Your search keyword '"Ramsahoye, Bernard"' showing total 78 results

51. Extracting DNA Demethylase Activity from MamMalian Cells.

Author

Walker, John M., Mills, Ken I., Ramsahoye, Bernard H., Szyf, Moshe, and Bhattacharya, Sanjoy K.

Abstract

Purification of an enzymatic activity requires a simple and relatively expeditious assay of its activity. However, the nature of the demethylase reaction has been elusive for decades. Although a large body of evidence supported the hypothesis that active demethylation takes place during development and differentiation (1), the nature of the reaction was unknown. The main problem with understanding demethylaion of DNA is that true demethylation of DNA would involve cleavage of a stable carbon-carbon bond, which had been considered highly unlikely. Different laboratories have suggested that demethylation of DNA is accomplished by different repair mechanisms. These alternative routes involve either a cleavage of the bond between the methylated cytosine base and the deoxyribose (2) or nucleotide excision (3) (Fig. 1). We have recently shown that mamMalian cancer-cell lines bear a bona fide demethylase activity and we defined the reactants and products of the demethylation reaction. The demethylation reaction involves the hydrolytic cleavage of the bond between the methyl-carbon and the carbon at the 5 position of the cytosine ring (Fig. 1 and Fig. 2) producing unmethylated cytosine while the methyl group is released as methanol (4). [ABSTRACT FROM AUTHOR]

Published

2002

52. Measuring DNA Demethylase Activity In Vitro.

Author

Walker, John M., Mills, Ken I., Ramsahoye, Bernard H., Szyf, Moshe, and Bhattacharya, Sanjoy K.

Abstract

The reaction catalyzing direct demethylation of DNA involves the removal of a methyl group residue from the 5′ position on cytosine; the products of the reaction are nonmethylated cytosine in the dinucleotide CpG and methanol (1). The study of the proteins involved in demethylation requires an assay for measuring enzymatic DNA demethylation. A number of assays were previously described for determining the state of methylation of CpG sequences DNA. For example, certain restriction enzymes such as HpaII or HhaI recognize subsets of CpG sequences only when the C is not methylated; thus, cleavage by this enzymes indicates demethylation of their recognition sequences (2) This assay is, however, obviously indirect and can only measure the state of methylation of a subset of CG sequences contained in the enzyme-specific recognition site. An additional problem is that this assay does not differentiate between DNA that is directly demethylated, and repair processes that remove methylated cytosines in DNA and replace them with other unmethylated cytosines found in the extracts. An additional assay is the bisulfite-mapping method, which can determine the state of methylation of cytosines at a single nucleotide resolution (3). This assay is based on the fact that nonmethylated cytosines are modified by bisulfite and converted to thymidine, whereas methylated cytosines are protected. This assay, similar to the restriction enzyme-based assays, is indirect; it does not measure demethylation but rather the conversion of cytosines. [ABSTRACT FROM AUTHOR]

Published

2002

53. DNA-Methylation Analysis by the Bisulfite-Assisted Genomic Sequencing Method.

Author

Walker, John M., Mills, Ken I., Ramsahoye, Bernard H., Hajkova, Petra, El-Maarri, Osman, Engemann, Sabine, Oswald, Joachim, Olek, Alexander, and Walter, Jörn

Abstract

The postreplicative methylation of DNA at the C5 position of cytosines is found in a broad spectrum of organisms ranging from prokaryotes to human (1). In prokaryotes the major role of cytosine C5 methylation (like adenine N6 and cytosine N4 methylation) is to protect the genome against DNA degrading nucleases (restriction/modification), whereas in many eukaryotes cytosine C5 methylation (found within CpG dinucleotides) plays a pivotal role in the control of gene expression, inactivation of repetitive sequences, stability of chromosomes, and in cell transformation leading to development of cancer. The growing evidence that the cytosine methylation is also crucial in embryonic development of mammals regulating genomic imprinting, X inactivation and cell differentiation (2) has caused a demand for effective methods that would detect this modification with high sensitivity and reliability. [ABSTRACT FROM AUTHOR]

Published

2002

54. Purification of MeCP2-Containing Deacetylase from Xenopus laevis.

Author

Walker, John M., Mills, Ken I., Ramsahoye, Bernard H., Jones, Peter L., Wade, Paul A., and Wolffe, Alan P.

