Gene Identification and Expression Analysis of 86,136 Expressed Sequence Tags(EST)from the Rice Genome 被引量：4

Gene Identification and Expression Analysis of 86,136 Expressed Sequence Tags (EST) from the Rice Genome

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摘要 Expressed Sequence Tag (EST) analysis has pioneered genome-wide gene discovery and expression profiling. In order to establish a gene expression index in the rice cultivar indica, we sequenced and analyzed 86,136 ESTs from nine rice cDNA libraries from the super hybrid cultivar LYP9 and its parental cultivars. We assembled these ESTs into 13,232 contigs and leave 8,976 singletons. Overall, 7,497 sequences were found similar to the existing sequences in GenBank and 14,711 are novel. These sequences are classified by molecular function, biological process and pathways according to the Gene Ontology. We compared our sequenced ESTs with the publicly available 95,000 ESTs from japonica, and found little sequence variation, despite the large difference between genome sequences. We then assembled the combined 173,000 rice ESTs for further analysis. Using the pooled ESTs, we compared gene expression in metabolism pathway between rice and Arabidopsis according to KEGG. We further profiled gene expression patterns in different tissues, developmental stages, and in a conditional sterile mutant, after checking the libraries are comparable by means of sequence coverage. We also identified some possible library specific genes and a number of enzymes and transcription factors that contribute to rice development. Expressed Sequence Tag (EST) analysis has pioneered genome-wide gene discovery and expression profiling. In order to establish a gene expression index in the rice cultivar indica, we sequenced and analyzed 86,136 ESTs from nine rice cDNA libraries from the super hybrid cultivar LYP9 and its parental cultivars. We assembled these ESTs into 13,232 contigs and leave 8,976 singletons. Overall, 7,497 sequences were found similar to the existing sequences in GenBank and 14,711 are novel. These sequences are classified by molecular function, biological process and pathways according to the Gene Ontology. We compared our sequenced ESTs with the publicly available 95,000 ESTs from japonica, and found little sequence variation, despite the large difference between genome sequences. We then assembled the combined 173,000 rice ESTs for further analysis. Using the pooled ESTs, we compared gene expression in metabolism pathway between rice and Arabidopsis according to KEGG. We further profiled gene expression patterns in different tissues, developmental stages, and in a conditional sterile mutant, after checking the libraries are comparable by means of sequence coverage. We also identified some possible library specific genes and a number of enzymes and transcription factors that contribute to rice development.

机构地区 HangzhouGenomicsInstitute/InstituteofBioinformaticsofZhejiangUniversity/KeyLaboratoryofBioinformaticsofZhejiangProvince BeijingGenomicsInstitute/CenterofGenomics&Bioinformatics StanfordUniversity CollegeofLifeSciences NexusGenomics

出处《Genomics, Proteomics & Bioinformatics》 SCIE CAS CSCD 2003年第1期26-42,共17页 基因组蛋白质组与生物信息学报（英文版）

关键词 EST expression profile EST, expression profile

分类号 S511 [农业科学—作物学] Q949.714.2 [生物学—植物学]

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Gene Identification and Expression Analysis of 86,136 Expressed Sequence Tags(EST)from the Rice Genome 被引量：4

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