Your search keyword '"Greally JM"' showing total 9 results

1. Post-conversion targeted capture of modified cytosines in mammalian and plant genomes.

Author

Li Q, Suzuki M, Wendt J, Patterson N, Eichten SR, Hermanson PJ, Green D, Jeddeloh J, Richmond T, Rosenbaum H, Burgess D, Springer NM, and Greally JM

Subjects

Alleles, Animals, Cell Line, Cytosine analysis, DNA Methylation, Genomics methods, Humans, Mice, Polymorphism, Single Nucleotide, Sulfites, 5-Methylcytosine analysis, Cytosine analogs & derivatives, Genome, Plant, High-Throughput Nucleotide Sequencing methods, Sequence Analysis, DNA methods

Abstract

We present a capture-based approach for bisulfite-converted DNA that allows interrogation of pre-defined genomic locations, allowing quantitative and qualitative assessments of 5-methylcytosine (5mC) and 5-hydroxymethylcytosine (5hmC) at CG dinucleotides and in non-CG contexts (CHG, CHH) in mammalian and plant genomes. We show the technique works robustly and reproducibly using as little as 500 ng of starting DNA, with results correlating well with whole genome bisulfite sequencing data, and demonstrate that human DNA can be tested in samples contaminated with microbial DNA. This targeting approach will allow cell type-specific designs to maximize the value of 5mC and 5hmC sequencing., (© The Author(s) 2015. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2015

2. Genome-wide hydroxymethylation tested using the HELP-GT assay shows redistribution in cancer.

Author

Bhattacharyya S, Yu Y, Suzuki M, Campbell N, Mazdo J, Vasanthakumar A, Bhagat TD, Nischal S, Christopeit M, Parekh S, Steidl U, Godley L, Maitra A, Greally JM, and Verma A

Subjects

5-Methylcytosine analysis, Animals, Cell Line, Tumor, Cell Transformation, Neoplastic, Cytosine analysis, Cytosine metabolism, Gene Expression, Genome, Human, Genomics methods, Glycosyltransferases metabolism, Humans, Mice, Pancreatic Neoplasms genetics, Polymerase Chain Reaction, Cytosine analogs & derivatives, DNA, Neoplasm chemistry

Abstract

5-hydroxymethylcytosine (5-hmC) is a recently discovered epigenetic modification that is altered in cancers. Genome-wide assays for 5-hmC determination are needed as many of the techniques for 5-methylcytosine (5-mC) determination, including methyl-sensitive restriction digestion and bisulfite sequencing cannot distinguish between 5-mC and 5-hmC. Glycosylation of 5-hmC residues by beta-glucosyl transferase (β-GT) can make CCGG residues insensitive to digestion by MspI. Restriction digestion by HpaII, MspI or MspI after β-GT conversion, followed by adapter ligation, massive parallel sequencing and custom bioinformatic analysis allowed us determine distribution of 5-mC and 5-hmC at single base pair resolution at MspI restriction sites. The resulting HpaII tiny fragment Enrichment by Ligation-mediated PCR with β-GT (HELP-GT) assay identified 5-hmC loci that were validated at global level by liquid chromatography-mass spectrometry (LC-MS) and the locus-specific level by quantitative reverse transcriptase polymerase chain reaction of 5-hmC pull-down DNA. Hydroxymethylation at both promoter and intragenic locations correlated positively with gene expression. Analysis of pancreatic cancer samples revealed striking redistribution of 5-hmC sites in cancer cells and demonstrated enrichment of this modification at many oncogenic promoters such as GATA6. The HELP-GT assay allowed global determination of 5-hmC and 5-mC from low amounts of DNA and with the use of modest sequencing resources. Redistribution of 5-hmC seen in cancer highlights the importance of determination of this modification in conjugation with conventional methylome analysis.

Published

2013

3. Cytosine methylation changes in enhancer regions of core pro-fibrotic genes characterize kidney fibrosis development.

Author

Ko YA, Mohtat D, Suzuki M, Park AS, Izquierdo MC, Han SY, Kang HM, Si H, Hostetter T, Pullman JM, Fazzari M, Verma A, Zheng D, Greally JM, and Susztak K

Subjects

Aged, Base Sequence, Binding Sites, Case-Control Studies, Cluster Analysis, DNA Methylation, Fibrosis, Gene Expression Profiling, Gene Regulatory Networks, Humans, Middle Aged, Nucleotide Motifs, Position-Specific Scoring Matrices, Renal Insufficiency, Chronic genetics, Renal Insufficiency, Chronic pathology, Reproducibility of Results, Transcription Factors, Transcription, Genetic drug effects, Cytosine metabolism, Enhancer Elements, Genetic, Gene Expression Regulation drug effects, Kidney metabolism, Kidney pathology

