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大麦恢复基因 Rfm1 座位的高分辨率遗传图谱和物理图谱构建。

High-resolution genetic mapping and physical map construction for the fertility restorer Rfm1 locus in barley.

机构信息

Plant Genome Research Unit, National Institute of Agrobiological Sciences, 2-1-2, Kan-non-dai, Tsukuba, 305-8602, Japan.

出版信息

Theor Appl Genet. 2015 Feb;128(2):283-90. doi: 10.1007/s00122-014-2428-2. Epub 2014 Nov 21.

Abstract

High-resolution genetic linkage mapping and BAC physical mapping narrowed the fertility restorer locus Rfm1 in barley to a sub-centimorgan genetic interval and a 208-kb physical interval. Rfm1 restores the fertility of msm1 and msm2 male-sterile cytoplasms in barley. The fertility restoration gene is located on the short arm of chromosome 6H (6HS), and we pursued a positional cloning of this gene. Starting from a previous result that has delimited Rfm1 within a 10.8 cM region on 6HS, we developed novel CAPS and SSR markers tightly linked to the gene in barley using the sequence information from the syntenic region of rice and barley genome assemblies. Next, we performed fine mapping of the Rfm1 locus. To isolate recombinants, we surveyed 3,638 F2 plants derived from a cross between the CMS strain and the Rf strain with adjacent markers (NAS2090 and NAS1080). This analysis identified 175 recombinant plants from the F2 population to build a high-resolution map with nine markers tightly linked to the Rfm1 locus. Rfm1 was located within the 0.14 cM region delimited by two markers (NAS9113 and NAS9200). Using these flanking markers as well as marker cosegregating with Rfm1 (NAS9133), we screened the BAC libraries of the cultivar Morex, an rfm1 carrier. We isolated 11 BAC clones and constructed a BAC physical map using their fingerprints. Finally, we delimited the Rfm1 locus encompassing the rfm1 allele on a 208-kb contig composed of three minimally overlapping BAC clones. This precise localization of the Rfm1 locus in the barley genome is expected to greatly accelerate the future map-based cloning of the Rfm1 gene by sequence analysis and its genetic transformation for the complementation of cytoplasmic male-sterile plants.

摘要

高分辨率遗传连锁图谱和 BAC 物理图谱将大麦育性恢复基因 Rfm1 定位在一个亚厘摩遗传区间和 208kb 物理区间内。Rfm1 恢复了大麦 msm1 和 msm2 雄性不育细胞质的育性。育性恢复基因位于 6H 染色体的短臂上(6HS),我们对该基因进行了定位克隆。从先前已经将 Rfm1 限定在 6HS 上 10.8cM 区域的结果出发,我们利用水稻和大麦基因组序列信息,在大麦中开发了与该基因紧密连锁的新 CAPS 和 SSR 标记。接下来,我们对 Rfm1 基因座进行了精细作图。为了分离重组体,我们用相邻标记(NAS2090 和 NAS1080)对 CMS 品系和 Rf 品系杂交产生的 3638 株 F2 代植株进行了调查。该分析从 F2 群体中鉴定出 175 株重组体植株,构建了一个包含 9 个紧密连锁标记的高分辨率图谱。Rfm1 位于由两个标记(NAS9113 和 NAS9200)界定的 0.14cM 区域内。利用这些侧翼标记以及与 Rfm1 共分离的标记(NAS9133),我们筛选了 Morex 品种的 BAC 文库,该品种是 rfm1 携带者。我们分离了 11 个 BAC 克隆,并利用它们的指纹构建了一个 BAC 物理图谱。最后,我们将 Rfm1 基因座限定在由三个最小重叠 BAC 克隆组成的 208kb 连续体上,该连续体包含 rfm1 等位基因。该 Rfm1 基因座在大麦基因组中的精确定位有望极大地加速该基因的图谱克隆,通过序列分析和对细胞质雄性不育植物的遗传转化来实现其功能互补。

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