par Yang, Jun 
;Sharma, Sunny ;Watzinger, Peter;Hartmann, Johannes David;Kötter, Peter;Entian, Karl-Dieter
Référence PloS one, 12, 3, e0173940
Publication Publié, 2017-03
;Sharma, Sunny ;Watzinger, Peter;Hartmann, Johannes David;Kötter, Peter;Entian, Karl-DieterRéférence PloS one, 12, 3, e0173940
Publication Publié, 2017-03
Article révisé par les pairs
| Résumé : | Ribosomes are large ribonucleoprotein complexes that are fundamental for protein synthesis. Ribosomes are ribozymes because their catalytic functions such as peptidyl transferase and peptidyl-tRNA hydrolysis depend on the rRNA. rRNA is a heterogeneous biopolymer comprising of at least 112 chemically modified residues that are believed to expand its topological potential. In the present study, we established a comprehensive modification profile of Saccharomyces cerevisiae's 18S and 25S rRNA using a high resolution Reversed-Phase High Performance Liquid Chromatography (RP-HPLC). A combination of mung bean nuclease assay, rDNA point mutants and snoRNA deletions allowed us to systematically map all ribose and base modifications on both rRNAs to a single nucleotide resolution. We also calculated approximate molar levels for each modification using their UV (254nm) molar response factors, showing sub-stoichiometric amount of modifications at certain residues. The chemical nature, their precise location and identification of partial modification will facilitate understanding the precise role of these chemical modifications, and provide further evidence for ribosome heterogeneity in eukaryotes. |