Abstract

Background: One in eleven people is affected by chronic kidney disease, a condition characterized by kidney fibrosis and progressive loss of kidney function. Epidemiological studies indicate that adverse intrauterine and postnatal environments have a long-lasting role in chronic kidney disease development. Epigenetic information represents a plausible carrier for mediating this programming effect. Here we demonstrate that genome-wide cytosine methylation patterns of healthy and chronic kidney disease tubule samples obtained from patients show significant differences., Results: We identify differentially methylated regions and validate these in a large replication dataset. The differentially methylated regions are rarely observed on promoters, but mostly overlap with putative enhancer regions, and they are enriched in consensus binding sequences for important renal transcription factors. This indicates their importance in gene expression regulation. A core set of genes that are known to be related to kidney fibrosis, including genes encoding collagens, show cytosine methylation changes correlating with downstream transcript levels., Conclusions: Our report raises the possibility that epigenetic dysregulation plays a role in chronic kidney disease development via influencing core pro-fibrotic pathways and can aid the development of novel biomarkers and future therapeutics.

Published

2013

4. Late-replicating heterochromatin is characterized by decreased cytosine methylation in the human genome.

Author

Suzuki M, Oda M, Ramos MP, Pascual M, Lau K, Stasiek E, Agyiri F, Thompson RF, Glass JL, Jing Q, Sandstrom R, Fazzari MJ, Hansen RS, Stamatoyannopoulos JA, McLellan AS, and Greally JM

Subjects

Cell Line, Gene Expression Profiling, Gene Expression Regulation, Humans, Time Factors, Transcription, Genetic, Cytosine metabolism, DNA Methylation, DNA Replication, Genome, Human, Heterochromatin metabolism

Abstract

Heterochromatin is believed to be associated with increased levels of cytosine methylation. With the recent availability of genome-wide, high-resolution molecular data reflecting chromatin organization and methylation, such relationships can be explored systematically. As well-defined surrogates for heterochromatin, we tested the relationship between DNA replication timing and DNase hypersensitivity with cytosine methylation in two human cell types, unexpectedly finding the later-replicating, more heterochromatic regions to be less methylated than early replicating regions. When we integrated gene-expression data into the study, we found that regions of increased gene expression were earlier replicating, as previously identified, and that transcription-targeted cytosine methylation in gene bodies contributes to the positive correlation with early replication. A self-organizing map (SOM) approach was able to identify genomic regions with early replication and increased methylation, but lacking annotated transcripts, loci missed in simple two variable analyses, possibly encoding unrecognized intergenic transcripts. We conclude that the relationship of cytosine methylation with heterochromatin is not simple and depends on whether the genomic context is tandemly repetitive sequences often found near centromeres, which are known to be heterochromatic and methylated, or the remaining majority of the genome, where cytosine methylation is targeted preferentially to the transcriptionally active, euchromatic compartment of the genome.

Published

2011

5. Cytosine methylation dysregulation in neonates following intrauterine growth restriction.

Author

Einstein F, Thompson RF, Bhagat TD, Fazzari MJ, Verma A, Barzilai N, and Greally JM

Subjects

Hepatocyte Nuclear Factor 4 genetics, Humans, In Situ Hybridization, Fluorescence, Infant, Newborn, Polymerase Chain Reaction, Promoter Regions, Genetic, Cytosine metabolism, DNA Methylation, Fetal Growth Retardation genetics

Abstract

Background: Perturbations of the intrauterine environment can affect fetal development during critical periods of plasticity, and can increase susceptibility to a number of age-related diseases (e.g., type 2 diabetes mellitus; T2DM), manifesting as late as decades later. We hypothesized that this biological memory is mediated by permanent alterations of the epigenome in stem cell populations, and focused our studies specifically on DNA methylation in CD34+ hematopoietic stem and progenitor cells from cord blood from neonates with intrauterine growth restriction (IUGR) and control subjects., Methods and Findings: Our epigenomic assays utilized a two-stage design involving genome-wide discovery followed by quantitative, single-locus validation. We found that changes in cytosine methylation occur in response to IUGR of moderate degree and involving a restricted number of loci. We also identify specific loci that are targeted for dysregulation of DNA methylation, in particular the hepatocyte nuclear factor 4alpha (HNF4A) gene, a well-known diabetes candidate gene not previously associated with growth restriction in utero, and other loci encoding HNF4A-interacting proteins., Conclusions: Our results give insights into the potential contribution of epigenomic dysregulation in mediating the long-term consequences of IUGR, and demonstrate the value of this approach to studies of the fetal origin of adult disease.

Published

2010

6. Optimized design and data analysis of tag-based cytosine methylation assays.

Author

Suzuki M, Jing Q, Lia D, Pascual M, McLellan A, and Greally JM

Subjects

Base Sequence, Cells, Cultured, Cytosine chemistry, DNA Methylation, DNA-Cytosine Methylases chemistry, DNA-Cytosine Methylases metabolism, Genome, Human, Humans, Polymorphism, Genetic, Site-Specific DNA-Methyltransferase (Adenine-Specific) chemistry, Site-Specific DNA-Methyltransferase (Adenine-Specific) metabolism, Cytosine metabolism, Sequence Analysis, DNA

Abstract

Using the type III restriction-modification enzyme EcoP15I, we isolated sequences flanking sites digested by the methylation-sensitive HpaII enzyme or its methylation-insensitive MspI isoschizomer for massively parallel sequencing. A novel data transformation allows us to normalise HpaII by MspI counts, resulting in more accurate quantification of methylation at >1.8 million loci in the human genome. This HELP-tagging assay is not sensitive to sequence polymorphism or base composition and allows exploration of both CG-rich and depleted genomic contexts.

