Startseite Differential methylation kinetics of individual target site strands by T4Dam DNA methyltransferase
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Differential methylation kinetics of individual target site strands by T4Dam DNA methyltransferase

  • Victor V. Zinoviev , Alexey A. Evdokimov , Ernst G. Malygin , Bianca Sclavi , Malcolm Buckle und Stanley Hattman
Veröffentlicht/Copyright: 2. November 2007
Biological Chemistry
Aus der Zeitschrift Band 388 Heft 11

Abstract

Prokaryote DNA methyltransferases (MTases) of the Dam family (including those of bacteriophages T2 and T4) catalyze methyl group transfer from S-adenosyl-L-methionine (AdoMet), producing S-adenosyl-L-homocysteine (AdoHcy) and methylated adenine residues in palindromic GATC sequences. Dam DNA MTases, as all site-specific enzymes interacting with polymeric DNA, require a mechanism of action that ensures a rapid search for specific targets for catalytic action, during both the initial and subsequent rounds of methylation. The results of pre-steady-state (reaction burst) and steady-state methylation analyses of individual targets permitted us to monitor the action of T4Dam, which has three degrees of freedom: sliding, reorientation and adaptation to the canonical GATC sequence. The salient results are as follows: (i) 40mer substrate duplexes containing two canonical GATC sites showed differential methylation of the potential targets, i.e., T4Dam exhibited a preference for one site/target, which may present the better ‘kinetic trap’ for the enzyme. (ii) Prior hemimethylation of the two sites made both targets equally capable of being methylated during the pre-steady-state reaction. (iii) Although capable of moving in either direction along double-stranded DNA, there are some restrictions on T4Dam reorientation/adaptation on 40mer duplexes.

Keywords: hemimethylation; pre-steady-state methylation; reaction burst; S-adenosyl-L-homocysteine; S-adenosyl-L-methionine
Corresponding author
Received: 2007-5-11
Accepted: 2007-7-7
Published Online: 2007-11-02
Published in Print: 2007-11-01

©2007 by Walter de Gruyter Berlin New York

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  3. Cysteine cathepsin non-inhibitory binding partners: modulating intracellular trafficking and function
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https://doi.org/10.1515/BC.2007.142
Schlagwörter für diesen Artikel
hemimethylation; pre-steady-state methylation; reaction burst; S-adenosyl-L-homocysteine; S-adenosyl-L-methionine

Artikel in diesem Heft

  1. Proteinase Inhibitors and Biological Control – An Attractive International Symposia Series
  2. Two decades of thyroglobulin type-1 domain research
  3. Cysteine cathepsin non-inhibitory binding partners: modulating intracellular trafficking and function
  4. Cysteine proteases: destruction ability versus immunomodulation capacity in immune cells
  5. ‘Species’ of peptidases
  6. Protease research in the era of systems biology
  7. Human and mouse homo-oligomeric meprin A metalloendopeptidase: substrate and inhibitor specificities
  8. Association of cathepsin E with tumor growth arrest through angiogenesis inhibition and enhanced immune responses
  9. Characterization and comparative 3D modeling of CmPI-II, a novel ‘non-classical’ Kazal-type inhibitor from the marine snail Cenchritis muricatus (Mollusca)
  10. Cellular localization of MAGI-1 caspase cleavage products and their role in apoptosis
  11. Differential methylation kinetics of individual target site strands by T4Dam DNA methyltransferase
  12. Characterisation of zinc-binding domains of peroxisomal RING finger proteins using size exclusion chromatography/inductively coupled plasma-mass spectrometry
  13. Defining the extended substrate specificity of kallikrein 1-related peptidases
  14. Latent MMP-9 is bound to TIMP-1 before secretion
  15. Novel expression of kallikreins, kallikrein-related peptidases and kinin receptors in human pleural mesothelioma
  16. Activity of ulilysin, an archaeal PAPP-A-related gelatinase and IGFBP protease
  17. Clinical chemistry reference database for Wistar rats and C57/BL6 mice
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