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作 者:张娜[1] 杨文香[1] 李亚宁[1] 张汀[1] 刘大群[1]
机构地区:[1]河北农业大学植物保护学院植物病理学系/河北省农作物病虫害生物防治工程技术研究中心,河北保定071001
出 处:《作物学报》2007年第4期657-662,共6页Acta Agronomica Sinica
基 金:国家自然科学基金项目(30170602);国家重点基础研究发展计划(973计划)项目(2005CCA01600)
摘 要:用定位于2A染色体的59对SSR、EST-SSR引物,对小麦抗叶锈病基因Lr45进行分子标记,共筛选出11对揭示TcLr45多态性的引物。用157株F2抗感群体对这11对引物进一步检测,得到4个与Lr45共分离的SSR标记(Xgwm95、Xgwm47、Xgwm372和Xgwm122)。将经PAGE检测的标记Xgwm95的抗感差异带及Xgwm47的抗性片段进行克隆测序发现其中含有微卫星序列,且均为二核苷酸重复。Xgwm372和Xgwm122经琼脂糖凝胶电泳发现,与Lr45的供体黑麦有共同的标记片段,可直接用于分子标记辅助选择。Wheat ( Triticum aestivum L. ) leaf rest, caused by Puccinia triticina (formerly P. recondita f. sp. tritici), is one of the most destructive diseases on wheat production throughout the world. The exploitation of markers and locations of leaf rust resistance (Lr series) genes will facilitate marker-assisted selection, and benefit the breeding of effective leaf rust resistant cultivars and the gene cloning. Lr45 is a resistant gene against wheat leaf rust disease originated from Secale cereale and is located on the chromosome 2A. No vimlent isolate to the gene has been found to date. SSR are abundant, highly polymorphic, evenly distributed over the wheat genome, and required only small amounts of genomic DNA for analysis. Therefore, it is highly suitable for genetic markers in wheat for mapping agronomically important genes. And it provides a robust tool for verification and localization of wheat target genes. In this study, SSR markers were employed to tag the gene Lr45 and four NILs (TcLr11, TcLr17, TcLr37, and TcLr45), the original parent Secale cereale, the susceptible line Thatcher and 157 individuals of F2 progeny derived from a cross between TcLr45 and Thatcher were used to marker gene Lr45. The wheat seedlings of parents and F2 generation were inoculated solely with leaf rust spora, and cultured in greenhouse. At the 14th day after inoculation, infection type of all plant materials were scored in six grades with Roelfs' s system. Genomic DNA of wheat was isolated by CTAB. Fifty-nine SSR and EST-SSR primer pairs located on wheat chromosome 2A were screened, and the PCR-amplified products were either checked on 3.0% agrose gel or on a denaturing 6.0% poly-acrylamide gel. Eleven primer pairs displayed polyrnorphism of TcLr45 and four SSR markers (Xgwm95, Xgwm47, Xgwm372, and Xgwm122) co-segregated with Lr45 were acquired. Xgwm95 gave difference bands in F2 populations, and Xgwm47 have a resistance band of 133 bp. Resistance and susceptibility sequenced marker Xgwm95, resistance sequenced
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