Strong components of epigenetic memory by primary cell sampling location

We first characterized differences in DNAm levels from cultured fibroblasts derived from different locations (scalp versus dura). Many probes, targeting individual CpGs, were differentially methylated between scalp- and dura-derived fibroblasts– 101,989 (22%) at genome-wide significance (false discovery rate, FDR < 5%, see Methods). These significant DNAm differences between cultured fibroblasts from the scalp and dura were large in magnitude, with 57,704 probes having differences in DNAm levels greater than 10%, and 23,752 with differences greater than 20% (Fig 1A). The directionality of these DNAm differences was balanced, with approximately equal proportions of CpGs showing increased versus decreased methylation in cultured fibroblasts from scalp compared to dura. These differentially methylated probes (DMPs) were widely distributed across the genome, as 18,551 genes (defined by UCSC knownGene database) had at least one DMP within 5 kilobases (kb), as did 33,247 transcripts (see Methods). These widespread single CpG differences manifest as the largest component of variability in the entire dataset, as the first principal component (Fig 1B, explaining 38% and 62.3% of the variability before and after surrogate variable analysis, SVA [24]) represents the sampling location of these cultured fibroblasts, suggesting a strong epigenetic memory of original cell location.

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Fig 1. DNA methylation patterns in dura- and scalp-derived fibroblasts.

(A) Histogram of difference in DNAm levels at CpGs/probes between scalp and dura derived fibroblasts (on the proportion methylation scale). (B) The first principal component (PC1) of the DNAm data plotted against fibroblast sampling location (scalp versus dura). (C) Example significant differentially methylated region (DMR) that overlaps the gene RUNX3, with DNAm levels on the y-axis and genomic coordinates on the x-axis. (D) Example significant DNAm block, with DNAm levels on the y-axis and genomic coordinates on the x-axis. Gene annotation panels in C and D are based on Ensembl annotation–dark blue represents exons and light blue represents introns.

https://doi.org/10.1371/journal.pgen.1005819.g001

Since these differentially methylated CpGs tended to cluster in a smaller number of genes, we further identified 697 differentially methylated regions (DMRs) at stringent genome-wide significance (family-wise error rate, FWER < 10%)–these regions were identified based on adjacent probes showing directionally-consistent differences in DNAm > 10% between groups [25] (see Methods). For example, we identified a region of 24 contiguous probes hypermethylated in scalp-derived fibroblasts within the gene RUNX3 –a tumor suppressor that plays an integral role in regulating cell proliferation and the rate of apoptosis [26] (Fig 1C, see S2 Fig and S2 Table for all significant DMRs). Regional differences, particularly in CpG island shores, previously have been shown to better distinguish tissues and cell types [1] and correlate with neighboring gene expression levels [23] than individual CpGs. Unlike at the single CpG level, which had balanced directionality of differential methylation, the majority of DMRs had higher DNAm levels in fibroblasts derived from scalp compared to those derived from dura (N = 414, 59.4%). Using gene sets defined by biological processes [27], these neighboring genes (within 5 kb) were strongly enriched for morphogenesis (including morphogenesis of the epithelium), developmental processes, cell differentiation, and epithelium and connective tissue development, among other more general gene sets (all p < 10⁻⁸, S3 Table).

In addition to the extensive differential methylation at both the CpG and regional level, we identified 243 long-range regions with consistent significant methylation change (FWER < 10%), called “blocks” [28], using an algorithm adapted from whole genome bisulfite sequencing (WGBS) data to Illumina 450k [23]. A representative significant block is shown in Fig 1D (see S3 Fig for all significant blocks at FWER < 10%). Blocks have now been identified across many cancer types [29], and tend to associate with higher order chromatin structure including nuclear lamin-associated domains (LADs) [30] and large organized chromatin K9 modification (LOCKs) [28]. The 243 significant blocks in our data represent 41 Mb of sequence and contain 298 annotated genes. These blocks contain 41 of the significant DMRs that differentiate sampling location of the fibroblasts, and more interestingly, every block overlaps at least one “dynamic” cell/tissue DMR identified using WGBS data from Ziller et al (2013) [3].

While these cultured fibroblasts were several generations/passages removed from the primary tissue and morphologically indistinguishable, we nevertheless found widespread epigenetic differences by sampling location of the primary fibroblasts at varying spatial scales, suggesting a strong epigenetic memory of the original cell location.