Abstract

DNA methylation has long been associated with stable transcriptional silencing and a repressive chromatin structure (review refs. 1,2). Differential methylation is associated with imprinting, carcinogenesis, silencing of repetitive DNA, and allows for differentiating cells to efficiently shut off unnecessary genes. In vertebrates, where 60-90% of genomic CpG dinucleotides are methylated, methylation-dependent repression is vital for proper embryonic development (3). Microinjection experiments using methylated DNA templates implicate chromatin structure as an underlying mechanism of methylation-dependent silencing (4,5). Methyl-specific transcriptional repression requires chromatin assembly, and can be partially relieved by the histone deacetylase inhibitor Trichostatin A. In addition, two proteins have been identified, MeCP1 (6) and MeCP2 (7), that specifically bind to methylated DNA and mediate transcriptional repression. MeCP1 is a relatively uncharacterized complex that requires at least 12 symmetrical methyl-CpGs for DNA binding (6). MeCP2 is a single polypeptide containing a methyl-binding domain capable of binding a single methyl-CpG, and a transcriptional repression domain (8). Recently MeCP2 was shown to interact with the Sin3 corepressor and histone deacetylase (9,10). Changes in the acetylation state of the core histone tails correlates with changes in transcription (reviewed in refs. 11,12), and several transcriptional repression complexes containing histone deacetylases have recently been described (9,13,14) [ABSTRACT FROM AUTHOR]

Published

2002

55. Differential Methylation Hybridization Using CpG Island Arrays.

Author

Walker, John M., Mills, Ken I., Ramsahoye, Bernard H., Yan, Pearlly S., Wei, Susan H., and Huang, Tim Hui-sing

Abstract

Differential hybridization and its related techniques have been developed to identify genes whose expressions are altered during different physiological conditions or in dissimilar cell or tissue types (1-3). High-throughput DNA array technologies have further advanced these analyses, providing for simultaneous examinations of expressions of thousands of genes between two different cell types in a single experiment (4-6). Recently, we have adapted the hybridization approach to devise an array-based technique, called differential methylation hybridization (DMH), to identify changes in DNA methylation patterns commonly observed in cancer (7). Methylation of DNA is the addition of a methyl group to the 5th carbon position of cytosine that is 5′ to a guanine in GC-rich regions known as CpG islands, which are frequently located in the 5′-end of regulatory regions of genes (8,9) This epigenetic reaction does not usually change nucleotide sequences nor affect the specificity of DNA base pairing, but it can have inhibitory effects on gene expression (8,9). [ABSTRACT FROM AUTHOR]

Published

2002

56. Combined Bisulfite Restriction Analysis (COBRA).

Author

Walker, John M., Mills, Ken I., Ramsahoye, Bernard H., Eads, Cindy A., and Laird, Peter W.

Abstract

Most molecular biological techniques used to analyze specific loci in complex genomic DNA involve some form of sequence-specific amplification, whether it is biological amplification by cloning in Escherichia coli, direct amplification by polymerase chain reaction (PCR), or signal amplification by hybridization with a probe that can be visualized. Since DNA methylation is added postreplicatively by a dedicated maintenance DNA methyltransferase that is not present in either E. coli or in the PCR reaction, the methylation information is lost during molecular cloning or PCR amplification. Molecular hybridization does not discriminate between methylated and unmethylated DNA, since the methyl group on the cytosine does not participate in base pairing. The lack of a facile way to amplify the methylation information in complex genomic DNA has been a significant impediment to DNA methylation research. [ABSTRACT FROM AUTHOR]

Published

2002

57. Restriction Landmark Genome Scanning.

Author

Walker, John M., Mills, Ken I., Ramsahoye, Bernard H., Costello, Joseph F., Plass, Christoph, and Cavenee, Webster K.

Abstract

Restriction landmark genomic scanning (RLGS) is a method that provides both a quantitative genetic and epigenetic (cytosine methylation) assessment of thousands of CpG islands in a single gel without prior knowledge of gene sequence (1). The method is a two-dimensional separation of radiolabeled genomic DNA into nearly 2,000 discrete fragments that have a high probability of containing gene sequences and are ideal in length for cloning and sequence analysis. Genomic DNA is digested with an infrequently cutting restriction enzyme such as NotI, radiolabeled at the cleaved ends, digested with a second restriction enzyme, and then electrophoresed through a narrow, 60 cm-long agarose tube-shaped gel. The DNA in the tube gel is then digested by a third, more frequently cutting restriction enzyme and electrophoresed, in a direction perpendicular to the first separation, through a 5% nondenaturing polyacrylamide gel, and the gel is autoradiographed. Radiolabeled NotI sites are frequently used as "landmarks" because Note can not cleave methylated sites and since an estimated 89% of NotI sites are within CpG islands (2). Using a methylation-sensitive enzyme, the technique has been termed RLGS-M (3). The resulting RLGS profile displays both the copy number and methylation status of the CpG islands. These profiles are highly reproducible and are therefore amenable to inter- and intra-individual DNA sample comparisons. [ABSTRACT FROM AUTHOR]

Published

2002

58. Methylation Analysis by Chemical DNA Sequencing.

Author

Walker, John M., Mills, Ken I., Ramsahoye, Bernard H., Szabó, Piroska E., Mann, Jeffrey R., and Pfeifer, Gerd P.

