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Cloning and Characterization of a New Site-Specific Methyl-Directed ElmI Endonuclease Recognizing and Cleaving C5-methylated DNA Sequence 5’-G(5mC)^NG(5mC)-3’

Putative open reading frames of MD-endonucleases have been identified in Enterobacteria genomes as a result of the search for amino acid sequences homologous to MD-endonuclease BisI. A highly conserved DNA primary structure of these open reading frames in different genera of Enterobacteria (Escheric...

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Autores principales: Chernukhin, V. A., Gonchar, D. A., Abdurashitov, M. A., Belichenko, O. A., Dedkov, V. S., Mikhnenkova, N. A., Lomakovskaya, E. N., Udal’yeva, S. G., Degtyarev, S. Kh.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: A.I. Gordeyev 2016
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4837579/
https://www.ncbi.nlm.nih.gov/pubmed/27099792
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author Chernukhin, V. A.
Gonchar, D. A.
Abdurashitov, M. A.
Belichenko, O. A.
Dedkov, V. S.
Mikhnenkova, N. A.
Lomakovskaya, E. N.
Udal’yeva, S. G.
Degtyarev, S. Kh.
author_facet Chernukhin, V. A.
Gonchar, D. A.
Abdurashitov, M. A.
Belichenko, O. A.
Dedkov, V. S.
Mikhnenkova, N. A.
Lomakovskaya, E. N.
Udal’yeva, S. G.
Degtyarev, S. Kh.
author_sort Chernukhin, V. A.
collection PubMed
description Putative open reading frames of MD-endonucleases have been identified in Enterobacteria genomes as a result of the search for amino acid sequences homologous to MD-endonuclease BisI. A highly conserved DNA primary structure of these open reading frames in different genera of Enterobacteria (Escherichia, Klebsiella and Cronobacter) has allowed researchers to create primers for PCR screening, which was carried out on Enterobacteria DNA collected from natural sources. The DNA fragment, about 440 bp in length, was amplified by use of the genomic DNA of a wild E.coli LM N17 strain as a template and was inserted into the pMTL22 vector. Endonuclease activity was detected in an E.coli ER 2267 strain transformed with the obtained construction. A new enzyme named ElmI was purified by chromatographic techniques from the recombinant strain biomass. It was discovered that similarly to BisI this enzyme specifically cleaves the methylated DNA sequence 5’-GCNGC- 3’ before the central nucleotide “N” if this sequence contains two 5-methylcytosines. However, unlike BisI, ElmI more efficiently cleaves this sequence if more than two cytosine residues are methylated.
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spelling pubmed-48375792016-04-20 Cloning and Characterization of a New Site-Specific Methyl-Directed ElmI Endonuclease Recognizing and Cleaving C5-methylated DNA Sequence 5’-G(5mC)^NG(5mC)-3’ Chernukhin, V. A. Gonchar, D. A. Abdurashitov, M. A. Belichenko, O. A. Dedkov, V. S. Mikhnenkova, N. A. Lomakovskaya, E. N. Udal’yeva, S. G. Degtyarev, S. Kh. Acta Naturae Research Article Putative open reading frames of MD-endonucleases have been identified in Enterobacteria genomes as a result of the search for amino acid sequences homologous to MD-endonuclease BisI. A highly conserved DNA primary structure of these open reading frames in different genera of Enterobacteria (Escherichia, Klebsiella and Cronobacter) has allowed researchers to create primers for PCR screening, which was carried out on Enterobacteria DNA collected from natural sources. The DNA fragment, about 440 bp in length, was amplified by use of the genomic DNA of a wild E.coli LM N17 strain as a template and was inserted into the pMTL22 vector. Endonuclease activity was detected in an E.coli ER 2267 strain transformed with the obtained construction. A new enzyme named ElmI was purified by chromatographic techniques from the recombinant strain biomass. It was discovered that similarly to BisI this enzyme specifically cleaves the methylated DNA sequence 5’-GCNGC- 3’ before the central nucleotide “N” if this sequence contains two 5-methylcytosines. However, unlike BisI, ElmI more efficiently cleaves this sequence if more than two cytosine residues are methylated. A.I. Gordeyev 2016 /pmc/articles/PMC4837579/ /pubmed/27099792 Text en Copyright ® 2016 Park-media Ltd. http://creativecommons.org/licenses/by/2.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Research Article
Chernukhin, V. A.
Gonchar, D. A.
Abdurashitov, M. A.
Belichenko, O. A.
Dedkov, V. S.
Mikhnenkova, N. A.
Lomakovskaya, E. N.
Udal’yeva, S. G.
Degtyarev, S. Kh.
Cloning and Characterization of a New Site-Specific Methyl-Directed ElmI Endonuclease Recognizing and Cleaving C5-methylated DNA Sequence 5’-G(5mC)^NG(5mC)-3’
title Cloning and Characterization of a New Site-Specific Methyl-Directed ElmI Endonuclease Recognizing and Cleaving C5-methylated DNA Sequence 5’-G(5mC)^NG(5mC)-3’
title_full Cloning and Characterization of a New Site-Specific Methyl-Directed ElmI Endonuclease Recognizing and Cleaving C5-methylated DNA Sequence 5’-G(5mC)^NG(5mC)-3’
title_fullStr Cloning and Characterization of a New Site-Specific Methyl-Directed ElmI Endonuclease Recognizing and Cleaving C5-methylated DNA Sequence 5’-G(5mC)^NG(5mC)-3’
title_full_unstemmed Cloning and Characterization of a New Site-Specific Methyl-Directed ElmI Endonuclease Recognizing and Cleaving C5-methylated DNA Sequence 5’-G(5mC)^NG(5mC)-3’
title_short Cloning and Characterization of a New Site-Specific Methyl-Directed ElmI Endonuclease Recognizing and Cleaving C5-methylated DNA Sequence 5’-G(5mC)^NG(5mC)-3’
title_sort cloning and characterization of a new site-specific methyl-directed elmi endonuclease recognizing and cleaving c5-methylated dna sequence 5’-g(5mc)^ng(5mc)-3’
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4837579/
https://www.ncbi.nlm.nih.gov/pubmed/27099792
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