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基于PCR的标记检测方法的开发与验证,用于小麦中高分子量谷蛋白等位基因Glu-B1-1d(Bx-6)的阴性选择。

Development and validation of a PCR-based marker assay for negative selection of the HMW glutenin allele Glu-B1-1d (Bx-6) in wheat.

作者信息

Schwarz G, Felsenstein F G, Wenzel G

机构信息

EpiGene GmbH, Biotechnology in Plant Protection, Hohenbachernstrasse 19-21, 85354 Freising, Germany.

出版信息

Theor Appl Genet. 2004 Sep;109(5):1064-9. doi: 10.1007/s00122-004-1718-5. Epub 2004 Jun 3.

Abstract

Polymorphisms between the coding sequences of high-molecular-weight (HMW) glutenin x-type genes at the Glu-1 locus were used to amplify Glu-1B x-type-specific PCR fragments. PCR analysis in a wheat cultivar subset carrying different Glu-1B x-type alleles resulted in PCR fragments that differed in size for Glu-B1-1d (B-x6) and non -Glu-B1-1d (B-x6) genotypes. Subsequent sequencing analysis revealed a 15-bp in-frame insertion in the coding regions of all Glu-B1-1d (B-x6) genotypes which allowed the development of a B-x6-specific PCR assay for high-throughput allele sizing by ion-pair reversed-phase high-performance liquid chromatography. The assay was validated in a set of 86 German wheat cultivars, and genotyping data unequivocally verified the presence of HMW glutenin subunits GLU-B1-1D (Bx-6) + GLU-B1-2A (By-8) by means of sodium dodecyl sulphate-polyacrylamide gel electrophoresis. These results demonstrate that the PCR assay can be applied for the detection and negative selection of the 'poor breadmaking quality' Glu-B1-1d (B-x6) alleles in wheat breeding programs.

摘要

利用Glu-1位点高分子量(HMW)谷蛋白x型基因编码序列之间的多态性来扩增Glu-1B x型特异性PCR片段。对携带不同Glu-1B x型等位基因的小麦品种子集进行PCR分析,结果显示,对于Glu-B1-1d(B-x6)和非Glu-B1-1d(B-x6)基因型,PCR片段大小不同。随后的测序分析表明,所有Glu-B1-1d(B-x6)基因型的编码区存在一个15bp的框内插入,这使得能够开发一种B-x6特异性PCR检测方法,通过离子对反相高效液相色谱法进行高通量等位基因大小测定。该检测方法在一组86个德国小麦品种中得到验证,基因分型数据通过十二烷基硫酸钠-聚丙烯酰胺凝胶电泳明确验证了高分子量谷蛋白亚基GLU-B1-1D(Bx-6)+GLU-B1-2A(By-8)的存在。这些结果表明,该PCR检测方法可用于小麦育种计划中“面包制作品质差”的Glu-B1-1d(B-x6)等位基因的检测和负向选择。

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