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Transgene-induced CCWGG methylation does not alter CG methylation patterning in human kidney cells

Several reports suggest that C(m)CWGG methylation tends not to co-exist with (m)CG methylation in human cells. We have asked whether or not methylation at CCWGG sites can influence CG methylation. DNA from cells expressing an M.EcoRII–GFP fusion was actively methylated at CCWGG sites. CG methylation...

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Autores principales: Shevchuk, Taras, Kretzner, Leo, Munson, Kristofer, Axume, John, Clark, Jarrod, Dyachenko, Olga V., Caudill, Marie, Buryanov, Yaroslav, Smith, Steven S.
Formato: Texto
Lenguaje:English
Publicado: Oxford University Press 2005
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC1266073/
https://www.ncbi.nlm.nih.gov/pubmed/16246913
http://dx.doi.org/10.1093/nar/gki920
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author Shevchuk, Taras
Kretzner, Leo
Munson, Kristofer
Axume, John
Clark, Jarrod
Dyachenko, Olga V.
Caudill, Marie
Buryanov, Yaroslav
Smith, Steven S.
author_facet Shevchuk, Taras
Kretzner, Leo
Munson, Kristofer
Axume, John
Clark, Jarrod
Dyachenko, Olga V.
Caudill, Marie
Buryanov, Yaroslav
Smith, Steven S.
author_sort Shevchuk, Taras
collection PubMed
description Several reports suggest that C(m)CWGG methylation tends not to co-exist with (m)CG methylation in human cells. We have asked whether or not methylation at CCWGG sites can influence CG methylation. DNA from cells expressing an M.EcoRII–GFP fusion was actively methylated at CCWGG sites. CG methylation as measured by R.HpaII/R.MspI ratios was unchanged in cells expressing the transgene. Cloned representatives of C(m)CWGG methylated DNA often contained, or were adjacent to an ALU repeat, suggesting that M.EcoRII-GFP actively methylated gene-rich R-band DNA. The transgenic methyltransferase applied C(m)CWGG methylation to a representative human promoter that was heavily methylated at CG dinucleotides (the SERPINB5 promoter) and to a representative promoter that was essentially unmethylated at CG dinucleotides (the APC promoter). In each case, the CG methylation pattern remained in its original state, unchanged by the presence of neighboring C(m)CWGG sites. Q-PCR measurements showed that RNA expression from the APC gene was not significantly altered by the presence of C(m)CWGG in its promoter. Kinetic studies suggested that an adjacent C(m)CWGG methylation site influences neither the maintenance nor the de novo methylation activities of purified human Dnmt1. We conclude that C(m)CWGG methylation does not exert a significant effect on CG methylation in human kidney cells.
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spelling pubmed-12660732005-10-26 Transgene-induced CCWGG methylation does not alter CG methylation patterning in human kidney cells Shevchuk, Taras Kretzner, Leo Munson, Kristofer Axume, John Clark, Jarrod Dyachenko, Olga V. Caudill, Marie Buryanov, Yaroslav Smith, Steven S. Nucleic Acids Res Article Several reports suggest that C(m)CWGG methylation tends not to co-exist with (m)CG methylation in human cells. We have asked whether or not methylation at CCWGG sites can influence CG methylation. DNA from cells expressing an M.EcoRII–GFP fusion was actively methylated at CCWGG sites. CG methylation as measured by R.HpaII/R.MspI ratios was unchanged in cells expressing the transgene. Cloned representatives of C(m)CWGG methylated DNA often contained, or were adjacent to an ALU repeat, suggesting that M.EcoRII-GFP actively methylated gene-rich R-band DNA. The transgenic methyltransferase applied C(m)CWGG methylation to a representative human promoter that was heavily methylated at CG dinucleotides (the SERPINB5 promoter) and to a representative promoter that was essentially unmethylated at CG dinucleotides (the APC promoter). In each case, the CG methylation pattern remained in its original state, unchanged by the presence of neighboring C(m)CWGG sites. Q-PCR measurements showed that RNA expression from the APC gene was not significantly altered by the presence of C(m)CWGG in its promoter. Kinetic studies suggested that an adjacent C(m)CWGG methylation site influences neither the maintenance nor the de novo methylation activities of purified human Dnmt1. We conclude that C(m)CWGG methylation does not exert a significant effect on CG methylation in human kidney cells. Oxford University Press 2005 2005-10-24 /pmc/articles/PMC1266073/ /pubmed/16246913 http://dx.doi.org/10.1093/nar/gki920 Text en © The Author 2005. Published by Oxford University Press. All rights reserved
spellingShingle Article
Shevchuk, Taras
Kretzner, Leo
Munson, Kristofer
Axume, John
Clark, Jarrod
Dyachenko, Olga V.
Caudill, Marie
Buryanov, Yaroslav
Smith, Steven S.
Transgene-induced CCWGG methylation does not alter CG methylation patterning in human kidney cells
title Transgene-induced CCWGG methylation does not alter CG methylation patterning in human kidney cells
title_full Transgene-induced CCWGG methylation does not alter CG methylation patterning in human kidney cells
title_fullStr Transgene-induced CCWGG methylation does not alter CG methylation patterning in human kidney cells
title_full_unstemmed Transgene-induced CCWGG methylation does not alter CG methylation patterning in human kidney cells
title_short Transgene-induced CCWGG methylation does not alter CG methylation patterning in human kidney cells
title_sort transgene-induced ccwgg methylation does not alter cg methylation patterning in human kidney cells
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC1266073/
https://www.ncbi.nlm.nih.gov/pubmed/16246913
http://dx.doi.org/10.1093/nar/gki920
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