Abstract
Heterogeneity of the main ribosomal composition represents an emerging, yet debatable, mechanism of gene expression regulation with a purported role in ribosomopathies, a group of disorders caused by mutations in ribosomal protein genes (RPs). Ribosomopathies, mysteriously relate with tissue-specific symptoms (mainly anemia and cancer predisposition), despite the ubiquitous expression and necessity of the associated RPs. An outstanding question that may shed light into disease pathogenicity and provide potential pharmacological interventions, is whether and how the ribosomal composition is modified during, the highly affected by RP mutations, process of erythroid differentiation. To address this issue, we analyzed ribosome stoichiometry using an established model of erythroid differentiation, through sucrose gradient ultracentrifugation and quantitative proteomics. We found that differentiation associates with an extensive reprogramming of the overall ribosomal levels, characterized by an increase in monosomes and a decrease in polysomes. However, by calculating a stoichiometry score for each independent ribosomal protein, we found that the main ribosomal architecture remained invariable between immature and differentiated cells. In total, none of the 78 Ribosomal Proteins (RPs- 74 core RPs, Rack1, Fau and 2 paralogs) detected was statistically different between the samples. This data was further verified through antibody-mediated quantification of 6 representative RPs. Moreover, bioinformatic analysis of whole cell proteomic data derived out of 4 additional models of erythropoiesis revealed that RPs were co-regulated across these cell types, too. In conclusion, ribosomes maintain an invariant protein stoichiometry during differentiation, thus excluding ribosome heterogeneity from a potential mechanism of toxicity in ribosomopathies and other erythroid disorders.
Highlights
Ribosomes constitute the main macromolecular machines that catalyze protein synthesis within the cells of all domains of life
To elucidate ribosome composition and regulation during erythroid differentiation we performed a detailed examination of the ribosomal population in MEL cells, along with a whole cell data analysis derived from 4 additional models of differentiation
Our data strongly supports that, while the Erythro-Riboproteomics ribosome population is re-organized the main ribosomal composition remains unaltered during differentiation
Summary
Ribosomes constitute the main macromolecular machines that catalyze protein synthesis within the cells of all domains of life. The small subunit is responsible for the recognition and binding of ribosomes to cytosolic mRNAs, while the large subunit catalyzes peptide bond formation. This core ribosomal structure is highly conserved across bacteria, archaea, and eukaryotes (Bowman et al, 2020). It has been proposed that some ribosomal subgroups may demonstrate alterations that differentiate them from the typical ribosomal machinery This kind of ribosome heterogeneity may arise through quantitative alterations of one or more RPs that disrupt the equimolar (1:1) ratio between the RPs in each ribosomal entity (Sauert et al, 2015; Guimaraes and Zavolan, 2016; Genuth and Barna, 2018; Sulima and Dinman, 2019; Li and Wang, 2020). Heterogeneous ribosomes may show increased affinity for selected 5-untraslated regions in transcripts and be specialized to preferentially translate distinct mRNA subgroups (Xue and Barna, 2012)
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