The Kinetics of PDZ Domain-Ligand Interactions and Implications for the Binding Mechanism

Gianni, Stefano; Engström, Åke; Larsson, Mårten; Calosci, Nicoletta; Malatesta, Francesco; Eklund, Lars; Ngang, Chi Celestine; Travaglini-Allocatelli, Carlo; Jemth, Per

doi:10.1074/jbc.m506017200

Cited by 88 publications

(140 citation statements)

References 38 publications

Supporting

Mentioning

129

Contrasting

Unclassified

Order By: Relevance

“…The numbering of residues refers to full length PSD-95α without exon b and is the same as used in Doyle et al 13 The F337W mutation serves as a fluorescence probe in ligand binding experiments and does not affect the affinity of the PDZ3-peptide interaction. [16][17][18] It also does not affect the energetic coupling pattern between side-chain residues in the PDZ domain and in the peptide ligand 9 , since the coupling energy for F337W is zero with regard to a second mutation in the peptide ligand, either at the C-terminal Val 0 or at Ser -2 (not shown). The sequence corresponding to the α3-helix (residues 396-401) was deleted from the cDNA of PDZ3 to generate the α3-helix-deleted mutant PDZ3∆α3.…”

Section: Methodsmentioning

confidence: 99%

Interactions outside the Boundaries of the Canonical Binding Groove of a PDZ Domain Influence Ligand Binding

et al. 2012

Self Cite

View full text Add to dashboard Cite

Section: Methodsmentioning

confidence: 99%

Interactions outside the Boundaries of the Canonical Binding Groove of a PDZ Domain Influence Ligand Binding

et al. 2012

Self Cite

View full text Add to dashboard Cite

“…k on is the association or on-rate constant, k off is the dissociation or off-rate constant, and [A] 0 and n are the initial concentrations of the varied and constant species, respectively (20,21). The slow phase observed upon mixing PDZ1-2* with dimeric peptide, which increased up to a constant value with peptide concentration, was analyzed with a model-free polynomial equation (Equation 4), to calculate k obs at 15 M dimeric peptide by intrapolation.…”

Section: Methodsmentioning

confidence: 99%

Deciphering the Kinetic Binding Mechanism of Dimeric Ligands Using a Potent Plasma-stable Dimeric Inhibitor of Postsynaptic Density Protein-95 as an Example

Celestine

Bach

Gottschalk

et al. 2010

Journal of Biological Chemistry

Self Cite

View full text Add to dashboard Cite

Dimeric ligands can be potent inhibitors of protein-protein or enzyme-substrate interactions. They have increased affinity and specificity toward their targets due to their ability to bind two binding sites simultaneously and are therefore attractive in drug design. However, few studies have addressed the kinetic mechanism of interaction of such bivalent ligands. We have investigated the binding interaction of a recently identified potent plasma-stable dimeric pentapeptide and PDZ1-2 of postsynaptic density protein-95 (PSD-95) using protein engineering in combination with fluorescence polarization, isothermal titration calorimetry, and stopped-flow fluorimetry. We demonstrate that binding occurs via a two-step process, where an initial binding to either one of the two PDZ domains is followed by an intramolecular step, which produces the bidentate complex. We have determined all rate constants involved in the binding reaction and found evidence for a conformational transition of the complex. Our data demonstrate the importance of a slow dissociation for a successful dimeric ligand but also highlight the possibility of optimizing the intramolecular association rate. The results may therefore aid the design of dimeric inhibitors in general.Biological molecules that comprise two or more binding units enable di-or multivalent binding to their protein partners. This concept is well known in nature as a way to increase affinity and selectivity, such as in virus-cell and antibody-antigen recognition (1). Consequently, linking two ligands together can be a strategy to enhance binding of drug candidates to therapeutically relevant proteins by exploiting a bivalent binding site (2-5). It is proposed that such dimeric inhibitors will foster a more potent response by increasing the affinity toward their targets by some hundred-fold (6, 7). Indeed, in vitro binding studies have shown improved affinities of dimeric inhibitors toward their targets as compared with their monomeric counterparts (5, 8 -11). It is complex to predict the overall affinity enhancement by linking two ligands because the observed binding energy is not a direct summation of the binding energies of individual components, and the entropy and enthalpy compensation are difficult to estimate (6,7,12). Therefore, experimental determination of the binding mechanism of dimeric ligands is useful for future design of dimeric ligands. However, there are only a few cases where in solution methods have been used to determine the mechanism of interaction of such ligands (5,7,10). One class of proteins where dimeric ligands have been exploited in an attempt to develop potential inhibitors for therapeutically relevant interactions in the cell is the PDZ (PSD-95/Dlg/Zonula occludens-1) domain family of proteins (5, 8). PDZ domains constitute a class of protein-protein interacting modules that functions as scaffolds and adapters in signaling cascades, and they are found in a few hundred proteins in the human genome (13). PDZ domains generally bind to the C termini of thei...

