Boron‐dependent regulation of translation through AUGUAA sequence in yeast

Under high boron (B) conditions, nodulin 26‐like intrinsic protein 5;1 (NIP5;1) mRNA, a boric acid channel, is destabilized to avoid excess B entry into roots of Arabidopsis thaliana. In this regulation, the minimum upstream open reading frame (uORF), AUGUAA, in its 5′‐untranslated region (5′‐UTR) i...

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Published inYeast (Chichester, England) Vol. 37; no. 12; pp. 638 - 646
Main Authors Tsednee, Munkhtsetseg, Tanaka, Mayuki, Kasai, Koji, Fujiwara, Toru
Format Journal Article
LanguageEnglish
Published England Wiley Subscription Services, Inc 01.12.2020
Subjects
5' Untranslated Regions
animals
Arabidopsis thaliana
AUGUAA
Biodegradation
Boric acid
Boron
eukaryotic cells
evolution
gene expression
mRNA
NIP5;1
Open reading frames
Reporter gene
reporter genes
ribosomes
Saccharomyces cerevisiae
Translation
translational regulation
Yeast
yeasts
AUGUAA
translational regulation
NIP5;1
Saccharomyces cerevisiae
boron
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ISSN0749-503X
1097-0061
1097-0061
DOI10.1002/yea.3526

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Summary:Under high boron (B) conditions, nodulin 26‐like intrinsic protein 5;1 (NIP5;1) mRNA, a boric acid channel, is destabilized to avoid excess B entry into roots of Arabidopsis thaliana. In this regulation, the minimum upstream open reading frame (uORF), AUGUAA, in its 5′‐untranslated region (5′‐UTR) is essential, and high B enhances ribosome stalling at AUGUAA and leads to suppression of translation and mRNA degradation. This B‐dependent AUGUAA‐mediated regulation occurs also in animal transient expression and reticulocyte lysate translation systems. Thus, uncovering the ubiquitousness of B‐dependent unique regulation is important to reveal the evolution of translational regulation. In the present study, we examined the regulation in Saccharomyces cerevisiae. Reporter assay showed that in yeast, carrying ATGTAA in 5′‐UTR of NIP5;1 upstream of the reporter gene, the relative reporter activities were reduced significantly under high B conditions compared with control, whereas deletion of ATGTAA abolished such responses. This suggests that AUGUAA mediates B‐dependent regulation of translation in Saccharomyces cerevisiae. Moreover, the deletion of ATGTAA resulted in up to 10‐fold increase in general reporter activities indicating the suppression effect of AUGUAA on translation of the main ORF. Interestingly, mRNA level of the reporter gene was not affected by B in both yeast cells with and without AUGUAA. This finding reveals that in yeast, unlike the case in plants, mRNA degradation is not associated with AUGUAA regulation. Together, results suggest that B‐dependent AUGUAA‐mediated translational regulation is common among eukaryotes.
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ISSN:0749-503X
1097-0061
1097-0061
DOI:10.1002/yea.3526