Proteopedia

Nitrogenase: Difference between revisions

← Older edit
Student (talk | contribs)
students
33,700 edits
No edit summary
Michal Harel (talk | contribs)
31,761 edits
No edit summary
 
(45 intermediate revisions by 5 users not shown)
Line 1: Line 1:
Please do NOT make changes to this sandbox. Sandboxes 10-30 are currently reserved by Prof. Sheila Jaswal at Amherst College.
<StructureSection load="1N2C" size="350" color="white" caption="Nitrogenase complex: α (grey and green) and β (pink and yellow) chains, nitrogenase iron protein ( purple,cyan, red and gold), showing Fe-Mo-S cluster complex with ADP, adipic acid, AlF4, Ca+2 and Mg+2 ions [[1n2c]]">
__TOC__
==Function==


 
'''Nitrogenase''' (Nase) is an enzyme that fixes atmospheric nitrogen (N<sub>2</sub>) into ammonia. Though abundantly present in the atmosphere, most organisms cannot utilize N<sub>2</sub> directly, and must instead take it in through other forms, like ammonia or nitrate. The triple bond in N<sub>2</sub> is highly resistant to changes in oxidation state, and nitrogenases, found only in nitrogen-fixing bacteria, are the only proteins capable of reducing N<sub>2</sub> to ammonia.
== <p style="font-size:x-large;">Nitrogenase</p> ==
<applet load="1N2C" size="400" color="white" frame="true" align="right" caption="Nitrogenase"/>
'''Nitrogenase''' is an enzyme that fixes atmospheric nitrogen (N<sub>2</sub>) into ammonia. Though abundantly present in the atmosphere, most organisms cannot utilize N<sub>2</sub> directly, and must instead take it in through other forms, like ammonia or nitrate. The triple bond in N<sub>2</sub> is highly resistant to changes in oxidation state, and nitrogenases, found only in nitrogen-fixing bacteria, are the only proteins capable of reducing N<sub>2</sub> to ammonia.




Line 11: Line 10:
N<sub>2</sub> + 8 H<sup>+</sup> + 16 MgATP + 8 e<sup>-</sup> &rarr; 2NH<sub>3</sub> + H<sub>2</sub> + 16 MgADP + 16 P<sub>i</sub>
N<sub>2</sub> + 8 H<sup>+</sup> + 16 MgATP + 8 e<sup>-</sup> &rarr; 2NH<sub>3</sub> + H<sub>2</sub> + 16 MgADP + 16 P<sub>i</sub>


Two different proteins comprise the nitrogenase complex. The FeMo protein binds substrate and reduces H<sup>+</sup> and N<sub>2</sub> to H<sub>2</sub> and ammonia, while the Fe protein receives electrons from ferredoxin, hydrolyzes ATP, and reduces the FeMo protein. To the right is shown a crystal structure (PDB entry [[1n2c]]) where two complexes of FeMo protein bound to Fe protein were crystallized together. Click here to see only <scene name='Sandbox_10/1n2c_single_complex/2'>one complex</scene>.
Two different proteins comprise the nitrogenase complex. The FeMo protein binds substrate and reduces H<sup>+</sup> and N<sub>2</sub> to H<sub>2</sub> and ammonia, while the Fe protein receives electrons from ferredoxin, hydrolyzes ATP, and reduces the FeMo protein. To the right is shown a crystal structure (PDB entry [[1n2c]]<ref>PMID:9163420</ref>) where two complexes of FeMo protein bound to Fe protein were crystallized together. Click here to see only <scene name='Sandbox_10/1n2c_single_complex/2'>one complex</scene>.


The <scene name='Sandbox_10/1n2c_fe_protein/1'>Fe protein</scene> is here bound to two <scene name='Sandbox_10/1n2c_atp/3'>ADP x AlF<sub>4</sub><sup>-</sup></scene>, an analog for the planar transition state of ATP hydrolysis. The motif that binds ATP is a conserved nucleotide binding motif called Walker's motif A. Coloring by <scene name='Sandbox_10/1n2c_atp_evolutionary/1'>evolutionary conservation</scene>, the nucleotide binding pocket is clear.


At the bottom of the protein, where the Fe protein comes into contact with the FeMo protein, is a <scene name='Sandbox_10/1n2c_fes_cluster_cys/1'>4Fe:4S cluster</scene>, held in place by cysteines. This cluster accepts electrons from ferredoxin and gives electrons to the FeMo protein.
The <scene name='Sandbox_10/1n2c_fe_protein/1'>Fe protein</scene> is here bound to two <scene name='Sandbox_10/1n2c_atp/3'>ADP x AlF4-</scene>, an analog for the planar transition state of ATP hydrolysis. The motif that binds ATP is a conserved nucleotide binding motif called Walker's motif A. Coloring by <scene name='Sandbox_10/1n2c_atp_evolutionary/1'>evolutionary conservation</scene>, the nucleotide binding pocket is clear. At the bottom of the protein, where the Fe protein comes into contact with the FeMo protein, is a <scene name='Sandbox_10/1n2c_fes_cluster_cys/1'>4Fe:4S cluster</scene>, held in place by cysteines. This cluster accepts electrons from ferredoxin and gives electrons to the FeMo protein.


