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[http://media.axon.es/pdf/90977_2.pdf] pockets
[http://media.axon.es/pdf/90977_2.pdf] pockets
[http://www.enzim.hu/~lbarna/articles/17275314.pdf]
[http://www.enzim.hu/~lbarna/articles/17275314.pdf]
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== Structure and domains ==
== Structure and domains ==
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Unfortunately, no structure of the full MMP8 protein have been crystallized yet, but <scene name='71/719866/Human_prommp-1_structure/1'>here</scene> you can see in orange the hemopexin domain of human pro-MMP1 which is very well conserved between these two proteins, by the way you can find in this article: [http://www.fasebj.org/content/12/12/1075.full#ref-27 Matrix metalloproteinases: structures, evolution, and diversification,Irina Massova, Lakshmi P. Kotra, Rafael Fridman and Shahriar Mobashery], good pieces of information on conservations among the MMPs family.
Unfortunately, no structure of the full MMP8 protein have been crystallized yet, but <scene name='71/719866/Human_prommp-1_structure/1'>here</scene> you can see in orange the hemopexin domain of human pro-MMP1 which is very well conserved between these two proteins, by the way you can find in this article: [http://www.fasebj.org/content/12/12/1075.full#ref-27 Matrix metalloproteinases: structures, evolution, and diversification,Irina Massova, Lakshmi P. Kotra, Rafael Fridman and Shahriar Mobashery], good pieces of information on conservations among the MMPs family.
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To express collagenolytic activity, MMP-8 needs to have both the catalytic and hemopexin domains. The linker peptide can position the hemopexin domain in such a way that it bends over the active site of the catalytic domain. But understanding how the Hemopexin domain assists in the cleavage of collagen is elusive.<ref>PMID:15257288</ref> Thus, the collagen would be captured between these two domains. However, the active site cannot accommodate the entire triple helix in a native state. The linker peptide would, by means of its collagen-like conformation, change the quaternary structure of the captured collagen. Interactions between proline residues of the collagenase and a specific region of the collagen would generate a “proline zipper,” resulting in destabilization of the cleavage site area of the collagen. After destabilization, one chain of the triple helix fits in the specificity pocket or <scene name='71/719866/S1prime_pocket/1'>S1' pocket</scene> to the right of the active-site zinc. At first, the Gly residue of the substrate binds the <scene name='71/719866/Catalytic_site/4'>active site</scene> thanks to the Zn2+ atom. When it binds it takes the place of unstable water molecules and establishes stabilizing interactions with the active site thanks to its C terminal part.<ref>PMID:17185359</ref> The carboxyl group of the glutamate serves as a general base to draw a proton from the displaced water molecule, thereby facilitating the nucleophilic attack of the water molecule on the carbonyl carbon of the peptide scissile bond. Then, the Alanine residue of the enzyme makes a hydrogen bond with the NH group of the substrate. Moreover, this NH group becomes the new N-terminus after cleavage.<ref name="inhibitor">PMID:12730128</ref>
To express collagenolytic activity, MMP-8 needs to have both the catalytic and hemopexin domains. The linker peptide can position the hemopexin domain in such a way that it bends over the active site of the catalytic domain. But understanding how the Hemopexin domain assists in the cleavage of collagen is elusive.<ref>PMID:15257288</ref> Thus, the collagen would be captured between these two domains. However, the active site cannot accommodate the entire triple helix in a native state. The linker peptide would, by means of its collagen-like conformation, change the quaternary structure of the captured collagen. Interactions between proline residues of the collagenase and a specific region of the collagen would generate a “proline zipper,” resulting in destabilization of the cleavage site area of the collagen. After destabilization, one chain of the triple helix fits in the specificity pocket or <scene name='71/719866/S1prime_pocket/1'>S1' pocket</scene> to the right of the active-site zinc. At first, the Gly residue of the substrate binds the <scene name='71/719866/Catalytic_site/4'>active site</scene> thanks to the Zn2+ atom. When it binds it takes the place of unstable water molecules and establishes stabilizing interactions with the active site thanks to its C terminal part.<ref>PMID:17185359</ref> The carboxyl group of the glutamate serves as a general base to draw a proton from the displaced water molecule, thereby facilitating the nucleophilic attack of the water molecule on the carbonyl carbon of the peptide scissile bond. Then, the Alanine residue of the enzyme makes a hydrogen bond with the NH group of the substrate. Moreover, this NH group becomes the new N-terminus after cleavage.<ref name="inhibitor">PMID:12730128</ref>