Epigenetic memory related to original cell location manifests in the transcriptome

We next sought to determine the functional correlates of the widespread epigenetic differences identified between scalp- and dura-derived fibroblasts by performing RNA sequencing (RNA-seq) on polyadenylated (polyA+) mRNA from the same cultured samples (see Methods). Briefly, we aligned the reads to the transcriptome using TopHat [31] and generated normalized gene counts (as fragments per kb per million mapped reads, FPKM) based on the Illumina iGenome hg19 annotation using the featureCounts software [32]. A median of 88.0% (interquartile range, IQR: 85.5%– 88.8%) of reads mapped to the genome, of which a median of 84.7% (IQR: 84.4%–85.5%) mapped to the annotated transcriptome (see S1 Table for sample-specific percentages). We identified 11,218 expressed genes with average FPKM expression greater than 1.0. Initial clustering of the gene FPKM values separated the fibroblast samples by location in the first principal component (PC), which explained 35.4% of the variance (S4 Fig), mirroring the first principal component of the DNAm data (Fig 1B). We could further cluster our samples by sampling location using a set of 337 genes (of which 210 were in our dataset) that were previously identified by Rinn et al [17] to group largely dermal fibroblasts by their anatomical sites of origin (S5 Fig)–these genes better clustered the samples by sampling location than random sets of 210 genes (p<0.001, see Methods). Differential expression analysis of the RNA-seq data, independent of the results from the epigenetic analyses above, identified many genes that differed by the source of the primary fibroblast– 5,830 genes at FDR < 5%. Both scalp- and dura-derived fibroblasts expressed high levels of Fibroblast Specific Protein-1 (FSP-1) and this gene was more highly expressed scalp-derived fibroblasts (fold change = 5.5, FDR = 5.6x10^-6) in line with increased higher proliferation rates in the scalp-derived versus dura-derived fibroblasts [15]. The differentially expressed genes were strongly enriched for signaling and cell communication, cell proliferation, apoptotic processes, and epithelium development and morphogenesis via gene ontology (GO) analysis (all p < 10⁻⁸, S4 Table)–these gene sets were similar, and much more significant, to those identified comparing gene expression profiles across positional-identity genes in dermal fibroblasts [17].

We next used the gene expression data as a functional readout of the differentially methylated loci identified between fibroblasts cultured from scalp and dura. The majority of significant DMPs (76,971/101,989, 75.47%) were inside or near (within 5kb of) a UCSC annotated gene, and 28.2% (21,742/76,971) were significantly associated with gene expression levels (at p < 0.05). This percentage of DMPs with significant expression readout was elevated (34.9%) among those DMPs with larger DNAm differences by sampling location (greater than 10% difference in DNAm levels). These DMPs were strongly significantly enriched among the CpG sites that associated with expression levels at the p < 0.05 (48,062 probes within 5kb of genes, odds ratio, OR = 3.99, p < 2.2x10^-16) and FDR < 0.05 (6,559 probes within 5kb of genes, OR = 19.54, p < 2.2x10^-16) significance thresholds. Surprisingly, we found that the DNAm levels at the majority of these expression-associated differentially methylated CpGs tended to be positively associated with gene expression, regardless of overall methylation levels (un-, partially-, or highly-methylated) or their location in the gene (islands, shores and shelves)–these biases towards positive associations were statistically significant for many of these comparisons (see S5 Table, panels A and B). We hypothesize these positive correlations could be due to the probe design of the Illumina 450 (the majority of probes are in lowly methylated regions) combined with the majority of genes having low expression (38.75% had mean FPKMs < 1).

We identified similar associations using transcript-level expression data using the Sailfish program [33] (see Methods) on the above transcriptome– 76.5% (77,981/101,989) of the DMPs were within 5 kb of a transcript, and 30.4% of them (23,672/77,981) correlated with expression (at p < 0.05). 33,247 unique transcripts overlapped or were within 5 kb of DMPs, and of them, 27.0% (8,981/33,247) exhibited significant correlation between DNAm and expression (at p < 0.05). The 33,247 transcripts proximal to the DMRs corresponded to 18,699 genes, the majority of which (84.3%, 15,761/18,699) contained more than one transcript. Interestingly, these associations often appear in a transcript-specific manner—6,190 genes (39.3%) had ≥ 1 transcript with significant correlation between DNAm and expression (at p < 0.05), with ≥ 1 transcripts that were not associated with nearby CpG levels. These results suggest that genes, and their underlying transcripts, can functionally validate many of the differentially methylated CpGs for sampling location.

