Altered -3 Substrate Specificity of Escherichia coli Signal Peptidase 1 Mutants as Revealed by Screening a Combinatorial Peptide Library

Ekici, Özlem Doğan; Karla, Andrew; Paetzel, Mark; Lively, Mark O.; Pei, Dehua; Dalbey, Ross E.

doi:10.1074/jbc.m608779200

Cited by 18 publications

(30 citation statements)

References 42 publications

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“…One possible explanation for the lack of fidelity is that the cysteine mutation in the binding site results in sliding of the substrate within the active site such that alternative peptide bonds can be hydrolyzed. Moreover, Ile144 and Ile86 control substrate specificity, because mutation of these residues results in substrate cleavage even with an arginine at the Ϫ3 position (35).…”

Section: Signal Peptidase Imentioning

confidence: 99%

Membrane Proteases in the Bacterial Protein Secretion and Quality Control Pathway

Dalbey

Wang

Dijl

2012

Microbiol Mol Biol Rev

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130

129

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SUMMARY Proteolytic cleavage of proteins that are permanently or transiently associated with the cytoplasmic membrane is crucially important for a wide range of essential processes in bacteria. This applies in particular to the secretion of proteins and to membrane protein quality control. Major progress has been made in elucidating the structure-function relationships of many of the responsible membrane proteases, including signal peptidases, signal peptide hydrolases, FtsH, the rhomboid protease GlpG, and the site 1 protease DegS. These enzymes employ very different mechanisms to cleave substrates at the cytoplasmic and extracytoplasmic membrane surfaces or within the plane of the membrane. This review highlights the different ways that bacterial membrane proteases degrade their substrates, with special emphasis on catalytic mechanisms and substrate delivery to the respective active sites.

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Section: Signal Peptidase Imentioning

confidence: 99%

Membrane Proteases in the Bacterial Protein Secretion and Quality Control Pathway

Dalbey

Wang

Dijl

2012

Microbiol Mol Biol Rev

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130

129

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“…The residues with altered chemical shifts were mapped onto the crystal structure of the SPase I Δ2–75 (Figure 3) (5). Virtually all of the perturbed residues are located in one groove on the surface of the protein (Figure 3A).…”

Section: Resultsmentioning

confidence: 99%

“…A model of a wild-type alkaline phosphatase signal peptide cleavage region plus the C-terminal most core region Phe residue (Phe-Cys-Pro-Val-Thr-Lys-Ala) bound to the binding site of SPase I Δ2–75 was prepared using the atomic coordinates from the model of the SPase I Δ2–75 complex with the cleavage region of the beta-lactamase signal peptide deduced from molecular modeling and generously provided by Mark Paetzel (5). Backbone-dependent changes in the signal peptide sequence of the model were prepared using the PyMOL Viewer Software.…”

Section: Methodsmentioning

confidence: 99%

“…The enzyme is thought to catalyze peptide bond hydrolysis via a catalytic dyad involving the hydroxyl of Ser90 for nucleophilic attack and the ε-amine of Lys145 as the general base to cleave the preprotein. Crystal structures of the soluble catalytic domain (SPase I Δ2–75) in the apo-form (3) and with bound inhibitors (4,5) revealed two shallow hydrophobic cavities adjacent to the Ser–Lys dyad that would be appropriate for docking residues −1 and −3 of the signal peptide.…”

mentioning

confidence: 99%

“…To date, these interactions have been inferred from co-crystals of SPase I Δ2–75 with 5 S , 6 S β-lactam (penem) (4) or with the fatty acid derivative, Arylomycin A2 (5), both inhibitors of SPase I activity, and from molecular modeling using the β-lactamase signal peptide to predict its binding locale (5). However, no direct structural analysis of the enzyme with bound signal peptide or preprotein has been accomplished.…”

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confidence: 99%

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A Small Subset of Signal Peptidase Residues are Perturbed by Signal Peptide Binding

