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Yorodumi- EMDB-28512: Cryo-ET 3D reconstruction of an individual tetra-nucleosome-H1 pa... -
+Open data
-Basic information
Entry | Database: EMDB / ID: EMD-28512 | |||||||||
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Title | Cryo-ET 3D reconstruction of an individual tetra-nucleosome-H1 particle in 5 mM NaCl and 20 mM HEPES buffer --- Particle #217 | |||||||||
Map data | Cryo-ET 3D reconstruction of an individual tetra-nucleosome-H1 particle in 5 mM NaCl and 20 mM HEPES buffer --- Particle #217 | |||||||||
Sample |
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Keywords | Nucleosome Array / DNA BINDING PROTEIN | |||||||||
Biological species | Xenopus laevis (African clawed frog) | |||||||||
Method | electron tomography / cryo EM | |||||||||
Authors | Zhang M / Celis CD / Liu JF / Bustamante C / Ren G | |||||||||
Funding support | United States, 1 items
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Citation | Journal: Nat Commun / Year: 2024 Title: Angle between DNA linker and nucleosome core particle regulates array compaction revealed by individual-particle cryo-electron tomography. Authors: Meng Zhang / César Díaz-Celis / Jianfang Liu / Jinhui Tao / Paul D Ashby / Carlos Bustamante / Gang Ren / Abstract: The conformational dynamics of nucleosome arrays generate a diverse spectrum of microscopic states, posing challenges to their structural determination. Leveraging cryogenic electron tomography (cryo- ...The conformational dynamics of nucleosome arrays generate a diverse spectrum of microscopic states, posing challenges to their structural determination. Leveraging cryogenic electron tomography (cryo-ET), we determine the three-dimensional (3D) structures of individual mononucleosomes and arrays comprising di-, tri-, and tetranucleosomes. By slowing the rate of condensation through a reduction in ionic strength, we probe the intra-array structural transitions that precede inter-array interactions and liquid droplet formation. Under these conditions, the arrays exhibite irregular zig-zag conformations with loose packing. Increasing the ionic strength promoted intra-array compaction, yet we do not observe the previously reported regular 30-nanometer fibers. Interestingly, the presence of H1 do not induce array compaction; instead, one-third of the arrays display nucleosomes invaded by foreign DNA, suggesting an alternative role for H1 in chromatin network construction. We also find that the crucial parameter determining the structure adopted by chromatin arrays is the angle between the entry and exit of the DNA and the corresponding tangents to the nucleosomal disc. Our results provide insights into the initial stages of intra-array compaction, a critical precursor to condensation in the regulation of chromatin organization. | |||||||||
History |
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-Structure visualization
Supplemental images |
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-Downloads & links
-EMDB archive
Map data | emd_28512.map.gz | 27.9 MB | EMDB map data format | |
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Header (meta data) | emd-28512-v30.xml emd-28512.xml | 8.2 KB 8.2 KB | Display Display | EMDB header |
Images | emd_28512.png | 28.2 KB | ||
Filedesc metadata | emd-28512.cif.gz | 3.7 KB | ||
Archive directory | http://ftp.pdbj.org/pub/emdb/structures/EMD-28512 ftp://ftp.pdbj.org/pub/emdb/structures/EMD-28512 | HTTPS FTP |
-Validation report
Summary document | emd_28512_validation.pdf.gz | 250.9 KB | Display | EMDB validaton report |
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Full document | emd_28512_full_validation.pdf.gz | 250.4 KB | Display | |
Data in XML | emd_28512_validation.xml.gz | 5.8 KB | Display | |
Data in CIF | emd_28512_validation.cif.gz | 6.6 KB | Display | |
Arichive directory | https://ftp.pdbj.org/pub/emdb/validation_reports/EMD-28512 ftp://ftp.pdbj.org/pub/emdb/validation_reports/EMD-28512 | HTTPS FTP |
-Related structure data
Related structure data | C: citing same article (ref.) |
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-Links
EMDB pages | EMDB (EBI/PDBe) / EMDataResource |
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-Map
File | Download / File: emd_28512.map.gz / Format: CCP4 / Size: 30.5 MB / Type: IMAGE STORED AS FLOATING POINT NUMBER (4 BYTES) | ||||||||||||||||||||||||||||||||
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Annotation | Cryo-ET 3D reconstruction of an individual tetra-nucleosome-H1 particle in 5 mM NaCl and 20 mM HEPES buffer --- Particle #217 | ||||||||||||||||||||||||||||||||
Projections & slices | Image control
Images are generated by Spider. | ||||||||||||||||||||||||||||||||
Voxel size | X=Y=Z: 7.4 Å | ||||||||||||||||||||||||||||||||
Density |
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Symmetry | Space group: 1 | ||||||||||||||||||||||||||||||||
Details | EMDB XML:
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-Supplemental data
-Sample components
-Entire : Tetranucleosome array in the presence of H1
Entire | Name: Tetranucleosome array in the presence of H1 |
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Components |
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-Supramolecule #1: Tetranucleosome array in the presence of H1
Supramolecule | Name: Tetranucleosome array in the presence of H1 / type: complex / ID: 1 / Parent: 0 |
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Source (natural) | Organism: Xenopus laevis (African clawed frog) |
-Experimental details
-Structure determination
Method | cryo EM |
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Processing | electron tomography |
Aggregation state | particle |
-Sample preparation
Buffer | pH: 7.5 / Details: 5 mM NaCl 20 mM HEPES 1 mM DTT 1 mM EDTA |
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Vitrification | Cryogen name: ETHANE / Chamber humidity: 99 % / Chamber temperature: 277 K |
Sectioning | Other: NO SECTIONING |
-Electron microscopy
Microscope | FEI TITAN KRIOS |
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Image recording | Film or detector model: GATAN K2 QUANTUM (4k x 4k) / Average exposure time: 2.0 sec. / Average electron dose: 5.4 e/Å2 |
Electron beam | Acceleration voltage: 300 kV / Electron source: FIELD EMISSION GUN |
Electron optics | Illumination mode: FLOOD BEAM / Imaging mode: BRIGHT FIELD / Nominal defocus max: 3.5 µm / Nominal defocus min: 2.5 µm |
Experimental equipment | Model: Titan Krios / Image courtesy: FEI Company |
-Image processing
Final reconstruction | Software - Name: SPIDER / Number images used: 35 |
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-Atomic model buiding 1
Refinement | Protocol: FLEXIBLE FIT |
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