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Substrate binding and specificity of rhomboid intramembrane protease revealed by substrate-peptide complex structures
S. Zoll, S. Stanchev, J. Began, J. Skerle, M. Lepšík, L. Peclinovská, P. Majer, K. Strisovsky,
Language English Country England, Great Britain
Document type Journal Article, Research Support, Non-U.S. Gov't
NLK
Free Medical Journals
from 1982 to 1 year ago
Nature Open Access
from 2003-10-01
PubMed Central
from 1982
Europe PubMed Central
from 1982 to 1 year ago
Open Access Digital Library
from 1997-01-01
Open Access Digital Library
from 1997-01-01
Medline Complete (EBSCOhost)
from 1997-01-02 to 1 year ago
Wiley Free Content
from 1997 to 1 year ago
Springer Nature OA/Free Journals
from 2003-10-01
- MeSH
- Amino Acid Chloromethyl Ketones chemical synthesis pharmacology MeSH
- DNA-Binding Proteins antagonists & inhibitors chemistry genetics metabolism MeSH
- Endopeptidases chemistry genetics metabolism MeSH
- Escherichia coli chemistry enzymology genetics MeSH
- Catalytic Domain MeSH
- Crystallography, X-Ray MeSH
- Membrane Proteins antagonists & inhibitors chemistry genetics metabolism MeSH
- Models, Molecular * MeSH
- Mutation MeSH
- Escherichia coli Proteins antagonists & inhibitors chemistry genetics metabolism MeSH
- Providencia chemistry MeSH
- Recombinant Proteins MeSH
- Molecular Dynamics Simulation * MeSH
- Substrate Specificity MeSH
- Protein Binding MeSH
- Binding Sites MeSH
- Publication type
- Journal Article MeSH
- Research Support, Non-U.S. Gov't MeSH
The mechanisms of intramembrane proteases are incompletely understood due to the lack of structural data on substrate complexes. To gain insight into substrate binding by rhomboid proteases, we have synthesised a series of novel peptidyl-chloromethylketone (CMK) inhibitors and analysed their interactions with Escherichia coli rhomboid GlpG enzymologically and structurally. We show that peptidyl-CMKs derived from the natural rhomboid substrate TatA from bacterium Providencia stuartii bind GlpG in a substrate-like manner, and their co-crystal structures with GlpG reveal the S1 to S4 subsites of the protease. The S1 subsite is prominent and merges into the 'water retention site', suggesting intimate interplay between substrate binding, specificity and catalysis. Unexpectedly, the S4 subsite is plastically formed by residues of the L1 loop, an important but hitherto enigmatic feature of the rhomboid fold. We propose that the homologous region of members of the wider rhomboid-like protein superfamily may have similar substrate or client-protein binding function. Finally, using molecular dynamics, we generate a model of the Michaelis complex of the substrate bound in the active site of GlpG.
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- $a The mechanisms of intramembrane proteases are incompletely understood due to the lack of structural data on substrate complexes. To gain insight into substrate binding by rhomboid proteases, we have synthesised a series of novel peptidyl-chloromethylketone (CMK) inhibitors and analysed their interactions with Escherichia coli rhomboid GlpG enzymologically and structurally. We show that peptidyl-CMKs derived from the natural rhomboid substrate TatA from bacterium Providencia stuartii bind GlpG in a substrate-like manner, and their co-crystal structures with GlpG reveal the S1 to S4 subsites of the protease. The S1 subsite is prominent and merges into the 'water retention site', suggesting intimate interplay between substrate binding, specificity and catalysis. Unexpectedly, the S4 subsite is plastically formed by residues of the L1 loop, an important but hitherto enigmatic feature of the rhomboid fold. We propose that the homologous region of members of the wider rhomboid-like protein superfamily may have similar substrate or client-protein binding function. Finally, using molecular dynamics, we generate a model of the Michaelis complex of the substrate bound in the active site of GlpG.
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