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Microarrays for global expression constructed with a low redundancy set of 27,500 sequenced cDNAs representing an array of developmental stages and physiological conditions of the soybean plant

机译:用低冗余度的27,500个测序cDNA集构建的用于全球表达的微阵列,这些序列代表了大豆植物的发育阶段和生理状况

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摘要

BACKGROUND:Microarrays are an important tool with which to examine coordinated gene expression. Soybean (Glycine max) is one of the most economically valuable crop species in the world food supply. In order to accelerate both gene discovery as well as hypothesis-driven research in soybean, global expression resources needed to be developed. The applications of microarray for determining patterns of expression in different tissues or during conditional treatments by dual labeling of the mRNAs are unlimited. In addition, discovery of the molecular basis of traits through examination of naturally occurring variation in hundreds of mutant lines could be enhanced by the construction and use of soybean cDNA microarrays.RESULTS:We report the construction and analysis of a low redundancy 'unigene' set of 27,513 clones that represent a variety of soybean cDNA libraries made from a wide array of source tissue and organ systems, developmental stages, and stress or pathogen-challenged plants.The set was assembled from the 5' sequence data of the cDNA clones using cluster analysis programs. The selected clones were then physically reracked and sequenced at the 3' end. In order to increase gene discovery from immature cotyledon libraries that contain abundant mRNAs representing storage protein gene families, we utilized a high density filter normalization approach to preferentially select more weakly expressed cDNAs. All 27,513 cDNA inserts were amplified by polymerase chain reaction. The amplified products, along with some repetitively spotted control or 'choice' clones, were used to produce three 9,728-element microarrays that have been used to examine tissue specific gene expression and global expression in mutant isolines.CONCLUSIONS:Global expression studies will be greatly aided by the availability of the sequence-validated and low redundancy cDNA sets described in this ++
机译:背景:微阵列是检查协调基因表达的重要工具。大豆(Glycine max)是世界粮食供应中最具经济价值的作物品种之一。为了加速大豆的基因发现以及假设驱动的研究,需要开发全球表达资源。微阵列用于通过mRNA的双重标记来确定不同组织中或条件治疗期间的表达模式的应用是无限的。此外,通过构建和使用大豆cDNA微阵列可以增强通过检查数百个突变系中自然发生的变异而发现性状的分子基础。结果:我们报告了低冗余“单基因”集的构建和分析包含27,513个代表大豆大豆cDNA文库的克隆,这些大豆cDNA文库由多种来源的组织和器官系统,发育阶段以及受胁迫或病原体攻击的植物组成。该集合使用cDNA克隆的5'序列数据进行聚类分析程序。然后将选定的克隆进行物理分离,并在3'端测序。为了增加从不成熟子叶文库中发现基因的发现,该子叶文库包含代表存储蛋白基因家族的丰富mRNA,我们使用了高密度过滤器归一化方法来优先选择表达较弱的cDNA。通过聚合酶链反应扩增所有27,513个cDNA插入片段。扩增后的产物与一些重复发现的对照或“选择”克隆一起,用于生产三个9,728个元素的微阵列,用于检测突变体等位基因中的组织特异性基因表达和整体表达。借助此++中描述的经过序列验证的低冗余cDNA集的可用性

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