Journal:JBIC:8

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A hydrogen-bonding network formed by the B10-E7-E11 residues of a truncated hemoglobin from Tetrahymena pyriformis is critical for stability of bound oxygen and nitric oxide detoxification

Jotaro Igarashi, Kazuo Kobayashi and Ariki Matsuoka^[1]

Molecular Tour
A wide diversity of both structure and function has been discovered in the study of . Hbs transport in the red blood cells of higher organisms. Even though oxygen molecules can diffuse into cells, unicellular organisms also have Hb-like molecules. Here, we consider the term 'hemoglobins' to include such molecules. Three classes of Hb have been found in unicellular organisms. First, single-domain globins are comprised of three-over-three (3/3) α-helical folds, as is myoglobin (Mb). Second, flavohemoglobins are distinguished by the presence of an N-terminal globin domain and an additional C-terminal FAD-containing reductase region. Finally, truncated Hbs (trHbs) have been discovered recently and are widely distributed in unicellular organisms.

, also known as 2/2 hemoglobins, can be further classified into three different groups (I, II, and III). Genomic sequences of bacteria, cyanobacteria, and plants indicate that trHbs are rather common. Group I, Group II, and Group III trHbs have distinct phylogenetic trees and show different ligand-binding properties. The Group I trHb of the ciliated protozoan Tetrahymena pyriformis (Tp trHb) was first discovered by Keilin and Ryley in 1953.

It is known that trHbs exist in ciliates of the Tetrahymena group, but trHb structure and function remain poorly understood. To investigate trHb function with respect to stability of bound oxygen and protein structure, we measured the oxygen binding kinetics of Tetrahymena pyriformis trHb, and determined the crystal structure of the protein.

The three-dimensional structure of an was determined at 1.73 Å resolution (3aq9). . Tyr25 donated a hydrogen bond to the terminal oxygen atom, whereas Gln46 hydrogen-bonded to the proximal oxygen atom. Furthermore, .

The O₂ association and dissociation rate constants of T. pyriformis trHb were 5.5 μM^-1 s^-1, and 0.18 s^-1, respectively. The oxygen affinity was determined to be 33 nM. The autooxidation rate constant was 3.8 x 10^-3 h^-1. These values are similar to those of .

Mutations:

Mutation at Tyr25: and .
Mutation at Gln46:
Mutation at increased the O₂ dissociation and autooxidation rate constants, and partly disrupted the hydrogen-bonding network.

An , in a crystal state, with nitric oxide. This suggests that Tp trHb functions in nitric oxide detoxification.

PDB reference: Crystal structure of truncated hemoglobin from Tetrahymena pyriformis, Fe(II)-O2 form 3aq5; Crystal structure of truncated hemoglobin from Tetrahymena pyriformis, Fe(III) form 3aq6; Crystal structure of truncated hemoglobin from Tetrahymena pyriformis, Y25F mutant, Fe(III) form 3aq7; Crystal structure of truncated hemoglobin from Tetrahymena pyriformis, Q46E mutant, Fe(III) form 3aq8; Crystal structure of truncated hemoglobin from Tetrahymena pyriformis, Q50E mutant, Fe(III) form 3aq9.

↑ Igarashi J, Kobayashi K, Matsuoka A. A hydrogen-bonding network formed by the B10-E7-E11 residues of a truncated hemoglobin from Tetrahymena pyriformis is critical for stability of bound oxygen and nitric oxide detoxification. J Biol Inorg Chem. 2011 Feb 5. PMID:21298303 doi:10.1007/s00775-011-0761-3

