Induced Fit of an Epitope Peptide to a Monoclonal Antibody Probed with a Novel Parallel Surface Plasmon Resonance Assay

Baggio, Rick; Carven, Gregory J.; Chiulli, Anthony; Palmer, Michelle; Stern, Lawrence J.; Arenas, Jaime

doi:10.1074/jbc.m410687200

Cited by 24 publications

(13 citation statements)

References 27 publications

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“…In the following data evaluation, we therefore initially focused on k off values, which seemed reasonable, as this rate constant furthermore yielded the largest contribution to the global change in the Gibbs free energy of binding (⌬⌬G). The impact of specific side chain deletion primarily on k off rather than on k on is concordant with reports for other protein/protein interactions probed by alanine scanning mutagenesis (46,47). The quality of the data evaluation for these interactions is illustrated in supplemental Fig.…”

Section: Resultssupporting

confidence: 71%

Characterization of the Functional Epitope on the Urokinase Receptor

Gårdsvoll

Gilquin

et al. 2006

Journal of Biological Chemistry

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The high affinity interaction between the serine protease urokinase-type plasminogen activator (uPA) and its glycolipid-anchored receptor (uPAR) represents one of the key regulatory steps in cell surface-associated plasminogen activation. On the basis on our crystal structure solved for uPAR in complex with a peptide antagonist, we recently proposed a model for the corresponding complex with the growth factor-like domain of uPA (Llinas et al. (2005) EMBO J. 24, 1655-1663). In the present study, we provide experimental evidence that consolidates and further develops this model using data from a comprehensive alanine scanning mutagenesis of uPAR combined with low resolution distance constraints defined within the complex using chemical cross-linkers as molecular rulers. The kinetic rate constants for the interaction between pro-uPA and 244 purified uPAR mutants with single-site replacements were determined by surface plasmon resonance. This complete alanine scanning of uPAR highlighted the involvement of 20 surface-exposed side chains in this interaction. Mutations causing ⌬⌬G > 1 kcal/mol for the uPA interaction are all located within or at the rim of the central cavity uniquely formed by the assembly of all three domains in uPAR, whereas none are found outside this crevice. Identification of specific cross-linking sites in uPAR and pro-uPA enabled us to build a model of the uPAR⅐uPA complex in which the kringle domain of uPA was positioned by the constraints established by the range of these cross-linkers. The nature of this interaction is predominantly hydrophobic and highly asymmetric, thus emphasizing the importance of the shape and size of the central cavity when designing low molecular mass antagonists of the uPAR/uPA interaction.The urokinase-type plasminogen activator receptor (uPAR) 2 is a glycosylphosphatidylinositol-anchored membrane glycoprotein (1) that has a primary role in focalizing plasminogen activation at the cell surface through its specific high affinity interaction with the urokinase-type plasminogen activator (uPA). Besides facilitating the generation of plasmin activity in the vicinity of uPAR-expressing cells, which is directly or indirectly involved in remodeling of the extracellular matrix (2, 3), the uPAR/pro-uPA interaction also assists in regulating other aspects of cell adhesion and migration. Among these molecular processes is the direct interaction with matrix-deposited vitronectin (4); the modulation of integrin function, in particular ␣ M ␤ 2 , ␣ 5 ␤ 1 , and ␣ 3 ␤ 1 (5-8); and the activation of the chemotactic FPRL1 receptor (9). As an increased expression level of uPAR is often found in the invasive areas of various human cancers and correlates with poor prognosis (10), the uPAR/uPA interaction and uPA catalytic activity are considered relevant molecular targets for drug development (11-13). Intervention strategies developed for targeting the uPAR/uPA interaction with a view to cancer therapy include recombinant fusion proteins containing the receptor-binding module of uPA (14,...

