Dissection of cell cycle–dependent dynamics of Dnmt1 by FRAP and diffusion-coupled modeling

Schneider, Katja; Fuchs, Christiane; Dobay, Akos; Rottach, Andrea; Qin, Weihua; Wolf, Patricia; Álvarez-Castro, José M.; Nalaskowski, Marcus M.; Kremmer, Elisabeth; Schmid, Volker; Leonhardt, Heinrich; Schermelleh, Lothar

doi:10.1093/nar/gkt191

Cited by 57 publications

(61 citation statements)

References 69 publications

(63 reference statements)

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“…S3B and S3D), indicating that hypoxia stress substantially reduced their binding to chromatin. As chromatin organizing proteins and molecular platforms such as the condensin complex are closely associated with cell cycle regulation, it is possible that reduced chromatin binding by proteins in clusters a and c could be attributed to cell cycle disruption due to hypoxia stress (26,27). Consistent with these proteomic data, our cell cycle analysis of cancer cells that had been subjected to hypoxia revealed a corresponding cell cycle arrest in G 0 -G 1 phase (supplemental Figs.…”

Section: Resultssupporting

confidence: 81%

Quantitative Profiling of Chromatome Dynamics Reveals a Novel Role for HP1BP3 in Hypoxia-induced Oncogenesis

Dutta

Ren

Lim

et al. 2014

Molecular & Cellular Proteomics

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In contrast to the intensely studied genetic and epigenetic changes that induce host cell transformation to initiate tumor development, those that promote the malignant progression of cancer remain poorly defined. As emerging evidence suggests that the hypoxic tumor microenvironment could re-model the chromatin-associated proteome (chromatome) to induce epigenetic changes and alter gene expression in cancer cells, we hypothesized that hypoxia-driven evolution of the chromatome promotes malignant changes and the development of therapy resistance in tumor cells. To test this hypothesis, we isolated chromatins from tumor cells treated with varying conditions of normoxia, hypoxia, and re-oxygenation and then partially digested them with DNase I and analyzed them for changes in euchromatin-and heterochromatinassociated proteins using an iTRAQ-based quantitative proteomic approach. We identified a total of 1446 proteins with a high level of confidence, including 819 proteins that were observed to change their chromatin association topology under hypoxic conditions. These hypoxia-sensitive proteins included key mediators of chromatin organization, transcriptional regulation, and DNA repair. Furthermore, our proteomic and functional experiments revealed a novel role for the chromatin organizer protein HP1BP3 in mediating chromatin condensation during hypoxia, leading to increased tumor cell viability, radio-resistance, chemo-resistance, and self-renewal. Taken together, our findings indicate that HP1BP3 is a key mediator of tumor progression and cancer cell acquisition of therapy-resistant traits, and thus might represent a novel therapeutic target in a range of human malignancies. Molecular &

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Section: Resultssupporting

confidence: 81%

Quantitative Profiling of Chromatome Dynamics Reveals a Novel Role for HP1BP3 in Hypoxia-induced Oncogenesis

Dutta

Ren

Lim

et al. 2014

Molecular & Cellular Proteomics

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“…We considered that the main site of demethylation might occur in Satellite 2 repeat sequences (SAT2) for 3 reasons. First, the RFTS domain mediates association of DNMT1 to pericentromeric heterochromatin to maintain dense methylation 47,48 and SAT2 is the most abundant repeat in the region. 49 Second, SAT2-specific hypomethylation has been found in DNMT1-null cells 50,51 and in patients with RFTS-mutated DNMT1.…”

Section: Dnmt1-drfts Cells Exhibit Genomic Hypomethylationmentioning

confidence: 99%

RFTS-deleted DNMT1 enhances tumorigenicity with focal hypermethylation and global hypomethylation