2008

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Perturbations of the chemical shifts of a small subset of residues in the catalytically active domain of Escherichia coli signal peptidase I (SPase I) upon binding signal peptide suggest the contact surface on the enzyme for the substrate. SPase I, an integral membrane protein, is vital to preprotein transport in prokaryotic and eukaryotic secretory systems; it binds and proteolyses the N-terminal signal peptide of the preprotein, permitting folding and localization of the mature protein. Employing isotopically labeled C-terminal E. coli SPase I Δ2-75 and an unlabeled soluble synthetic alkaline phosphatase signal peptide, SPase I Δ2-75 was titrated with the signal peptide and 2Δ 1 H-15 N heteronuclear single-quantum correlation nuclear magnetic resonance spectra revealed chemical shifts of specific enzyme residues sensitive to substrate binding. These residues were identified by 3D HNCACB, 3D CBCA(CO)NH, and 3D HN(CO) experiments. Residues Ile80, Glu82, Gln85, Ile86, Ser88, Gly89, Ser90, Met91, Leu95, Ile101, Gly109, Val132, Lys134, Asp142, Ile144, Lys145, and Thr234, alter conformation and are likely all in, or adjacent to, the substrate binding site. The remainder of the enzyme structure is unperturbed. Ramifications for conformational changes for substrate docking and catalysis are discussed. Keywords membrane protein; NMR; signal peptidase; signal peptide; substrate binding Virtually all proteins destined for extracytoplasmic locations are synthesized as preproteins with a cleavable N-terminal extension sequence called the signal peptide. The signal peptide earmarks the preprotein for entry into the appropriate transport pathway and promotes the membrane translocation process via interactions with components of the transport machinery. In the penultimate step of transport, recognition by a signal peptidase is critical for proteolytic removal of the signal peptide and sets the stage for folding of the mature protein and its final localization.The Escherichia coli signal peptidase I (SPase I) is an integral membrane protein of 37 kDa with two transmembrane segments (residues 4-28 and 58-76), a periplasmic N-terminus and C-terminal catalytic domain (residues 77-323) (1,2). The enzyme is thought to catalyze peptide bond hydrolysis via a catalytic dyad involving the hydroxyl of Ser90 for nucleophilic attack and the ε-amine of Lys145 as the general base to cleave the preprotein. Crystal structures of the soluble catalytic domain (SPase I Δ2-75) in the apo-form (3) and with bound inhibitors

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Specificity Profiling of Protein‐Binding Domains Using One‐Bead‐One‐Compound Peptide Libraries

Kunys

Lian

Pei

2012

CP Chemical Biology

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One‐bead‐one‐compound (OBOC) libraries consist of structurally related compounds (e.g., peptides) covalently attached to a solid support, with each resin bead carrying a unique compound. OBOC libraries of high structural diversity can be rapidly synthesized and screened without the need for any special equipment, and therefore can be employed in any chemical or biochemical laboratory. OBOC peptide libraries have been widely used to map the ligand specificity of proteins, to determine the substrate specificity of enzymes, and to develop inhibitors against macromolecular targets. They have proven particularly useful in profiling the binding specificity of protein modular domains (e.g., SH2 domains, BIR domains, and PDZ domains); subsequently, the specificity information can be used to predict the protein targets of these domains. The protocols outlined in this article describe the methodologies for synthesizing and screening OBOC peptide libraries against SH2 and PDZ domains, and the related data analysis. Curr. Protoc. Chem. Biol. 4:331‐355 © 2012 by John Wiley & Sons, Inc.

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Altered -3 Substrate Specificity of Escherichia coli Signal Peptidase 1 Mutants as Revealed by Screening a Combinatorial Peptide Library

Cited by 18 publications

References 42 publications

Membrane Proteases in the Bacterial Protein Secretion and Quality Control Pathway

Membrane Proteases in the Bacterial Protein Secretion and Quality Control Pathway

A Small Subset of Signal Peptidase Residues are Perturbed by Signal Peptide Binding

Specificity Profiling of Protein‐Binding Domains Using One‐Bead‐One‐Compound Peptide Libraries

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