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基于 ddRAD-seq 衍生 SNPs 的八倍体草莓(Fragaria ×ananassa)匍匐茎产量的高密度连锁图谱构建和 QTL 定位。

High density linkage map construction and QTL mapping for runner production in allo-octoploid strawberry Fragaria × ananassa based on ddRAD-seq derived SNPs.

机构信息

Department of Horticulture, Suncheon National University, 255 Jungang-ro, Suncheon, Jeonnam, 57922, South Korea.

Department of Genetics and Plant Breeding, Bangladesh Agricultural University, Mymensingh, 2202, Bangladesh.

出版信息

Sci Rep. 2019 Mar 1;9(1):3275. doi: 10.1038/s41598-019-39808-9.

Abstract

Recent advances in high-throughput genome sequencing technologies are now making the genetic dissection of the complex genome of cultivated strawberry easier. We sequenced Maehyang (short-day cultivar) × Albion (day-neutral cultivar) crossing populations using double digest restriction-associated DNA (ddRAD) sequencing technique that yielded 978,968 reads, 80.2% of which were aligned to strawberry genome allowing the identification of 13,181 high quality single nucleotide polymorphisms (SNPs). Total 3051 SNPs showed Mendelian segregation in F, of which 1268 were successfully mapped to 46 linkage groups (LG) spanning a total of 2581.57 cM with an average interval genetic distance of 2.22 cM. The LGs were assigned to the 28 chromosomes of Fragaria × ananassa as determined by positioning the sequence tags on F. vesca genome. In addition, seven QTLs namely, qRU-5D, qRU-3D1, qRU-1D2, qRU-4D, qRU-4C, qRU-5C and qRU-2D2 were identified for runner production with LOD value ranging from 3.5-7.24 that explained 22-38% of phenotypic variation. The key candidate genes having putative roles in meristem differentiation for runnering and flowering within these QTL regions were identified. These will enhance our understanding of the vegetative vs sexual reproductive behavior in strawberry and will aid in setting breeding targets for developing perpetual flowering and profuse runnering cultivar.

摘要

高通量基因组测序技术的最新进展使得对栽培草莓复杂基因组的遗传分析变得更加容易。我们使用双酶切相关 DNA 测序 (ddRAD) 技术对 Maehyang(短日照品种)×Albion(日中性品种)杂交群体进行测序,共产生了 978968 个reads,其中 80.2%与草莓基因组序列匹配,从而鉴定出 13181 个高质量的单核苷酸多态性 (SNP)。F1 代中共有 3051 个 SNP 表现出孟德尔分离,其中 1268 个 SNP 成功定位到 46 个连锁群 (LG),总长度为 2581.57cM,平均遗传距离为 2.22cM。通过将序列标签定位在 F. vesca 基因组上,LG 被分配到 Fragaria ×ananassa 的 28 条染色体上。此外,鉴定到了 7 个与匍匐茎产生相关的 QTL,即 qRU-5D、qRU-3D1、qRU-1D2、qRU-4D、qRU-4C、qRU-5C 和 qRU-2D2,其 LOD 值范围为 3.5-7.24,解释了 22-38%的表型变异。鉴定到了在这些 QTL 区域内与匍匐茎和开花的分生组织分化有关的关键候选基因,这些基因具有假定的作用。这些将有助于我们理解草莓的营养生长和有性生殖行为,并有助于制定培育永久性开花和大量匍匐茎品种的目标。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d8d7/6397268/8199ccd9a7e0/41598_2019_39808_Fig1_HTML.jpg

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