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A universal karyotypic system for hexaploid and diploid Avena species brings oat cytogenetics into the genomics era

机译:用于六倍体和二倍体Avena物种的通用核型系统将燕麦细胞遗传学与基因组学时

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摘要

Abstract Background The identification of chromosomes among Avena species have been studied by C-banding and in situ hybridization. However, the complicated results from several cytogenetic nomenclatures for identifying oat chromosomes are often contradictory. A universal karyotyping nomenclature system for precise chromosome identification and comparative evolutionary studies would be essential for genus Avena based on the recently released genome sequences of hexaploid and diploid Avena species. Results Tandem repetitive sequences were predicted and physically located on chromosomal regions of the released Avena sativa OT3098 genome assembly v1. Eight new oligonucleotide (oligo) probes for sequential fluorescence in situ hybridization (FISH) were designed and then applied for chromosome karyotyping on mitotic metaphase spreads of A. brevis, A. nuda, A. wiestii, A. ventricosa, A. fatua, and A. sativa species. We established a high-resolution standard karyotype of A. sativa based on the distinct FISH signals of multiple oligo probes. FISH painting with bulked oligos, based on wheat-barley collinear regions, was used to validate the linkage group assignment for individual A. sativa chromosomes. We integrated our new Oligo-FISH based karyotype system with earlier karyotype nomenclatures through sequential C-banding and FISH methods, then subsequently determined the precise breakage points of some chromosome translocations in A. sativa. Conclusions This new universal chromosome identification system will be a powerful tool for describing the genetic diversity, chromosomal rearrangements and evolutionary relationships among Avena species by comparative cytogenetic and genomic approaches.
机译:摘要通过C型和原位杂交研究了Avena物种中染色体的鉴定。然而,用于鉴定燕麦染色体的几种细胞遗传学命令的复杂结果通常是矛盾的。基于最近释放的六倍体和二倍体Avena物种的最近释放的基因组序列,养殖型鉴定和比较进化研究的通用核型鉴定和比较进化研究至关重要。结果预测串联重复序列,物理位于释放的Avena Sativa OT3098基因组组件V1的染色体区域上。设计了八种新的寡核苷酸(oligo)原位杂交(鱼类)的荧光(鱼类)探针,然后施用于染色体核型核型核型核型核苷酸型核苷酸型核苷酸,A. Brevis,A. NUDA,A.Viestii,A.Fortricosa,A. Fatua和A. Sativa物种。我们建立了基于多种寡粒探针的不同鱼信号的A.苜蓿的高分辨率标准核型。使用基于麦克利共线区域的膨胀寡核苷酸的鱼绘用于验证单个A.苜蓿染色体的联动组分配。我们通过顺序C键和鱼类方法将新的核心型核型系统与早期的核型术语进行整合,随后确定了A.苜蓿中一些染色体易位的精确破坏点。结论这种新的通用染色体识别系统将是通过比较细胞遗传学和基因组方法描述艾美娜物种中遗传多样性,染色体重排和进化关系的强大工具。

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