Influence of Charge Distribution at the Active Site Surface on the Substrate Specificity of Human Neutrophil Protease 3 and Elastase

Korkmaz, Brice; Hajjar, Eric; Kalupov, Timofey; Reuter, Nathalie; Brillard-Bourdet, Michèle; Moreau, Thierry; Juliano, Luiz; Gauthier, Francis

doi:10.1074/jbc.m608700200

Cited by 53 publications

(85 citation statements)

References 43 publications

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“…4B). In agreement with structural data, HNE and PR3 preferentially accommodate small hydrophobic residues (Val, Cys, Ala, Met, Ile) (Brubaker et al, 1992;Koehl et al, 2003;Korkmaz et al, 2007;Wysocka et al, 2007) in the S1 pocket, whereas CG has both a chymotrypsin-like and a trypsin-like specificity, permitting both large, hydrophobic P1 residues (Phe, Leu, Met) and positive Lys or Arg residues (Tanaka et al, 1985). The S2 subsites of HNE and CG are bordered by Phe215, Leu99, and the flat side of the imidazole ring of the catalytic triad His57, which is quite hydrophobic.…”

Section: Structural Characteristics and Proteolytic Specificitysupporting

confidence: 61%

“…Indeed, most commercially available chromogenic and/or fluorogenic substrates used to measure HNE and CG display a proline at the P2 position. Because of the presence of Lys99, PR3 preferentially accommodates a negatively charged residue at P2 (Hajjar et al, 2006;Korkmaz et al, 2007). The S3 subsite of CG is formed by a Lys at position 192, which favors interaction with an acidic P3 residue (Tanaka et al, 1985).…”

Section: Neutrophil Serine Proteasesmentioning

confidence: 99%

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Neutrophil Elastase, Proteinase 3, and Cathepsin G as Therapeutic Targets in Human Diseases

et al. 2010

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Section: Structural Characteristics and Proteolytic Specificitysupporting

confidence: 61%

Section: Neutrophil Serine Proteasesmentioning

confidence: 99%

Neutrophil Elastase, Proteinase 3, and Cathepsin G as Therapeutic Targets in Human Diseases

et al. 2010

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“…Substrate hydrolysis was followed by measuring the fluorescence at ex ϭ 320 nm and em ϭ 420 nm, as reported earlier (18,21).…”

Section: Methodsmentioning

confidence: 99%

Structural Characterization of Mouse Neutrophil Serine Proteases and Identification of Their Substrate Specificities

Kalupov

Brillard-Bourdet

Dadé

et al. 2009

Journal of Biological Chemistry

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It is widely accepted that neutrophil serine proteases (NSPs) play a critical role in neutrophil-associated lung inflammatory and tissue-destructive diseases. To investigate NSP pathogenic role(s), various mouse experimental models have been developed that mimic acutely or chronically injured human lungs. We and others are using mouse exposure to cigarette smoke as a model for chronic obstructive pulmonary disease with or without exacerbation. However, the relative contribution of NSPs to lung disease processes as well as their underlying mechanisms remains still poorly understood. And the lack of purified mouse NSPs and their specific substrates have hampered advances in these studies. In this work, we compared mouse and human NSPs and generated three-dimensional models of murine NSPs based on three-dimensional structures of their human homologs. Analyses of these models provided compelling evidence that peptide substrate specificities of human and mouse NSPs are different despite their conserved cleft and close structural resemblance. These studies allowed us to synthesize for the first time novel sensitive fluorescence resonance energy transfer substrates for individual mouse NSPs. Our findings and the newly identified substrates should better our understanding about the role of NSPs in the pathogenesis of cigarette-associated chronic obstructive pulmonary disease as well as other neutrophils-associated inflammatory diseases.Neutrophil serine proteases (NSPs), 3 neutrophil elastase (NE), cathepsin G (CG), and proteinase 3 (Pr3), are mainly stored in neutrophil primary granules in readily active forms. NSPs are structurally related and share the conserved chargerelay triad, His 57 -Asp , where Ser is the active residue (chymotrypsinogen numbering) (1). NSPs contribute to neutrophil oxygen-independent system-mediated protection of the host against invading pathogens (2). Indeed, NSPs serve a physiological role for killing of microbes (3). Activated neutrophils are also known to release NSPs in the setting of inflammation. In vitro, NSPs are capable of cleaving a panoply of substrates. These include extracellular matrix proteins, pro-inflammatory mediators, coagulation factors, and immunoglobulins (4). NE degrades pro-inflammatory mediators such as tumor necrosis factor-␣ and interleukin-1␤, hence could alter the inflammatory response. The enzyme is capable of inducing the secretion of granulocyte macrophage-colony stimulating factor and interleukin-8, which could amplify the inflammation. Consequently, the release of these potent proteinases in diseased situations could create a proteolytic environment where degradation of different host molecules might occur and result in inappropriate inflammatory response. Because of their large substrate repertoire, NSPs have been implicated in the pathogenesis of various inflammatory and tissue-destructive diseases, including acute lung injury, cystic fibrosis, and COPD (5-7).COPD is recognized as a major health problem whose worldwide incidence is increasing dramatically...