Abstract

The presence of 5-methylcytosine as a modified base in DNA was discovered many decades ago. Surprisingly, however, and despite intense research efforts, the principal function of DNA methylation is still unknown. The CpG dinucleotide is the predominant if not exclusive target sequence for methylation by mammalian DNA methyltransferases. The analysis of DNA methylation at single-nucleotide resolution (genomic sequencing) has long been considered technically difficult, at least in mammalian cells. Recently, techniques have been developed that give a sufficient specificity and sensitivity for analysis of the methylation of single-copy genes by DNA-sequencing techniques (1,2). Currently, the most widely used method is based on bisulfite-induced deamination of cytosines followed by polymerase chain reaction (PCR) and DNA sequencing (2). Chemical DNA sequencing combined with ligation-mediated PCR (LM-PCR) is an alternative method for determination of genomic methylation patterns (1). LM-PCR is based on the ligation of an oligonucleotide linker onto the 5′ end of each DNA molecule that was created by a strand-cleavage reaction during chemical DNA sequencing. This ligation reaction provides a common sequence on all 5′ ends allowing exponential PCR to be used for signal amplification. One microgram of mammalian DNA per lane is more than sufficient to obtain good-quality DNA sequence ladders. The general LM-PCR procedure used for methylation analysis by chemical DNA sequencing is outlined in Fig. 1 [ABSTRACT FROM AUTHOR]

Published

2002

59. Methylation-Sensitive Restriction Fingerprinting.

Author

Walker, John M., Mills, Ken I., Ramsahoye, Bernard H., and Davies, Catherine S.

Abstract

Methylation of cytosine residues is an almost ubiquitous finding of higher organisms (1). The majority of this methylation occurs at the dinucleotide CpG (where p denotes a phosphate group) (2). CpG sites are distributed throughout the genome with clusters of the sequence being found in the 5′ promoter region of housekeeping genes, in groups known as CpG islands. These short stretches of DNA have a have a C and G base composition, which in mammals and avians is estimated to be 10 times higher than in bulk DNA (3) [ABSTRACT FROM AUTHOR]

Published

2002

60. Measurement of Genome-Wide DNA Cytosine-5 Methylation by Reversed-Phase High-Pressure Liquid Chromatography.

Author

Walker, John M., Mills, Ken I., and Ramsahoye, Bernard H.

Abstract

In health, approx 4% of cytosines are methylated. Tissues can vary in their levels of DNA methylation and the overall level is often reduced in malignancy (1). The level of DNA methylation is usually obtained by chromatographic separation of the constituent nucleotide bases or their related deoxyribonucleotides or deoxyribonucleosides, and is usually represented as a fraction of total cytosine. Quantification of 5mC by chromatographic separation of deoxyribonucleotides has the advantage that, as deoxyribonucleotides can be easily distinguished from ribonucleotides, contamination of the DNA by RNA is less likely to cause error. This can be the case if 5mC is assayed after chemical hydrolysis of the DNA to bases. [ABSTRACT FROM AUTHOR]

Published

2002

61. Nearest-Neighbor Analysis.

Author

Walker, John M., Mills, Ken I., and Ramsahoye, Bernard H.

Abstract

Nearest-neighbor analysis can be used to identify the 3′ nearest neighbors of 5mC residues in DNA (1,2). It can also be used to measure the level of methylation of a specific methylated dinucleotide in DNA. Typically, in the case of mammalian DNA, this means quantifying the degree of methylation at CpG dinucleotides. It has the added advantage of being applicable to small samples of the order of 1 microgram of genomic DNA. The only drawback is that it is a radioactive technique and the appropriate facilities and techniques for handling radioactive substances must be available. [ABSTRACT FROM AUTHOR]

Published

2002

62. Overview.

Author

Walker, John M., Mills, Ken I., and Ramsahoye, Bernard H.

Abstract

In the last decade great strides have been made in understanding the molecular biology of the cell. The entire sequence of the human genome, and the entire genomes of a number of other organisms and microorganisms, are now available to researchers on the World Wide Web. As we enter the postgenome era, research efforts will increasingly focus on the mechanisms that control the expression of genes and the interactions between proteins encoded by the genomic DNA. Most of what we know about DNA methylation in mammals indicates that it is likely to be part of a system affecting chromatin structure and transcriptional control. As such, mammalian DNA methylation has traditionally attracted intense research interest from scientists in the fields of Development and Cancer biology. The recent discovery that two human diseases, ICF syndrome (1) (Immunodeficiency, Centromeric region instability, Facial abnormalities) and Rett syndrome (2), a form of X-linked mental retardation, are caused by mutations in genes coding for a methyltransferase and a methyl-CpG binding protein, respectively, has broadened and intensified interest further. This book has been compiled in the hope that it will be a useful technical manual for those in the field of DNA methylation. What follows is a brief review of key facts and developments in the field in the hope that, for the uninitiated, this will help to set the technical chapters in context. [ABSTRACT FROM AUTHOR]

Published

2002

63. DNA methylation in Drosophila melanogaster

Author

Lyko, Frank, primary, Ramsahoye, Bernard H., additional, and Jaenisch, Rudolf, additional

Published

2000

64. DNMT3A mutations at R882 hotspot are only found in major clones of acute myeloid leukemia.

Author

Bisling, Kathrin E., Brewin, John N., McGovern, Andrew P., Horne, Gillian A., Rider, Tom, Stewart, Helen J., Ramsahoye, Bernard H., and Chevassut, Timothy J.