Moving beyond individual CpGs, 587/697 (84.2%) DMRs were in or near (<5kb) genes, and many had DNAm levels that were significantly associated with gene expression levels (306/587, 52.1% at p < 0.05). For instance, a DMR overlapping an intronic sequence of the SIM1 gene (Fig 2A) was unmethylated with low corresponding expression of the gene in the cultured fibroblasts from dura, and highly methylated with corresponding high expression levels of the gene in the scalp-derived fibroblasts (Fig 2B and S2 Table). This is in line with previous reports suggesting that gene body methylation levels positively associate with local gene expression [34], unlike CpG island shore methylation that tends to be negatively associated with gene expression levels [1]. Of the 478 unique genes in or within 5kb of DMRs, the expression of 235 (49.2%) of them was significantly correlated with DNAm (p < 0.05). These 235 unique genes tended to exhibit stronger differential expression between the scalp- and dura-derived fibroblasts (median fold change = 1.59, IQR = 1.23–2.68) than individual CpG results, in line with previously published findings [23]. GO analysis on expression-associated genes proximal to DMRs revealed enrichment for multiple important biological processes such as connective tissue development, epithelium morphogenesis and development, cell differentiation (specifically including epithelial cell differentiation), and cell proliferation (including epithelial cell proliferation), among other more general sets (all p < 10⁻⁸, see S6 Table). Unlike at the single CpG-level, we found that the majority of DMRs in and around the transcriptional start sites of genes (CpGs islands and shores) were negatively correlated with gene expression (S5 Table), in line with previous research [1]. We observed similar methylation-expression associations using transcript-level expression measurements– 312/599 DMRs (52.1%) near ≥ 1 transcripts associated with expression, and like at the single CpG level, found evidence for transcript-specific epigenetic regulation of expression (among 28.9% of genes containing multiple transcripts and associated with DNAm levels within the DMRs).

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Fig 2. Regional DNA methylation changes manifest in the transcriptome.

(A) Plot of the DNAm levels (proportion methylation) of an example significant DMR, which overlaps the gene SIM1. (B) Plot of the average DMR DNAm levels versus the expression level of SIM1, showing high positive correlation (p = 4.67x10⁻⁸).

https://doi.org/10.1371/journal.pgen.1005819.g002

Lastly, we found that the majority of differentially methylated blocks contained at least one gene and transcript differentially expressed between scalp- and dura-derived fibroblasts. The majority of blocks contained at least one gene (N = 188/243, 77.4%); 63.8% (N = 120/188) had at least one gene and 66.66% (N = 124/186) at least one transcript that was differentially expressed (at p < 0.05).

As a representative example, one of the blocks, hypermethylated in scalp-derived fibroblasts, overlaps the HOXB gene cluster (Fig 3A), which has previously been shown to be play a role in the position identities of fibroblasts [17]. In this block, expression levels of the HOXB genes are significantly greater in fibroblasts cultured from scalp than those from dura (Fig 3B), which contrasted previous microarray-based data showing these genes were not expressed in dermal samples taken from the head [17] highlighting the improved precision of RNA-sequencing data to quantify expression levels. Similarly, the 188 significant blocks contained 298 unique genes, and 126 of them (42.3%) were differentially expressed (at FDR < 0.05) which is a higher proportion than the rest of the transcriptome (0.42 vs. 0.32, p = 3.79x10^-9).

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Fig 3. Long-range DNA methylation changes manifest in the transcriptome.

(A) Plot of the DNAm levels (proportion methylation) of a significant DNAm block overlapping genes in the HOX family. Y-axis: proportion DNAm levels, x-axis: genomic coordinates on chromosome 17. (B) Corresponding expression levels of the HOX genes within the DNAm block are more highly expressed in the scalp. Y-axis: log₂ transformed fragments per kilobase per million mapped (FPKM), x-axis: sampling location.

https://doi.org/10.1371/journal.pgen.1005819.g003

Given the strong association between DNAm levels and local expression levels, we sought to more fully examine the epigenetic states of these sampling location-associated DNAm differences. We downloaded chromatin state data (18 states) from the NIH Roadmap Epigenomics Consortium on the four available fibroblast samples (2 primary foreskin, 1 adult dermal, and 1 lung) [35], and mapped our DMPs, DMRs, and blocks for fibroblast sampling location onto these states (S7 Table). The CpGs differentially methylated by sampling location were largely enriched for enhancer chromatin states, including preferential enrichment of genic (EnhG2) and active (EnhA1) enhancer states and depleted for active transcriptional start site (TSS) states (TssA). At the region level, DMRs were largely enriched for bivalent TSS (EnhBiv) and repressive polycomb (ReprPC) states and depleted for transcription (Tx) genic enhancer (EnhG2) states, and blocks were strongly enriched for quiescent (Quies) and heterochromatin (Het) states and depleted for transcriptional states. These enrichments were relatively conserved across the four Roadmap fibroblast samples, further suggesting distinct epigenetic states in scalp- compared to dura-derived fibroblasts. These results suggest that epigenetic memory related to original cell location manifests in genomic state differences and largely reads out in the transcriptome, particularly among regional changes in DNAm related to fibroblast sampling location.

