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首页> 外文期刊>Theoretical and Applied Genetics >Allelic variation of polyphenol oxidase (PPO) genes located on chromosomes 2A and 2D and development of functional markers for the PPO genes in common wheat
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Allelic variation of polyphenol oxidase (PPO) genes located on chromosomes 2A and 2D and development of functional markers for the PPO genes in common wheat

机译:2A和2D染色体上多酚氧化酶(PPO)基因的等位变异和普通小麦PPO基因功能标记的建立

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摘要

Polyphenol oxidase (PPO) activity is highly related to the undesirable browning of wheat-based end products, especially Asian noodles. Characterization of PPO genes and the development of their functional markers are of great importance for marker-assisted selection in wheat breeding. In the present study, complete genomic DNA sequences of two PPO genes, one each located on chromosomes 2A and 2D and their allelic variants were characterized by means of in silico cloning and experimental validation. Sequences were aligned at both DNA and protein levels. Two haplotypes on chromosome 2D showed 95.2% sequence identity at the DNA level, indicating much more sequence diversity than those on chromosome 2A with 99.6% sequence identity. Both of the PPO genes on chromosomes 2A and 2D contain an open reading frame (ORF) of 1,731 bp, encoding a PPO precursor peptide of 577 amino acids with a predicted molecular mass of ∼64 kD. Two complementary dominant STS markers, PPO16 and PPO29, were developed based on the PPO gene haplotypes located on chromosome 2D; they amplify a 713-bp fragment in cultivars with low PPO activity and a 490-bp fragment in those with high PPO activity, respectively. The two markers were mapped on chromosome 2DL using a doubled haploid population derived from the cross Zhongyou 9507/CA9632, and a set of nullisomic–tetrasomic lines and ditelosomic line 2DS of Chinese Spring. QTL analysis indicated that the PPO gene co-segregated with the two STS markers and was closely linked to SSR marker Xwmc41 on chromosome 2DL, explaining from 9.6 to 24.4% of the phenotypic variance for PPO activity across three environments. In order to simultaneously detect PPO loci on chromosomes 2A and 2D, a multiplexed marker combination PPO33/PPO16 was developed and yielded distinguishable DNA patterns in a number of cultivars. The STS marker PPO33 for the PPO gene on chromosome 2A was developed from the same gene sequences as PPO18 that we reported previously, and can amplify a 481-bp and a 290-bp fragment from cultivars with low and high PPO activity, respectively. A total of 217 Chinese wheat cultivars and advanced lines were used to validate the association between the polymorphic fragments and grain PPO activity. The results showed that the marker combination PPO33/PPO16 is efficient and reliable for evaluating PPO activity and can be used in wheat breeding programs aimed for noodle and other end product quality improvement.
机译:多酚氧化酶(PPO)活性与基于小麦的最终产品(尤其是亚洲面条)的不良褐变高度相关。 PPO基因的表征及其功能标记的开发对于小麦育种中标记辅助选择非常重要。在本研究中,通过计算机克隆和实验验证来表征两个PPO基因的完整基因组DNA序列,每个基因位于2A和2D染色体上,以及它们的等位基因变异体。在DNA和蛋白质水平上比对序列。 2D染色体上的两个单倍型在DNA水平上显示95.2%的序列同一性,表明其序列多样性比2A染色体上具有99.6%的序列同一性的多。染色体2A和2D上的两个PPO基因均含有1,731 bp的开放阅读框(ORF),编码577个氨基酸的PPO前体肽,预测分子量约为64 kD。基于位于2D染色体上的PPO基因单倍型,开发了两个互补的优势STS标记PPO16和PPO29。它们分别在低PPO活性的品种中扩增713 bp的片段,在高PPO活性的品种中扩增490 bp的片段。使用来自中游9507 / CA9632的双倍单倍体群体以及中国春季的一组无效等位基因-四体性系和双端体系2DS,将这两个标记物定位在2DL染色体上。 QTL分析表明,PPO基因与两个STS标记共分离,并与2DL染色体上的SSR标记Xwmc41密切相关,解释了在三种环境下PPO活性的表型变异占9.6%至24.4%。为了同时检测2A和2D染色体上的PPO基因座,开发了多重标记组合PPO33 / PPO16,并在许多品种中产生了可区分的DNA模式。 2A染色体上PPO基因的STS标记PPO33是从与我们先前报道的PPO18相同的基因序列开发而来的,可以分别从具有低和高PPO活性的品种中扩增481-bp和290-bp片段。共有217个中国小麦品种和高级品系用于验证多态性片段与籽粒PPO活性之间的关系。结果表明,标记物组合PPO33 / PPO16可有效,可靠地评估PPO活性,可用于小麦改良计划中,以改善面条和其他最终产品的质量。

著录项

  • 来源
    《Theoretical and Applied Genetics》 |2007年第1期|47-58|共12页
  • 作者单位

    Beijing Engineering and Technique Research Center of Hybrid Wheat Beijing Academy of Agricultural and Forestry Sciences Beijing 100097 China;

    College of Agronomy Northwest Sci-Tech University of Agriculture and Forestry Yangling 712100 Shaanxi Province China;

    USDA-ARS Western Wheat Quality Laboratory Washington State University P.O. Box 646394 Pullman WA 99164-6394 USA;

    Department of Crop and Soil Sciences Affiliated with the Western Wheat Quality Laboratory Washington State University Pullman WA 99164-6394 USA;

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