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“…The only exception is the very conservative Ile-208 substitution on the back side of the hPR3 molecule by a Val, which is one methyl group shorter. Active site residues K99, D61, and R143 implicated in the substrate binding of hPR3 and conferring its specificity are not substituted on gPR3 (24)(25)(26). Fig.…”

Section: Structural Characteristics Of Gpr3mentioning

confidence: 96%

Mapping of Conformational Epitopes on Human Proteinase 3, the Autoantigen of Wegener’s Granulomatosis

Kuhl

Korkmaz

Utecht³

et al. 2010

The Journal of Immunology

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Anti-neutrophil cytoplasmic Abs (cANCAs) against conformational epitopes of proteinase 3 (PR3) are regarded as an important pathogenic marker in Wegener’s granulomatosis (WG). Although the three-dimensional structure of PR3 is known, binding sites of mAbs and cANCAs have not been mapped to date. Competitive binding and biosensor experiments suggested the existence of four nonoverlapping areas on the PR3 surface. In this paper, we present an approach to identify these discontinuous surface regions that cannot be mimicked by linear peptides. The very few surface substitutions found in closely related PR3 homologs from primates, which were further varied by the construction of functional human-gibbon hybrids, resulted in the differential loss of three Ab binding sites, two of which were mapped to the N-terminal β-barrel and one to the linker segment connecting the N- and C-terminal barrels of PR3. The sera from WG patients differed in their binding to gibbon PR3 and the gibbon-human PR3 hybrid, and could be divided into two groups with similar or significantly reduced binding to gibbon PR3. Binding of almost all sera to PR3–α1-protease inhibitor (α1–PI) complexes was even more reduced and often absent, indicating that major antigenic determinants overlap with the active site surface on PR3 that associates with α1-PI. Similarly, the mouse mAbs CLB12.8 and 6A6 also did not react with gibbon PR3 and PR3–α1-PI complexes. Our data strongly suggest that cANCAs from WG patients at least in part recognize similar surface structures as do mouse mAbs and compete with the binding of α1-PI to PR3.

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Influence of Charge Distribution at the Active Site Surface on the Substrate Specificity of Human Neutrophil Protease 3 and Elastase

Cited by 53 publications

References 43 publications

Neutrophil Elastase, Proteinase 3, and Cathepsin G as Therapeutic Targets in Human Diseases

Neutrophil Elastase, Proteinase 3, and Cathepsin G as Therapeutic Targets in Human Diseases

Structural Characterization of Mouse Neutrophil Serine Proteases and Identification of Their Substrate Specificities

Mapping of Conformational Epitopes on Human Proteinase 3, the Autoantigen of Wegener’s Granulomatosis

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