Glutaraldehyde Modified Mica: A New Surface for Atomic Force Microscopy of Chromatin

Wang, Hongda; Bash, R.; Yodh, Jaya G.; Hager, Gordon L.; Lohr, D.; Lindsay, Stuart

doi:10.1016/s0006-3495(02)75362-9

Cited by 126 publications

(143 citation statements)

References 29 publications

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“…Atomic Force Microscopy-To minimize the surface influence on the structure of TrmBL2-and histone-DNA complexes in our AFM experiments, we used glutaraldehyde-coated mica, which better preserves the native conformation of protein-DNA samples compared with freshly cleaved or (3-aminopropyl)triethoxysilane-modified mica (27,28). To prepare it, freshly cleaved mica was treated with 0.1% (3-aminopropyl)triethoxysilane solution for 15 min, then rinsed with deionized water, dried with nitrogen gas, and incubated in a desiccator overnight.…”

Section: Methodsmentioning

confidence: 99%

Transcriptional Repressor TrmBL2 from Thermococcus kodakarensis Forms Filamentous Nucleoprotein Structures and Competes with Histones for DNA Binding in a Salt- and DNA Supercoiling-dependent Manner

Efremov

Maruyama

et al. 2015

Journal of Biological Chemistry

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Background: TrmBL2 and histones maintain the genome functioning in hyperthermophilic euryarchaeal cells. Results: TrmBL2 forms filaments on DNA through cooperative binding and competes with histones in a salt-and DNA supercoiling-dependent manner. Conclusion: TrmBL2-histone collective behavior dynamically controls DNA organization. Significance: The discovered mechanisms provide insights into the regulation of the genome structure and global transcription profile by TrmBL2 and histones.

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Section: Methodsmentioning

confidence: 99%

Transcriptional Repressor TrmBL2 from Thermococcus kodakarensis Forms Filamentous Nucleoprotein Structures and Competes with Histones for DNA Binding in a Salt- and DNA Supercoiling-dependent Manner

Efremov

Maruyama

et al. 2015

Journal of Biological Chemistry

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“…AUC experiments describe the unperturbed, global conformation of chromatin fibers under physiological conditions (37)(38)(39)(40)(41)(42)(43)(44)(45)(46), and SFM allows it to identify changes of the fiber geometry at the single nucleosomal level (47)(48)(49)(50)(51)(52)(53)(54)(55)(56)(57). By using a combination of these two biophysical techniques in conjunction with biochemical characterizations, it is shown here that NAP1 mediates the reversible removal of the linker histones from chromatin fibers.…”

mentioning

confidence: 99%

NAP1 Modulates Binding of Linker Histone H1 to Chromatin and Induces an Extended Chromatin Fiber Conformation