When the Fe protein is bound to the FeMo protein (<scene name='Sandbox_10/1n2c_single_complex/2'>zoom out</scene>), ATP is hydrolyzed and electrons that were transferred to the 4Fe:4S cluster of the Fe protein by ferredoxin are transferred to the FeMo protein. The crystal structure of the complete nitrogenase complex reveals how the binding of the Fe and FeMo proteins, the hydrolysis of ATP, and the transfer of electrons are all coupled.


Compared to the crystal structure of Fe protein that is not bound to FeMo protein, Fe protein complexed with FeMo protein  
When the Fe protein is bound to the FeMo protein (<scene name='Sandbox_10/1n2c_single_complex/2'>zoom out</scene>), ATP is hydrolyzed and electrons that were transferred to the 4Fe:4S cluster of the Fe protein by ferredoxin are transferred to the FeMo protein. The crystal structure of the complete nitrogenase complex reveals how the binding of the Fe and FeMo proteins, the hydrolysis of ATP, and the transfer of electrons are all coupled. The figure below summarizes how these processes are linked.


[[Image:clip_image002.jpg]]
[[Image:clip_image002.jpg]]


the two subunits of the Fe protein are pushed closer together. When this happens
Before this crystal structure showing the complete nitrogenase complex was solved, crystal structures of the Fe and FeMo proteins had been solved, but the mechanisms of ATP hydrolysis and electron transfer were still unknown. In this structure, as indicated in the figure above, the two subunits of the Fe protein were observed to have swung closer together. This movement results from Fe protein binding to FeMo protein. Focusing in on the <scene name='Sandbox_10/1n2c_atp/3'>ATP binding pocket</scene> discussed above, especially on the <scene name='Sandbox_10/1n2c_atp_lys_10/1'>AlF4-</scene> that is an analog for the negatively charged planar transition state reveals that there are several positive charges in this vicinity that stabilize the transition state. Importantly, Lys 10 from the opposite subunit is an important source of stabilizing positive charge. Only in this structure where the two subunits have swung closer together is this residue in position to help catalyze the hydrolysis of the terminal phosphate of ATP.
 
<scene name='Sandbox_10/1n2c_atp_lys_10/1'>TextToBeDisplayed</scene>
 
 
 
 
 




Green fluorescent protein ('''GFP'''), originally isolated from the jellyfish Aequorea victoria (PDB entry [[1ema]]), fluorsceses green (509nm) when exposed to blue light (395nm and 475nm). It is one of the most important proteins used in biological research because it can be used to tag otherwise invisible gene products of interest and thus observe their existence, location and movement.
For these reasons, binding of Fe protein to FeMo protein results in hydrolysis of ATP. Additionally, the 4Fe:4S cluster is lowered close enough to the metal-sulfur clusters of the FeMo protein that electron transfer can occur. All three clusters found in the Fe protein-FeMo protein complex can be seen <scene name='Sandbox_10/1n2c_clusters/2'>here</scene>. Once the electrons have passed from the 4Fe:4S cluster of the Fe protein to the 8Fe:7S cluster of the FeMo protein, they then transfer to the 7Fe:Mo:9S:homocitrate:X cluster where X is an unidentified light atom. It is at this cluster where reduction of N<sub>2</sub> and H<sup>+</sup> occur. The exact mechanism of reduction, however, is still unknown.


== Exploring the Structure ==
==3D structure of Nitrogenase==
<applet load='1ema' size='300' frame='true' align='right' caption='Insert caption here' />
[[Nitrogenase 3D structures]]


GFP is a beta barrel protein with 11 beta sheets. It is a 26.9kDa protein made up of 238 amino acids. The <scene name='Sandbox_10/Gfp/1'>chromophore</scene>, responsible for the fluorescent properties of the protein, is buried inside the beta barrel as part of the central alpha helix passing through the barrel. The chromophore forms via spontaneous cyclization and oxidation of three residues in the central alpha helix: -Thr65 (or Ser65)-Tyr66-Gly67. This cyclization and oxidation creates the chromophore's five-membered ring via a new bond between the threonine and the glycine residues.<ref>PMID:8703075 </ref>
</StructureSection>


== References ==
== References ==
<references/>
<references/>
[[Category:Topic Page]]

Proteopedia Page Contributors and Editors (what is this?)Proteopedia Page Contributors and Editors (what is this?)

Student, Eran Hodis, David Canner, Michal Harel, Alexander Berchansky, Joel L. Sussman
Retrieved from "https://proteopedia.openfox.io/w/Nitrogenase"