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pm42的鉴定与基因定位,pm42是一个源自野生二粒小麦(Triticum turgidum var. dicoccoides)的新型隐性小麦抗白粉病基因。

Identification and genetic mapping of pm42, a new recessive wheat powdery mildew resistance gene derived from wild emmer (Triticum turgidum var. dicoccoides).

作者信息

Hua Wei, Liu Ziji, Zhu Jie, Xie Chaojie, Yang Tsomin, Zhou Yilin, Duan Xiayu, Sun Qixin, Liu Zhiyong

机构信息

Department of Plant Genetics and Breeding, China Agricultural University, Beijing 100193, People's Republic of China.

出版信息

Theor Appl Genet. 2009 Jul;119(2):223-30. doi: 10.1007/s00122-009-1031-4. Epub 2009 Apr 30.

Abstract

Powdery mildew, caused by Blumeria graminis f. sp. tritici, is one of the most important wheat diseases worldwide in areas with cool or maritime climates. Wild emmer (Triticum turgidum var. dicoccoides) is an important potential donor of disease resistances and other traits for common wheat improvement. A powdery mildew resistance gene was transferred from wild emmer accession G-303-1M to susceptible common wheat by crossing and backcrossing, resulting in inbred line P63 (Yanda1817/G-303-1 M//3*Jing411, BC(2)F(6)). Genetic analysis of an F(2) population and the F(2:3) families developed from a cross of P63 and a susceptible common wheat line Xuezao showed that the powdery mildew resistance in P63 was controlled by a single recessive gene. Molecular markers and bulked segregant analysis were used to characterize and map the powdery mildew resistance gene. Nine genomic SSR markers (Xbarc7, Xbarc55, Xgwm148, Xgwm257, Xwmc35, Xwmc154, Xwmc257, Xwmc382, Xwmc477), five AFLP-derived SCAR markers (XcauG3, XcauG6, XcauG10, XcauG20, XcauG22), three EST-STS markers (BQ160080, BQ160588, BF146221) and one RFLP-derived STS marker (Xcau516) were linked to the resistance gene, designated pm42, in P63. pm42 was physically mapped on chromosome 2BS bin 0.75-0.84 using Chinese Spring nullisomic-tetrasomic, ditelosomic and deletion lines, and was estimated to be more than 30 cM proximal to Xcau516, a RFLP-derived STS marker that co-segregated with the wild emmer-derived Pm26 which should be physically located in 2BS distal bin 0.84-1.00. pm42 was highly effective against 18 of 21 differential Chinese isolates of B. graminis f. sp. tritici. The closely linked molecular markers will enable the rapid transfer of pm42 to wheat breeding populations thus adding to their genetic diversity.

摘要

由小麦白粉菌小麦专化型(Blumeria graminis f. sp. tritici)引起的白粉病,是凉爽气候或海洋性气候地区全球最重要的小麦病害之一。野生二粒小麦(Triticum turgidum var. dicoccoides)是普通小麦改良中抗病性及其他性状的重要潜在供体。通过杂交和回交,将一个白粉病抗性基因从野生二粒小麦材料G - 303 - 1M转移到感病的普通小麦中,获得了自交系P63(偃大1817/G - 303 - 1M//3×京411,BC(2)F(6))。对P63与感病普通小麦品系薛早杂交产生的F(2)群体及其F(2:3)家系进行遗传分析,结果表明P63中的白粉病抗性由单个隐性基因控制。利用分子标记和集群分离分析法对该白粉病抗性基因进行了鉴定和定位。9个基因组SSR标记(Xbarc7、Xbarc55、Xgwm148、Xgwm257、Xwmc35、Xwmc154、Xwmc257、Xwmc382、Xwmc477)、5个AFLP衍生的SCAR标记(XcauG3、XcauG6、XcauG10、XcauG20、XcauG22)、3个EST - STS标记(BQ160080、BQ160588、BF146221)和1个RFLP衍生的STS标记(Xcau516)与P63中名为pm42的抗性基因连锁。利用中国春缺体 - 四体、双端体和缺失系,将pm42物理定位到2BS染色体臂的0.75 - 0.84区间,估计它位于与野生二粒小麦衍生的Pm26共分离的RFLP衍生STS标记Xcau516近端超过30 cM处,Pm26应位于物理位置2BS染色体臂远端的0.84 - 1.00区间。pm42对21个中国小麦白粉菌小麦专化型鉴别菌系中的18个表现出高抗性。紧密连锁的分子标记将使pm42能够快速转移到小麦育种群体中,从而增加其遗传多样性。

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