The cleavage is at Gly775–Ile776 or Leu776 in each alpha-chain of the collagen molecule<ref name="hinge"/> and takes place at neutral pH. It generates fragments that spontaneously lose their helical conformation, denature to gelatin, and become soluble. The gelatin is then susceptible to attack by gelatinases and other proteases.<ref>[http://www.ebi.ac.uk/interpro/entry/IPR028709 "Neutrophil collagenase"]</ref>
The cleavage is at Gly775–Ile776 or Leu776 in each alpha-chain of the collagen molecule<ref name="hinge"/> and takes place at neutral pH. It generates fragments that spontaneously lose their helical conformation, denature to gelatin, and become soluble. The gelatin is then susceptible to attack by gelatinases and other proteases.<ref>[http://www.ebi.ac.uk/interpro/entry/IPR028709 "Neutrophil collagenase"]</ref>
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== Inhibitors of MMP-8 ==
== Inhibitors of MMP-8 ==
=== Endogenous inhibitors ===
=== Endogenous inhibitors ===
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The tissue inhibitors of metalloproteinases (TIMPs) are specific inhibitors of the whole family of MMPs proteins. Currently, four TIMPs were identified (TIMP-1, TIMP-2, TIMP-3, TIMP-4).
The tissue inhibitors of metalloproteinases (TIMPs) are specific inhibitors of the whole family of MMPs proteins. Currently, four TIMPs were identified (TIMP-1, TIMP-2, TIMP-3, TIMP-4).
They are 21 to 29kDa proteins, contain 2 subdomains (N-ter and C-ter) and have a "wedge-like" shape.
They are 21 to 29kDa proteins, contain 2 subdomains (N-ter and C-ter) and have a "wedge-like" shape.
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=== Synthetic inhibitors ===
=== Synthetic inhibitors ===
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Because endogenous TIMPs have a broad spectrum of action over MMPs, researches were conducted to produce engineered TIMPs and modify their affinity for MMPs. For instance, mutation of the Thr2 of TIMP-1 modify the specificity of this inhibitor as this residue interacts with the S1' pocket of the MMPs.<ref>PMID:20080133</ref>
Because endogenous TIMPs have a broad spectrum of action over MMPs, researches were conducted to produce engineered TIMPs and modify their affinity for MMPs. For instance, mutation of the Thr2 of TIMP-1 modify the specificity of this inhibitor as this residue interacts with the S1' pocket of the MMPs.<ref>PMID:20080133</ref>
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Recently, new range of inhibitors which do not chelate the catalytic zinc were developped. Those compounds target the selectivity regions for substrates of the MMPs rather than binding to the catalytic zinc. For instance, they can interact with the S1' pocket and induce a conformational change like <scene name='71/719866/Non-chelating_inhibitor/2'>new inhibitors</scene> of MMP-8.<ref>[http://www.rcsb.org/pdb/explore/explore.do?structureId=3DPE 'Crystal structure of the complex between MMP-8 and a non-zinc chelating inhibitor']</ref>
Recently, new range of inhibitors which do not chelate the catalytic zinc were developped. Those compounds target the selectivity regions for substrates of the MMPs rather than binding to the catalytic zinc. For instance, they can interact with the S1' pocket and induce a conformational change like <scene name='71/719866/Non-chelating_inhibitor/2'>new inhibitors</scene> of MMP-8.<ref>[http://www.rcsb.org/pdb/explore/explore.do?structureId=3DPE 'Crystal structure of the complex between MMP-8 and a non-zinc chelating inhibitor']</ref>
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== Function ==
== Function ==
A major function of MMPs is thought to be the removal of ECM in tissue resorption. Because of their recognized role in disease (see below) the MMPs have long been considered as pharmacological targets, but their multiplicity, associated with their variable expression in different tissues and their apparently overlapping substrate specificities, has presented considerable challenges to those hoping to design suitable therapeutic inhibitors.
A major function of MMPs is thought to be the removal of ECM in tissue resorption. Because of their recognized role in disease (see below) the MMPs have long been considered as pharmacological targets, but their multiplicity, associated with their variable expression in different tissues and their apparently overlapping substrate specificities, has presented considerable challenges to those hoping to design suitable therapeutic inhibitors.
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== Disease ==
== Disease ==
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== References ==
== References ==
<references />
<references />
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RESSOURCE : Image:2oy4 mm1.pdb ( la structure du monomère )
 

