Cell. 2008 May 2;133(3):523-36.

Highly integrated single-base resolution maps of the epigenome in Arabidopsis.

Lister R, O'Malley RC, Tonti-Filippini J, Gregory BD, Berry CC, Millar AH, Ecker JR.

Source

Plant Biology Laboratory, The Salk Institute for Biological Studies, 10010 North Torrey Pines Road, La Jolla, CA 92037, USA.

Abstract

Deciphering the multiple layers of epigenetic regulation that control transcription is critical to understanding how plants develop and respond to their environment. Using sequencing-by-synthesis technology we directly sequenced the cytosine methylome (methylC-seq), transcriptome (mRNA-seq), and small RNA transcriptome (smRNA-seq) to generate highly integrated epigenome maps for wild-type Arabidopsis thaliana and mutants defective in DNA methyltransferase or demethylase activity. At single-base resolution we discovered extensive, previously undetected DNA methylation, identified the context and level of methylation at each site, and observed local sequence effects upon methylation state. Deep sequencing of smRNAs revealed a direct relationship between the location of smRNAs and DNA methylation, perturbation of smRNA biogenesis upon loss of CpG DNA methylation, and a tendency for smRNAs to direct strand-specific DNA methylation in regions of RNA-DNA homology. Finally, strand-specific mRNA-seq revealed altered transcript abundance of hundreds of genes, transposons, and unannotated intergenic transcripts upon modification of the DNA methylation state.

Comment in

Cell. 2008 May 2;133(3):395-7.

PMID:: 18423832; [PubMed - indexed for MEDLINE]
PMCID: PMC2723732

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Figure 4

Distribution of smRNA Lenghts and Overlap between DNA Methylation and 24-mer smRNAs

(A) Nucleotide frequency and distribution flanking and within uniquely aligning 24-mer smRNAs.
(B) Methylcytosine distribution presented as the ratio of methylcytosines to all cytosines located at each position flanking and within uniquely aligning 24-mer smRNAs. Abbreviations: mC, methylcytosine on the sense strand relative to the smRNA sequence; C, total cytosine on the sense strand; mC*, methylcytosine on the antisense strand; C*, total cytosine on the antisense strand.

Highly Integrated Single-Base Resolution Maps of the Epigenome in Arabidopsis

Cell. Cell;133(3):523-536.

Figure 7

Identification of Upregulated Transposons and Intergenic Transcripts Regulated by DNA Methylation through mRNA-Seq

(A) The percentage of transposons/pseudogenes in the Arabidopsis genome for which mRNA-seq-based evidence of transcription was present or absent in each genotype.
(B) Hypermethylation of transposons in rdd. Browser visualization of methylcytosines located within and proximal to the copia-like retrotransposon At2g24660. Dense methylation is present within the retrotransposon only in rdd.
(C) An upregulated intergenic transcript identified in the DNA methyltransferase mutant met1 (indicated by arrow). Sites of DNA methylation are shown, and the color reflects the methylation context, as indicated.

Highly Integrated Single-Base Resolution Maps of the Epigenome in Arabidopsis

Cell. Cell;133(3):523-536.

Figure 6

Diverse Patterns of Interaction between DNA Methylation and smRNAs

(A) Hierarchical clustering of all 1 kb regions of the nuclear genome that have significantly different DNA methylation and/or smRNA density between Col-0 and met1 or ddc, and regions that show no difference (see Experimental Procedures). Yellow indicates >3-fold mC density and/or >5-fold smRNA difference;black indicates no difference above thresholds (<2-fold change in mC density or sequenced bases of smRNA). Minimum Col-0 mC: 8 per kilobase, minimum Col-0 smRNA: 300 sequenced bases per kilobase.
(B–F) Typical examples from various clusters visualized in the AnnoJ browser. Tracks are shown for DNA methylation sites and smRNA. smRNAs are colored as in Figure 5. Abbreviations: mC, methylcytosine.

Highly Integrated Single-Base Resolution Maps of the Epigenome in Arabidopsis

Cell. Cell;133(3):523-536.

Figure 1

DNA Methylation Context and Chromosomal Distribution in Wild-Type Col-0

(A) Methylcytosines identified (top panel) in Col-0 from bisulfite-converted sequencing reads (bottom panel) for a region of chromosome 1, as represented in the AnnoJ browser.
(B) The fraction of methylcytosines identified in each sequence context for Col-0, where H = A, C, or T.
(C) The density of methylcytosines identified in each context, on each strand throughout chromosome 1, counted in 50 kb bins.
(D) Distribution of the percentage methylation at each sequence context. The y axis indicates the fraction of the total methylcytosines that display each percentage of methylation (x axis), where percentage methylation was determined as the fraction of reads at a reference cytosine containing cytosines following bisulfite conversion. Fractions were calculated within bins of 10%, as indicated on the x axis.

