Abstract
YoeB is a toxin encoded by the yefM-yoeB antitoxin-toxin operon in the Escherichia coli genome. Here we show that YoeB, a highly potent protein synthesis inhibitor, specifically blocks translation initiation. In in vivo primer extension experiments using two different mRNAs, a major band was detected after YoeB induction at three bases downstream of the initiation codon at 2.5 min. An identical band was also detected in in vitro toeprinting experiments after the addition of YoeB to the reaction mixtures containing 70 S ribosomes and the same mRNAs, even in the absence of tRNA(f)(Met). Notably, this band was not detected in the presence of YoeB alone, indicating that YoeB by itself does not have endoribonuclease activity under the conditions used. The 70 S ribosomes increased upon YoeB induction, and YoeB was found to be specifically associated with 50 S subunits. Using tetracycline and hygromycin B, we demonstrated that YoeB binds to the 50 S ribosomal subunit in 70 S ribosomes and interacts with the A site leading to mRNA cleavage at this site. As a result, the 3'-end portion of the mRNA was released from ribosomes, and translation initiation was effectively inhibited. These results demonstrate that YoeB primarily inhibits translation initiation.
Highlights
When YoeB forms a complex with 70 S ribosomes and mRNA in vitro, partial cleavage of mRNAs is observed at positions three and four bases downstream of the initiation codon as observed in in vivo experiments
Using tetracycline and hygromycin B, we demonstrated that YoeB binds to the 50 S ribosomal subunit in 70 S ribosomes and interacts with the A site leading to mRNA cleavage at this site
These results indicate that the binding of 70 S ribosomes to the mRNA is absolutely required for the YoeB-mediated cleavage of mRNAs. tRNAfMet Is not Required for YoeB-Mediated A Site Cleavage— we examined if the initiator tRNAfMet is required for YoeB-mediated mRNA cleavage in the presence of YoeB
Summary
Strains and Plasmids—E. coli BL21(DE3), BW25113 (⌬araBAD) (8), and MRE600 (9) were used. For in vivo primer extension, the lpp and ompA mRNAs were prepared from E. coli BW25113 cells containing pBADYoeB at various time points as indicated in C and D before and after the induction of YoeB. Primer Extension Analysis in Vivo—For primer extension analysis of mRNA cleavage sites in vivo, total RNAs were extracted from the E. coli BW25113 cells containing pBADYoeB at different time points as indicated, C and D. At 37 °C for 10 min, and reverse transcriptase (2 units) was mRNA produced from this DNA fragment was 151 bases in length
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