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Nucleosome positioning from tiling microarray data
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AbstractMotivation: The packaging of DNA around nucleosomes in eukaryotic cells plays a crucial role in regulation of gene expression, and other DNA-related processes. To better understand the regulatory role of nucleosomes, it is important to pinpoint their position in a high (5–10 bp) resolution. Toward this end, several recent works used dense tiling arrays to map nucleosomes in a high-throughput manner. These data were then parsed and hand-curated, and the positions of nucleosomes were assessed.Results: In this manuscript, we present a fully automated algorithm to analyze such data and predict the exact location of nucleosomes. We introduce a method, based on a probabilistic graphical model, to increase the resolution of our predictions even beyond that of the microarray used. We show how to build such a model and how to compile it into a simple Hidden Markov Model, allowing for a fast and accurate inference of nucleosome positions.We applied our model to nucleosomal data from mid-log yeast cells reported by Yuan et al. and compared our predictions to those of the original paper; to a more recent method that uses five times denser tiling arrays as explained by Lee et al.; and to a curated set of literature-based nucleosome positions. Our results suggest that by applying our algorithm to the same data used by Yuan et al. our fully automated model traced 13% more nucleosomes, and increased the overall accuracy by about 20%. We believe that such an improvement opens the way for a better understanding of the regulatory mechanisms controlling gene expression, and how they are encoded in the DNA.Contact: nir@cs.huji.ac.il
Oxford University Press (OUP)
Title: Nucleosome positioning from tiling microarray data
Description:
AbstractMotivation: The packaging of DNA around nucleosomes in eukaryotic cells plays a crucial role in regulation of gene expression, and other DNA-related processes.
To better understand the regulatory role of nucleosomes, it is important to pinpoint their position in a high (5–10 bp) resolution.
Toward this end, several recent works used dense tiling arrays to map nucleosomes in a high-throughput manner.
These data were then parsed and hand-curated, and the positions of nucleosomes were assessed.
Results: In this manuscript, we present a fully automated algorithm to analyze such data and predict the exact location of nucleosomes.
We introduce a method, based on a probabilistic graphical model, to increase the resolution of our predictions even beyond that of the microarray used.
We show how to build such a model and how to compile it into a simple Hidden Markov Model, allowing for a fast and accurate inference of nucleosome positions.
We applied our model to nucleosomal data from mid-log yeast cells reported by Yuan et al.
and compared our predictions to those of the original paper; to a more recent method that uses five times denser tiling arrays as explained by Lee et al.
; and to a curated set of literature-based nucleosome positions.
Our results suggest that by applying our algorithm to the same data used by Yuan et al.
our fully automated model traced 13% more nucleosomes, and increased the overall accuracy by about 20%.
We believe that such an improvement opens the way for a better understanding of the regulatory mechanisms controlling gene expression, and how they are encoded in the DNA.
Contact: nir@cs.
huji.
ac.
il.
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