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首页> 外文期刊>Plant Molecular Biology >Monitoring of gene expression profiles and isolation of candidate genes involved in pollination and fertilization in rice (Oryza sativa L.) with a 10K cDNA microarray
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Monitoring of gene expression profiles and isolation of candidate genes involved in pollination and fertilization in rice (Oryza sativa L.) with a 10K cDNA microarray

机译:用10K cDNA微阵列监测水稻(Oryza sativa L.)的授粉和受精基因表达谱并分离候选基因

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To monitor gene expression profiles during pollination and fertilization in rice at a genome scale, we generated 73 424 high-quality expressed sequence tags ( ESTs) derived from the green/etiolated shoot and pistil (0-5 h after pollination, 5hP) of rice, which were subsequently used to construct a cDNA microarray containing ca. 10 000 unique rice genes. This microarray was used to analyze gene expression in pistil unpollinated (UP), 5hP and 5DAP(5 days after pollination), anther, shoot, root, 10-day-old embryo (10EM) and 10-day-old endosperm (10EN). Clustering analysis revealed that the anther has a gene-expression pro. le more similar to root than to pistil and most pistil-preferentially expressed genes respond to pollination and/or fertilization. There are 253 ESTs exhibiting differential expression (e +/- 2-fold changes) during pollination and fertilization, and about 70% of them can be assigned a putative function. We also recovered 20 genes similar to pollination-related and/or fertility-related genes previously identified as well as genes that were not implicated previously. Microarray and real-time PCR analyses showed that the array sensitivity was estimated at 1-5 copies of mRNA per cell, and the differentially expressed genes showed a high correlation between the two methods. Our results indicated that this cDNA microarray constructed here is reliable and can be used for monitoring gene expression profiles in rice. In addition, the genes that differentially expressed during pollination represent candidate genes for dissecting molecular mechanism of this important biological process in rice.
机译:为了在基因组规模上监测水稻授粉和受精过程中的基因表达谱,我们从水稻的绿色/离生芽和雌蕊(授粉后0-5小时,授粉5hP)产生了73 424个高质量表达序列标签(EST) ,随后用于构建含有ca.的cDNA微阵列。 10,000个独特的水稻基因。该微阵列用于分析未授粉雌蕊(UP),5hP和5DAP(授粉后5天),花药,枝条,根,10日龄胚(10EM)和10日龄胚乳(10EN)的基因表达。聚类分析表明该花药具有基因表达亲。与雌蕊相比,它更类似于根,并且多数雌蕊优先表达的基因对授粉和/或受精产生反应。有253个EST在授粉和受精过程中表现出差异表达(e +/- 2倍变化),其中约70%的EST被赋予推定功能。我们还回收了20个与先前鉴定的与授粉相关和/或与生育相关的基因相似的基因,以及先前未涉及的基因。微阵列和实时PCR分析表明,阵列敏感性估计为每个细胞1-5个mRNA,并且差异表达的基因显示出两种方法之间的高度相关性。我们的结果表明,此处构建的cDNA微阵列是可靠的,可用于监测水稻中的基因表达谱。另外,在授粉过程中差异表达的基因代表了解析水稻这一重要生物过程的分子机制的候选基因。

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