Sandbox Reserved 1508
From Proteopedia
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{{Sandbox_Reserved_ESBS}}<!-- PLEASE ADD YOUR CONTENT BELOW HERE --> | {{Sandbox_Reserved_ESBS}}<!-- PLEASE ADD YOUR CONTENT BELOW HERE --> | ||
| - | =='''The protein 5C04''' | + | =='''The protein 5C04''' == |
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<StructureSection load='5C04' size='340' side='right' caption='Caption for this structure' scene=''> | <StructureSection load='5C04' size='340' side='right' caption='Caption for this structure' scene=''> | ||
<div align="justified">The protein 5C04 is classified as an oxidoreductase. We found it in the ''Mycobacterium tuberculosis'' organism, especially in the strain ATCC 25618/H37Rv. It can be expressed in ''Escherichia Coli'' bacteria. This is a pathogenic protein which is involved in the tuberculosis. Its pathogenicity is due to a specific mutation in the active site of peroxiredoxins.</div> | <div align="justified">The protein 5C04 is classified as an oxidoreductase. We found it in the ''Mycobacterium tuberculosis'' organism, especially in the strain ATCC 25618/H37Rv. It can be expressed in ''Escherichia Coli'' bacteria. This is a pathogenic protein which is involved in the tuberculosis. Its pathogenicity is due to a specific mutation in the active site of peroxiredoxins.</div> | ||
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In oxidative stress, the organism manage to do a reduction of peroxides. This reaction is catalyzed by the peroxiredoxins. From a structural point of view, a specific amino acid is involved in this reaction: its a nucleophilic cystein, called peroxidatic cystein. In order to understand the mechanism and the specificity of this reaction according to its specific chemical environment, researchers used the ''Mycobacterium tuberculosis'' alkyl hydroperoxide reductase E (MtAhpE) as model (Pedre et al, 2016). The mutational effects of key residues in its environment are located in the active site. These amino acids create an environment favorising the reaction with peroxides. | In oxidative stress, the organism manage to do a reduction of peroxides. This reaction is catalyzed by the peroxiredoxins. From a structural point of view, a specific amino acid is involved in this reaction: its a nucleophilic cystein, called peroxidatic cystein. In order to understand the mechanism and the specificity of this reaction according to its specific chemical environment, researchers used the ''Mycobacterium tuberculosis'' alkyl hydroperoxide reductase E (MtAhpE) as model (Pedre et al, 2016). The mutational effects of key residues in its environment are located in the active site. These amino acids create an environment favorising the reaction with peroxides. | ||
| - | Peroxiredoxins are peroxidases which catalyze the reduction of peroxides (organic peroxide H2O2 or organic hydroperoxides). | + | Peroxiredoxins are peroxidases which catalyze the reduction of peroxides (organic peroxide H2O2 or organic hydroperoxides). |
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The molecular function of the protein are: protein binding, peroxidase, thioredoxin, antioxidant, oxidoreductase and peroxiredoxin activities. | The molecular function of the protein are: protein binding, peroxidase, thioredoxin, antioxidant, oxidoreductase and peroxiredoxin activities. | ||
The biological processes may become involved as a cellular response to oxidative stress, cell redox homeostasis, response to nitrosative stress, evasion or tolerance by symbiont of host produced nitric oxide, oxidation reduction process and cellular oxidant detoxification. | The biological processes may become involved as a cellular response to oxidative stress, cell redox homeostasis, response to nitrosative stress, evasion or tolerance by symbiont of host produced nitric oxide, oxidation reduction process and cellular oxidant detoxification. | ||
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== Structure highlights == | == Structure highlights == | ||
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== Catalytic site == | == Catalytic site == | ||
The article architecture in peroxiredoxins: a case study on ''Mycobacterium tuberculosis'' AhpE (Zeida et al, 2015) describe the active site <scene name='80/802682/Cys45/1'>The active site</scene> of the protein 5C04 by using the model ''Mycobacterium tuberculosis'' AhpE (alkyl hydroperoxide reductases E). Researchers noticed that cysteine is not essential for the binding of H2O2 to the active site of peroxiredoxin. There are conserved residues in the active site which are important for H2O2 binding and reduction: the threonine from the PxxxTxxC sequence motif and an arginine distant in a sequence but close to the active site (Zeida et al, 2015). The conserved arginine plays a pivotal role in bringing the oxygen of the peroxide closer to the catalytic site, weakening the O–O bond and stabilizing the transition state between the proximal O (Zeida et al, 2015). | The article architecture in peroxiredoxins: a case study on ''Mycobacterium tuberculosis'' AhpE (Zeida et al, 2015) describe the active site <scene name='80/802682/Cys45/1'>The active site</scene> of the protein 5C04 by using the model ''Mycobacterium tuberculosis'' AhpE (alkyl hydroperoxide reductases E). Researchers noticed that cysteine is not essential for the binding of H2O2 to the active site of peroxiredoxin. There are conserved residues in the active site which are important for H2O2 binding and reduction: the threonine from the PxxxTxxC sequence motif and an arginine distant in a sequence but close to the active site (Zeida et al, 2015). The conserved arginine plays a pivotal role in bringing the oxygen of the peroxide closer to the catalytic site, weakening the O–O bond and stabilizing the transition state between the proximal O (Zeida et al, 2015). | ||
