost-efficient. Confirmed applicability of LTR markers in map construction and genetic mapping will facilitate genetic research in chokecherry and other rosaceous species.
机译:逆转座子是在植物基因组中普遍存在且分布良好的最大的转座因子(TEs)组。 TE在染色体上的转位/插入通常会在TE及其侧翼序列之间产生独特的重复连接(RJ)。长末端重复序列(LTR)在植物基因组中非常保守且丰富,这使得LTR逆转座子对于开发基于TE接头的标记物非常有价值。在这项研究中,从通过Roche 454测序产生的窒息基因组序列中检测到LTR逆转座子及其RJ。总共鉴定出1246个LTR反转录转座子,并设计了338个聚合酶链反应引物对。其中336个被用于扩增来自窒息物和其他蔷薇科物种的DNA。 336个LTR引物对中的平均283个(84.2%)有效地扩增了窒息物的DNA。在其他李属(99)或酒渣鼻物种(19)中,也有一百一十七种窒息LTR引物也产生了扩增。 78个多态LTR标记中的总共59个符合根据分离失真卡方(chi(2))测试进行连锁图构建的条件。 48个LTR标记已成功定位在先前构建的扼流圈地图上。大多数LTR标记都被绘制在窒息地图的LG XI上。我们的结果表明,使用随机基因组序列开发LTR标记是快速且具有成本效益的。 LTR标记物在地图构建和遗传图谱中的确定的适用性将有助于窒息和其他蔷薇科物种的遗传研究。

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