Long Reads Capture Simultaneous Enhancer-Promoter Methylation Status for Cell-type Deconvolution

Author:

Margalit Sapir,Abramson Yotam,Sharim Hila,Manber Zohar,Bhattacharya Surajit,Chen Yi-Wen,Vilain Eric,Barseghyan Hayk,Elkon RanORCID,Sharan Roded,Ebenstein Yuval

Abstract

AbstractMotivationWhile promoter methylation is associated with reinforcing fundamental tissue identities, the methylation status of distant enhancers was shown by genome-wide association studies to be a powerful determinant of cell-state and cancer. With recent availability of long-reads that report on the methylation status of enhancer-promoter pairs on the same molecule, we hypothesized that probing these pairs on the single-molecule level may serve the basis for detection of rare cancerous transformations in a given cell population. We explore various analysis approaches for deconvolving cell-type mixtures based on their genome-wide enhancer-promoter methylation profiles.ResultsTo evaluate our hypothesis we examine long-read optical methylome data for the GM12787 cell line and myoblast cell lines from two donors. We identified over 100,000 enhancer-promoter pairs that co-exist on at least 30 individual DNA molecules per pair. We developed a detailed methodology for mixture deconvolution and applied it to estimate the proportional cell compositions in synthetic mixtures based on analyzing their enhancer-promoter pairwise methylation. We found our methodology to lead to very accurate estimates, outperforming our promoter-based deconvolutions. Moreover, we show that it can be generalized from deconvolving different cell types to subtle scenarios where one wishes to deconvolve different cell populations of the same cell-type.AvailabilityThe code used in this work to analyze single-molecule Bionano Genomics optical maps is available via the GitHub repositoryhttps://github.com/ebensteinLab/Single_molecule_methylation_in_EP.Contactuv@post.tau.ac.il(Y.E),roded@tauex.tau.ac.il(R.S)

Publisher

Cold Spring Harbor Laboratory

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