AI Article Synopsis

  • Promoters are key transcriptional regulatory sequences located upstream of gene start sites, but identifying all human transcription start sites and their functional elements remains incomplete.
  • A study examined 74 promoters related to inflammatory bowel disease using a transfected-cell array in HEK293T cells, revealing that 21.6% were active.
  • The study found that 75% of these active promoters corresponded with their gene's transcriptional activity, highlighting the importance of promoter activity in gene expression regulation and showcasing a novel large-scale approach to studying regulatory sequences.

Article Abstract

Promoters are the best characterized transcriptional regulatory sequences in complex genomes because of their predictable location immediately upstream of transcription start sites. Despite a substantial body of literature describing transcriptional promoters, the identification of true start sites for all human transcripts is far from complete. The same is true of the key structural and functional elements responsible for promoter action in different cell types. In order to identify elements responsible for promoter activity, we applied transfected-cell array technology to functionally evaluate promoters for genes involved in inflammatory bowel disease. Seventy-four promoters were examined by reverse transfection of a promoter-fluorescent reporter constructs into a human embryonic kidney cell line (HEK293T). Sixteen (21.6%) promoters were found to be active in HEK293 T cells. Correlations between promoter activity and endogenous transcript level were calculated, and 75% of active promoters were found to be associated with transcriptional activity of their gene counterparts. These results provide experimental evidence of promoter activity, which may aid in understanding the regulation of gene expression. Moreover, this is the first large-scale functional study of regulatory sequences to use a high-throughput transfected-cell array technique.

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Source
http://dx.doi.org/10.1016/j.gene.2009.10.003DOI Listing

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