Genomic landscape of human allele-specific DNA methylation

Fang, Fang; Hodges, Emily; Molaro, Antoine; Dean, Matthew D.; Hannon, Gregory J.; Smith, Andrew D.

doi:10.1073/pnas.1201310109

Cited by 104 publications

(127 citation statements)

References 44 publications

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“…Notably, we found that one ASM region located within the promoter of ZNF718 was also common to all 9 tissues. Although conclusive experimental data are not available for characterizing ZNF718 as an imprinting gene, our findings agree with those of a statistical model developed by Fang et al., which identified ZNF718 as a candidate imprinting gene 22 . Nevertheless, our results demonstrate that Q-RRBS can be used to accurately identify ASM regions by using UMIs.…”

Section: Q-rrbs Can Be Used To Identify Asms In the Absence Of Heterosupporting

confidence: 93%

Q-RRBS: a quantitative reduced representation bisulfite sequencing method for single-cell methylome analyses

Wang

Dong

et al. 2015

Epigenetics

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Reduced representation bisulfite sequencing (RRBS) is a powerful method of DNA methylome profiling that can be applied to single cells. However, no previous report has described how PCR-based duplication-induced artifacts affect the accuracy of this method when measuring DNA methylation levels. For quantifying the effects of duplication-induced artifacts on methylome profiling when using ultra-trace amounts of starting material, we developed a novel method, namely quantitative RRBS (Q-RRBS), in which PCR-induced duplication is excluded through the use of unique molecular identifiers (UMIs). By performing Q-RRBS on varying amounts of starting material, we determined that duplication-induced artifacts were more severe when small quantities of the starting material were used. However, through using the UMIs, we successfully eliminated these artifacts. In addition, Q-RRBS could accurately detect allele-specific methylation in absence of allele-specific genetic variants. Our results demonstrate that Q-RRBS is an optimal strategy for DNA methylation profiling of single cells or samples containing ultra-trace amounts of cells.

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Section: Q-rrbs Can Be Used To Identify Asms In the Absence Of Heterosupporting

confidence: 93%

Q-RRBS: a quantitative reduced representation bisulfite sequencing method for single-cell methylome analyses

Wang

Dong

et al. 2015

Epigenetics

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“…DNA methylation is an important epigenetic mark controlling gene expression, thus playing pivotal roles in many cellular processes including embryonic development [1], genomic imprinting [2,3], X-chromosome inactivation [4], transposable element repression [5], and preservation of chromosome stability [6]. Aberrant DNA methylations are known to be associated with human diseases such as cancers, lupus, muscular dystrophy, and imprintingrelated birth defects [7][8][9][10][11][12][13][14].…”

Section: Introductionmentioning

confidence: 99%

MethylPurify: tumor purity deconvolution and differential methylation detection from single tumor DNA methylomes

Zheng

Zhao

et al. 2014

Genome Biol

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We propose a statistical algorithm MethylPurify that uses regions with bisulfite reads showing discordant methylation levels to infer tumor purity from tumor samples alone. MethylPurify can identify differentially methylated regions (DMRs) from individual tumor methylome samples, without genomic variation information or prior knowledge from other datasets. In simulations with mixed bisulfite reads from cancer and normal cell lines, MethylPurify correctly inferred tumor purity and identified over 96% of the DMRs. From patient data, MethylPurify gave satisfactory DMR calls from tumor methylome samples alone, and revealed potential missed DMRs by tumor to normal comparison due to tumor heterogeneity.

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“…Another open problem in the analysis of single-cell methylation data is the resolution (known as phasing) of epi-haplotypes to allow recovery of a single-chromosome methylome in diploid cells 44 . Phasing can be important for physically linking the methylation state of promoters, regulatory elements and transcribed units in cis.…”

Section: Lamina-associated Domainsmentioning

confidence: 99%

Single-cell epigenomics: techniques and emerging applications

2015

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Epigenomics is the study of the physical modifications, associations and conformations of genomic DNA sequences, with the aim of linking these with epigenetic memory, cellular identity and tissue-specific functions. While current techniques in the field are characterizing the average epigenomic features across large cell ensembles, the increasing interest in the epigenetics within complex and heterogeneous tissues is driving the development of single-cell epigenomics. We review emerging single-cell methods for capturing DNA methylation, chromatin accessibility, histone modifications, chromosome conformation and replication dynamics. Together, these techniques are rapidly becoming a powerful tool in studies of cellular plasticity and diversity, as seen in stem cells and cancer.

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Genomic landscape of human allele-specific DNA methylation

Cited by 104 publications

References 44 publications

Q-RRBS: a quantitative reduced representation bisulfite sequencing method for single-cell methylome analyses

Q-RRBS: a quantitative reduced representation bisulfite sequencing method for single-cell methylome analyses

MethylPurify: tumor purity deconvolution and differential methylation detection from single tumor DNA methylomes

Single-cell epigenomics: techniques and emerging applications

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