Revision as of 15:20, 30 January 2016

Matrix metalloproteinase-8

MMP-8, also called, Neutrophil collagenase or Collagenase 2, is a zinc-dependent and calcium-dependent enzyme. It belongs to the Matrix metalloproteinase (MMP) family which is involved in the breakdown of extracellular matrix in embryonic development, reproduction, and tissue remodeling, as well as in disease processes. The gene coding this family is localized on the chromosome 11 of Homo sapiens with 467 residues.[1]

is the initial structure of the catalytic domain of MMP-8.

MMP-8 catalytic domain

Drag the structure with the mouse to rotate

References

  1. "MMP-8 matrix metallopeptidase 8 (neutrophil collagenase)"
  2. "Metalloendopeptidase activity"
  3. Stams T, Spurlino JC, Smith DL, Wahl RC, Ho TF, Qoronfleh MW, Banks TM, Rubin B. Structure of human neutrophil collagenase reveals large S1' specificity pocket. Nat Struct Biol. 1994 Feb;1(2):119-23. PMID:7656015
  4. 4.0 4.1 Substrate specificity of MMPs
  5. 5.0 5.1 5.2 Bode W, Reinemer P, Huber R, Kleine T, Schnierer S, Tschesche H. The X-ray crystal structure of the catalytic domain of human neutrophil collagenase inhibited by a substrate analogue reveals the essentials for catalysis and specificity. EMBO J. 1994 Mar 15;13(6):1263-9. PMID:8137810
  6. 6.0 6.1 Knauper V, Docherty AJ, Smith B, Tschesche H, Murphy G. Analysis of the contribution of the hinge region of human neutrophil collagenase (HNC, MMP-8) to stability and collagenolytic activity by alanine scanning mutagenesis. FEBS Lett. 1997 Mar 17;405(1):60-4. PMID:9094424
  7. Hirose T, Patterson C, Pourmotabbed T, Mainardi CL, Hasty KA. Structure-function relationship of human neutrophil collagenase: identification of regions responsible for substrate specificity and general proteinase activity. Proc Natl Acad Sci U S A. 1993 Apr 1;90(7):2569-73. PMID:8464863
  8. Van Wart HE, Birkedal-Hansen H. The cysteine switch: a principle of regulation of metalloproteinase activity with potential applicability to the entire matrix metalloproteinase gene family. Proc Natl Acad Sci U S A. 1990 Jul;87(14):5578-82. PMID:2164689
  9. Chung L, Dinakarpandian D, Yoshida N, Lauer-Fields JL, Fields GB, Visse R, Nagase H. Collagenase unwinds triple-helical collagen prior to peptide bond hydrolysis. EMBO J. 2004 Aug 4;23(15):3020-30. Epub 2004 Jul 15. PMID:15257288 doi:http://dx.doi.org/10.1038/sj.emboj.7600318
  10. Piccard H, Van den Steen PE, Opdenakker G. Hemopexin domains as multifunctional liganding modules in matrix metalloproteinases and other proteins. J Leukoc Biol. 2007 Apr;81(4):870-92. Epub 2006 Dec 21. PMID:17185359 doi:http://dx.doi.org/10.1189/jlb.1006629
  11. 11.0 11.1 Visse R, Nagase H. Matrix metalloproteinases and tissue inhibitors of metalloproteinases: structure, function, and biochemistry. Circ Res. 2003 May 2;92(8):827-39. PMID:12730128 doi:http://dx.doi.org/10.1161/01.RES.0000070112.80711.3D
  12. "Neutrophil collagenase"
  13. Nagase H, Visse R, Murphy G. Structure and function of matrix metalloproteinases and TIMPs. Cardiovasc Res. 2006 Feb 15;69(3):562-73. Epub 2006 Jan 5. PMID:16405877 doi:http://dx.doi.org/10.1016/j.cardiores.2005.12.002
