Dynamic changes in the secondary structure of ECE-1 and XCE account for their different substrate specificities

Dynamic changes in the secondary structure of ECE-1 and XCE account for their different substrate specificities

<p>Abstract</p> <p>Background</p> <p>X-converting enzyme (XCE) involved in nervous control of respiration, is a member of the M13 family of zinc peptidases, for which no natural substrate has been identified yet. In contrast, it’s well characterized homologue endothelin...

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Main Authors: Ul-Haq Zaheer, Iqbal Sadaf, Moin Syed
Format: Article
Language:English
Published: BMC 2012-11-01
Series:BMC Bioinformatics
Online Access:http://www.biomedcentral.com/1471-2105/13/285
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spelling doaj-092b3268d3274f5ab21de5d731e917352020-11-24T23:28:06ZengBMCBMC Bioinformatics1471-21052012-11-0113128510.1186/1471-2105-13-285Dynamic changes in the secondary structure of ECE-1 and XCE account for their different substrate specificitiesUl-Haq ZaheerIqbal SadafMoin Syed<p>Abstract</p> <p>Background</p> <p>X-converting enzyme (XCE) involved in nervous control of respiration, is a member of the M13 family of zinc peptidases, for which no natural substrate has been identified yet. In contrast, it’s well characterized homologue endothelin-converting enzyme-1 (ECE-1) showed broad substrate specificity and acts as endopeptidase as well as dipeptidase. To explore the structural differences between XCE and ECE-1, homology model of XCE was built using the complex structure of ECE-1 with phosphoramidon (pdb-id: 3DWB) as template. Phosphoramidon was docked into the binding site of XCE whereas phosphate oxygen of the inhibitor was used as water molecule to design the apo forms of both enzymes. Molecular dynamics simulation of both enzymes was performed to analyze the dynamic nature of their active site residues in the absence and presence of the inhibitor.</p> <p>Results</p> <p>Homology model of XCE explained the role of non-conserved residues of its S2’ subsite. Molecular dynamics (MD) simulations identified the flexible transitions of F149/I150, N566/N571, W714/W719, and R145/R723 residues of ECE-1/XCE for the strong binding of the inhibitor. Secondary structure calculations using DSSP method reveals the folding of R145/R723 residue of ECE-1/XCE into β-sheet structure while unfolding of the S2’ subsite residues in aECE-1 and sustained compact folding of that of aXCE. The results evaluated are in good agreement with available experimental data, thus providing detailed molecular models which can explain the structural and specificities differences between both zinc peptidases.</p> <p>Conclusions</p> <p>Secondary structure changes of both enzymes during the simulation time revealed the importance of β-sheet structure of R145/R723 for its binding with the terminal carboxylate group of the inhibitor. Unfolding of the α-helix comprising the S2’ subsite residues in aECE-1 correlate well with its endopeptidase activity while their compact folding in aXCE may account for the inactivity of the enzyme towards large C-terminal containing substrates.</p> http://www.biomedcentral.com/1471-2105/13/285
collection DOAJ
language English
format Article
sources DOAJ
author Ul-Haq Zaheer
Iqbal Sadaf
Moin Syed
spellingShingle Ul-Haq Zaheer
Iqbal Sadaf
Moin Syed
Dynamic changes in the secondary structure of ECE-1 and XCE account for their different substrate specificities
BMC Bioinformatics
author_facet Ul-Haq Zaheer
Iqbal Sadaf
Moin Syed
author_sort Ul-Haq Zaheer
title Dynamic changes in the secondary structure of ECE-1 and XCE account for their different substrate specificities
title_short Dynamic changes in the secondary structure of ECE-1 and XCE account for their different substrate specificities
title_full Dynamic changes in the secondary structure of ECE-1 and XCE account for their different substrate specificities
title_fullStr Dynamic changes in the secondary structure of ECE-1 and XCE account for their different substrate specificities
title_full_unstemmed Dynamic changes in the secondary structure of ECE-1 and XCE account for their different substrate specificities
title_sort dynamic changes in the secondary structure of ece-1 and xce account for their different substrate specificities
publisher BMC
series BMC Bioinformatics
issn 1471-2105
publishDate 2012-11-01
description <p>Abstract</p> <p>Background</p> <p>X-converting enzyme (XCE) involved in nervous control of respiration, is a member of the M13 family of zinc peptidases, for which no natural substrate has been identified yet. In contrast, it’s well characterized homologue endothelin-converting enzyme-1 (ECE-1) showed broad substrate specificity and acts as endopeptidase as well as dipeptidase. To explore the structural differences between XCE and ECE-1, homology model of XCE was built using the complex structure of ECE-1 with phosphoramidon (pdb-id: 3DWB) as template. Phosphoramidon was docked into the binding site of XCE whereas phosphate oxygen of the inhibitor was used as water molecule to design the apo forms of both enzymes. Molecular dynamics simulation of both enzymes was performed to analyze the dynamic nature of their active site residues in the absence and presence of the inhibitor.</p> <p>Results</p> <p>Homology model of XCE explained the role of non-conserved residues of its S2’ subsite. Molecular dynamics (MD) simulations identified the flexible transitions of F149/I150, N566/N571, W714/W719, and R145/R723 residues of ECE-1/XCE for the strong binding of the inhibitor. Secondary structure calculations using DSSP method reveals the folding of R145/R723 residue of ECE-1/XCE into β-sheet structure while unfolding of the S2’ subsite residues in aECE-1 and sustained compact folding of that of aXCE. The results evaluated are in good agreement with available experimental data, thus providing detailed molecular models which can explain the structural and specificities differences between both zinc peptidases.</p> <p>Conclusions</p> <p>Secondary structure changes of both enzymes during the simulation time revealed the importance of β-sheet structure of R145/R723 for its binding with the terminal carboxylate group of the inhibitor. Unfolding of the α-helix comprising the S2’ subsite residues in aECE-1 correlate well with its endopeptidase activity while their compact folding in aXCE may account for the inactivity of the enzyme towards large C-terminal containing substrates.</p>
url http://www.biomedcentral.com/1471-2105/13/285
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AT moinsyed dynamicchangesinthesecondarystructureofece1andxceaccountfortheirdifferentsubstratespecificities
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