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Identification of stop codon readthrough genes in Saccharomyces cerevisiae.


ABSTRACT: We specifically sought genes within the yeast genome controlled by a non-conventional translation mechanism involving the stop codon. For this reason, we designed a computer program using the yeast database genomic regions, and seeking two adjacent open reading frames separated only by a unique stop codon (called SORFs). Among the 58 SORFs identified, eight displayed a stop codon bypass level ranging from 3 to 25%. For each of the eight sequences, we demonstrated the presence of a poly(A) mRNA. Using isogenic [PSI(+)] and [psi(-)] yeast strains, we showed that for two of the sequences the mechanism used is a bona fide readthrough. However, the six remaining sequences were not sensitive to the PSI state, indicating either a translation termination process independent of eRF3 or a new stop codon bypass mechanism. Our results demonstrate that the presence of a stop codon in a large ORF may not always correspond to a sequencing error, or a pseudogene, but can be a recoding signal in a functional gene. This emphasizes that genome annotation should take into account the fact that recoding signals could be more frequently used than previously expected.

SUBMITTER: Namy O 

PROVIDER: S-EPMC154216 | biostudies-literature | 2003 May

REPOSITORIES: biostudies-literature

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Identification of stop codon readthrough genes in Saccharomyces cerevisiae.

Namy Olivier O   Duchateau-Nguyen Guillemette G   Hatin Isabelle I   Hermann-Le Denmat Sylvie S   Termier Michel M   Rousset Jean-Pierre JP  

Nucleic acids research 20030501 9


We specifically sought genes within the yeast genome controlled by a non-conventional translation mechanism involving the stop codon. For this reason, we designed a computer program using the yeast database genomic regions, and seeking two adjacent open reading frames separated only by a unique stop codon (called SORFs). Among the 58 SORFs identified, eight displayed a stop codon bypass level ranging from 3 to 25%. For each of the eight sequences, we demonstrated the presence of a poly(A) mRNA.  ...[more]

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