Highly Integrated Single-Base Resolution Maps of the Epigenome in Arabidopsis

Cell. Cell;133(3):523-536.

Figure 2

The Effect on Cytosine Methylation Frequency by Neighboring Bases

(A–C) The methylation frequency of cytosines in the (A) CHG, (B) CHH, and (C) CG contexts are shown as a function of proximal base composition. Base composition effects two positions upstream (−2) to four bases downstream (+4) of a particular cytosine are interrogated by dividing the number of methylcytosines to total cytosines of each base at each position.
(D) The percent contribution of each CG tetramer (−1 to +2) was calculated in five 200 bp pair sections in the 1 kb region immediately upstream of all genes in the genome. For each tetramer, the percent contribution in the 800–1000 bp region was used to normalize all other regions.

Highly Integrated Single-Base Resolution Maps of the Epigenome in Arabidopsis

Cell. Cell;133(3):523-536.

Figure 5

Methylcytosine Density Correlates with smRNA Abundance

(A–C) Hierarchical clustering of all 1 kb regions of the nuclear genome that have significantly different methylcytosine and smRNA density between Col-0 and (A) met1, (B) ddc, and (C) rdd (see Experimental Procedures). Yellow indicates >3-fold change in methylcytosine density and >5-fold difference in number of sequenced bases of smRNA; black indicates no change above fold change thresholds. Minimum methylcytosines: 8 per kilo-base, minimum smRNA: 300 sequenced bases per kilo-base.
(D) DNA methylation and smRNAs in Col-0 and met1.
(E) DNA methylation and smRNAs in Col-0 and rdd. Tracks are shown for DNA methylation sites and smRNA. smRNAs are colored internally by their uniqueness (red: maps to a single location, greyscale: maps to multiple locations), and a surrounding box indicates the size class (orange:21-mer, black: 24-mer), and the shading represents the copy number (darker: more copies, lighter: fewer copies). Abbreviations: mC, methylcytosine.

Highly Integrated Single-Base Resolution Maps of the Epigenome in Arabidopsis

Cell. Cell;133(3):523-536.

Figure 3

Methylation in DNA Methyltransferase and DNA Demethylase Mutant Plants

(A) The fraction of methylcytosines in each sequence context for each genotype. Positions were compared only where all genotypes had a sequence read depth between 6 and 10.
(B) Ratio of the number of methylcytosines in each mutant versus Col-0 per 200 kb, where read depth was 6–10. The horizontal line represents Col-0, the plotted line represents percentage methylation in the mutant versus Col-0.
(C) Average distribution of DNA methylation in each context throughout genes and 1 kb upstream and downstream in Col-0 and met1. Values are normalized to the highest point within each profile.
(D) Density of sites of hypermethylation in rdd. The number of sites of DNA methylation present in rdd and absent in Col-0 was tabulated for promoters (1 kb upstream), 5′UTRs, gene bodies, and 3′UTRs, and the density of methylation in each normalized to the length of each feature. The number of features that contained hypermethylation above different lower thresholds of density was calculated, and the number of features of each type normalized relative to the feature with the most counts, for each lower threshold.

Highly Integrated Single-Base Resolution Maps of the Epigenome in Arabidopsis

Cell. Cell;133(3):523-536.

Data from this publication

Epigenomics

Experiments, by feature type.See all experiments (8)

gene expression (4)

small RNA analysis (4)

Publication Types, MeSH Terms, Substances, Grant Support

Publication Types

Research Support, N.I.H., Extramural
Research Support, Non-U.S. Gov't
Research Support, U.S. Gov't, Non-P.H.S.

MeSH Terms

Arabidopsis/genetics*
CpG Islands
DNA Methylation*
DNA Modification Methylases/genetics
DNA Modification Methylases/metabolism
Epigenesis, Genetic*
Gene Expression Profiling
Genome, Plant*
Mutation
RNA, Plant/metabolism
RNA, Untranslated/metabolism
Sequence Analysis, DNA/methods

Substances

RNA, Plant
RNA, Untranslated
DNA Modification Methylases

Grant Support

R01 HG003523-01/HG/NHGRI NIH HHS/United States
R01 HG003523-02/HG/NHGRI NIH HHS/United States
R01 HG003523-03/HG/NHGRI NIH HHS/United States

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Highly integrated single-base resolution maps of the epigenome in Arabidopsis.

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Epigenomics

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