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At the active site of the enzyme, a pyrodoxal-phosphate cofactor is covalently linked to the Lysine 51 an invariant residue. A parallel β-sheet associated with three α-helices are part of the N terminal domain (residues 46 to 153). Two of those α-helices are part of the dimer interface and the third one is partly forming the entrance of the active site as on the other side of the β-sheet. On the other hand the C-terminal domain is made of 6-stranded mixed β-sheets surrounded by four α-helices (two on each sides) and of residues with a unique insertion of eight amino acids within them. (Ågren et al, 2008) | At the active site of the enzyme, a pyrodoxal-phosphate cofactor is covalently linked to the Lysine 51 an invariant residue. A parallel β-sheet associated with three α-helices are part of the N terminal domain (residues 46 to 153). Two of those α-helices are part of the dimer interface and the third one is partly forming the entrance of the active site as on the other side of the β-sheet. On the other hand the C-terminal domain is made of 6-stranded mixed β-sheets surrounded by four α-helices (two on each sides) and of residues with a unique insertion of eight amino acids within them. (Ågren et al, 2008) | ||
All those compounds allow the enzyme to have several conformations : an open one, a closed one (when a substrate is bound to the enzyme) and an inhibited form (when there is a chlorite bound at an allosteric site). (Ågren et al, 2008) | All those compounds allow the enzyme to have several conformations : an open one, a closed one (when a substrate is bound to the enzyme) and an inhibited form (when there is a chlorite bound at an allosteric site). (Ågren et al, 2008) | ||
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The cysteine are polar uncharged amino acids. It has the particularity to be easily oxidized to form a dimer containing disulfide bridge between two cysteine. Important protein nonpolar residues in the dimer interface have been shown. The proximity between this hydrophobic region and Cys residues allows this kind of substrates to lay most of their aliphatic carbon chains over the patch, supporting the direct interaction of the peroxide group with the reactive thiolate group (Zeida et al, 2015). There is a complex hydrogen bound network which is involved in the Thr and oxygen bonding. | The cysteine are polar uncharged amino acids. It has the particularity to be easily oxidized to form a dimer containing disulfide bridge between two cysteine. Important protein nonpolar residues in the dimer interface have been shown. The proximity between this hydrophobic region and Cys residues allows this kind of substrates to lay most of their aliphatic carbon chains over the patch, supporting the direct interaction of the peroxide group with the reactive thiolate group (Zeida et al, 2015). There is a complex hydrogen bound network which is involved in the Thr and oxygen bonding. | ||
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== Disease == | == Disease == | ||
The Tuberculosis begins with a dormant phase in which ''Mycobacterium tuberculosis'' is surviving within granulomas in the lungs of infected individuals where the environment is characterized by oxidative stress (characterized among other things by the reduction of peroxides). This one leads to the formation of nitrogen monoxide which are used by phagocytic cells to kill internalized bacteria. The first targets of reactive nitrogen intermediates (which comes from the transformation of nitrogen monoxide) are cysteine and tyrosine side chains. | The Tuberculosis begins with a dormant phase in which ''Mycobacterium tuberculosis'' is surviving within granulomas in the lungs of infected individuals where the environment is characterized by oxidative stress (characterized among other things by the reduction of peroxides). This one leads to the formation of nitrogen monoxide which are used by phagocytic cells to kill internalized bacteria. The first targets of reactive nitrogen intermediates (which comes from the transformation of nitrogen monoxide) are cysteine and tyrosine side chains. | ||
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The cysteine synthase (CysM) of Mycobacterium tuberculosis is an ''O''-Phosphoserine Sulfhydrylase (Ägren et al, 2008). The metabolic pathways of biosynthesis of cysteine are important for the synthesis of de novo proteins and for reduced thiol as a component of the oxidative defense mechanisms. That occurs in the dormant state of ''Mycobacterium tuberculosis''. | The cysteine synthase (CysM) of Mycobacterium tuberculosis is an ''O''-Phosphoserine Sulfhydrylase (Ägren et al, 2008). The metabolic pathways of biosynthesis of cysteine are important for the synthesis of de novo proteins and for reduced thiol as a component of the oxidative defense mechanisms. That occurs in the dormant state of ''Mycobacterium tuberculosis''. | ||