Subjects

GENETIC mutation, ACUTE myeloid leukemia, BONE marrow

Abstract

A letter to the editor is presented that focuses on research on the role of mutations on the gene DNMT3A in initiating events in acute myeloid leukemia (AML), stating that bone marrow samples were studied from 19 patients with AML, and mentions mutations of R882 on DNMT3A were not found in secondary subclones.

Published

2014

65. Mammalian (cytosine-5) methyltransferases cause genomic DNA methylation and lethality in Drosophila

Author

Lyko, Frank, primary, Ramsahoye, Bernard H., additional, Kashevsky, Helena, additional, Tudor, Matthew, additional, Mastrangelo, Mary-Ann, additional, Orr-Weaver, Terry L., additional, and Jaenisch, Rudolf, additional

Published

1999

66. EPSTEIN-BARR VIRUS IN SQUAMOUS CELL CARCINOMA AFTER RENAL TRANSPLANTATION

Author

THOMAS, DAVID W., primary, RAMSAHOYE, BERNARD, additional, JASANI, BHARAT, additional, and LIM, SEAH H., additional

Published

1995

67. The relationship between chromatin structure and transcriptional activity in mammalian genomes.

Author

Gilbert, Nick and Ramsahoye, Bernard

Subjects

*CHROMATIN, *GENETIC transcription, *MAMMALIAN artificial chromosomes, *HUMAN genome, *NUCLEOSIDES

Abstract

In cells, chromatin is folded into a 30 nm fibre. Recent genome-wide studies have shown that DNasel-sensitive sites are present in both transcribed and non-transcribed genes and are enriched in the gene-dense regions of the human genome. The distribution of open chromatin has also been shown to correlate with gene density rather than transcription. In this review it is suggested that open chromatin corresponds to a 30 nm fibre interspersed with discontinuities, and that blocks of open chromatin might facilitate gene transcription, but are neither necessary nor sufficient. The nature of these discontinuities is not known but could correspond to alterations in chromatin fibre structure caused by irregular nucleosome positioning, nucleosome remodelling activities, variant histones or the binding of specific transcription factors. [ABSTRACT FROM AUTHOR]

Published

2005

68. Dnmt1Overexpression Causes Genomic Hypermethylation, Loss of Imprinting, and Embryonic Lethality

Author

Biniszkiewicz, Detlev, Gribnau, Joost, Ramsahoye, Bernard, Gaudet, François, Eggan, Kevin, Humpherys, David, Mastrangelo, Mary-Ann, Jun, Zhan, Walter, Jörn, and Jaenisch, Rudolf

Abstract

Biallelic expression of Igf2is frequently seen in cancers because Igf2functions as a survival factor. In many tumors the activation of Igf2expression has been correlated with de novo methylation of the imprinted region. We have compared the intrinsic susceptibilities of the imprinted region of Igf2and H19, other imprinted genes, bulk genomic DNA, and repetitive retroviral sequences to Dnmt1overexpression. At low Dnmt1methyltransferase levels repetitive retroviral elements were methylated and silenced. The nonmethylated imprinted region of Igf2and H19was resistant to methylation at low Dnmt1levels but became fully methylated when Dnmt1was overexpressed from a bacterial artificial chromosome transgene. Methylation caused the activation of the silent Igf2allele in wild-type and Dnmt1knockout cells, leading to biallelic Igf2expression. In contrast, the imprinted genes Igf2r, Peg3, Snrpn, and Grf1were completely resistant to de novo methylation, even when Dnmt1was overexpressed. Therefore, the intrinsic difference between the imprinted region of Igf2and H19and of other imprinted genes to postzygotic de novo methylation may be the molecular basis for the frequently observed de novo methylation and upregulation of Igf2in neoplastic cells and tumors. Injection of Dnmt1-overexpressing embryonic stem cells in diploid or tetraploid blastocysts resulted in lethality of the embryo, which resembled embryonic lethality caused by Dnmt1deficiency.

