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Article Dans Une Revue Biochemical Journal Année : 2006

Direct comparison of nick-joining activity of the nucleic acid ligases from bacteriophage T4

Desmond R. Bullard
  • Fonction : Auteur

Résumé

The genome of bacteriophage T4 encodes three polynucleotide ligases, which seal the backbone of nucleic acids during infection of host bacteria. The DNA ligase (T4Dnl) and two RNA ligases (T4Rnl1 and T4Rnl2) join a diverse array of substrates, including nicks that are present in double-stranded nucleic acids, albeit with different efficiencies. To unravel the biochemical and functional relationship between these proteins, a systematic analysis of their substrate specificity was performed using recombinant proteins. The ability of each protein to ligate 20 base-pair double-stranded oligonucleotides containing a single-strand break was determined. Between 4 and 37 °C, all proteins ligated substrates containing various combinations of DNA and RNA. The RNA ligases ligated a more diverse set of substrates than T4Dnl and, generally, T4Rnl1 had 50-1,000-fold lower activity than T4Rnl2. In assays using identical conditions, optimal ligation of all substrates was at pH 8 for T4Dnl and T4Rnl1 and pH 7 for T4Rnl2, demonstrating that the protein dictates the pH optimum for ligation. All proteins ligated a substrate containing DNA as the unbroken strand, with the nucleotides at the nick of the broken strand being RNA at the 3‘-hydroxyl and DNA at the 5‘-phosphate. Since this RNA:DNA hybrid was joined at a similar maximal rate by T4Dnl and T4Rnl2 at 37 °C, we consider the possibility that this could be an unexpected physiological substrate used during some pathways of "DNA repair".

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Dates et versions

hal-00478543 , version 1 (30-04-2010)

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Desmond R. Bullard, Richard P. Bowater. Direct comparison of nick-joining activity of the nucleic acid ligases from bacteriophage T4. Biochemical Journal, 2006, 398 (1), pp.135-144. ⟨10.1042/BJ20060313⟩. ⟨hal-00478543⟩

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