Mei

Brenner

2014

Cell Cycle

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Site-specific hypermethylation of tumor suppressor genes accompanied by genome-wide hypomethylation are epigenetic hallmarks of malignancy. However, the molecular mechanisms that drive these linked changes in DNA methylation remain obscure. DNA methyltransferase 1 (DNMT1), the principle enzyme responsible for maintaining methylation patterns is commonly dysregulated in tumors. Replication foci targeting sequence (RFTS) is an N-terminal domain of DNMT1 that inhibits DNA-binding and catalytic activity, suggesting that RFTS deletion would result in a gain of DNMT1 function. However, a substantial body of data suggested that RFTS is required for DNMT1 activity. Here, we demonstrate that deletion of RFTS alters DNMT1-dependent DNA methylation during malignant transformation. Compared to full-length DNMT1, ectopic expression of hyperactive DNMT1-DRFTS caused greater malignant transformation and enhanced promoter methylation with condensed chromatin structure that silenced DAPK and DUOX1 expression. Simultaneously, deletion of RFTS impaired DNMT1 chromatin association with pericentromeric Satellite 2 (SAT2) repeat sequences and produced DNA demethylation at SAT2 repeats and globally. To our knowledge, RFTS-deleted DNMT1 is the first single factor that can reprogram focal hypermethylation and global hypomethylation in parallel during malignant transformation. Our evidence suggests that the RFTS domain of DNMT1 is a target responsible for epigenetic changes in cancer.

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“…In this paper, we use FRAP data sets of GFP-Dnmt1 expressed in mouse C2C12 myoblast cells (Schneider et al, 2013), which were obtained from multiple cell nuclei and can therefore be utilized to illustrate how our nonlinear regression model can be used to fit all available data at once. DNA methylation at position 5 of cytosines within CpG dinocleotide sequences is an important biochemical process for the stable epigenetic gene silencing in vertebrates (Bird, 2002, Spada et al, 2006.…”

Section: Datamentioning

confidence: 99%

“…To date, for the analysis of data from FRAP experiments for the same molecule on multiple similar cell nuclei with a mathematical model, either the data of each recovery curve is analyzed separately, and the results for all cell nuclei are regarded together (e.g., Schneider et al, 2013), or the data of the different cell nuclei are pooled, averaged and then analyzed (e.g., McNally, 2008). In the second case, the recovery curves of the cell nuclei are averaged to obtain a smooth curve that can then be analyzed by the same mathematical model that is usually used for the analysis of one recovery curve.…”

Section: Introductionmentioning

confidence: 99%

“…See Sprague and McNally (2005) for more information on FRAP experiments. In this paper, we concentrate on half-nucleus FRAP [as opposed to circle FRAP or strip FRAP (Sprague et al, 2004;Mueller et al, 2008)], which should cover representative fractions of heterogeneously distributed binding sites in all cell cycle stages (Schneider et al, 2013). An example for such data is given in Figure 1.…”

Section: Introductionmentioning

confidence: 99%

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Bayesian mixed-effects model for the analysis of a series of FRAP images

Feilke

Schneider

Schmid

2015

Statistical Applications in Genetics and Molecular Biology

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Abstract:The binding behavior of molecules in nuclei of living cells can be studied through the analysis of images from fluorescence recovery after photobleaching experiments. However, there is still a lack of methodology for the statistical evaluation of FRAP data, especially for the joint analysis of multiple dynamic images. We propose a hierarchical Bayesian nonlinear model with mixed-effect priors based on local compartment models in order to obtain joint parameter estimates for all nuclei as well as to account for the heterogeneity of the nuclei population. We apply our method to a series of FRAP experiments of DNA methyltransferase 1 tagged to green fluorescent protein expressed in a somatic mouse cell line and compare the results to the application of three different fixed-effects models to the same series of FRAP experiments. With the proposed model, we get estimates of the off-rates of the interactions of the molecules under study together with credible intervals, and additionally gain information about the variability between nuclei. The proposed model is superior to and more robust than the tested fixedeffects models. Therefore, it can be used for the joint analysis of data from FRAP experiments on various similar nuclei.

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Dissection of cell cycle–dependent dynamics of Dnmt1 by FRAP and diffusion-coupled modeling

Cited by 57 publications

References 69 publications

Quantitative Profiling of Chromatome Dynamics Reveals a Novel Role for HP1BP3 in Hypoxia-induced Oncogenesis

Quantitative Profiling of Chromatome Dynamics Reveals a Novel Role for HP1BP3 in Hypoxia-induced Oncogenesis

RFTS-deleted DNMT1 enhances tumorigenicity with focal hypermethylation and global hypomethylation

Bayesian mixed-effects model for the analysis of a series of FRAP images

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