Published

2010

7. High-resolution genome-wide cytosine methylation profiling with simultaneous copy number analysis and optimization for limited cell numbers.

Author

Oda M, Glass JL, Thompson RF, Mo Y, Olivier EN, Figueroa ME, Selzer RR, Richmond TA, Zhang X, Dannenberg L, Green RD, Melnick A, Hatchwell E, Bouhassira EE, Verma A, Suzuki M, and Greally JM

Subjects

Cells, Cultured, DNA chemistry, Deoxyribonuclease HpaII, Genome, Human, Humans, Cytosine metabolism, DNA analysis, DNA Methylation, Polymerase Chain Reaction methods

Abstract

Many genome-wide assays involve the generation of a subset (or representation) of the genome following restriction enzyme digestion. The use of enzymes sensitive to cytosine methylation allows high-throughput analysis of this epigenetic regulatory process. We show that the use of a dual-adapter approach allows us to generate genomic representations that includes fragments of <200 bp in size, previously not possible when using the standard approach of using a single adapter. By expanding the representation to smaller fragments using HpaII or MspI, we increase the representation by these isoschizomers to more than 1.32 million loci in the human genome, representing 98.5% of CpG islands and 91.1% of refSeq promoters. This advance allows the development of a new, high-resolution version of our HpaII-tiny fragment Enrichment by Ligation-mediated PCR (HELP) assay to study cytosine methylation. We also show that the MspI representation generates information about copy-number variation, that the assay can be used on as little as 10 ng of DNA and that massively parallel sequencing can be used as an alternative to microarrays to read the output of the assay, making this a powerful discovery platform for studies of genomic and epigenomic abnormalities.

Published

2009

8. An analytical pipeline for genomic representations used for cytosine methylation studies.

Author

Thompson RF, Reimers M, Khulan B, Gissot M, Richmond TA, Chen Q, Zheng X, Kim K, and Greally JM

Subjects

Artifacts, Reproducibility of Results, Sensitivity and Specificity, Chromosome Mapping methods, Cytosine, DNA Methylation, Oligonucleotide Array Sequence Analysis methods, Polymerase Chain Reaction methods, Sequence Analysis, DNA methods, Software

Abstract

Motivation: Representations of the genome can be generated by the selection of a subpopulation of restriction fragments using ligation-mediated PCR. Such representations form the basis for a number of high-throughput assays, including the HELP assay to study cytosine methylation. We find that HELP data analysis is complicated not only by PCR amplification heterogeneity but also by a complex and variable distribution of cytosine methylation. To address this, we created an analytical pipeline and novel normalization approach that improves concordance between microarray-derived data and single locus validation results, demonstrating the value of the analytical approach. A major influence on the PCR amplification is the size of the restriction fragment, requiring a quantile normalization approach that reduces the influence of fragment length on signal intensity. Here we describe all of the components of the pipeline, which can also be applied to data derived from other assays based on genomic representations.

Published

2008

9. Comparative isoschizomer profiling of cytosine methylation: the HELP assay.

Author

Khulan B, Thompson RF, Ye K, Fazzari MJ, Suzuki M, Stasiek E, Figueroa ME, Glass JL, Chen Q, Montagna C, Hatchwell E, Selzer RR, Richmond TA, Green RD, Melnick A, and Greally JM

Subjects

Animals, CpG Islands, Genome, In Situ Hybridization, Fluorescence, Mice, Multigene Family, Nucleic Acid Hybridization, Promoter Regions, Genetic, Reverse Transcriptase Polymerase Chain Reaction, Cytosine metabolism, DNA Methylation

Abstract

The distribution of cytosine methylation in 6.2 Mb of the mouse genome was tested using cohybridization of genomic representations from a methylation-sensitive restriction enzyme and its methylation-insensitive isoschizomer. This assay, termed HELP (HpaII tiny fragment Enrichment by Ligation-mediated PCR), allows both intragenomic profiling and intergenomic comparisons of cytosine methylation. The intragenomic profile shows most of the genome to be contiguous methylated sequence with occasional clusters of hypomethylated loci, usually but not exclusively at promoters and CpG islands. Intergenomic comparison found marked differences in cytosine methylation between spermatogenic and brain cells, identifying 223 new candidate tissue-specific differentially methylated regions (T-DMRs). Bisulfite pyrosequencing confirmed the four candidates tested to be T-DMRs, while quantitative RT-PCR for two genes with T-DMRs located at their promoters showed the HELP data to be correlated with gene activity at these loci. The HELP assay is robust, quantitative, and accurate and is providing new insights into the distribution and dynamic nature of cytosine methylation in the genome.

Published

2006