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Section: Resultssupporting

confidence: 71%

Characterization of the Functional Epitope on the Urokinase Receptor

Gårdsvoll

Gilquin

et al. 2006

Journal of Biological Chemistry

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“…(Tables 1 and 2). The on rates of the three peptides are very similar, as is typically observed for the structurally similar peptide analogs (1). In contrast, the off rates vary by an order of magnitude, consistent with the various stabilities of the bound peptides as reflected by a well-positioned thioether tether (104-2) versus a poorly positioned thioether tether (74-2) compared to the linear peptide 84-1.…”

Section: Resultssupporting

confidence: 48%

Structure-Function Analysis of the Epitope for 4E10, a Broadly Neutralizing Human Immunodeficiency Virus Type 1 Antibody

Brunel¹,

Zwick²,

Cardoso³

et al. 2006

J Virol

124

121

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The human immunodeficiency virus type 1 (HIV-1) neutralizing antibody 4E10 binds to a linear, highly conserved epitope within the membrane-proximal external region of the HIV-1 envelope glycoprotein gp41. We have delineated the peptide epitope of the broadly neutralizing 4E10 antibody to gp41 residues 671 to 683, using peptides with different lengths encompassing the previously suggested core epitope (NWFDIT). Peptide binding to the 4E10 antibody was assessed by competition enzyme-linked immunosorbent assay, and the K d values of selected peptides were determined using surface plasmon resonance. An Ala scan of the epitope indicated that several residues, W672, F673, and T676, are essential (>1,000-fold decrease in binding upon replacement with alanine) for 4E10 recognition. In addition, five other residues, N671, D674, I675, W680, and L679, make significant contributions to 4E10 binding. In general, the Ala scan results agree well with the recently reported crystal structure of 4E10 in complex with a 13-mer peptide and with our circular dichroism analyses. Neutralization competition assays confirmed that the peptide NWFDITNWLWYIKKKK-NH 2 could effectively inhibit 4E10 neutralization. Finally, to limit the conformational flexibility of the peptides, helix-promoting 2-aminoisobutyric acid residues and helix-inducing tethers were incorporated. Several peptides have significantly improved affinity (>1,000-fold) over the starting peptide and, when used as immunogens, may be more likely to elicit 4E10-like neutralizing antibodies. Hence, this study represents the first stage toward iterative development of a vaccine based on the 4E10 epitope.

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“…Here, incident light hits the metal sensor layer from the top passing through the analyte containing low refractive index medium. This eliminates on the one hand the need for a high refractive index prism for every measurement channel and so makes this architecture attractive for high-throughput screening purposes [25]. But on the other hand, it also exhibits the big disadvantage that the exciting light has to incite through the analyte matrix, which will very often interfere with the light in terms of absorption or diffraction rendering a SPR measurement difficult if not impossible.…”

Section: Spr Sensors For Cell Detectionmentioning

confidence: 98%

“…3b) [25][26][27]. Here, incident light hits the metal sensor layer from the top passing through the analyte containing low refractive index medium.…”

Section: Spr Sensors For Cell Detectionmentioning

confidence: 99%

Surface plasmon resonance sensors in cell biology: basics and application

Robelek

2009

Bioanal Rev

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Optical sensors based on the excitation of surface plasmons, referred to as surface plasmon resonance (SPR) sensors, have become a central analytical tool for characterizing and quantifying a wide variety of macromolecular interactions, like receptor-ligand contacts. Besides this classical field of application, in the last 15 years, the development of SPR sensors aiming for the detection and analysis of ligand/cell or host/pathogen interactions, cell/ cell contacts, and cellular reactions gained considerable momentum. The number of publications reporting about applications of SPR sensors implementing vital prokaryotic or eukaryotic cells as biorecognition elements for medical diagnostics, environmental monitoring, or biological safety is steadily growing. This review gives a short introduction to the technique of surface plasmon resonance and the parameters that are important for its application in the field of vital cell sensors. Furthermore, the publications concerning the application of such sensors in the analysis of cellular interactions and cellular reactions to extra-and intracellular stimuli are summarized.

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Induced Fit of an Epitope Peptide to a Monoclonal Antibody Probed with a Novel Parallel Surface Plasmon Resonance Assay

Cited by 24 publications

References 27 publications

Characterization of the Functional Epitope on the Urokinase Receptor

Characterization of the Functional Epitope on the Urokinase Receptor

Structure-Function Analysis of the Epitope for 4E10, a Broadly Neutralizing Human Immunodeficiency Virus Type 1 Antibody

Surface plasmon resonance sensors in cell biology: basics and application

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