| Literature DB >> 20627892 |
Tingting Lu1, Guojun Lu, Danlin Fan, Chuanrang Zhu, Wei Li, Qiang Zhao, Qi Feng, Yan Zhao, Yunli Guo, Wenjun Li, Xuehui Huang, Bin Han.
Abstract
The functional complexity of the rice transcriptome is not yet fully elucidated, despite many studies having reported the use of DNA microarrays. Next-generation DNA sequencing technologies provide a powerful approach for mapping and quantifying the transcriptome, termed RNA sequencing (RNA-seq). In this study, we applied RNA-seq to globally sample transcripts of the cultivated rice Oryza sativa indica and japonica subspecies for resolving the whole-genome transcription profiles. We identified 15,708 novel transcriptional active regions (nTARs), of which 51.7% have no homolog to public protein data and >63% are putative single-exon transcripts, which are highly different from protein-coding genes (<20%). We found that approximately 48% of rice genes show alternative splicing patterns, a percentage considerably higher than previous estimations. On the basis of the available rice gene models, 83.1% (46,472 genes) of the current rice gene models were validated by RNA-seq, and 6228 genes were identified to be extended at the 5' and/or 3' ends by at least 50 bp. Comparative transcriptome analysis demonstrated that 3464 genes exhibited differential expression patterns. The ratio of SNPs with nonsynonymous/synonymous mutations was nearly 1:1.06. In total, we interrogated and compared transcriptomes of the two rice subspecies to reveal the overall transcriptional landscape at maximal resolution.Entities:
Mesh:
Year: 2010 PMID: 20627892 PMCID: PMC2928502 DOI: 10.1101/gr.106120.110
Source DB: PubMed Journal: Genome Res ISSN: 1088-9051 Impact factor: 9.043