High-affinity urokinase receptor antagonists identified with bacteriophage peptide display.

Goodson, Robert J.; Doyle, Michael; Kaufman, Susan; Rosenberg, Steven

doi:10.1073/pnas.91.15.7129

Cited by 178 publications

(129 citation statements)

References 42 publications

(37 reference statements)

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“…Using the cyclic disulfide-bridged form of the minimal uPAR-binding region as lead structure (cyclo 19,31 uPA 19-31 ), we have identified cyclo 19,31 ]-uPA 19-31 as -to our knowledge -the most potent competitive uPA-antagonist presently known that displays only a 20-to 40-fold lower uPAR-binding capacity as compared to the natural uPAR ligands uPA or ATF. Cyclo 19,31 ]-uPA 19-31 inhibits binding of uPA to uPAR on human tumor cells with more than 3-fold higher efficiency compared to the lead structure and at least with 10-fold higher efficiency compared to a high affinity uPAR ligand (clone 20 peptide) derived from bacteriophage display (Goodson et al, 1994;Bürgle et al, 1997). Furthermore, cyclo 19,31 ]-uPA 19-31 efficiently displaces uPAR-bound uPA from the cell surface of human cells and inhibits uPA-mediated, cell-associated plasminogen activation and fibrin degradation.…”

Section: Discussionmentioning

confidence: 99%

“…Other types of peptide antagonists of uPA/uPAR-interaction, which show no obvious similarity to uPA [19][20][21][22][23][24][25][26][27][28][29][30][31] , have been identified by a bacteriophage peptide display approach (Goodson et al, 1994). All of the reactive peptides (with the clone 20 peptide being most active) harbor relatively short common motifs, such as LWXXY and FXXYLW, which may represent a variation of the motif 24 YFXXIXW 30 within the uPA molecule (only the critical hydrophobic amino acids for uPAR-binding are depicted) (Magdolen et al, 1996;Bürgle et al, 1997).…”

Section: Introductionmentioning

confidence: 99%

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Cyclo19,31[D-Cys19]-uPA19-31 Is a Potent Competitive Antagonist of the Interaction of Urokinase-Type Plasminogen Activator with Its Receptor (CD87)

Magdolen

Bürgle²,

Na³

et al. 2001

Biological Chemistry

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IntroductionThe serine proteases urokinase-type plasminogen activator (uPA) and plasmin, in concert with other proteolytic enzymes (e. g. matrix metalloproteases, cysteine proteases), are involved in tumor-associated processes such as cell invasion and regulation of cell/cell and cell/matrix contacts Schmitt et al., 2000;Andreasen et al., 2000). (pro-)uPA binds to a specific, high-affinity cell surface receptor, uPAR (CD87), which is composed of three structurally homologous, independently folded domains (Dear and Medcalf, 1998). In addition, there are also cellular binding sites for plasmin(ogen) (Félez, 1998). In consequence, binding of (pro-) uPA to cell membrane-anchored uPAR significantly increases plasmin generation due to a distinct increase of reciprocal activation of pro-uPA and plasminogen (Ellis et al., 1991). Plasmin not only degrades a variety of components of the extracellular matrix (e. g. fibrin and laminin), but also activates certain matrix metalloproteases (in addition to pro-uPA) which break down additional structural proteins of the extracellular matrix such as various collagens. Thus, cell surface-triggered plasminogen activation plays a fundamental role in tissue remodeling, which is a prerequisite for tumor cell invasion and metastasis Schmitt et al., 2000;Andreasen et al., 2000).The interaction of pro-uPA or its activated form high molecular weight (HMW-)uPA with uPAR has been characterised in detail. Although the N-terminal domain I of uPAR contains major determinants for uPA-binding, high affinity interaction with uPA is dependent on the multidomain structure of the receptor, indicating that all three protein domains are involved in the formation of a composite ligand binding site (Ploug, 1998;Gårdsvoll et al., 1999;Bdeir et al., 2000). In contrast, uPA binds to uPAR via a defined continuous peptide sequence

