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水稻Rf-1基因的定位克隆,该基因是BT型细胞质雄性不育的恢复基因,编码一种定位于线粒体的PPR蛋白。

Positional cloning of the rice Rf-1 gene, a restorer of BT-type cytoplasmic male sterility that encodes a mitochondria-targeting PPR protein.

作者信息

Akagi H, Nakamura A, Yokozeki-Misono Y, Inagaki A, Takahashi H, Mori K, Fujimura T

机构信息

Laboratory of Plant Breeding and Genetics, Department of Biological Production, Faculty of Bioresource Sciences, Akita Prefectural University, Kaidoubata-Nishi 241-7, Shimoshinjyo-Nakano, 010-0195 Akita, Japan.

出版信息

Theor Appl Genet. 2004 May;108(8):1449-57. doi: 10.1007/s00122-004-1591-2. Epub 2004 Feb 14.

DOI:10.1007/s00122-004-1591-2
PMID:14968308
Abstract

The combination of cytoplasmic male sterility (CMS) in one parent and a restorer gene ( Rf) to restore fertility in another are indispensable for the development of hybrid varieties. We have found a rice Rf-1 gene that restores BT-type CMS by applying a positional cloning strategy. Using linkage analysis in combination with 6,104 BC(1)F(3) progeny derived from a cross between two near-isogenic lines (NILs) differing only at the Rf-1 locus, we delimited the Rf-1 gene to a 22.4-kb region in the rice genome. Duplicate open reading frames ( Rf-1A and Rf-1B) with a pentatricopeptide (PPR) motif were found in this region. Since several insertions and/or deletions were found in the regions corresponding to both the Rf-1A and Rf-1B genes in the maintainer's allele, they may have lost their function. Rf-1A protein had a mitochondria-targeting signal, whereas Rf-1B did not. The Rf-1B gene encoded a shorter polypeptide that was determined by a premature stop codon. Based on the function of the Rf-1 gene, its product is expected to target mitochondria and may process the transcript from an atp6/orf79 region in the mitochondrial genome. Since the Rf-1A gene encodes a 791-amino acid protein with a signal targeting mitochondria and has 16 repeats of the PPR motif, we concluded that Rf-1A is the Rf-1 gene. Nine duplications of Rf-1A homologs were found around the Rf-1 locus in the Nipponbare genome. However, while some of them encoded proteins with the PPR motif, they do not restore BT-type CMS based on the lack of co-segregation with the restoration phenotype. These duplicates may have played diversified roles in RNA processing and/or recombination in mitochondria during the co-evolution of these genes and the mitochondrial genome.

摘要

一个亲本中的细胞质雄性不育(CMS)与另一个亲本中用于恢复育性的恢复基因(Rf)相结合,对于杂交品种的培育是必不可少的。我们通过应用定位克隆策略发现了一个水稻Rf-1基因,它能恢复BT型CMS。利用连锁分析,结合两个仅在Rf-1位点不同的近等基因系(NILs)杂交产生的6104个BC(1)F(3)后代,我们将Rf-1基因定位到水稻基因组中的一个22.4 kb区域。在该区域发现了具有五肽重复序列(PPR)基序的重复开放阅读框(Rf-1A和Rf-1B)。由于在保持系等位基因中与Rf-1A和Rf-1B基因对应的区域发现了几个插入和/或缺失,它们可能已经失去了功能。Rf-1A蛋白具有线粒体靶向信号,而Rf-1B没有。Rf-1B基因编码的多肽较短,由一个提前的终止密码子决定。基于Rf-1基因的功能,其产物预计靶向线粒体,并可能加工线粒体基因组中atp6/orf79区域的转录本。由于Rf-1A基因编码一个具有线粒体靶向信号的791个氨基酸的蛋白质,并且有16个PPR基序重复,我们得出结论,Rf-1A就是Rf-1基因。在日本晴基因组的Rf-1位点周围发现了9个Rf-1A同源物的重复序列。然而,虽然其中一些编码具有PPR基序的蛋白质,但由于缺乏与恢复表型的共分离,它们不能恢复BT型CMS。这些重复序列可能在这些基因与线粒体基因组的共同进化过程中,在线粒体的RNA加工和/或重组中发挥了多样化的作用。

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