Published

2002

69. DNA hypomethylation leads to cGAS-induced autoinflammation in the epidermis

Author

Beck, Mirjam A., Fischer, Heinz, Grabner, Lisa M., Groffics, Tamara, Winter, Mircea, Tangermann, Simone, Meischel, Tina, Zaussinger-Haas, Barbara, Wagner, Patrick, Fischer, Carina, Folie, Christina, Arand, Julia, Schoefer, Christian, Ramsahoye, Bernard, Lagger, Sabine, Machat, Georg, Eisenwort, Gregor, Schneider, Stephanie, Podhornik, Alexandra, Kothmayer, Michael, Reichart, Ursula, Gloesmann, Martin, Tamir, Ido, Mildner, Michael, Sheibani-Tezerji, Raheleh, Kenner, Lukas, Petzelbauer, Peter, Egger, Gerda, Sibilia, Maria, Ablasser, Andrea, and Seiser, Christian

Subjects

skin, epigenetics, innate immune system, methylation causes, dna methylation, autoinflammation, cytosolic dna, stem-cells, self, dnmt1, inflammation, sting pathway, expression, cancer, roles

Abstract

DNA methylation is a fundamental epigenetic modification, important across biological processes. The maintenance methyltransferase DNMT1 is essential for lineage differentiation during development, but its functions in tissue homeostasis are incompletely understood. We show that epidermis-specific DNMT1 deletion severely disrupts epidermal structure and homeostasis, initiating a massive innate immune response and infiltration of immune cells. Mechanistically, DNA hypomethylation in keratinocytes triggered transposon derepression, mitotic defects, and formation of micronuclei. DNA release into the cytosol of DNMT1-deficient keratinocytes activated signaling through cGAS and STING, thus triggering inflammation. Our findings show that disruption of a key epigenetic mark directly impacts immune and tissue homeostasis, and potentially impacts our understanding of autoinflammatory diseases and cancer immunotherapy.

70. EPSTEINBARR VIRUS IN SQUAMOUS CELL CARCINOMA AFTER RENAL TRANSPLANTATION

Author

THOMAS, DAVID W., RAMSAHOYE, BERNARD, JASANI, BHARAT, and LIM, SEAH H.

Published

1995

71. Identifying somatic structural rearrangements in leukaemia by tumour-only paired-end whole genome sequencing

Author

Bibby, Lloyd, Ramsahoye, Bernard, and Gilbert, Nicholas

Abstract

Our understanding of the molecular pathogenesis of acute and chronic leukaemia has been greatly advanced by high-throughput next generation DNA sequencing. Nowadays, lymphoid, and myeloid malignancies are characterised by many somatically acquired genomic structural rearrangements including chromosomal translocations, inversions, large deletions or insertions, and internal tandem duplications, as well as chromosomal copy number changes. The ultimate effect of these is the deregulation of oncogenes or tumour suppressor genes which promotes transformation to disease. Clinically, the presence of structural abnormalities in a leukaemia patient's tumour genome predict treatment response and patient survival, so it is necessary to conduct investigations at presentation to better understand a patient's tumour genome and inform patient risk stratification and care. The detection of the genomic structural rearrangements vital for clinical management are currently detected using conventional cytogenetic analysis (G-banding), and many structural rearrangements can be detected in this manner, but many others are too subtle and evade detection. Gene-centric techniques such as PCR or FISH can focus detection on specific rearrangements to confirm or refute their presence in a genome, but other less common potentially significant rearrangements will be missed simply because they are not known to be looked for. Overall, conventional cytogenetic techniques are laborious and time consuming, and are of inadequate through-put to determine all genomic rearrangements present in a sample with ease. With the development of 2 x 150 bp paired-end whole genome sequencing however, it is theoretically possible to identify all disease-relevant structural abnormalities with base-pair precision and resolution in a single experiment, reducing the cost and time spent per mutation to generate a complete genomic profile from which clinical decisions can be made. Effective whole genome sequencing analysis is not trivial however, and many approaches outside of clinical practice rely on sequencing both a tumour DNA sample and patient-matched germline DNA sample to discriminate the somatic rearrangements from polymorphic structural variants restricted to the tumour. Similarly, paired tumour and germline DNA sequencing is relied upon to limit the number of technical artefacts that otherwise masquerade as structural rearrangements when analysed by the current publicly available structural variant calling algorithms. Without paired-sample DNA sequencing, current computational approaches detect thousands of structural abnormalities in a single patient by comparison to the reference genome. Most of which are simply not real somatic changes and have the potential to mislead and waste resources in their confirmation. However, the collection of a matched germline DNA sample is simply impractical in haematology-oncology as there is no suitable tissue in which to easily sample, limiting the uptake of whole genome sequencing as a suitable replacement for cytogenetics. The associated costs of sequencing a second DNA sample further limits the use of whole genome sequencing in clinical practice also. Therefore, novel methods and analytical approaches for the detection of structural rearrangements in leukaemia without a germline DNA sample in which to compare to is an unmet clinical need. To that end, we have developed a computational method to detect and identify somatic structural rearrangements of clinical significance in leukaemia, using a tumour-only paired-end whole genome sequencing approach. This approach was developed using a 64-core computer server to enable massively parallel data processing, but the algorithm is scalable and can be implemented on systems with fewer resources. This approach uses discordant and split reads to identify and model structural rearrangements in paired-end whole genome sequencing data but differs from other less specific algorithms because it performs a series of internal validation steps to identify only those discordant split reads that give reliable evidence of structural rearrangement. To identify structural polymorphisms which persist after structural variant detection, each putative breakpoint sequence is compared with publicly available databases of polymorphic structural variation. This approach has been tested on 17 tumour-only leukaemia samples obtained at presentation and demonstrates a higher rate of specificity than the current structural variant algorithms available. It also exceeds the level of sensitivity of cytogenetics. This work demonstrates the superiority of whole genome sequencing in a clinical setting, and the ease of which tumour-only whole genome sequencing analysis can be conducted routinely in clinical haematology-oncology.

