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Obtaining retrotransposon sequences analysis of their genomic distribution and use of retrotransposon-derived genetic markers in lentil (Lens culinaris Medik.)

机译:在小扁豆中获得反转录转座子序列分析其基因组分布并使用反转录转座子衍生的遗传标记(Lens culinaris Medik。)

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摘要

Retrotransposons with long terminal repeats (LTR-RTs) are widespread mobile elements in eukaryotic genomes. We obtained a total of 81 partial LTR-RT sequences from lentil corresponding to internal retrotransposon components and LTRs. Sequences were obtained by PCR from genomic DNA. Approximately 37% of the LTR-RT internal sequences presented premature stop codons, pointing out that these elements must be non-autonomous. LTR sequences were obtained using the iPBS technique which amplifies sequences between LTR-RTs. A total of 193 retrotransposon-derived genetic markers, mainly iPBS, were used to obtain a genetic linkage map from 94 F7 inbred recombinant lines derived from the cross between the cultivar Lupa and the wild ancestor L. culinaris subsp. orientalis. The genetic map included 136 markers located in eight linkage groups. Clusters of tightly linked retrotransposon-derived markers were detected in linkage groups LG1, LG2, and LG6, hence denoting a non-random genomic distribution. Phylogenetic analyses identified the LTR-RT families in which internal and LTR sequences are included. Ty3-gypsy elements were more frequent than Ty1-copia, mainly due to the high Ogre element frequency in lentil, as also occurs in other species of the tribe Vicieae. LTR and internal sequences were used to analyze in silico their distribution among the contigs of the lentil draft genome. Up to 8.8% of the lentil contigs evidenced the presence of at least one LTR-RT similar sequence. A statistical analysis suggested a non-random distribution of these elements within of the lentil genome. In most cases (between 97% and 72%, depending on the LTR-RT type) none of the internal sequences flanked by the LTR sequence pair was detected, suggesting that defective and non-autonomous LTR-RTs are very frequent in lentil. Results support that LTR-RTs are abundant and widespread throughout of the lentil genome and that they are a suitable source of genetic markers useful to carry out further genetic analyses.
机译:具有长末端重复序列(LTR-RT)的逆转座子是真核生物基因组中广泛的移动元件。我们从小扁豆中获得了总共81个部分LTR-RT序列,对应于内部反转录转座子成分和LTR。通过PCR从基因组DNA获得序列。大约37%的LTR-RT内部序列出现过早的终止密码子,指出这些元素必须是非自治的。使用iPBS技术获得LTR序列,该技术可扩增LTR-RT之间的序列。总共193个反转录转座子衍生的遗传标记(主要是iPBS)被用于从94个F7自交重组系获得遗传连锁图谱,该重组系衍生自栽培品种Lupa和野生祖先culinaris亚种之间的杂交。东方人。遗传图谱包括位于八个连锁群中的136个标记。在链接组LG1,LG2和LG6中检测到紧密连接的逆转座子衍生标记的簇,因此表示非随机基因组分布。系统发育分析确定了LTR-RT家族,其中包括内部和LTR序列。 Ty3-吉普赛元素比Ty1-copia更为频繁,这主要是由于小扁豆中的食人魔元素频率较高,在Vicieae部落的其他物种中也是如此。 LTR和内部序列被用于计算机分析它们在扁豆吃水基因组的重叠群中的分布。高达8.8%的小扁豆重叠群证明存在至少一个LTR-RT类似序列。统计分析表明,这些元素在小扁豆基因组中是非随机分布的。在大多数情况下(取决于LTR-RT类型,介于97%和72%之间),没有检测到LTR序列对侧翼的内部序列,这表明扁豆中有缺陷的和非自主的LTR-RT非常常见。结果支持LTR-RT在整个小扁豆基因组中丰富且分布广泛,并且它们是可用于进行进一步遗传分析的遗传标记的合适来源。

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