Increased stochastic variability in scalp-derived fibroblasts

We hypothesized that scalp-derived fibroblasts might have more variable levels of DNAm than dura-derived fibroblasts, given the chronic exposure to environmental factors (e.g. sunlight, chemicals) in the primary tissue across the lifespan. At the individual CpG level, we tested for differences in variance between the scalp- and dura-derived fibroblasts independent of the underlying mean methylation levels [36] (see Methods section). While only two probes reached genome-wide significance (at FDR < 0.05) for differences in variance, at marginal levels of significance (p < 0.05), fibroblasts cultured from scalp had more variable DNAm levels than fibroblasts cultured from dura (N = 13,169/16,330, 80.6%).

We next sought to characterize methylome-wide patterns of DNAm across these fibroblasts in the context of other diverse cell types. After downloading and normalizing Illumina 450k data from sorted blood [20] and frontal cortex [21], as well as skin-derived fibroblasts [19] and melanoma samples (SKCM) from the Cancer Genome Atlas (TCGA) [37], we computed methylome-wide Euclidean distances between and across each of the 11 cell types (see Methods section). We noted that these cell types largely cluster by tissue source (brain, blood, and fibroblasts in the first two principal components and largest dendrogram splits, S6 Fig).

The inter-individual epigenomic distances, and their variability, were much greater in the scalp-derived (as well as skin-derived) fibroblasts than dura-derived fibroblasts (p = 1.34x10^-9 and p = 1.77x10^-14 respectively, see Fig 4). The distances within scalp- and skin-derived fibroblasts were significantly larger than those calculated within pure blood and cortex cell types (p-values range from 1.04x10^-21 to <10⁻¹⁰⁰). Interestingly, the inter-individual distances between fibroblasts cultured from scalp samples were greater than the distances between different cell types within a blood cell lineage (e.g. natural killer cells versus CD4+ T-cells) which were previously suggested for different dermal fibroblasts [16] and instead more similar to distances across lineage (e.g. natural kill cells versus monocytes). Note that comparing inter-individual distance between two cell types (e.g. scalp- versus dura-derived fibroblasts) reflects the extensive differential methylation between these two cell types (see Fig 1)—the inter-individual distances are large but the variability in distances was low.

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Fig 4. Increased methylome distances within scalp-derived fibroblasts.

Y-axis: methylome (Euclidean) distance between pairs of samples stratified by cell and tissue types. CD4T: CD4+ T-cell, NK: natural killer cell, Mono: monocyte, NeuN+: neuronal DLPC cell, NeuN-: non-neuronal DLPFC cell.

https://doi.org/10.1371/journal.pgen.1005819.g004

As another example, the distances across scalp-derived fibroblasts were lower than the inter-individual variability between neurons and non-neurons (via NeuN+ sorting), which reflects the extensive methylation differences between these two cell types [21]. As expected, we found the greatest methylome-wide distances and largest inter-individual variability in the melanoma samples [28,36], which highlights the relative scale of these methylome-wide distances (ranging from pure cell types to cancer). These increased epigenomic distances may relate to the rate of cell division, which is non-existent in neuronal cells [38] and infrequent in T-lymphocytes at the population level [39]. The increased epigenetic variability in the scalp samples was further not associated with differences in donor age (p > 0.05, S7 Fig), suggesting increased epigenetic stochastic variability in scalp- (and skin-) derived fibroblasts.

Epigenetic memory related to donor age

We hypothesized that a subset of this increased variability might result from age-related divergence in DNAm at individual loci that were differential by sampling location, such that young donors would have lesser difference in DNAm levels, and older donors would have larger differences in DNAm. By fitting linear models on the difference in DNAm levels across sampling location as a function of donor age (see Methods), we identified 7,265 CpGs associated with diverging DNAm levels across aging (at FDR < 10%, S8 Fig). These loci appeared to be clustered into representative patterns of their age-related changes (Fig 5). The majority of these CpGs had significant age-related changes in fibroblasts derived from the scalp (64.0%), but not dura (17.4%), and the magnitude of change across age was larger in scalp-derived fibroblasts–the average change in percent DNAm per decade of life was 3.13% (IQR = 1.81%-4.29%) in fibroblasts derived from scalp compared to 1.13% (IQR = 0.295%-1.61%) in those from the dura mater.

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Fig 5. Representative patterns of age-associated changes in DNAm by sampling location.

Each panel (A-H) shows mean adjusted expression levels versus age for each of eight clusters of location-specific age-related changes in DNAm levels. Y-axis: mean-centered DNAm levels, x-axis: sample age, p-value represents the statistical interaction between sampling location and age on DNAm levels. N: number of CpGs in the cluster. Vertical lines at each sample indicate +/- 3 times the standard error by cluster.

