Measuring cell-type specific differential methylation in human brain tissue

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Abstract

The behavior of epigenetic mechanisms in the brain is obscured by tissue heterogeneity and disease-related histological changes. Not accounting for these confounders leads to biased results. We develop a statistical methodology that estimates and adjusts for celltype composition by decomposing neuronal and non-neuronal differential signal. This method provides a conceptual framework for deconvolving heterogeneous epigenetic data from postmortem brain studies. We apply it to find cell-specific differentially methylated regions between prefrontal cortex and hippocampus. We demonstrate the utility of the method on both Infinium 450k and CHARM data. © 2013 Montaño et al.; licensee BioMed Central Ltd.

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Montaño, C. M., Irizarry, R. A., Kaufmann, W. E., Talbot, K., Gur, R. E., Feinberg, A. P., & Taub, M. A. (2013). Measuring cell-type specific differential methylation in human brain tissue. Genome Biology, 14(8). https://doi.org/10.1186/gb-2013-14-8-r94

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