Please use this identifier to cite or link to this item: http://hdl.handle.net/2122/15526
Authors: De Lise, Federica* 
Iacono, Roberta* 
Strazzulli, Andrea* 
Giglio, Rosa* 
Curci, Nicola* 
Maurelli, Luisa* 
Avino, Rosario* 
Carandente, Antonio* 
Caliro, Stefano* 
Tortora, Alessandra* 
Lorenzini, Fabio* 
Di Donato, Paola* 
Moracci, Marco* 
Cobucci-Ponzano, Beatrice* 
Title: Transcript Regulation of the Recoded Archaeal α-l-Fucosidase In Vivo
Journal: Molecules 
Series/Report no.: /26 (2021)
Publisher: MDPI
Issue Date: 25-Mar-2021
DOI: 10.3390/molecules26071861
Keywords: Archaea; extremophiles; limits of life; programmed frameshifting; recoding
Subject Classification03.04. Chemical and biological 
Abstract: Genetic decoding is flexible, due to programmed deviation of the ribosomes from standard translational rules, globally termed "recoding". In Archaea, recoding has been unequivocally determined only for termination codon readthrough events that regulate the incorporation of the unusual amino acids selenocysteine and pyrrolysine, and for -1 programmed frameshifting that allow the expression of a fully functional α-l-fucosidase in the crenarchaeon Saccharolobus solfataricus, in which several functional interrupted genes have been identified. Increasing evidence suggests that the flexibility of the genetic code decoding could provide an evolutionary advantage in extreme conditions, therefore, the identification and study of interrupted genes in extremophilic Archaea could be important from an astrobiological point of view, providing new information on the origin and evolution of the genetic code and on the limits of life on Earth. In order to shed some light on the mechanism of programmed -1 frameshifting in Archaea, here we report, for the first time, on the analysis of the transcription of this recoded archaeal α-l-fucosidase and of its full-length mutant in different growth conditions in vivo. We found that only the wild type mRNA significantly increased in S. solfataricus after cold shock and in cells grown in minimal medium containing hydrolyzed xyloglucan as carbon source. Our results indicated that the increased level of fucA mRNA cannot be explained by transcript up-regulation alone. A different mechanism related to translation efficiency is discussed.
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