Published

2021

72. Investigating epigenetic mechanisms of acquired endocrine resistance in an in vitro model of breast cancer

Author

Skerry, Benjamin James Oliver, Ramsahoye, Bernard, and Gilbert, Nick

Subjects

epigenetics, methylation, breast cancer, fulvestrant

Abstract

I have investigated epigenetic mechanisms of acquired endocrine-resistance in breast cancer using an in vitro model system based on estrogen-dependent MCF7 cells and their derivatives, LCC1 and LCC9. LCC1 cells, derived from MCF7 after passage in ovariectomised mice and routinely cultured in vitro in the absence of estrogen, exhibit estrogen-independent growth. They retain sensitivity to tamoxifen and fulvestrant. LCC9 cells, derived from LCC1 cells by growing them in increasing concentrations of fulvestrant, are completely estrogen-independent and are resistant to fulvestrant and cross-resistant to tamoxifen. When compared to MCF7 cells, LCC1 cells have marked up-regulation of the estrogen receptor α (ERα) protein that is not concomitant with increased estrogen receptor 1 (ESR1) transcription, suggesting a role for estrogen in controlling the proteasomal degradation of ERα. However, despite being grown in the same estrogen-deprived conditions, LCC9 cells do not have up-regulated ERα levels. As LCC1 cells retain sensitivity to tamoxifen and fulvestrant, these data suggest that LCC1 have developed estrogen-independence through ERα uncoupled from its ligand. However, LCC9 cells appear to have developed an alternative mechanism which is not dependent on ERα, presumably explaining their resistance to fulvestrant. I have studied global gene expression changes in the presence and absence of estrogen in these cell lines, using oligonucleotide microarrays, and correlated these data with global DNA methylation data derived from methylation arrays, which interrogate the methylation status of approximately 27,000 CpG dinucleotides in the genome. The analysis led to the discovery of more than 5,000 genes that were potentially either up-regulated or down-regulated by estrogen in MCF7 cells, either directly or indirectly. The transcriptional response to estrogen was generally muted in LCC1 and LCC9 compared with MCF7, but was not completely absent. I used various methods based on differential gene expression to parse the data, including gene ontology analysis, aiming to select genes for further mechanistic study. However, none of these methods led to the conclusive identification of a specific gene (or set of genes) that might have accounted for the physiological differences between the cell lines. In one strategy, I reasoned that, as the endocrine-resistant cells had lost their estrogen-dependence, genes involved might be regulated in an estrogen-dependent manner in MCF7 cells, without exhibiting misregulation in LCC9. This led to the identification of DUSP1 as a candidate gene, which was taken forward for mechanistic study because of its potential role in regulating ERα expression. However, when over-expressing DUSP1 in LCC9 cells, I could not demonstrate any effect on ERα levels. The final approach taken was to identify genes that might have been epigenetically deregulated, being both estrogen-regulated and deregulated in association with aberrant DNA methylation in the estrogen-independent cell lines. Surprisingly, given the phenotypic differences between the cell lines, only a very few genes were significantly methylated between cell lines. Of those that were differentially methylated between MCF7 cells and LCC1/9, only three exhibited the expected inverse correlation between methylation and expression. Of these, the gene CYBA was selected for further investigation. CYBA is a critical component of the NAPDH oxidase complex which is involved in generating oxygen free-radicals. My work suggests CYBA expression is estrogen-dependent, and that chronic estrogen deprivation leads to the epigenetic inactivation of CYBA in breast cancer cells. I speculate that the epigenetic suppression of CYBA may protect cells from the oxidant damage that results from estrogen deprivation and may be part of the mechanism that leads to acquired endocrine-resistance in previously sensitive cells.

