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利用水稻作为基因组间克隆载体进行基于图谱的大麦抗秆锈病基因Rpg1和rpg4的克隆

Towards map-based cloning of the barley stem rust resistance genes Rpg1 and rpg4 using rice as an intergenomic cloning vehicle.

作者信息

Kilian A, Chen J, Han F, Steffenson B, Kleinhofs A

机构信息

Dept. of Crop & Soil Sciences, Washington State University, Pullman 99164, USA.

出版信息

Plant Mol Biol. 1997 Sep;35(1-2):187-95.

PMID:9291972
Abstract

The barley stem rust resistance genes Rpg1 and rpg4 were mapped in barley on chromosomes 1P and 7M, respectively and the syntenous rice chromosomes identified as 6P and 3P by mapping common probes in barley and rice. Rice yeast artificial chromosome (YAC), bacterial artificial chromosome (BAC) and cosmid clones were used to isolate probes mapping to the barley Rpg1 region. The rice BAC isolated with the pM13 probe was a particularly excellent source of probes. A high-resolution map of the Rpg1 region was established with 1400 gametes yielding a map density of 3.6 markers per 0.1 cM. A detailed physical map was established for the rice BAC fragment containing the Rpg1-flanking markers pM13 and B24. This fragment covers a barley genetic distance of 0.6 cM and a rice DNA physical distance of ca. 70 kb. The distribution of barley cross-overs in relation to the rice DNA physical distances was extremely uneven. The barley genetic distance between the pM13 marker and Rpg1 was 0.1 cM per ca. 55 kb, while on the proximal side it was 0.5 cm per ca. 15 kb. Three probes from the distal end of the pM13 BAC mapped 3.0 cm proximal of Rpg1 and out of synteny with rice. These experiments confirm the validity of using large insert rice clones as probe sources to saturate small barley (and other large genome cereals) genome regions with markers. They also establish a note of caution that even in regions of high microsynteny, there may be small DNA fragments that have transposed and are no longer in syntenous positions.

摘要

大麦抗秆锈病基因Rpg1和rpg4分别定位在大麦的1P和7M染色体上,通过在大麦和水稻中定位共同探针,确定与之同线的水稻染色体为6P和3P。利用水稻酵母人工染色体(YAC)、细菌人工染色体(BAC)和黏粒克隆来分离定位到大麦Rpg1区域的探针。用pM13探针分离出的水稻BAC是特别优良的探针来源。利用1400个配子构建了Rpg1区域的高分辨率图谱,图谱密度为每0.1 cM有3.6个标记。为包含Rpg1侧翼标记pM13和B24的水稻BAC片段构建了详细的物理图谱。该片段覆盖大麦遗传距离0.6 cM和水稻DNA物理距离约70 kb。大麦交叉与水稻DNA物理距离的分布极不均匀。pM13标记与Rpg1之间的大麦遗传距离约为每55 kb 0.1 cM,而在近端一侧约为每15 kb 0.5 cM。来自pM13 BAC远端的三个探针定位在Rpg1近端3.0 cM处,且与水稻不同线。这些实验证实了使用大型插入水稻克隆作为探针来源,用标记饱和小的大麦(以及其他大基因组谷类作物)基因组区域的有效性。它们还提醒注意,即使在高度微观同线的区域,可能也有小的DNA片段发生了转座,不再处于同线位置。

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