https://doi.org/10.1371/journal.pgen.1005819.g005

A subset of these CpGs showing sampling location-dependent age-related changes associated with nearby gene expression levels. Most of the probes (N = 5,185/7,265, 71.4%) were annotated to 3,553 unique genes (within 5kb) and 21.8% of these (N = 775/3,555) showed significant correlation between DNAm and gene expression (p < 0.05). These DNAm associated genes were enriched for multiple general developmental processes including cell development, morphogenesis, and differentiation (all p<10⁻⁸, S8 Table). Several of the age-related CpGs showing expression association were within genes that are involved in cell proliferation and apoptosis. For instance, DNAm levels at two significant probes inside the gene TEAD1, which regulates notochord development and cell proliferation [40], were significantly associated with gene expression levels (p = 8.60x10^-4 and 0.045, respectively). Another significant DNAm-expression pair (p = 0.02) involved AVEN, a gene shown to inhibit Caspase activation in apoptosis [41]. Interestingly, while we identified a large number of age-related CpGs, “DNA methylation ages” [8] were very similar to the chronological ages of the samples (see Methods and S9 Fig)–these associations did not differ by sampling location (p = 0.72) and there was further no association between “DNA methylation age” and sampling location alone (p = 0.96). The age-associated CpGs identified here therefore suggest that altered regulation of DNAm levels across aging occurs primarily in fibroblasts derived from scalp but not from dura, perhaps through altered cell proliferation and apoptosis, and possibly reflecting greater exposure to environmental agents that can affect the methylome.

Epigenetic memory related to sampling location and age do not implicate genetic mosaicism

Lastly, we characterized the expressed sequences of the scalp- and dura-derived fibroblasts within each individual to examine the extent of genetic mosaicism, which may contribute to differences in DNAm through changing the underlying genetic sequence in the fibroblasts taken from scalp. De novo variants were called directly from the RNAseq data, and after filtering by many quality metrics (see Methods) we identified 64 high-confidence candidate variants that were discordant by sampling location in at least a single individual (S9 Table), including 22 annotated coding variants (13 synonymous and 9 non- synonymous) [42]. We found no association between coding variant burden and subject age (p = 0.71, S10 Fig). These results suggest that many of the location- and age-associated DNAm differences are not due to somatic mosaicism and likely arise through epigenetic mechanisms that are maintained through cell culture and multiple passages.

Human tissue collection

Human dural and scalp fibroblasts on which the methylation and gene expression studies were performed were obtained from fibroblast lines derived from human post mortem scalp and dura mater tissues. For this study, tissues from 11 individuals were used, with the ages of individuals ranging from 0.1 to 85 years of age (see S1 Table for additional demographics). The post-mortem tissues from 2 of the subjects were collected by the Lieber Institute for Brain Development (LIBD) and the tissues from the remaining 9 subjects were collected by National Institute for Mental Health (NIMH) (Clinical Brain Disorders Branch (CBDB), Division of Intramural Research Programs (DIRP)). The NIMH tissues were collected from two medical examiners (Washington, DC office and Commonwealth of Virginia, Northern District office); the LIBD tissues were obtained the Office of the Chief Medical Examiner (Baltimore, MD). A preliminary neurological or psychiatric diagnosis was given to each case after demographic, medical, and clinical histories were gathered via a telephone screening on the day of donation. For each case, the postmortem interval (PMI) (the time (in hours) elapsed between death and tissue freezing) was recorded. (See S1 Table for PMIs and demographics for every subject used in this study). Every case underwent neuropathological examinations to screen for neurological pathology. Additionally, the medical examiner’s office performed toxicology analysis of every subject’s blood to screen for drugs.

Dura and scalp tissue were collected at the time of autopsy. From the autopsy room, the tissues were transported in separate bags: one containing cerebral dura mater and the other a 1 in X 1 in scalp segment with hair attached. Both bags were transported on wet ice to the lab, where the culture procedure was immediately started.

Scalp and dura tissue cultures

The dura culture medium was prepared out of 1X DMEM (Ref#11960–044, GIBCO) with 10% by volume fetal bovine serum, 2% by volume 100X GlutaMAX (Cat#: 35050, GIBCO), 1% by volume Penicillin-Streptomycin/Amphotercin solution (Ref# 15140–122, GIBCO), and 1% by volume Gentamicin solution (Cat# 17105–041, Quality Biological). This culture medium was used in all subsequent steps of the dura culturing procedure. The scalp culture medium used for all subsequent steps of the scalp culturing procedure was made the same way except without the 1% Gentamycin. A rinsing solution was prepared out of 1X PBS (pH 7.2) (Ref# 21-040-CV, Corning Life Sciences), 1% by volume Penicillin-Streptomycin/Amphotericin solution (Ref# 15140–122, GIBCO), and 1% by volume Gentamicin (Cat# 17105–041, Quality Biological).

