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首页> 外文期刊>Генетика: Ежемес. журн. >The use of RAPD and STS analyses for marking genes of homeologous group 5 chromosomes of common wheat.
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The use of RAPD and STS analyses for marking genes of homeologous group 5 chromosomes of common wheat.

机译:RAPD和STS分析用于标记普通小麦同源5组染色体的基因。

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摘要

The search for STS (sequence-tagged site) and RAPD (random amplified polymorphic DNA) markers tightly linked to some genes of homoeologous group 5 chromosomes of common wheat Triticum aestivum, more specifically, awns inhibitor genes (B1), vernalization response gene (Vrn1) and homoeologous chromosome pairing gene (Ph1), was conducted. To estimate the linkage of the gene with the marker, wheat lines marked with recessive alleles b1 and vrn1 were used. RFLP (restriction fragment length polymorphism)and SSR (simple sequence repeat) analyses of isogenic wheat lines were conducted to characterize the chromosomal region transferred to the isogenic line from the donor parent. In RAPD analysis of isogenic wheat lines marked with recessive alleles b1 andvrn1, 95 arbitrary primers were used. To develop STS markers, analysis of the primary structure of RFLP markers Xpsr426 and Xcdo504, tightly linked to the Vrn1 gene, and the Xpsr1201 marker, located at the Ph1 locus, was carried out. Two markers that are tightly linked to the Vrn1 gene (5AL) - RAPD marker Xr405 and STS marker Xsts426 - were obtained in this work. In addition, there is every reason to believe that Xsts426 can be used as a PCR marker of genes Vrn2 (5BL) and Vrn3 (5DL), while Xsts1201 isa marker of Ph1 (5BL).
机译:寻找与普通小麦小麦5号同源同源基因的一些基因紧密相连的STS(序列标记位点)和RAPD(随机扩增的多态DNA)标记,更确切地说是芒抑制基因(B1),春化反应基因(Vrn1) ),并进行了同源染色体配对基因(Ph1)。为了估计该基因与标记的连锁,使用了标记有隐性等位基因b1和vrn1的小麦品系。对同基因小麦品系进行RFLP(限制性片段长度多态性)和SSR(简单序列重复)分析,以表征从供体亲本转移到同基因品系的染色体区域。在标记有隐性等位基因b1和vrn1的等基因小麦品系的RAPD分析中,使用了95个任意引物。为了开发STS标记,分析了与Vrn1基因紧密相连的RFLP标记Xpsr426和Xcdo504的一级结构,以及位于Ph1位点的Xpsr1201标记。在这项工作中获得了两个与Vrn1基因(5AL)紧密相连的标记-RAPD标记Xr405和STS标记Xsts426。另外,有充分理由相信Xsts426可以用作基因Vrn2(5BL)和Vrn3(5DL)的PCR标记,而Xsts1201是Ph1(5BL)的标记。

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