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@@ Line 1: / Line 1: @@
-<StructureSection load='Jbic8.pdb' size='500' side='right' scene='Journal:JBIC:8/Cv/1' caption=''>
+<StructureSection load='Jbic8.pdb' size='450' side='right' scene='Journal:JBIC:8/Cv/1' caption=''>
 === A hydrogen-bonding network formed by the B10-E7-E11 residues of a truncated hemoglobin from Tetrahymena pyriformis is critical for stability of bound oxygen and nitric oxide detoxification ===
 <big>Jotaro Igarashi, Kazuo Kobayashi and Ariki Matsuoka</big><ref>DOI 10.1007/s00775-011-0761-3</ref>
 <hr/>
 <b>Molecular Tour</b><br>
 A wide diversity of both structure and function has been discovered in the study of <scene name='Journal:JBIC:8/Rabbit_hb/1'>hemoglobins (Hbs) from many species</scene>. Hbs transport <scene name='Journal:JBIC:8/Rabbit_hb/5'>oxygen</scene> in the red blood cells of higher organisms. Even though oxygen molecules can diffuse into cells, unicellular organisms also have Hb-like molecules. Here, we consider the term 'hemoglobins' to include such molecules. Three classes of Hb have been found in unicellular organisms. First, single-domain globins are comprised of three-over-three (3/3) α-helical folds, as is myoglobin (Mb). Second, flavohemoglobins are distinguished by the presence of an N-terminal globin domain and an additional C-terminal FAD-containing reductase region. Finally, truncated Hbs (trHbs) have been discovered recently and are widely distributed in unicellular organisms.
@@ Line 13: / Line 10: @@
 It is known that trHbs exist in ciliates of the Tetrahymena group, but trHb structure and function remain poorly understood. To investigate trHb function with respect to stability of bound oxygen and protein structure, we measured the oxygen binding kinetics of Tetrahymena pyriformis trHb, and determined the crystal structure of the protein.
-The three-dimensional structure of an <scene name='Journal:JBIC:8/Trhb/2'>Fe(II)-O2 complex of Tp trHb</scene> was determined at 1.73 Å resolution. <scene name='Journal:JBIC:8/Trhb/3'>Tyr25 (B10) and Gln46 (E7) were hydrogen-bonded to a heme-bound dioxygen molecule</scene>. Tyr25 donated a hydrogen bond to the terminal oxygen atom, whereas Gln46 hydrogen-bonded to the proximal oxygen atom. Furthermore, <scene name='Journal:JBIC:8/Trhb/4'>Tyr25 was hydrogen-bonded to the Gln46 and Gln50 (E11) residues</scene>.
+The three-dimensional structure of an <scene name='Journal:JBIC:8/Trhb/2'>Fe(II)-O2 complex of Tp trHb</scene> was determined at 1.73 Å resolution ([[3aq9]]). <scene name='Journal:JBIC:8/Trhb/3'>Tyr25 (B10) and Gln46 (E7) were hydrogen-bonded to a heme-bound dioxygen molecule</scene>. Tyr25 donated a hydrogen bond to the terminal oxygen atom, whereas Gln46 hydrogen-bonded to the proximal oxygen atom. Furthermore, <scene name='Journal:JBIC:8/Trhb/4'>Tyr25 was hydrogen-bonded to the Gln46 and Gln50 (E11) residues</scene>.
+The O<sub>2</sub> association and dissociation rate constants of ''T. pyriformis'' trHb were 5.5 μM<sup>-1</sup> s<sup>-1</sup>, and 0.18 s<sup>-1</sup>, respectively. The oxygen affinity was determined to be 33 nM. The autooxidation rate constant was 3.8 x 10<sup>-3</sup> h<sup>-1</sup>. These values are similar to those of <scene name='Journal:JBIC:8/Hbn/3'>HbN from Mycobacterium tuberculosis</scene>.
-The O<sub>2</sub> association and dissociation rate constants of ''T. pyriformis'' trHb were 5.5 μM<sup>-1</sup> s<sup>-1</sup>, and 0.18 s<sup>-1</sup>, respectively. The oxygen affinity was determined to be 33 nM. The autooxidation rate constant was 3.8 x 10<sup>-3</sup> h<sup>-1</sup>. These values are similar to those of HbN from ''Mycobacterium tuberculosis''. Mutations at <scene name='Journal:JBIC:8/Trhb/8'>Tyr25</scene>, <scene name='Journal:JBIC:8/Trhb/9'>Gln46</scene>, and <scene name='Journal:JBIC:8/Trhb/10'>Gln50</scene> increased the O<sub>2</sub> dissociation and autooxidation rate constants, and <scene name='Journal:JBIC:8/Al/5'>partly disrupted the hydrogen-bonding network</scene>.
+'''Mutations:'''
+*Mutation at Tyr25: <scene name='43/435485/As/6'>Wildtype Y25 and mutant Y25F together</scene> and <scene name='43/435485/As/5'>animation of this scene</scene>. <jmol><jmolButton>
+<script>if (_animating); anim pause;set echo bottom left; color echo white; font echo 20 sansserif;echo Animation Paused; else; anim resume; set echo off;endif;</script>
+<text>Toggle Animation</text>
+</jmolButton></jmol>
+*Mutation at Gln46: <scene name='43/435485/Ad/4'>Wildtype Q46 and mutant Q46E together (animation)</scene> <jmol><jmolButton>
+<script>if (_animating); anim pause;set echo bottom left; color echo white; font echo 20 sansserif;echo Animation Paused; else; anim resume; set echo off;endif;</script>
+<text>Toggle Animation</text>
+</jmolButton></jmol>
+*Mutation at <scene name='Journal:JBIC:8/Trhb/11'>Gln50</scene> increased the O<sub>2</sub> dissociation and autooxidation rate constants, and partly disrupted the hydrogen-bonding network.
-An Fe(III)-H<sub>2</sub>O complex of ''Tp'' trHb was formed following reaction of the Fe(II)-O<sub>2</sub> complex of ''Tp'' trHb, in a crystal state, with nitric oxide. This suggests that ''Tp'' trHb functions in nitric oxide detoxification.
+An <scene name='Journal:JBIC:8/Ag/4'>Fe(III)-H2O complex of Tp trHb was formed following reaction of the Fe(II)-O2 complex of Tp trHb</scene>, in a crystal state, with nitric oxide. This suggests that ''Tp'' trHb functions in nitric oxide detoxification.
+'''PDB reference:''' Crystal structure of truncated hemoglobin from ''Tetrahymena pyriformis'', Fe(II)-O2 form [[3aq5]]; Crystal structure of truncated hemoglobin from ''Tetrahymena pyriformis'', Fe(III) form [[3aq6]]; Crystal structure of truncated hemoglobin from ''Tetrahymena pyriformis'', Y25F mutant, Fe(III) form [[3aq7]]; Crystal structure of truncated hemoglobin from ''Tetrahymena pyriformis'', Q46E mutant, Fe(III) form [[3aq8]]; Crystal structure of truncated hemoglobin from ''Tetrahymena pyriformis'', Q50E mutant, Fe(III) form [[3aq9]].
 </StructureSection>
 <references/>
 __NOEDITSECTION__

Journal:JBIC:8

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A hydrogen-bonding network formed by the B10-E7-E11 residues of a truncated hemoglobin from Tetrahymena pyriformis is critical for stability of bound oxygen and nitric oxide detoxification

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