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定位水稻中负责抗纹枯病的数量性状基因座。

Mapping quantitative trait Loci responsible for resistance to sheath blight in rice.

作者信息

Liu G, Jia Y, Correa-Victoria F J, Prado G A, Yeater K M, McClung A, Correll J C

机构信息

Rice Research and Extension Center, University of Arkansas, 2900 Hwy 130E, Stuttgart, AR 72160, USA.

出版信息

Phytopathology. 2009 Sep;99(9):1078-84. doi: 10.1094/PHYTO-99-9-1078.

Abstract

Rice sheath blight (ShB), caused by the soilborne pathogen Rhizoctonia solani, annually causes severe losses in yield and quality in many rice production areas worldwide. Jasmine 85 is an indica cultivar that has proven to have a high level of resistance to this pathogen. The objective of this study was to determine the ability of controlled environment inoculation assays to detect ShB resistance quantitative trait loci (QTLs) in a cross derived from the susceptible cv. Lemont and the resistant cv. Jasmine 85. The disease reactions of 250 F(5) recombinant inbred lines (RILs) were measured on the seedlings inoculated using microchamber and mist-chamber assays under greenhouse conditions. In total, 10 ShB-QTLs were identified on chromosomes 1, 2, 3, 5, 6, and 9 using these two methods. The microchamber method identified four of five new ShB-QTLs, one on each of chromosomes 1, 3, 5, and 6. Both microchamber and mist-chamber methods identified two ShB-QTLs, qShB1 and qShB9-2. Four of the ShB-QTLs or ShB-QTL regions identified on chromosomes 2, 3, and 9 were previously reported in the literature. The major ShB-QTL qShB9-2, which cosegregated with simple sequence repeat (SSR) marker RM245 on chromosome 9, contributed to 24.3 and 27.2% of total phenotypic variation in ShB using microchamber and mistchamber assays, respectively. qShB9-2, a plant-stage-independent QTL, was also verified in nine haplotypes of 10 resistant Lemont/Jasmine 85 RILs using haplotype analysis. These results suggest that multiple ShB-QTLs are involved in ShB resistance and that microchamber and mist-chamber methods are effective for detecting plant-stage-independent QTLs. Furthermore, two SSR markers, RM215 and RM245, are robust markers and can be used in marker-assisted breeding programs to improve ShB resistance.

摘要

由土传病原菌立枯丝核菌引起的水稻纹枯病(ShB),每年在全球许多水稻产区都会导致产量和品质的严重损失。茉莉85是一个籼稻品种,已被证明对这种病原菌具有高度抗性。本研究的目的是确定在可控环境接种试验中检测由感病品种莱蒙特和抗病品种茉莉85杂交得到的后代中水稻纹枯病抗性数量性状位点(QTL)的能力。在温室条件下,使用微室和雾室试验对接种的250个F(5)重组自交系(RIL)的幼苗进行了病害反应测定。使用这两种方法,在第1、2、3、5、6和9号染色体上总共鉴定出10个水稻纹枯病QTL。微室法鉴定出了5个新的水稻纹枯病QTL中的4个,分别位于第1、3、5和6号染色体上。微室法和雾室法都鉴定出了2个水稻纹枯病QTL,即qShB1和qShB9-2。在第2、3和9号染色体上鉴定出的4个水稻纹枯病QTL或水稻纹枯病QTL区域先前已在文献中报道。主要的水稻纹枯病QTL qShB9-2与第9号染色体上的简单序列重复(SSR)标记RM245共分离,在微室和雾室试验中分别占水稻纹枯病总表型变异的24.3%和27.2%。qShB9-2是一个与植物生长阶段无关的QTL,通过单倍型分析在10个抗性莱蒙特/茉莉85 RIL的9个单倍型中也得到了验证。这些结果表明,多个水稻纹枯病QTL参与了水稻纹枯病抗性,微室法和雾室法对于检测与植物生长阶段无关的QTL是有效的。此外,两个SSR标记RM215和RM245是可靠的标记,可用于标记辅助育种计划以提高水稻纹枯病抗性。

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