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Nucleosome structure

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Nucleosomes are the basic building blocks of chromatin fibers. A nucleosome consists of a core containing an octamer of histone proteins and a DNA molecule 146 bp long wound around this core in two complete turns. The includes four types of proteins: , , and . Histone proteins are organized in dimers so:

Two H3-H4 dimers
Two H2A-H2B dimers

molecule wound in around octamer. Some complete the whole structure.

The main secondary structure in is .

If we highlight the different types of amino acid residues on the we can see that and are arranged so positively charged residues are in , where they can form ionic interactions (salt bridges) with . This distribution of electric charges stabilizes the whole structure.

References

This page is based on 1aoi file from Proteopedia.

1aoi is a 10 chain structure with sequence from Xenopus laevis. The July 2000 RCSB PDB Molecule of the Month feature on Nucleosome by David S. Goodsell is 10.2210/rcsb_pdb/mom_2000_7. Full crystallographic information is available from OCA. For a guided tour on the structure components use FirstGlance.

Proteopedia Page Contributors and Editors (what is this?)

Alejandro Porto, Eric Martz, Michal Harel

Retrieved from "http://52.214.119.220/wiki/index.php/Nucleosome_structure"

@@ Line 1: / Line 1: @@
-[[es:Nucleosome structure (spanish)]]
+[[es:Nucleosome structure (Spanish)]]
 ----
-<Structure load='1aoi' size='800' frame='true' align='right' caption='Nucleosoma' scene='60/602771/Proteinas/5'/>
+<Structure load='1aoi' size='450' frame='true' align='right' caption='Nucleosome [[1aoi]]' scene='60/602771/Nucleosoma/3'/>
-<big><big>'''Nucleosome''' is the basic structure of '''chromatin fiber'''. A nucleosome consists of a core with a '''histonic proteins octamer''' and a '''DNA''' molecule 146 bp long  wound around this core in two complete turns.
+<big><big>'''Nucleosomes''' are the basic building blocks of '''chromatin fibers'''. A nucleosome consists of a core containing '''an octamer of histone proteins''' and a '''DNA''' molecule 146 bp long  wound around this core in two complete turns.
-Histonic protein octamer includes four types of proteins: <scene name='60/602771/Histonah2a/1'>H2A</scene>, <scene name='60/602771/Histonah2b/1'>H2B</scene>, <scene name='60/602771/Histonah3/1'>H3</scene> y <scene name='60/602771/Histonah4/1'>H4</scene>. Histonic proteins are organized in dimers so:
+The <scene name='60/602771/Proteinas/5'>histone protein octamer</scene>  includes four types of proteins: <scene name='60/602771/Histonah2a/1'>H2A</scene>, <scene name='60/602771/Histonah2b/1'>H2B</scene>, <scene name='60/602771/Histonah3/1'>H3</scene> and <scene name='60/602771/Histonah4/1'>H4</scene>. Histone proteins are organized in dimers so:
 *Two H3-H4 dimers
@@ Line 13: / Line 13: @@
 *<scene name='60/602771/Octamero/1'>Whole octamer</scene>
-*<scene name='60/602771/Nucleosoma/3'>DNA</scene> molecule wound in<scene name='60/602771/Nucleosoma/4'>two complete turns</scene> around octamer. Some<scene name='60/602771/Nucleosoma/5'>manganese ions</scene> complete the whole structure.
+*<scene name='60/602771/Nucleosoma/3'>DNA</scene> molecule wound in <scene name='60/602771/Nucleosoma/4'>two complete turns</scene> around octamer. Some <scene name='60/602771/Nucleosoma/5'>manganese ions</scene> complete the whole structure.
-The more widespread secondary structure in <scene name='60/602771/Octamero/2'>histonic proteins</scene> is <scene name='60/602771/Secondarystructure/1'>alfa helix</scene>.
+The main secondary structure in <scene name='60/602771/Octamero/2'>histones</scene> is <scene name='60/602771/Secondarystructure/1'>alpha helices</scene>.
- If we situate the different types of amino acid residues in <scene name='60/602771/Esqueleto/1'>protein skeleton</scene> we can see that <scene name='60/602771/Residuosnegativos/1'>negatively charged residues</scene> and <scene name='60/602771/Residuospositivos/1'>positively charged residues</scene> are arranged so positively  charged residues are in peripherycal positions <scene name='60/602771/Periferia/1'>peripherycal positions</scene>, where they can stablish ionic interations with <scene name='60/602771/Interacciones/1'>phosphate groups on DNA molecule</scene>. Such electric charges distribution, gives stability to the whole structure.
+If we highlight the different types of amino acid residues on the <scene name='60/602771/Esqueleto/1'>protein backbone</scene> we can see that <scene name='60/602771/Residuosnegativos/1'>negatively charged residues</scene> and <scene name='60/602771/Residuospositivos/1'>positively charged residues</scene> are arranged so positively  charged residues are in <scene name='60/602771/Periferia/1'>peripheral positions</scene>, where they can form ionic interactions ([[salt bridges]]) with <scene name='60/602771/Interacciones/1'>phosphate groups on the DNA molecule</scene>. This distribution of electric charges stabilizes the whole structure.
 <small>
+==See Also==
+*[[Nucleosome structure (Spanish)]]
+*[[Nucleosomes]]
+*[[User:Eric Martz/Nucleosomes]]
 == References ==
 <references/>

Nucleosome structure

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