  14. [http://www.rcsb.org/pdb/explore/explore.do?structureId=1UEA "Metalloprotease-Inhibitor Complex
  15. Brew K, Nagase H. The tissue inhibitors of metalloproteinases (TIMPs): an ancient family with structural and functional diversity. Biochim Biophys Acta. 2010 Jan;1803(1):55-71. doi: 10.1016/j.bbamcr.2010.01.003. , Epub 2010 Jan 15. PMID:20080133 doi:http://dx.doi.org/10.1016/j.bbamcr.2010.01.003
  16. Jacobsen JA, Major Jourden JL, Miller MT, Cohen SM. To bind zinc or not to bind zinc: an examination of innovative approaches to improved metalloproteinase inhibition. Biochim Biophys Acta. 2010 Jan;1803(1):72-94. doi: 10.1016/j.bbamcr.2009.08.006. , Epub 2009 Aug 25. PMID:19712708 doi:http://dx.doi.org/10.1016/j.bbamcr.2009.08.006
  17. 'Crystal structure of the complex between MMP-8 and a N-hydroxyurea inhibitor'
  18. 'Crystal structure of the complex between MMP-8 and a non-zinc chelating inhibitor'
  19. "Extra Binding Region Induced by Non-Zinc Chelating Inhibitors into the S1′ Subsite of Matrix Metalloproteinase 8"
  20. Savill NJ, Weller R, Sherratt JA. Mathematical modelling of nitric oxide regulation of rete peg formation in psoriasis. J Theor Biol. 2002 Jan 7;214(1):1-16. PMID:11786028 doi:http://dx.doi.org/10.1006/jtbi.2001.2400
  21. Larochelle C, Alvarez JI, Prat A. How do immune cells overcome the blood-brain barrier in multiple sclerosis? FEBS Lett. 2011 Dec 1;585(23):3770-80. doi: 10.1016/j.febslet.2011.04.066. Epub, 2011 May 4. PMID:21550344 doi:http://dx.doi.org/10.1016/j.febslet.2011.04.066
  22. Westermarck J, Kahari VM. Regulation of matrix metalloproteinase expression in tumor invasion. FASEB J. 1999 May;13(8):781-92. PMID:10224222
  23. Liu KZ, Hynes A, Man A, Alsagheer A, Singer DL, Scott DA. Increased local matrix metalloproteinase-8 expression in the periodontal connective tissues of smokers with periodontal disease. Biochim Biophys Acta. 2006 Aug;1762(8):775-80. Epub 2006 Jul 22. PMID:16928431 doi:http://dx.doi.org/10.1016/j.bbadis.2006.05.014
  24. Balbin M, Fueyo A, Knauper V, Pendas AM, Lopez JM, Jimenez MG, Murphy G, Lopez-Otin C. Collagenase 2 (MMP-8) expression in murine tissue-remodeling processes. Analysis of its potential role in postpartum involution of the uterus. J Biol Chem. 1998 Sep 11;273(37):23959-68. PMID:9727011
  25. Brand KH, Ahout IM, de Groot R, Warris A, Ferwerda G, Hermans PW. Use of MMP-8 and MMP-9 to assess disease severity in children with viral lower respiratory tract infections. J Med Virol. 2012 Sep;84(9):1471-80. doi: 10.1002/jmv.23301. PMID:22825827 doi:http://dx.doi.org/10.1002/jmv.23301
  26. Gao M, Nguyen TT, Suckow MA, Wolter WR, Gooyit M, Mobashery S, Chang M. Acceleration of diabetic wound healing using a novel protease-anti-protease combination therapy. Proc Natl Acad Sci U S A. 2015 Dec 8;112(49):15226-31. doi:, 10.1073/pnas.1517847112. Epub 2015 Nov 23. PMID:26598687 doi:http://dx.doi.org/10.1073/pnas.1517847112
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