Literature DB >> 21324908

Bacterial toxin RelE mediates frequent codon-independent mRNA cleavage from the 5' end of coding regions in vivo.

Jennifer M Hurley1, Jonathan W Cruz, Ming Ouyang, Nancy A Woychik.   

Abstract

The enzymatic activity of the RelE bacterial toxin component of the Escherichia coli RelBE toxin-antitoxin system has been extensively studied in vitro and to a lesser extent in vivo. These earlier reports revealed that 1) RelE alone does not exhibit mRNA cleavage activity, 2) RelE mediates mRNA cleavage through its association with the ribosome, 3) RelE-mediated mRNA cleavage occurs at the ribosomal A site and, 4) Cleavage of mRNA by RelE exhibits high codon specificity. More specifically, RelE exhibits a preference for the stop codons UAG and UGA and sense codons CAG and UCG in vitro. In this study, we used a comprehensive primer extension approach to map the frequency and codon specificity of RelE cleavage activity in vivo. We found extensive cleavage at the beginning of the coding region of five transcripts, ompA, lpp, ompF, rpsA, and tufA. We then mapped RelE cleavage sites across one short transcript (lpp) and two long transcripts (ompF and ompA). RelE cut all of these transcripts frequently and efficiently within the first ∼100 codons, only occasionally cut beyond this point, and rarely cut at sites in proximity to the 3' end. Among 196 RelE sites in these five transcripts, there was no preference for CAG or UCG sense codons. In fact, bioinformatic analysis of the RelE cleavage sites failed to identify any sequence preferences. These results suggest a model of RelE function distinct from those proposed previously, because RelE directed frequent codon-independent mRNA cleavage coincident with the commencement of translation elongation.

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Year:  2011        PMID: 21324908      PMCID: PMC3083149          DOI: 10.1074/jbc.M110.108969

Source DB:  PubMed          Journal:  J Biol Chem        ISSN: 0021-9258            Impact factor:   5.157


  10 in total

1.  The bacterial toxin RelE displays codon-specific cleavage of mRNAs in the ribosomal A site.

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2.  Bacterial toxin YafQ is an endoribonuclease that associates with the ribosome and blocks translation elongation through sequence-specific and frame-dependent mRNA cleavage.

Authors:  Meredith H Prysak; Christopher J Mozdzierz; Angela M Cook; Ling Zhu; Yonglong Zhang; Masayori Inouye; Nancy A Woychik
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3.  The inhibitory mechanism of protein synthesis by YoeB, an Escherichia coli toxin.

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Journal:  J Biol Chem       Date:  2009-01-05       Impact factor: 5.157

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5.  Inhibitory mechanism of Escherichia coli RelE-RelB toxin-antitoxin module involves a helix displacement near an mRNA interferase active site.

Authors:  Guang-Yao Li; Yonglong Zhang; Masayori Inouye; Mitsuhiko Ikura
Journal:  J Biol Chem       Date:  2009-03-18       Impact factor: 5.157

6.  RelE toxins from bacteria and Archaea cleave mRNAs on translating ribosomes, which are rescued by tmRNA.

Authors:  Susanne K Christensen; Kenn Gerdes
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7.  Bacterial toxin HigB associates with ribosomes and mediates translation-dependent mRNA cleavage at A-rich sites.

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Authors:  Cajetan Neubauer; Yong-Gui Gao; Kasper R Andersen; Christine M Dunham; Ann C Kelley; Jendrik Hentschel; Kenn Gerdes; V Ramakrishnan; Ditlev E Brodersen
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  10 in total
  28 in total

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7.  Recommendations for bacterial ribosome profiling experiments based on bioinformatic evaluation of published data.

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8.  Structural and functional characterization of Escherichia coli toxin-antitoxin complex DinJ-YafQ.

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10.  Type II toxin/antitoxin MqsR/MqsA controls type V toxin/antitoxin GhoT/GhoS.

Authors:  Xiaoxue Wang; Dana M Lord; Seok Hoon Hong; Wolfgang Peti; Michael J Benedik; Rebecca Page; Thomas K Wood
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