What influences DNA replication rate in budding yeast?

BACKGROUND: DNA replication begins at specific locations called replication origins, where helicase and polymerase act in concert to unwind and process the single DNA filaments. The sites of active DNA synthesis are called replication forks. The density of initiation events is low when replication f...

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Main Authors: Thomas W Spiesser, Christian Diener, Matteo Barberis, Edda Klipp
Format: Article
Language:English
Published: Public Library of Science (PLoS) 2010-01-01
Series:PLoS ONE
Online Access:http://europepmc.org/articles/PMC2860512?pdf=render
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spelling doaj-a8cdcd13b5254194825957662d9e76592020-11-25T01:46:01ZengPublic Library of Science (PLoS)PLoS ONE1932-62032010-01-0154e1020310.1371/journal.pone.0010203What influences DNA replication rate in budding yeast?Thomas W SpiesserChristian DienerMatteo BarberisEdda KlippBACKGROUND: DNA replication begins at specific locations called replication origins, where helicase and polymerase act in concert to unwind and process the single DNA filaments. The sites of active DNA synthesis are called replication forks. The density of initiation events is low when replication forks travel fast, and is high when forks travel slowly. Despite the potential involvement of epigenetic factors, transcriptional regulation and nucleotide availability, the causes of differences in replication times during DNA synthesis have not been established satisfactorily, yet. METHODOLOGY/PRINCIPAL FINDINGS: Here, we aimed at quantifying to which extent sequence properties contribute to the DNA replication time in budding yeast. We interpreted the movement of the replication machinery along the DNA template as a directed random walk, decomposing influences on DNA replication time into sequence-specific and sequence-independent components. We found that for a large part of the genome the elongation time can be well described by a global average replication rate, thus by a single parameter. However, we also showed that there are regions within the genomic landscape of budding yeast with highly specific replication rates, which cannot be explained by global properties of the replication machinery. CONCLUSION/SIGNIFICANCE: Computational models of DNA replication in budding yeast that can predict replication dynamics have rarely been developed yet. We show here that even beyond the level of initiation there are effects governing the replication time that can not be explained by the movement of the polymerase along the DNA template alone. This allows us to characterize genomic regions with significantly altered elongation characteristics, independent of initiation times or sequence composition.http://europepmc.org/articles/PMC2860512?pdf=render
collection DOAJ
language English
format Article
sources DOAJ
author Thomas W Spiesser
Christian Diener
Matteo Barberis
Edda Klipp
spellingShingle Thomas W Spiesser
Christian Diener
Matteo Barberis
Edda Klipp
What influences DNA replication rate in budding yeast?
PLoS ONE
author_facet Thomas W Spiesser
Christian Diener
Matteo Barberis
Edda Klipp
author_sort Thomas W Spiesser
title What influences DNA replication rate in budding yeast?
title_short What influences DNA replication rate in budding yeast?
title_full What influences DNA replication rate in budding yeast?
title_fullStr What influences DNA replication rate in budding yeast?
title_full_unstemmed What influences DNA replication rate in budding yeast?
title_sort what influences dna replication rate in budding yeast?
publisher Public Library of Science (PLoS)
series PLoS ONE
issn 1932-6203
publishDate 2010-01-01
description BACKGROUND: DNA replication begins at specific locations called replication origins, where helicase and polymerase act in concert to unwind and process the single DNA filaments. The sites of active DNA synthesis are called replication forks. The density of initiation events is low when replication forks travel fast, and is high when forks travel slowly. Despite the potential involvement of epigenetic factors, transcriptional regulation and nucleotide availability, the causes of differences in replication times during DNA synthesis have not been established satisfactorily, yet. METHODOLOGY/PRINCIPAL FINDINGS: Here, we aimed at quantifying to which extent sequence properties contribute to the DNA replication time in budding yeast. We interpreted the movement of the replication machinery along the DNA template as a directed random walk, decomposing influences on DNA replication time into sequence-specific and sequence-independent components. We found that for a large part of the genome the elongation time can be well described by a global average replication rate, thus by a single parameter. However, we also showed that there are regions within the genomic landscape of budding yeast with highly specific replication rates, which cannot be explained by global properties of the replication machinery. CONCLUSION/SIGNIFICANCE: Computational models of DNA replication in budding yeast that can predict replication dynamics have rarely been developed yet. We show here that even beyond the level of initiation there are effects governing the replication time that can not be explained by the movement of the polymerase along the DNA template alone. This allows us to characterize genomic regions with significantly altered elongation characteristics, independent of initiation times or sequence composition.
url http://europepmc.org/articles/PMC2860512?pdf=render
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