Kepert

Mazurkiewicz

Heuvelman

et al. 2005

Journal of Biological Chemistry

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NAP1 (nucleosome assembly protein 1) is a histone chaperone that has been described to bind predominantly to the histone H2A⅐H2B dimer in the cell during shuttling of histones into the nucleus, nucleosome assembly/remodeling, and transcription. Here it was examined how NAP1 interacts with chromatin fibers isolated from HeLa cells. NAP1 induced a reversible change toward an extended fiber conformation as demonstrated by sedimentation velocity ultracentrifugation experiments. This transition was due to the removal of the linker histone H1. The H2A⅐H2B dimer remained stably bound to the native fiber fragments and to fibers devoid of linker histone H1. This was in contrast to mononucleosome substrates, which displayed a NAP1-induced removal of a single H2A⅐H2B dimer from the core particle. The effect of NAP1 on the chromatin fiber structure was examined by scanning/atomic force microscopy. A quantitative image analysis of ϳ36,000 nucleosomes revealed an increase of the average internucleosomal distance from 22.3 ؎ 0.4 to 27.6 ؎ 0.6 nm, whereas the overall fiber structure was preserved. This change reflects the disintegration of the chromatosome due to binding of H1 to NAP1 as chromatin fibers stripped from H1 showed an average nucleosome distance of 27.4 ؎ 0.8 nm. The findings suggest a possible role of NAP1 in chromatin remodeling processes involved in transcription and replication by modulating the local linker histone content.The dynamic organization of chromatin in the eukaryotic nucleus is tightly connected to transcription (1-3). Transcribed chromatin is thought to be in a more open conformation with a higher accessibility to DNase I or micrococcal nuclease (4 -7). On the other hand, highly compacted and dense chromatin regions, referred to as heterochromatin, are often transcriptionally inactive and contain a reduced number of genes (3,7,8). Several factors have been identified that promote a transition between a transcriptionally active and a more dense/inactive chromatin conformation. These include linker histones (9 -11), DNA methylation (2, 12), histone modifications (13-15), and the incorporation of histone variants (16 -19). The dynamic nature of chromatin manifests itself by continuous rearrangements of its three-dimensional structure. These changes involve the activity of histone chaperones that mediate the ordered deposition and the removal and exchange of histones (20 -23). The central carrier of the histone H2A⅐H2B dimer in the cell is NAP1 (nucleosome assembly protein 1) (24). NAP1 is involved in the transport of the histone H2A⅐H2B dimer from the cytoplasm to the nucleus and the deposition of histones onto the DNA as described in several reviews (20 -23). NAP1 and other histone chaperones stimulate the binding of transcription factors to chromatin templates (25, 26). In yeast, loss of NAP1 leads to an altered gene expression of about 10% of the genome (27), and several lines of evidence suggest that NAP1 has activities related to transcription. First, it has been shown that NAP1 is present in com...

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“…27 Since the structure of chromatin itself likely regulates aspects of gene transcription, 28 understanding these factors is of critical importance in probing epigenetics. Intensive research has been conducted to characterize the structural and functional properties of chromatin using diverse experimental and modeling techniques including atomic force microscopy (AFM), [29][30][31] optical/magnetic tweezers, 32,33 electron microscopy, 34,35 and X-ray scattering methods. 36,37 DNA is coiled around a nucleosome core comprising four pairs of histone proteins, and nucleosomes are connected to each other by linker DNA (often represented by a "beads-on-astring" model) ( Fig.…”

Section: Challenges In Chromatin Analysismentioning

confidence: 99%

Micro- and nanofluidic technologies for epigenetic profiling

et al. 2013

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This short review provides an overview of the impact micro- and nanotechnologies can make in studying epigenetic structures. The importance of mapping histone modifications on chromatin prompts us to highlight the complexities and challenges associated with histone mapping, as compared to DNA sequencing. First, the histone code comprised over 30 variations, compared to 4 nucleotides for DNA. Second, whereas DNA can be amplified using polymerase chain reaction, chromatin cannot be amplified, creating challenges in obtaining sufficient material for analysis. Third, while every person has only a single genome, there exist multiple epigenomes in cells of different types and origins. Finally, we summarize existing technologies for performing these types of analyses. Although there are still relatively few examples of micro- and nanofluidic technologies for chromatin analysis, the unique advantages of using such technologies to address inherent challenges in epigenetic studies, such as limited sample material, complex readouts, and the need for high-content screens, make this an area of significant growth and opportunity.

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Glutaraldehyde Modified Mica: A New Surface for Atomic Force Microscopy of Chromatin

Cited by 126 publications

References 29 publications

Transcriptional Repressor TrmBL2 from Thermococcus kodakarensis Forms Filamentous Nucleoprotein Structures and Competes with Histones for DNA Binding in a Salt- and DNA Supercoiling-dependent Manner

Transcriptional Repressor TrmBL2 from Thermococcus kodakarensis Forms Filamentous Nucleoprotein Structures and Competes with Histones for DNA Binding in a Salt- and DNA Supercoiling-dependent Manner

NAP1 Modulates Binding of Linker Histone H1 to Chromatin and Induces an Extended Chromatin Fiber Conformation

Micro- and nanofluidic technologies for epigenetic profiling

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