AI Article Synopsis

  • Complete deadenylation of polyA-tails in mRNAs is crucial for starting the decapping and degradation processes in cells.
  • Researchers conducted RNA sequencing in yeast and created a model estimating the rate of deadenylation, finding it to be about 10 adenines per minute.
  • The study revealed that while degradation rates of specific mRNAs, like ribosomal protein-coding mRNAs, increase under stress, these mRNAs can still degrade even if their deadenylation is inhibited, highlighting complex interactions between these processes.

Article Abstract

Complete cytoplasmic polyadenosine tail (polyA-tail) deadenylation is thought to be essential for initiating mRNA decapping and subsequent degradation. To investigate this prevalent model, we conducted direct RNA sequencing of S. cerevisiae mRNAs derived from chase experiments under steady-state and stress condition. Subsequently, we developed a numerical model based on a modified gamma distribution function, which estimated the transcriptomic deadenylation rate at 10 A/min. A simplified independent method, based on the delineation of quantile polyA-tail values, showed a correlation between the decay and deadenylation rates of individual mRNAs, which appeared consistent within functional transcript groups and associated with codon optimality. Notably, these rates varied during the stress response. Detailed analysis of ribosomal protein-coding mRNAs (RPG mRNAs), constituting 40% of the transcriptome, singled out this transcript group. While deadenylation and decay of RPG mRNAs accelerated under heat stress, their degradation could proceed even when deadenylation was blocked, depending entirely on ongoing nuclear export. Our findings support the general primary function of deadenylation in dictating the onset of decapping, while also demonstrating complex relations between these processes.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC11649921PMC
http://dx.doi.org/10.1038/s44318-024-00258-3DOI Listing

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