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Fine mapping and candidate gene analysis of purple pericarp gene Pb in rice (Oryza sativa L.)

机译:水稻(Oryza sativa L.)紫色果皮基因Pb的精细定位及候选基因分析

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Purple rice is a type of rice with anthocyanins deposited in its grain pericarp. The rice Pb gene controlling purple pericarp character is known to be on chromosome 4, and the purple color is dominant over white color. In this study, we fine mapped the Pb gene using two F_2 segregating populations, i.e. Pei'ai 64S (white) x Yunanheixiannuo (purple) and Pei'ai 64S x Chuanheinuo (purple). In the first-pass mapping, the Pb gene was located in the region downstream the SSR marker RM3820. In the fine mapping, the candidate region was saturated with In Del and CAPS markers developed specifically for this study. Eventually, the Pb gene was mapped within the 25-kb region delimited by the upstream marker RID3 and the downstream marker RID4. The delimited region contained two annotated genes, Ra and bhlh16 (TIGR Rice Genome, R.5). The former is a homologue of the Myc transcription factor Lc controlling anthocyanin biosynthesis in maize, and the latter is a homologue of the TT8 gene, which is also an Myc transcription factor gene controlling the pericarp pigmentation in Arabidopsis thaliana. Sequence analysis showed that the exon 7 of the Ra gene of Yunanheixiannuo and Chuanheinuo had a 2-bp (GT) deletion compared with those of the white rice varieties Pei'ai 64S, 9311 and Nipponbare. A CAPS marker, CAPSRa, was developed according to the GT deletion for analysis of the two F_2 segregating populations and 106 rice lines. The results showed that all F_2 plants with white pericarp, and all non-purple rice lines (63 white and 22 red) contained no GT deletion, but all 20 purple rice lines contained the GT deletion. These results suggested that the Ra gene may be the Pb gene and the purple pericarp characteristic of rice is caused by the GT deletion within exon7 of the Ra gene.
机译:紫米是一种在谷粒果皮中沉积有花青素的米。已知控制紫色果皮特征的水稻Pb基因在4号染色体上,紫色比白色占主导地位。在这项研究中,我们使用两个F_2隔离种群(即Pei'ai 64S(白色)x Yunanheixiannuo(紫色)和Pei'ai 64S x Chuanheinuo(紫色)对Pb基因进行了精细定位。在第一遍作图中,Pb基因位于SSR标记RM3820下游区域。在精细映射中,候选区域被In Del和专为该研究开发的CAPS标记饱和。最终,将Pb基因定位在由上游标记RID3和下游标记RID4界定的25-kb区域内。分隔区域包含两个带注释的基因Ra和bhlh16(TIGR水稻基因组,R.5)。前者是控制玉米花色苷生物合成的Myc转录因子Lc的同源物,后者是TT8基因的同源物,后者也是控制拟南芥果皮色素沉着的Myc转录因子基因。序列分析表明,与白色水稻品种培爱64S,9311和Nipponbare相比,Yunanheixiannuo和Chuanheinuo的Ra基因第7外显子缺失了2 bp(GT)。根据GT缺失,开发了CAPS标记CAPSRa,以分析两个F_2分离种群和106个水稻系。结果表明,所有带有白色果皮的F_2植株和所有非紫色水稻系(63个白色和22个红色)都没有GT缺失,但是所有20个紫色水稻系都带有GT缺失。这些结果提示Ra基因可能是Pb基因,而水稻的紫色果皮特性是由Ra基因第7外显子内的GT缺失引起的。

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