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The cysteine synthase CysM is a ''O''-phosphoserine-specific cysteine synthase which belongs to the fold type II pyridoxal 5’-phosphate-dependant enzymes (Ägren et al, 2008). The side chain of Arg220 interacts with the phosphate group by an hydrogen bound allowing the ''O''-phosphoserine bound to the enzyme. | The cysteine synthase CysM is a ''O''-phosphoserine-specific cysteine synthase which belongs to the fold type II pyridoxal 5’-phosphate-dependant enzymes (Ägren et al, 2008). The side chain of Arg220 interacts with the phosphate group by an hydrogen bound allowing the ''O''-phosphoserine bound to the enzyme. | ||
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Thus, the signaling pathway of the cysteine synthase (CysM) of ''Mycobacterium tuberculosis'' leads an ''O''-Phosphoserine binding with the enzyme ''O''-Phosphoserine Sulfhydrylase. This mechanism is independent from the ''O''-acetylserine and sulfate reduction pathway. | Thus, the signaling pathway of the cysteine synthase (CysM) of ''Mycobacterium tuberculosis'' leads an ''O''-Phosphoserine binding with the enzyme ''O''-Phosphoserine Sulfhydrylase. This mechanism is independent from the ''O''-acetylserine and sulfate reduction pathway. | ||
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According to researches on biosynthetic pathway in ''Mycobacterium tuberculosis'' (Burns et al, 2008), there are three pathways implicated cysteine in this disease: the sulfide dependent pathway, the cystathionine pathway and the CysO-thiocarboxylate pathway. For the CysO depending pathway, transcriptional profile analysis shown that cysM and cysO are upregulated under oxidative stress conditions. Moreover, the thiocarboxylate are much more resistant to oxidation than thiols. Thus, when the disease occurs, the environment becomes highly oxidizing due to the macrophages, leads to the cysteine biosynthesis. The CysO-thiocarboxylate evolves as an oxidation resistant form of sulfide, thiol is favored for the cysteine biosynthesis. | According to researches on biosynthetic pathway in ''Mycobacterium tuberculosis'' (Burns et al, 2008), there are three pathways implicated cysteine in this disease: the sulfide dependent pathway, the cystathionine pathway and the CysO-thiocarboxylate pathway. For the CysO depending pathway, transcriptional profile analysis shown that cysM and cysO are upregulated under oxidative stress conditions. Moreover, the thiocarboxylate are much more resistant to oxidation than thiols. Thus, when the disease occurs, the environment becomes highly oxidizing due to the macrophages, leads to the cysteine biosynthesis. The CysO-thiocarboxylate evolves as an oxidation resistant form of sulfide, thiol is favored for the cysteine biosynthesis. | ||
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</StructureSection> | </StructureSection> | ||
Revision as of 14:48, 11 January 2019
| This Sandbox is Reserved from 06/12/2018, through 30/06/2019 for use in the course "Structural Biology" taught by Bruno Kieffer at the University of Strasbourg, ESBS. This reservation includes Sandbox Reserved 1480 through Sandbox Reserved 1543. |
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The protein 5C04
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References
Ågren, Daniel, Robert Schnell, Wulf Oehlmann, Mahavir Singh, et Gunter Schneider. « Cysteine Synthase (CysM) of Mycobacterium Tuberculosis Is an O -Phosphoserine Sulfhydrylase: EVIDENCE FOR AN ALTERNATIVE CYSTEINE BIOSYNTHESIS PATHWAY IN MYCOBACTERIA ». Journal of Biological Chemistry 283, nᵒ 46 (14 novembre 2008): 31567‑74. https://doi.org/10.1074/jbc.M804877200.
Burns, Kristin E., Sabine Baumgart, Pieter C. Dorrestein, Huili Zhai, Fred W. McLafferty, et Tadhg P. Begley. « Reconstitution of a New Cysteine Biosynthetic Pathway in Mycobacterium t Uberculosis ». Journal of the American Chemical Society 127, nᵒ 33 (août 2005): 11602‑3. https://doi.org/10.1021/ja053476x.
Pedre, Brandán, Laura A. H. van Bergen, Anna Palló, Leonardo A. Rosado, Veronica Tamu Dufe, Inge Van Molle, Khadija Wahni, et al. « The Active Site Architecture in Peroxiredoxins: A Case Study on Mycobacterium Tuberculosis AhpE ». Chemical Communications 52, nᵒ 67 (2016): 10293‑96. https://doi.org/10.1039/C6CC02645A.
Rhee, Sue Goo, et Hyun Ae Woo. « Multiple Functions of Peroxiredoxins: Peroxidases, Sensors and Regulators of the Intracellular Messenger H 2 O 2 , and Protein Chaperones ». Antioxidants & Redox Signaling 15, nᵒ 3 (août 2011): 781‑94. https://doi.org/10.1089/ars.2010.3393.
Zeida, Ari, Aníbal M. Reyes, Pablo Lichtig, Martín Hugo, Diego S. Vazquez, Javier Santos, F. Luis González Flecha, Rafael Radi, Dario A. Estrin, et Madia Trujillo. « Molecular Basis of Hydroperoxide Specificity in Peroxiredoxins: The Case of AhpE from Mycobacterium Tuberculosis ». Biochemistry 54, nᵒ 49 (15 décembre 2015): 7237‑47. https://doi.org/10.1021/acs.biochem.5b00758.
