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亚麻(Linum usitatissimum L.)EST-SSR的开发与分析

Development and analysis of EST-SSRs for flax (Linum usitatissimum L.).

作者信息

Cloutier Sylvie, Niu Zhixia, Datla Raju, Duguid Scott

机构信息

Cereal Research Centre, Agriculture and Agri-Food Canada, Winnipeg, MB, Canada.

出版信息

Theor Appl Genet. 2009 Jun;119(1):53-63. doi: 10.1007/s00122-009-1016-3. Epub 2009 Apr 9.

Abstract

A set of 146,611 expressed sequence tags (ESTs) were generated from 10 flax cDNA libraries. After assembly, a total of 11,166 contigs and 11,896 singletons were mined for the presence of putative simple sequence repeats (SSRs) and yielded 806 (3.5%) non-redundant sequences which contained 851 putative SSRs. This is equivalent to one EST-SSR per 16.5 kb of sequence. Trinucleotide motifs were the most abundant (76.9%), followed by dinucleotides (13.9%). Tetra-, penta- and hexanucleotide motifs represented <10% of the SSRs identified. A total of 83 SSR motifs were identified. Motif (TTC/GAA)n was the most abundant (10.2%) followed by (CTT/AAG)n (8.7%), (TCT/AGA)n (8.6%), (CT/AG)n (6.7%) and (TC/GA)n (5.3%). A total of 662 primer pairs were designed, of which 610 primer pairs yielded amplicons in a set of 23 flax accessions. Polymorphism between the accessions was found for 248 primer pairs which detected a total of 275 EST-SSR loci. Two to seven alleles were detected per marker. The polymorphism information content value for these markers ranged from 0.08 to 0.82 and averaged 0.35. The 635 alleles detected by the 275 polymorphic EST-SSRs were used to study the genetic relationship of 23 flax accessions. Four major clusters and two singletons were observed. Sub-clusters within the main clusters correlated with the pedigree relationships amongst accessions. The EST-SSRs developed herein represent the first large-scale development of SSR markers in flax. They have potential to be used for the development of genetic and physical maps, quantitative trait loci mapping, genetic diversity studies, association mapping and fingerprinting cultivars for example.

摘要

从10个亚麻cDNA文库中生成了一组146,611个表达序列标签(EST)。组装后,共挖掘出11,166个重叠群和11,896个单拷贝序列,以寻找假定的简单序列重复(SSR),并产生了806个(3.5%)非冗余序列,其中包含851个假定的SSR。这相当于每16.5 kb序列中有一个EST-SSR。三核苷酸基序最为丰富(76.9%),其次是二核苷酸基序(13.9%)。四、五和六核苷酸基序占所鉴定SSR的比例不到10%。共鉴定出83个SSR基序。基序(TTC/GAA)n最为丰富(10.2%),其次是(CTT/AAG)n(8.7%)、(TCT/AGA)n(8.6%)、(CT/AG)n(6.7%)和(TC/GA)n(5.3%)。共设计了662对引物,其中610对引物在一组23个亚麻种质中产生了扩增子。在248对引物中发现了种质间的多态性,这些引物共检测到275个EST-SSR位点。每个标记检测到2至7个等位基因。这些标记的多态性信息含量值范围为0.08至0.82,平均为0.35。利用275个多态性EST-SSR检测到的635个等位基因研究了23个亚麻种质的遗传关系。观察到四个主要聚类和两个单拷贝。主要聚类中的亚聚类与种质间的系谱关系相关。本文开发的EST-SSR代表了亚麻中SSR标记的首次大规模开发。例如,它们有潜力用于遗传图谱和物理图谱的构建、数量性状位点定位、遗传多样性研究、关联作图以及品种指纹识别。

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