The dissected scalp sample was washed with the rinsing solution three times, the fat tissues were cut away, and all hair was plucked out with forceps. The scalp sample was then placed epidermis side down on a dish and floated with Dispase II enzyme solution (2.4 units of the Dispase II enzyme per mL of PBS, Dispase II enzyme: Cat#17105–041, GIBCO). (Dispase II enzyme is a proteolytic enzyme used to separate the dermis from the epidermis by cleaving the zone of the basement membrane.) The dish was covered with parafilm and foil, and placed in a 37°C incubator for 24 hours. After the 24-hour period, the epidermis was peeled away from the dermis. The dermis was washed with the rinsing solution, dried, and cut into 2–3 mm² pieces. The pieces were placed in a Falcon Easy Grip tissue culture 35×10 mm dish and one drop of scalp culture medium was added to each piece of scalp. The dish was placed in the incubator at 37°C and 5% CO₂ for culturing.

A similar procedure was followed for the dura samples. Dura samples were washed with the rinsing solution three times. Then, a few 2–3 mm² pieces were cut from the dura mater and placed together in an Easy Grip cell culture 35×10 mm dish. One drop of dura culture medium was added to each dura piece. The culture dish was then placed in an incubator (at 37°C and 5% CO₂) for culturing. The medium of each culture was changed to fresh medium 2–3 times per week to promote growth of the fibroblasts. On average, fibroblast cells started to proliferate at 7–14 days, however some samples took longer (up to 3 weeks).

Fibroblast cell cultures

The dura and scalp tissue cultures were monitored under a phase-contrast microscope. When the fibroblast growth reached 90–95% confluence, 1 mL of a 0.25% trypsin solution (Cat#T4049, Sigma) was added to each culture dish, and the cells were incubated for 5 to 8 min. Then, 1mL of media was added to each dish stop the enzymatic reaction. Next, the contents of each culture dish were transferred into separate 15 mL Falcon conical tubes and 8mL of media was added to each tube. The conical tubes were centrifuged for 5 min at 1100 rpm. The supernatant was discarded, 5mL of fresh media was added to each conical tube, and the contents of the tubes were transferred onto separate 25 cm³ cell culture Easy Flasks (Thermo Scientific, Cat# 156367), where they were kept in cultures for 3–5 days in an incubator (at 37°C and 5% CO₂). When the cells reached 90–95% confluence, the cells from each 25 cm³ flask were transferred onto two 75 cm³ cell culture easy flasks (Thermo Scientific, Cat# 156499) and kept in cultures for continued growth. When the cells reached 90–95% confluence, they were incubated with 3 mL of 0.25% trypsin solution for 5 to 8 min, after which 3mL of fresh culture media was added to stop the enzymatic reaction. Then, the contents of the flasks were transferred into separate 15 mL Falcon conical tube and 4mL of media was added to each tube. The tubes were centrifuged (5 min, 1100 rpm), the supernatant was discarded and the pellets containing the fibroblasts were removed from the centrifuge tubes and transferred to cryoTube vials (Cat#375418, Thermo Scientific). 0.5 mL of recovery cell culture freezing medium (Cat#12648–010, GIBCO) was added to each vial, after which the vials were insulated with Styrofoam and placed into a -80°C freezer. Later, the tubes were transferred to a -152°C liquid nitrogen freezer.

These frozen dura and scalp fibroblast cells were then used generate DNA methylation and gene expression levels. Genomic DNA was extracted from approximately 3 million cultured human fibroblast cells using the AllPrep DNA/RNA/miRNA Universal Kit (Qiagen). Bisulfite conversion was performed on 600 ng genomic DNA was done with the EZ DNA methylation kit (Zymo Research).

DNA methylation data generation

DNA methylation landscapes of the dura- and scalp-derived fibroblasts were analyzed using the Illumina HumanMethylation 450 BeadChip array (“450k”). The 450k array interrogates >485,000 DNA methylation sites (probes) and measures the proportion DNA methylation at each target site (the 450k array interrogates both CpG and CH sites). The microarray preparation and scanning were performed in accordance with the manufacturer’s protocols. The resulting data from the 450k consists of R(ed) and G(reen) intensities using two different probe chemistries [22], which we converted to M(ethylated) and U(nmethylated) intensities using the minfi Bioconductor package [23], version 1.14.0 using with R version3.2. One dura sample had lower median probe intensities and was removed prior to normalization and downstream analyses. After quality control (QC), the M and U intensities were normalized separately across samples using stratified quantile normalization [23]. Probes containing common SNPs (based on dbSNP 142) at the target CpG or single base extension site, and probes on the sex chromosomes were removed, leaving 456,513 probes on 21 samples for analysis.

Differential methylation analysis

We determined differential methylation using linear modeling on the normalized DNAm levels, using the model: (1) where y_ij is the normalized proportion methylation at probe i and sample j, α_i is the proportion methylation in the fibroblasts sampled from the dura mater, β_j is the difference in methylation in the scalp-derived fibroblast, and Loc_j is the sampling location represented by a binary variable (Dura = 0, Scalp = 1). These statistical models were adjusted for surrogate variables (6 SVs) estimated using surrogate variable analysis (SVA) [24].