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Section: Discussionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Cyclo19,31[D-Cys19]-uPA19-31 Is a Potent Competitive Antagonist of the Interaction of Urokinase-Type Plasminogen Activator with Its Receptor (CD87)

Magdolen

Bürgle²,

Na³

et al. 2001

Biological Chemistry

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“…Peptides are predicted to lack stability due to susceptibility to exoproteinase degradation in the plasma. High-affinity peptide ligands of uPAR that have been identified by phage display [112,113] may circumvent some of the pharmacological problems typically associated with peptide therapy. Alternatively, anti-uPAR antibodies [114] or non-peptidic small-molecule antagonists of uPA binding have been described [100].…”

Section: Inhibition Of Upa-upar Interactionsmentioning

confidence: 99%

Role of plasminogen activator-plasmin system in tumor angiogenesis

Rakic¹,

Maillard²,

Jost³

et al. 2003

Cellular and Molecular Life Sciences (CMLS)

118

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New blood formation or angiogenesis has become a key target in therapeutic strategies aimed at inhibiting tumor growth and other diseases associated with neovascularization. Angiogenesis is associated with important extracellular remodeling involving different proteolytic systems among which the plasminogen system plays an essential role. It belongs to the large serine proteinase family and can act directly or indirectly by activating matrix metalloproteinases or by liberating growth factors and cytokines sequestered within the extracellular matrix. Migration of endothelial cells is associated with significant upregulation of proteolysis and conversely, immunoneutralization or chemical inhibition of the system reduces angiogenesis in vitro. On the other hand genetically altered mice developed normally without overt vascular anomalies indicating the possibility of compensation by other proteases in vivo. Nevertheless, they have in some experimental settings revealed unanticipated roles for previously characterized proteinases or their inhibitors. In this review, the complex mechanisms of action of the serine proteases in pathological angiogenesis are summarized alongside possible therapeutic applications.

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“…And lots of antagonists were identified from phage displayed peptide libraries, such as urokinase receptor antagonists and the human type I interleukin (IL)-1 receptor antagonist [14][15][16][17]. However, there are some difficulties for membrane receptors to be purified and maintain the natural conformation.…”

Section: Introductionmentioning

confidence: 99%

Phage display selection on whole cells yields a small peptide specific for HCV receptor human CD81

Cao

Zhao

et al. 2003

Cell Res

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The human CD81 (hCD81), the most recently proposed receptor of hepatitis C virus (HCV), can especifically bind to HCV envelope glycoprotein 2 (E2). In this study, hCD81-expressing murine NIH/3T3 cells were used to select hCD81-binding peptides from a phage displayed nonapeptide library (PVIII9aaCys). Eighteen of the 75 clones selected from the library showed specific binding to the hCD81-expressing NIH/3T3 cells by enzyme linked immunosorbent assay (ELISA) and competitive inhibition test. Twelve out of the 18 clones shared the amino acid motif SPQYWTGPA. Sequence comparison of the motif showed no amino acid homology with the native HCV E2. The motif-containing phages could competitively inhibit the ability of HCV E2 binding to native hCD81-expressing MOLT-4 cells, and induce HCV E2 specific immune response in vivo. These results suggest that the selected motif SPQYWTGPA should be a mimotope of HCV E2 to bind to hCD81 molecules. Our findings cast new light on developing HCV receptor antagonists.

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High-affinity urokinase receptor antagonists identified with bacteriophage peptide display.

Cited by 178 publications

References 42 publications

Cyclo19,31[D-Cys19]-uPA19-31 Is a Potent Competitive Antagonist of the Interaction of Urokinase-Type Plasminogen Activator with Its Receptor (CD87)

Cyclo19,31[D-Cys19]-uPA19-31 Is a Potent Competitive Antagonist of the Interaction of Urokinase-Type Plasminogen Activator with Its Receptor (CD87)

Role of plasminogen activator-plasmin system in tumor angiogenesis

Phage display selection on whole cells yields a small peptide specific for HCV receptor human CD81

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