Published

2013

73. Transcriptional and epigenetic regulation of oestrogen signalling in breast cancer cells

Author

Bi, Jing, Gilbert, Nicholas, and Ramsahoye, Bernard

Subjects

oestrogen signalling, breast cancer

Abstract

Breast cancer is a common disease in women and has major impacts on health and quality of life. About 70% of breast cancers over express ERα, and are classified as ER positive breast cancer. Oestrogen receptor alpha (ERα) belongs to the nuclear receptor superfamily and is responsible for many effects of oestrogen on normal and cancerous breast tissue. Endocrine therapies that block the function of ERα or the synthesis of oestrogen have been a mainstay of ERα positive breast cancer treatment. However, their efficacy is limited by intrinsic and acquired drug resistance overtime, and endocrine resistance remains one of the biggest challenges in breast cancer treatment. In order to investigate the underlying mechanisms of acquired drug resistance, and to develop new strategies for breast cancer therapy, I generated a novel long-term oestrogen deprived cell line (DH) in serum-free condition. As DH cells are cultured in a defined media with known concentrations of growth factors, it provides an ideal system to identify and dissect changes in signalling pathways in response to hormones and inhibitors in vitro. At the same time, DH cells are representative of ER positive breast cancers treated with drugs that reduce the level of oestrogen. It enables the identification of survival pathways that could be activated during oestrogen deprivation. By using this cell model, I find that oestrogen stimulation enables cells to up-regulate the EGFR level and simultaneously reduces ERα expression at both mRNA and protein levels. Once up-regulated, EGFR expression is maintained despite oestrogen withdrawal indicating a stable transcriptional re-programming at the EGFR promoter. By using the whole genome expression microarrays, I identified a list of genes that also show stable changes in gene expression in response to oestrogen, suggesting that the oestrogen promotes transcriptional re-programming at multiple pathways in cells. In terms of signalling pathways, oestrogen activates the growth promoting MAPK pathway in an EGFR dependent manner and a 5-day oestrogen pulse substantially increases the resistance of cells to tamoxifen, while cells remain sensitive to the EGFR inhibitor, demonstrating a functional switch between ERα and EGFR survival pathways. Furthermore, microarray analysis of ERα and EGFR downstream target genes shows that there is a general activation of MAPK gene signature after 5 days of oestrogen stimulation in DH cells. In this thesis, I also investigate the molecular mechanism of oestrogen induced EGFR up-regulation in ER positive breast cancer cells. c-Myb is an oestrogen responsive transcription factor whose expression is regulated by ERα in breast cancer cells. I demonstrate that oestrogen treatment leads to ERα dependent c-Myb up-regulation in DH cells. I also find that c-Myb transiently locates upstream of the EGFR promoter to enhance its expression. As the up-regulation of EGFR in ER positive breast cancer could lead to survival pathway switching and endocrine therapy resistance, c-Myb could be a good drug target to prevent the likelihood these switches and subsequent relapse on endocrine therapies. The expression of EGFR remains high after the removal of oestrogen suggesting there may be epigenetic changes, which maintain the transcriptional re-programming stimulated by c-Myb. Bisulphite sequencing however demonstrates EGFR promoter DNA methylation pattern is not affected by oestrogen. Meanwhile, ChIP microarrays with four different histone modifications show no significant changes around the promoter area of EGFR in response to oestrogen. These observations suggest that alternative epigenetic modifications or epigenetic alternations at other genes may subsequently lead to the stable expression of EGFR in response to oestrogen.

Published

2013

74. Investigating the association between BRAFV600E and methylation in sporadic colon cancer

Author

Baxter, Eva Louise, Ramsahoye, Bernard., and Forrester, Lesley

Subjects

616.994, BRAF, methylation, colon cancer

Abstract

Aberrant methylation of CpG island promoters is a frequent observation in cancer and is known to affect many genes, including tumour suppressor genes. Genes with methylated promoters are usually repressed and inactive, and there is good evidence that most genes that become methylated in cancer are already repressed in the normal tissues from which tumours arise. However, the methylation of some genes appears to arise at previously active loci, suggesting either a stochastic epigenetic event or that these genes are somehow predisposed to becoming methylated. The DNA mismatch repair gene MLH1 is expressed in normal colonic epithelial cells but methylated and down-regulated in some sporadic mismatch repair-deficient colon tumours. These tumours are almost invariably associated with the simultaneous methylation of multiple cancer-specific loci, termed the CpG island methylator phenotype (CIMP) and an activating mutation of BRAF (V600E), raising the possibility that a hypermethylator phenotype may arise in cancer in direct association with a specific genetic alteration. The possibility that MLH1-deficiency caused BRAF mutation was discounted as genetic deficiency of MLH1 is not associated with BRAFV600E. I explored the possibility that BRAFV600E might induce MLH1 methylation but found no evidence in support of this. I then focused on factors that might mediate CIMP gene methylation, of which MLH1 methylation is known to be a part. Bioinformatic analysis of the genes methylated in BRAFV600E colon tumours indicated a significant enrichment in binding sites for the transcription factor MAZ (MYC-associated zinc finger protein). I hypothesised that loss of MAZ might lead to MLH1 down-regulation and its subsequent methylation. In this thesis I provide evidence that both MAZ and MLH1 expression are deregulated during normal colonic epithelial differentiation. The down-regulation of MAZ by RNA interference led to a reduction in MLH1 expression and methylation of its promoter. I speculate that MLH1 methylation may be associated with BRAF mutation because transformation by BRAFV600E allows progenitor cells to undergo a degree of differentiation whilst maintaining their malignant proliferation. I speculate that it is during this process of differentiation that MLH1 becomes susceptible to methylation.