Differentially methylation probes (DMPs) were identified by fitting Eq 1 to each probe, and obtaining the corresponding moderate t-statistic and p-value using the limma package [47]. P-values were adjusted for multiple testing using the false discovery rate (FDR) [48] and significant probes were called were FDR < 0.05. Principal component analysis (PCA) was performed after regressing out the surrogate variables from the DNAm levels of each probe, preserving the effect of fibroblast sampling location. Finding differentially methylated regions (DMRs) involves identifying contiguous probes where β ≠ 0 using the bumphunter Bioconductor package (version 1.6.0) [25], here requiring |β| > 0.1 (argument: cutoff = 0.1) and assessing statistical significance using linear modeling bootstrapping with 1000 iterations (argument: nullMethod = ‘bootstrap’ and B = 1000). DMRs were called statistically significant when the family wise error rate (FWER) ≤ 0.1. We identified blocks using the same model as above using the blockFinder function in the minfi package [23], which collapses nearby CpGs into a single measurement per sample, and then fits Eq.1 above, only here j represents probe group, not probe. Here we again required at least a 10% change in DNAm between groups and assessed statistical significance using the FWER based on 1000 iterations of the linear model bootstrap.

RNA extraction and sequencing

RNA was extracted from the cultured dura and scalp fibroblasts with the RNeasy kit (Qiagen), in accordance with the manufacturer’s protocol. RNA molecules were treated with DNase, polyadenylated (polyA+) RNA was isolated, and resulting sequencing libraries were constructed using the Illumina TruSeq RNA Sample Preparation Kit (v2) and sequenced on an Illumina HiSeq 2000. We note that while all samples were run on the same flow cell, the samples were somewhat imbalanced by lane–however, the first PC of the expression data did separate perfectly by sampling location. Sample-specific information on reads and alignments are available in S1 Table.

RNA-seq data generation

Resulting reads were mapped to the genome using TopHat2 [31] using the paired-ends procedure (we used the option—library-type fr-firststrand). Gene counts relative to the UCSC hg19 knownGene annotation were calculated using the featureCounts script of the Subread package (version 1.4.6) [32]. There were 23,710 genes in this annotation, and we dropped 305 genes that were annotated to more than 1 chromosome. Of the remaining 23,405 genes, 18,316 genes had non-zero expression counts in at least one sample. Counts were converted to FPKM (fragments per kilobase per million reads mapped) values to allow comparisons across genes with different lengths and libraries sequenced to different depths. These FPKMs were transformed prior to statistical analysis: log₂(FPKM + 1). The log transformed FPKM values were used in all subsequent gene-level analyses.

Next, we used the Sailfish software (33), version 0.7.6, to quantify isoforms from our RNA-seq reads. As a result, we obtained TPM (transcripts per million) values for each isoform, which we log transformed: log₂(TPM + 1). The log transformed TPM values were used in all subsequent transcript-level analyses.

RNA-seq data analysis

Differential expression for sampling location was identified using Eq 1 above, where y_ij represents transformed expression (rather than DNAm) levels, and different SVs (N = 4) were calculated from the expression data.

To test whether we could use a subset of genes to cluster our fibroblasts by sampling location, like reported by Rinn et all [17], we took the 337 genes published by the authors, which they found to group fibroblasts by anatomical location. Of these 337, we used only 210 genes, since a subset of the tabulated genes did not contain gene symbols, another subset was not interrogated by our RNAseq, and yet another subset was not expressed in any of our samples. We then perfumed Euclidean distance computations and clustering analysis by first using these 210 genes and then repeating the analysis 1000 times using 210 randomly chosen genes.

We carried out gene ontology analysis on the differentially expressed genes with the GOstats package [49]. Transformed FPKMs were next used to assess functional significance of differentially methylated features. We mapped the DMPs to genes in the UCSC knownGenes (hg19) and determined which DMPs exhibit correlation between DNAm and gene expression with the MatrixEQTL package [50]. We used Pearson's Chi-squared test with Yates' continuity correction to examine whether DMPs are more likely to exhibit correlations between DNAm and gene expression than non-DMPs. We then mapped significant DMRs to genes expressed in the RNA-seq data (e.g. showing non-zero expression levels in ≥ 1 samples), and correlated the average DNAm level within the DMR to the transformed expression level. When multiple genes were within or near a DMR, we retained the gene (and its correlation) with the largest absolute correlation. We carried out gene ontology analysis for the genes proximal to DMRs with the GOstats package. For each significant block, we found the UCSC annotated gene(s) containing within the block and their evidence for differential expression as calculated above. We used Pearson's Chi-squared test with Yates' continuity correction to test whether differentially expressed genes were enriched in blocks compared to the rest of the transcriptome. Finally, we analyzed the directionality of DNAm—expression correlations for DMPs and DMRs, as a function of DMR/DMP positions relative to genes. We used the binomial test to access the significance of distributions between positive and negative correlations of DNAm and gene expression.