show abstract

“…43) as well as a short His-tag, which does not influence the folding of PDZ3 (21). Expression and purification were as described earlier (37,46). The purity was checked by SDS/PAGE and the identity, by MALDI-TOF mass spectrometry.…”

Section: Methodsmentioning

confidence: 99%

Comparison of successive transition states for folding reveals alternative early folding pathways of two homologous proteins

Calosci

Celestine

Richter

et al. 2008

Proc. Natl. Acad. Sci. U.S.A.

Self Cite

View full text Add to dashboard Cite

The energy landscape theory provides a general framework for describing protein folding reactions. Because a large number of studies, however, have focused on two-state proteins with single well-defined folding pathways and without detectable intermediates, the extent to which free energy landscapes are shaped up by the native topology at the early stages of the folding process has not been fully characterized experimentally. To this end, we have investigated the folding mechanisms of two homologous threestate proteins, PTP-BL PDZ2 and PSD-95 PDZ3, and compared the early and late transition states on their folding pathways. Through a combination of ⌽ value analysis and molecular dynamics simulations we obtained atomic-level structures of the transition states of these homologous three-state proteins and found that the late transition states are much more structurally similar than the early ones. Our findings thus reveal that, while the native state topology defines essentially in a unique way the late stages of folding, it leaves significant freedom to the early events, a result that reflects the funneling of the free energy landscape toward the native state.energy landscape ͉ kinetics ͉ molecular dynamics ͉ phi analysis ͉ protein folding T he description of the folding process of a protein in terms of pathways on a free energy landscape has provided much insight into the mechanism of the folding reaction (1-4). Free energy landscapes of many proteins appear to resemble the shape of a funnel that guides the folding process toward the native state (5-7). According to this view, folding is considered a stochastic process so that a protein reaches its native conformation through folding pathways made up by an ensemble of different trajectories (6,(8)(9)(10). It has been difficult, however, to establish experimentally the extent to which these trajectories can differ from each other, in particular in the wider region of the free energy funnel corresponding to the initial stages of the folding process, where a considerable heterogeneity may be expected. Many proteins exhibit single folding pathways composed of families of closely related trajectories, but parallel folding pathways have also been observed (11), as well as significant changes of pathways and transition state structures upon circular permutation (12, 13) or solvent conditions (14-16). In addition, different transition state structures were characterized in two homologous proteins with a highly symmetric native structure (17).To obtain a glimpse of the width of the free energy landscape at the early stages of the folding reaction, we compared the folding pathways of two homologous three-state proteins. The study of homologous proteins represents a powerful approach to obtain insight into the process of protein folding (18-22), especially when combined with structural information on intermediate events (17,(23)(24)(25). The transition states of two-state proteins were compared in a series of studies (17, 23, 24, 26).Here we present a vivid illustration of...

show abstract

The Kinetics of PDZ Domain-Ligand Interactions and Implications for the Binding Mechanism

Cited by 88 publications

References 38 publications

Interactions outside the Boundaries of the Canonical Binding Groove of a PDZ Domain Influence Ligand Binding

Interactions outside the Boundaries of the Canonical Binding Groove of a PDZ Domain Influence Ligand Binding

Deciphering the Kinetic Binding Mechanism of Dimeric Ligands Using a Potent Plasma-stable Dimeric Inhibitor of Postsynaptic Density Protein-95 as an Example

Comparison of successive transition states for folding reveals alternative early folding pathways of two homologous proteins

Contact Info

Product

Resources

About