Published

2012

75. ITPase deficiency causes a Martsolf-like syndrome with a lethal infantile dilated cardiomyopathy.

Author

Handley MT, Reddy K, Wills J, Rosser E, Kamath A, Halachev M, Falkous G, Williams D, Cox P, Meynert A, Raymond ES, Morrison H, Brown S, Allan E, Aligianis I, Jackson AP, Ramsahoye BH, von Kriegsheim A, Taylor RW, Finch AJ, and FitzPatrick DR

Subjects

Animals, Base Sequence, Child, Preschool, DNA Mutational Analysis, DNA, Mitochondrial genetics, DNA, Mitochondrial metabolism, Female, Homozygote, Humans, Inosine metabolism, Male, Mice, Mice, Knockout, Mouse Embryonic Stem Cells enzymology, Mutation, Pedigree, Pyrophosphatases genetics, RNA genetics, RNA metabolism, Exome Sequencing, Cardiomyopathy, Dilated enzymology, Cardiomyopathy, Dilated genetics, Cataract enzymology, Cataract genetics, Hypogonadism enzymology, Hypogonadism genetics, Intellectual Disability enzymology, Intellectual Disability genetics, Metabolism, Inborn Errors enzymology, Metabolism, Inborn Errors genetics, Pyrophosphatases deficiency

Abstract

Typical Martsolf syndrome is characterized by congenital cataracts, postnatal microcephaly, developmental delay, hypotonia, short stature and biallelic hypomorphic mutations in either RAB3GAP1 or RAB3GAP2. Genetic analysis of 85 unrelated "mutation negative" probands with Martsolf or Martsolf-like syndromes identified two individuals with different homozygous null mutations in ITPA, the gene encoding inosine triphosphate pyrophosphatase (ITPase). Both probands were from multiplex families with a consistent, lethal and highly distinctive disorder; a Martsolf-like syndrome with infantile-onset dilated cardiomyopathy. Severe ITPase-deficiency has been previously reported with infantile epileptic encephalopathy (MIM 616647). ITPase acts to prevent incorporation of inosine bases (rI/dI) into RNA and DNA. In Itpa-null cells dI was undetectable in genomic DNA. dI could be identified at a low level in mtDNA without detectable mitochondrial genome instability, mtDNA depletion or biochemical dysfunction of the mitochondria. rI accumulation was detectable in proband-derived lymphoblastoid RNA. In Itpa-null mouse embryos rI was detectable in the brain and kidney with the highest level seen in the embryonic heart (rI at 1 in 385 bases). Transcriptome and proteome analysis in mutant cells revealed no major differences with controls. The rate of transcription and the total amount of cellular RNA also appeared normal. rI accumulation in RNA-and by implication rI production-correlates with the severity of organ dysfunction in ITPase deficiency but the basis of the cellulopathy remains cryptic. While we cannot exclude cumulative minor effects, there are no major anomalies in the production, processing, stability and/or translation of mRNA., Competing Interests: The authors have declared that no competing interests exist.

Published

2019

76. Measurement of genome-wide DNA cytosine-5 methylation by reversed-phase high-pressure liquid chromatography.

Author

Ramsahoye BH

Subjects

Animals, Bone Marrow Cells chemistry, Chromatography, High Pressure Liquid instrumentation, Deoxycytidine Monophosphate analysis, Humans, Hydrolysis, Mice, Reproducibility of Results, Spectrophotometry, Ultraviolet, Stem Cells chemistry, Chromatography, High Pressure Liquid methods, DNA chemistry, DNA Methylation, Deoxycytidine Monophosphate analogs & derivatives

Published

2002

77. DNA methylation protocols. Overview.

Author

Mills KI and Ramsahoye BH

Subjects

Animals, CpG Islands, DNA chemistry, DNA genetics, DNA metabolism, DNA (Cytosine-5-)-Methyltransferases deficiency, DNA (Cytosine-5-)-Methyltransferases genetics, DNA (Cytosine-5-)-Methyltransferases metabolism, Dosage Compensation, Genetic, Female, Gene Targeting, Genomic Imprinting, Humans, Male, Molecular Biology methods, Rett Syndrome genetics, Rett Syndrome metabolism, DNA Methylation

Published

2002

78. Nearest-neighbor analysis.

Author

Ramsahoye BH

Subjects

Animals, Chromatography, Gel, Chromatography, Thin Layer, CpG Islands, Methods, Phosphorus Radioisotopes, DNA chemistry, DNA Methylation

Published

2002