In addition to gene-level analysis, we studied transcript-level expression and its correlation with DNAm. We carried out the same analysis for isoform expression as for gene-level expression, with the exception that here we used relative isoform abundance values that we obtained with the Sailfish software (see above).

Chromatin state analysis

The 18-chromatin state data, derived using hidden Markov models (HMMs), was obtained for 4 fibroblast samples: samples E055 and E056 (foreskin primary fibroblasts), E126 (adult dermal fibroblast), and E128 (lung fibroblsts) in the Epigenome Roadmap project22 (http://egg2.wustl.edu/roadmap/web_portal/chr_state_learning.html). The chromatin states overlapping DMPs, DMRs, and blocks were obtained, and compared to a background of all 450k probes, considered probe groups, and collapsed probe groups respectively. Overlap was assessed based on the total coverage (in base pairs) of the chromatin states. Fold changes for enrichment of > 1.5 fold were highlighted. Prior to carrying out the enrichment analysis, the sex chromosomes and the mitochondrial chromosome were dropped.

Processing of public data and distance calculations

We performed a second larger data processing and normalization procedure on our scalp- and dura-derived fibroblasts after adding data from skin fibroblasts (GSE52025) [19], pure populations of blood [20] and prefrontal cortex cells [21] from the FlowSorted.Blood.450k and FlowSorted.DLPFC.450k Bioconductor packages respectively, and then melanoma data from TCGA [37]. The M and U channels were combined across all experiments and then normalized with stratified quantile normalization as described above. We then dropped the probes on the sex chromosomes as well as probes that are common SNPs (based on dbSNP 142) as described above. Within the normalized data, we then calculated all pairwise Euclidean distances on the proportion methylation scale, and selected specific comparisons to display in Fig 4.

Differential variability and age related changes by tissue type

We calculated differential variability between scalp and dura CpG DNAm levels using the Levene test [51] and subsequent p-values were adjusted for multiple testing using the FDR. We filtered out the 101,989 genome-wide significant probes showing mean methylation differences by sampling location, as there is a strong mean-variation relationship in DNAm data due to being constrained within 0 and 1 (e.g. gaining methylation from an unmethylated state or losing methylation from a fully methylated state increases variance).

We tested for probes that showed differential age-related divergence in DNAm by fibroblast sampling location. First, we calculated the difference in DNAm between scalp- and dura-derived fibroblasts from the same individual at every probe (creating a 456,513 probe by 10 individual matrix). We then computed 3 surrogate variables (the number estimated by the SVA algorithm) for a statistical model with donor age, and fit the following linear model: (2) where Δy_ji is the difference in DNAm levels between scalp and dura for probe i and individual j, γ_i is the difference in DNAm levels at birth, Age_i is the age of the donor, and δ_i is the change in the difference of DNAm per year of life. We then generated a Wald statistic and corresponding p-value for δ_i and adjusted for multiple testing via the FDR. Post hoc age-related changes, e.g. the change in DNAm levels per year of life, were calculated within the scalp and dura samples. We then associated expression of nearby genes (within 5kb) with the DNAm levels at the probes showing significant age-by-location effects and performed gene ontology on the significant genes with the GOstats package [49]. We lastly computed the “DNAm age” of our scalp and dura samples using the R code published by S. Horvath, (available at https://labs.genetics.ucla.edu/horvath/dnamage/) and fit a linear model containing main effects of biological age and sampling location, and an interaction term between these two variables on “DNAm age”.

Variant calling

We called expression variants directly from the RNA sequencing alignments using samtools (version 1.1) and mpileup across all samples [52]. We then filtered variants in the resulting variant call format (VCF) file based on coverage (<20), variant distance bias (p<0.05), read position bias (p<0.05), mapping quality bias (p<0.05), base quality bias (p<0.05), inbreeding coefficient binomial test (p<0.05), and homozygote bias (p>0.05). The resulting 64 high quality variants were annotated with SeattleSeq138 [42].

Study approval

For every subject from whom the post-mortem tissues were collected, informed consent was obtained verbally from the legal next-of-kin using a telephone script, and was both witnessed and audiotaped, in accordance with the IRB approved NIMH protocol 90-M-0142 and the Department of Health and Human Services for the State of Maryland (protocol # 12–24).

Data availability

DNA methylation data in both raw and processed forms are available on the Gene Expression Omnibus (GEO): GSE77136. RNA sequencing reads (raw data) are available on the Sequencing Read Archive (SRA): SRP068304 (BioProject: PRJNA286856) and the genes and transcript counts (processed data) are available on GEO at the above accession number (GSE77136).